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REFINEMENT AND INTEGRATION OF PCR-BASED DETECTION AND CLASSIC VIRUS ISOLATION METHODS FOR IMPROVED AEROVIROLOGY,
ARBOVIROLOGY, AND INFECTION CONTROL VIROLOGY RISK ASSESSMENTS
By
TANIA S. BONNY
A DISSERTATION PRESENTED TO THE GRADUATE SCHOOL OF THE UNIVERSITY OF FLORIDA IN PARTIAL FULFILLMENT
OF THE REQUIREMENTS FOR THE DEGREE OF DOCTOR OF PHILOSOPHY
UNIVERSITY OF FLORIDA
2017
© 2017 Tania S. Bonny
To almighty God. For creating me and taking care of me in every step of this eventful life. May I return to you as an enlightened soul.
4
ACKNOWLEDGMENTS
I would like to thank all who contributed to preparing this dissertation: my co-
authors, lab members, peers and officials at Environmental and Global Health
department. My profound gratitude to my respected committee members: Dr. John A.
Lednicky, Dr. Tara Sabo-Attwood, Dr. Song Liang, and Dr. Chang-Yu Wu, for their
constant support and guidance. Forever in debt to my wonderful mentor, Dr. John A.
Lednicky, I am blessed to have his guidance and inherit a tiny bit of his keen eye for
details, sense of humor, patience, kindness and an out of the box attitude to look at
everything.
I am grateful to my loving parents who always believed in my potential and let me
fly higher. I hope to make you proud in this life and hereafter. Hugs to my one and only
brother who has always been my best friend and lent his shoulder when I needed the
most. Finally, I must convey my sincere gratitude to almighty God for giving me a
privileged life with abundant love, care and strong support system.
This dissertation research was funded with multiple funding sources: (a) National
Science Foundation (Grant No. IDBR-1353423), (b) Aerosol Dynamics, Inc. and (c)
Internal funds from University of Florida to Dr. John A. Lednicky.
I declare an absence of competing interests with the information presented in this
dissertation. In addition, I also assume full responsibility for the collection and analysis
of all data.
5
TABLE OF CONTENTS page
ACKNOWLEDGMENTS .................................................................................................. 4
LIST OF TABLES ............................................................................................................ 8
LIST OF FIGURES ........................................................................................................ 10
LIST OF ABBREVIATIONS ........................................................................................... 12
ABSTRACT ................................................................................................................... 16
CHAPTER
1 BACKGROUND ...................................................................................................... 18
2 COLLECTION OF VIABLE VIRUS AEROSOLS USING THE SKC BIOSAMPLER: EVALUATION OF REVISED COLLECTION PROCEDURES ....... 27
Introduction ............................................................................................................. 27 Materials and Methods............................................................................................ 28
Sampling Sites and Dates ................................................................................ 28 Aerosol Collection System................................................................................ 29
Preparation of Cell Lines .................................................................................. 31 Virus Isolation ................................................................................................... 31 Rapid Detection of Influenza A and B Viruses .................................................. 32
GenMark Respiratory Viral Panel ..................................................................... 32 Identification of Influenza Virus Types and Subtypes and Genomic
Sequencing ................................................................................................... 33 Identification of Miscellaneous Respiratory Viruses ......................................... 33
Results .................................................................................................................... 33 Isolation and Identification of Viable Viruses in Aerosols Collected in Spring
2016 (April 4- 20) .......................................................................................... 33
Isolation and Identification of Viable Viruses in Aerosols Collected in Early Fall (August- September) 2016 ..................................................................... 34
Isolation and Identification of Viable Viruses in Aerosols Collected after Thanksgiving (December) 2016 .................................................................... 34
Discussion .............................................................................................................. 35
3 EVALUATION OF THE COLLECTION EFFICIENCY OF THE VIABLE VIRUS AEROSOL SAMPLER IN A STUDENT HEALTH CARE CENTER ......................... 50
Introduction ............................................................................................................. 50 Materials and Methods............................................................................................ 53
Healthcare Facility ............................................................................................ 53 Sampling Dates ................................................................................................ 53
6
Aerosol Collection System................................................................................ 53
Air Sampler Placement ..................................................................................... 54 Virology Laboratory .......................................................................................... 55
Air Sampler Collection Media Volume Reduction and Adjustment ................... 55 Cell Lines .......................................................................................................... 55 Cell Culture Media Formulations for Virus Isolation .......................................... 57 Inoculation, Maintenance, and Observation of Cell Cultures ............................ 57 Identification of Human Respiratory Viruses ..................................................... 58
GenMark Respiratory Virus Panel .................................................................... 58 Rapid Detection of Influenza A and B Viruses in Cell Cultures ......................... 59 Identification of Influenza Virus Types and Subtypes and Genomic
Sequencing ................................................................................................... 59 Identification of Respiratory Syncytial Virus Subtype A (RSV-A) ...................... 59
Identification of Miscellaneous Respiratory Viruses ......................................... 61
Results .................................................................................................................... 61
Isolation and Identification of Viable Viruses in Aerosols Collected March 11, 2016 ........................................................................................................ 61
Isolation and Identification of Viable Viruses Collected in Aerosols on March 28, 2016 ........................................................................................................ 63
Isolation of Only One Type of Viable Virus from Aerosols on April 8, 2016. ..... 63 Discussion .............................................................................................................. 63
4 ISOLATION AND IDENTIFICATION OF HUMAN CORONAVIRUS 229E FROM FREQUENTLY TOUCHED ENVIRONMENTAL SURFACES IN A CLASSROOM ......................................................................................................... 92
Introduction ............................................................................................................. 92
Materials and Methods............................................................................................ 93
Study Period and Site ....................................................................................... 93 Ethics................................................................................................................ 93
Environmental Surfaces ................................................................................... 94 Sample Collection ............................................................................................ 94 Cell Cultures for Virus Isolation ........................................................................ 94
GenMark RVP Assay ....................................................................................... 96 Whole Genome Sequencing of CoV-229E ....................................................... 96 Assessment of CoV-229E Stability under Classroom Ambient Light,
Temperature and Humidity Conditions .......................................................... 96 Results .................................................................................................................... 98
Discussion .............................................................................................................. 99
5 COMPLETE GENOME SEQUENCE OF ENTEROVIRUS D68 DETECTED IN CLASSROOM AIR AND ON ENVIRONMENTAL SURFACES ............................. 107
Introduction ........................................................................................................... 107
Methods and Materials.......................................................................................... 108 Results and Discussions ....................................................................................... 108
7
6 DETECTION OF ALPHACORONAVIRUS vRNA IN THE FECES OF BRAZILIAN FREE-TAILED BATS (TADARIDA BRASILIENSIS) FROM A COLONY IN FLORIDA, USA ................................................................................ 110
Introduction ........................................................................................................... 110 Materials and Methods.......................................................................................... 112
Collection and Processing of Bat Feces Samples .......................................... 112 Virus Isolation Attempts in Cell culture ........................................................... 113 Screening of Viral Nucleic Acids for Coronavirus RNA ................................... 113
Phylogenetic Analyses of the CoV RdRp Sequences .................................... 114 Results .................................................................................................................. 115 Discussion ............................................................................................................ 116
7 ISOLATION AND DETECTION OF ARBOVIRUSES AND HUMAN CORONAVIRUS 229E IN BLOOD COLLECTED FROM CHILDREN IN RURAL HAITI IN 2016 ....................................................................................................... 120
Introduction ........................................................................................................... 120 Methods and Materials.......................................................................................... 121
Initial Screen of Plasma Samples for Zika-, Dengue- and Chikungunya Viruses ........................................................................................................ 122
Virus Isolation in Cell Cultures ........................................................................ 122
RT-PCR of vRNA Purified from Spent Cell Growth Media and Infected Cells 123 Sequencing .................................................................................................... 123
GenMark RVP Assay ..................................................................................... 124 Results .................................................................................................................. 124
Isolation and Identification of ZIKV in Plasma Sample Cell Culture ................ 124
Isolation and Identification of DENV-3 in Plasma Sample Cell Culture .......... 125 Co-infection of Plasma Cell Culture with ZIKV and DENV-4 .......................... 125 Isolation and Identification of Human coronavirus 229E (CoV-229E) ............. 125
Discussion ............................................................................................................ 126
8 CONCLUDING REMARKS ................................................................................... 138
LIST OF REFERENCES ............................................................................................. 144
BIOGRAPHICAL SKETCH .......................................................................................... 163
8
LIST OF TABLES
Table page 2-1 Air sample collection during 2016 using the BioSampler .................................... 39
2-2 Air sample cell culture ........................................................................................ 40
2-3 Primers for the detection of and subtyping of influenza A virus. ......................... 41
2-4 Primers for the detection of and subtyping of human metapneumovirus, human parainfluenza virus and human coronaviruses. ...................................... 42
2-5 GenBank accession numbers for Influenza A virus gene sequences ................. 43
2-6 Amino acid changes in the deduced HA of H1N1 isolated December 05, 2016. .................................................................................................................. 43
2-7 Amino acid changes in the deduced NA of H1N1 isolated December 05, 2016. .................................................................................................................. 46
2-8 Amino acid changes in the deduced M proteins of H1N1 isolated December 05, 2016. ............................................................................................................ 49
3-1 Viable viruses in aerosols collected on March 11, 2016. .................................... 77
3-2 Viable viruses in aerosols collected on March 28, 2016. .................................... 77
3-3 Cell lines used for the isolation of common culturable human respiratory viruses. ............................................................................................................... 79
3-4 Primers for the detection of and subtyping of influenza A and B viruses. ........... 80
3-5 GenBank accession numbers for Influenza A and B virus sequences, March 11, 2016. ............................................................................................................ 81
3-6 GenBank accession numbers for RSV-A NS2 and N gene partial cds sequences. ......................................................................................................... 81
3-7 Amino acid substitutions in the HA protein of H1N1 viruses from March 11, 2016. .................................................................................................................. 82
3-8 Amino acid changes in the deduced NA of H1N1 isolated March 11. ................. 85
3-9 Amino acid changes in the deduced M proteins of H1N1 from March 11, 2016. .................................................................................................................. 87
3-10 Amino acid sequences at HA major immunogenic epitopes A and B1 of influenza H3N2 viruses in Gainesville, Florida, March 11, 2016. ........................ 89
9
3-11 Amino acid sequence differences in the NA of influenza H3N2 viruses, in Gainesville, Florida, March 11, 2016. ................................................................. 91
4-1 Development of virus induced CPE in inoculated cell lines. ............................. 106
7-1 Haiti plasma sample cell culture report ............................................................. 136
10
LIST OF FIGURES
Figure page 1-1 The five major global respiratory conditions: Forum of International
Respiratory Societies, 2013 ................................................................................ 26
1-2 Disease Burden of Influenza, CDC ..................................................................... 26
2-1 Schematic diagram of the SKC BioSampler (left) [image adapted from ............. 38
3-1 Schematic diagram of viable virus aerosol sampler (VIVAS) .............................. 69
3-2 Schematic diagram of the testing system ........................................................... 70
3-3 Schematic layout of the student infirmary lobby. Top: first floor, bottom: second floor. ....................................................................................................... 71
3-4 MDCK cells in serum-free cell culture medium plus trypsin.. .............................. 72
3-5 Solid-phase ELISA tests.. ................................................................................... 73
3-6 Representative GenMark RVP report of MDCK cells inoculated with collection medium from VIVAS sampling interval # 2, March 28, 2016.. ............. 74
3-7 MRC-5 and A549 cells in serum-free cell culture medium plus trypsin.. ............. 75
3-8 VERO E6 and LLC-MK2 cells in serum-free cell culture medium plus trypsin. ... 76
4-1 Isolation of CoV-229E in VERO E6 and A549 cells at 33°C. ............................ 103
4-2 eSensor Respiratory Viral Panel currents report for desk top7 (collected on 23 November 2016) inoculated cell culture sample. ......................................... 104
4-3 Stability of CoV-229E on different hard surfaces over a 7-day observation period. .............................................................................................................. 105
6-1 Representative results of RT-PCR detection of alphacoronavirus vRNA in Brazilian free-tailed bat feces. .......................................................................... 118
6-2 Maximum likelihood tree based on the nucleotide sequences of partial RdRp gene of bat CoVs .............................................................................................. 119
7-1 Appearance of ZIKV-induced CPE in LLC-MK2 and VERO E6 cells. ............... 129
7-2 Appearance of DENV-induced CPE in VERO E6 and MRC-5 cells .................. 130
7-3 Appearance of CPE in LLC-MK2 cells induced by ZIKV-DENV co-infection .... 131
11
7-4 Appearance of CPE in VERO E6 cells induced by ZIKV-DENV co-infection .... 132
7-5 Representative results of RT-PCR detection of Zika virus in LLC-MK2 cells inoculated with patient plasma samples. .......................................................... 133
7-6 Appearance of VERO E6 and MRC-5 cells during cell culture. ........................ 134
7-7 Representative eSensor Respiratory Viral Panel currents report (RUO) .......... 135
12
LIST OF ABBREVIATIONS
A549 Human adenocarcinomic alveolar basal epithelial cells
aDMEM Advanced Dulbecco's modified Eagle's medium
AE Alcohol ethoxylates
AGI All-glass impinger
AMV Avian myeloblastosis virus
ARIs Acute respiratory illnesses
ATCC American Type Culture Collection
BLAST Basic local alignment search tool
BSA Bovine serum albumin
BSL2 Biosafety level 2
BtCoVs Bat coronaviruses
CDC Centers for Disease Control and Prevention, United States
CHIKV Chikungunya virus
CO2 Carbon dioxide
COPD Chronic obstructive pulmonary disease
CoV Coronavirus
CoV-229E Human coronavirus 229E
CPC Condensation particle counter
CPE Cytopathic effect
DALY Disability-adjusted life years
DENV Dengue virus
dpi Days post-infection
EGH Environmental and Global Health
ELISA Enzyme-linked immunosorbent assay
13
EMEM Eagle's minimal essential medium
EV-D68 Enterovirus D68
FASTA Fast alignment (program)
FBS Fetal bovine serum
FWC Florida Fish and Wildlife Conservation Commission
HA Influenza virus Hemagglutinin
HCoV-NL63 Human coronavirus NL63
HeLa Human cervical epithelial adenocarcinoma cell line (transformed with human papillomavirus)
HEPA High-efficiency particulate air
HIV Human immunodeficiency virus
hMPV Human metapneumovirus
HPIV Human parainfluenza virus
HPNP Health Professions/Nursing/Pharmacy complex
HVAC Heating, ventilation and air conditioning
IACUC Institutional Animal Care and Use Committee
IFV Influenza virus
IgG Immunoglobulin G
IRB Institutional Review Board
L/min Liters per min
LLC-MK2 Rhesus monkey (Macaca mulatta) kidney epithelial cell
LRT Lower respiratory tract
M1 & M2 Influenza virus Matrix proteins 1 & 2
MDCK NBL2 Madin-Darby canine (Canis familiaris) epithelial kidney cell line
MERS-CoV Middle East respiratory syndrome coronavirus
14
MHV Mouse hepatitis virus
MRC-5 Normal male human lung fibroblast cell line
nA Nanoampere
NA Influenza virus neuraminidase
NCBI The National Center for Biotechnology Information
NCI-H292 Human mucoepidermoid pulmonary carcinoma cell line
NEP Influenza virus nuclear export protein
NIOSH The National Institute for Occupational Safety and Health
NP Nucleocapsid
NS1 Influenza A virus Nonstructural protein 1
PBS Phosphate buffered saline
PCIS Personal cascade impactor sampler
PCR Polymerase chain reaction
pdm09 Influenza pandemic 2009
PSN Penicillin, streptomycin and neomycin
PVDF Polyvinylidene difluoride
RdRp RNA-dependent RNA polymerase
RFR Revised flow rate
RH Relative humidity
RSV Respiratory syncytial virus
RT Reverse transcriptase
RT-PCR Reverse transcription polymerase chain reaction
RUO Research use only
RVP Respiratory viral panel
15
SARS-CoV Severe acute respiratory syndrome coronavirus
SFR Manufacturer recommended standard flow rate
SRA Student reception area
TB Tuberculosis
Tb1 Lu Tadarida brasiliensis lung epithelium cell line
Temp Temperature
TGEV Transmissible gastroenteritis virus
TPCK L-1-tosylamido-2-phenylethyl chloromethyl ketone
URT Upper respiratory tract
UTM Universal transport medium
VERO E6 African green monkey (Chlorocebus sp.) kidney epithelial cell line
VIVAS Viable Virus Aerosol Sampler
vRNA Virus ribonucleic acid
VTM Virus transport medium
w/v Weight to volume
WHO World Health Organization
WI-38 Human normal lung diploid fibroblast cell line
ZIKV Zika virus
16
Abstract of Dissertation Presented to the Graduate School of the University of Florida in Partial Fulfillment of the Requirements for the Degree of Doctor of Philosophy
REFINEMENT AND INTEGRATION OF PCR-BASED DETECTION AND CLASSIC
VIRUS ISOLATION METHODS FOR IMPROVED AEROVIROLOGY, ARBOVIROLOGY, AND INFECTION CONTROL VIROLOGY RISK ASSESSMENTS
By
Tania S. Bonny
August 2017
Chair: John A. Lednicky Major: Public Health
In preparation for a career in public health virology in Bangladesh, work detailed
in this dissertation focused on the development of knowledge and expertise in two
aspects of virology: (a) The collection of virus aerosols, and (b) Identification of
pandemic arboviruses.
The significance of respiratory virus transmission through inhalation of
aerosolized viruses remains contentious because effective tools and methods are
lacking to adequately assess the occurrence and risks thereof. A major technical
hindrance is the lack of air samplers that can efficiently collect virus aerosols. In this
dissertation, the efficiencies of the SKC BioSampler and that of a newly developed
device, the Viable Virus Aerosol Sampler (VIVAS), for the collection of aerosols of
viable virus in indoor settings, were evaluated. Separately, for insights on the
importance of contact transmission of respiratory viruses, swab samples of frequently
touched surfaces were collected and virus isolation attempted in cell cultures, and a
pilot study was conducted to discover potential viral respiratory pathogens in local bats.
The VIVAS out-performed the BioSampler at collecting viable virus aerosols, and is
17
potentially the best air sampling device currently available for the collection of virus
aerosols. Surface sampling revealed viable Human coronavirus 229E and other viruses
on frequently touched indoor surfaces, reinforcing that contact transmission may also be
a route of respiratory virus transmission. An alphacoronavirus RNA-dependent RNA
polymerase gene sequence was detected in bat feces, reinforcing the notion that
Florida bats may indeed be a source of potential respiratory pathogens.
The explosive spread of arthropod-borne viruses (arboviruses) into new
geographical areas is alarming. A contemporary and ongoing series of arbovirus
outbreaks over the past years in Haiti served as a training and learning platform.
Multiple arboviruses [Zika virus (ZIKV), Dengue virus (DENV) types 3 & 4] were isolated
from plasma samples collected between March and May 2016, indicating active co-
circulation of arboviruses during that period in Haiti, whereas only one virus was thought
responsible for that outbreak. Surprisingly, Human coronavirus 229E was isolated from
the plasma of one patient thought to have an arbovirus infection. This is the world’s first
record of that virus in human plasma.
18
CHAPTER 1 BACKGROUND
This dissertation work focused on the development of knowledge and expertise
in preparation for a career in public health virology in Bangladesh. In particular, two
virology topics of significant importance to Bangladesh were emphasized: (a) The
dynamics of airborne respiratory virus transmission, and (b) Identification of arboviruses
in acute human infections.
Acute respiratory infections continue to be the leading cause of morbidity and
mortality worldwide, especially in developing countries [1; Figure 1-1]. Notable human
respiratory diseases of the upper respiratory tract (URT) include influenza (“flu”) and
acute viral nasopharyngitis (“common cold”), which affect people across all age groups.
In the Unites States, influenza alone places a substantial burden on human health each
year. According to CDC estimates, influenza has been implicated in 9.2 - 60.8 million
illnesses, 40,000 - 710,000 hospitalizations and 12,000 - 56,000 deaths in the US
annually since 2010 [2; Figure 1-2]. Taken together, it is safe to assume that the overall
disease burden caused by influenza virus (IFV) and other human respiratory viruses is
likely to be much higher than current CDC estimates for influenza.
Influenza A, B and C viruses (and possibly the recently discovered Influenza D
virus) are the causative agents of influenza in humans. Severe influenza in the USA is
typically caused by influenza A and B viruses. The symptoms of influenza may include
chills, fever, cough, sore throat, runny nose, sneezing, muscle or body aches,
headache, fatigue and others such as chest pain. Clinically similar but generally less
severe manifestations of URT infection occur during episodes of the common cold. The
respiratory viruses most often implicated in the common cold are human rhinoviruses,
19
though coronaviruses, respiratory syncytial viruses, parainfluenza viruses, influenza
viruses, adenoviruses, metapneumovirus, and enteroviruses other than rhinoviruses are
possible causative agents [3]. Apart from common cold, many of these human
respiratory viruses also cause severe, often potentially life-threatening conditions
involving the lower respiratory tract (LRT). Human rhinoviruses, once thought to cause
relatively mild URT illness, are now also linked to exacerbations of chronic pulmonary
disease and asthma; bronchiolitis in infants and children; and pneumonia in the elderly
and immunocompromised patients [4]. Respiratory syncytial virus (RSV), and to a lesser
extent, human metapneumovirus (hMPV) can cause a range of LRT infections like
bronchiolitis, pneumonia and croup (laryngotracheobronchitis), primarily infecting
children, but also causing significant morbidity and mortality in the elderly,
immunocompromised patients and those with chronic cardiopulmonary disease [5, 6].
Human coronavirus, parainfluenzavirus, adenovirus and various enteroviruses can also
affect the LRT and cause similar disease manifestations [7-10].
During the course of a respiratory disease, a patient may generate a cloud of
airborne particles through breathing, coughing, sneezing and talking. The exhaled
particles containing viruses can vary in size from few millimeter (large droplets) to
submicron (<1 𝜇m) [11]. The larger respiratory droplets travel a short distance in the air
and settle quickly. However, some of the particles are too small to settle. They include
“droplet nuclei” that result from evaporated larger particles and remain suspended in the
air [12]. These potentially virus containing droplet nuclei may vary in size, from “naked
virus” particles (20-300 nm) to micrometer sized (<5 𝜇m) particles that are aggregated
to fomites or encased in respiratory secretions [13].
20
To initiate a respiratory infection, a virus must (a) remain viable (“live”; infectious)
in the ambient breathing air or on environmental surfaces, and (b) be able to transmit to
the respiratory tract of a susceptible person. Human respiratory viruses can be
transmitted from one person to another through various routes of infection. Four have
been identified as the major routes for many of these viruses:
1. Droplet infection occurs when respiratory droplets deposit on the mucous membranes of the upper respiratory tract (URT), such as the mouth and nose.
Droplets that are 10 m remain in the URT and do not reach the lower respiratory tract (LRT) [14].
2. Inhalation of small aerosols and droplet nuclei: Small aerosol particles (≤5 m) including the droplet nuclei can reach the LRT. These particles can also deposit on the URT surface, but the infection risk and disease severity may increase when they reach the lungs in the LRT [14-17].
3. Contact transmission: occurs as a result of direct contact between susceptible host and infected individual(s). It can also occur indirectly when virus-containing fomites are transferred to the mucous membrane of the URT of a susceptible host [14].
4. Ocular infection: may occur when airborne respiratory viruses (presumably either droplets or aerosols) come into contact with ocular surfaces. For instance, studies using animal models have shown that ocular surface can serve both as a site for virus entry and replication for airborne influenza viruses [18].
The relative importance of each of these routes remains poorly understood, with
the aerosol route being the most contentious one [11].
Infection risk analyses lack accuracy when they are solely based on detection of
virus genome [19], as breathing air and environmental surfaces always contain viruses
that have been inactivated through exposure to ultraviolet light, desiccation (drying), or
other means, and thus pose no health hazards [19]. Therefore, proof of virus viability
(i.e. presence of “live” virus) is important in order to assess the risk posed by respiratory
viruses transmitted via any of the above-mentioned routes. Current recommendations
for protection against the human respiratory viruses are mostly directed at prevention of
21
droplet transmissions assuming that viable (“live”), infectious viruses are transferred
only in large droplets that travel very short distance from the emitting source [20].
However, it is important to note that deposition of IFV-laden small particles into the
lower respiratory tract (LRT) may pose a greater health hazard compared to large
particle droplets deposited onto the URT [15-16, 21-23] because infection of the
alveolar cells in the LRT may lead to more severe diseases like pneumonia. It is,
therefore, important to assess the true inhalation or ocular biohazard risks posed by
airborne virus particles, especially aerosols and droplet nuclei, for the transmission of
respiratory diseases. For improved risk analyses and to partly fill critical knowledge
gaps regarding the transmission of respiratory viruses, environmental sampling aimed
at the isolation and identification of viable respiratory viruses in breathing air and on the
surfaces of living spaces is crucial. The knowledge gained from such studies would
inform policy makers and lead to the adoption and implementation of more effective
infection control and prevention strategies than currently exist. Otherwise, the fact that
respiratory viruses still exert a significant public health and economic burden even in
developed countries indicates that current infection control policies and procedures are
only partly effective.
The two commonly used methods for assessing microbiological quality of air are
passive monitoring and active sampling [24]. Passive monitoring using settle plates
have been used for detecting bacteria and fungi in the air. In active sampling, a known
volume of air is mechanically drawn in using an air sampling device and airborne
particles are collected onto a solid collection surface or into liquid collection medium.
The collected particles are subsequently removed from the device and analyzed. In
22
addition to collection of bacteria and fungi, active air sampling has also been used to
collect airborne virus particles [25]. However, several limiting factors pertaining to active
air sampling have impeded the collection of airborne respiratory viruses, namely: (1)
relatively low concentration of viruses in the ambient air, (2) low volume of air sample
collected by the sampling devices, (3) most air samplers do not separate collected
particles by size, (4) inefficiency at collecting submicron particles, and (5)
inactivation/loss of viability of the virus particles during collection [26-33]. All these
environmental factors and shortcomings in the existing air samplers signify the need for
an improved system for the effective collection of viable virus in submicron particles.
Apart from respiratory viruses, arthropod-borne viruses (arboviruses) are a
substantial threat to human and animal health worldwide due to a variety of evolving
factors such as climate change, anthropological behavior, commercial transportation
and land-remediation [34, 35]. Arboviruses are transmitted between arthropod vectors
(e.g. mosquitoes, ticks, sandflies, midges etc.) and vertebrates during the life cycle of
the virus [36]. Clinical manifestations of arbovirus infections can range from mild to life
threatening conditions [34]. The explosive spread of mosquito-borne viruses to new
geographical areas in the recent years has alarmed the public health community
worldwide. The continued presence of Dengue virus (DENV), Chikungunya virus
(CHIKV), and Zika virus (ZIKV) in endemic areas and their expansion through the
Americas place an estimated 3.9 billion people living in 120 different countries at risk
[37]. This has prompted researchers around the world to investigate arbovirus disease
epidemiology, prevention and control [37]. As part of the worldwide response to study
and eradicate arboviruses, researchers at University of Florida (UF) has initiated
23
projects to determine the causative agents and incidence of arbovirus infections in Haiti
and elsewhere in the Caribbean and in the Americas.
Specific aims: To advance our understanding of respiratory virus transmission
and to generate new insights on the etiology and incidence of arbovirus disease in the
New World, the work undertaken in this proposal had five specific aims:
1. To improve air sampling methods typically used for collection of viable human respiratory viruses using the SKC BioSampler.
Hypothesis: Based on cumulative experience at the laboratories of Drs. Lednicky
and Wu [including unpublished data], and from the published literature [11, 38-45], I
hypothesize that the collection of virus aerosols using the industry-standard device (the
SKC BioSampler) is inefficient and ineffective when the device is used according to the
manufacturer's instructions, and that the methodology can be improved by refining the
operating procedures. This will be tested by using the SKC BioSampler according to the
manufacturer’s instructions and by revised operating procedures for collection of virus
aerosol in indoor settings. Such experiments will facilitate comparisons between the
methodologies and help explain why previous studies using the BioSampler were not
very successful in collecting viable human respiratory viruses from breathing air.
2. To evaluate the viable virus collection efficiency of a newly developed Viable Virus Aerosol Sampler (VIVAS) in a student health care center.
Hypothesis: Based on the previous work at laboratories of Drs. Lednicky and Wu,
the VIVAS was reported to have a viable collection efficiency of ~74% for laboratory-
generated influenza A H1N1 virus [46]. I hypothesize that VIVAS will out-perform the
industry standard SKC BioSampler for the collection of viable virus aerosols. To test the
hypothesis, air samples will be collected using both devices operating simultaneously in
24
a student health care center and using these samples, attempts will be made to isolate
and identify respiratory viruses.
3. To collect, isolate and identify human respiratory viruses from frequently touched surfaces in classroom setting during influenza season.
Hypothesis: Frequently touched surfaces in classrooms harbor viable IFV and
other human respiratory viruses during outbreak of influenza viruses. This hypothesis
will be tested by collecting swab samples from surfaces in a classroom that is widely
used and frequently cleaned, and at a time when students are complaining of
respiratory infections.
4. To seek evidence of coronavirus shedding in the feces of Brazilian free-tailed bats in Florida.
Hypothesis: Bats are reservoirs of many emerging and reemerging zoonotic
viruses, some of which are highly pathogenic in humans. The probable origin of Severe
acute respiratory syndrome coronavirus (SARS-CoV) in bats [47, 48] and recent
findings of a bat coronavirus related to Middle East respiratory syndrome coronavirus
(MERS-CoV) in Mexican bats [49] suggest that the abundant, yet underexplored, bat
population in Florida could harbor coronaviruses, and it is possible they may be
pathogenic to humans. To test this hypothesis, feces samples of Brazilian free-tailed
bats will be obtained from a conservation site in Florida and tested if CoV can be
isolated after inoculation onto readily available cell lines and/or CoV vRNA detected in
the bat feces using molecular methods.
5. To identify the most probable causative agents and seek insights on the incidence of putative arbovirus infections in Haitians with undifferentiated febrile illnesses suspected to be due to arboviruses.
Hypothesis: The Haitian population continues to be vulnerable to arbovirus
diseases due to recurring natural disasters, poor infrastructures, and lack of resources
25
for disease diagnosis, prevention and control. Due to the abundance of mosquito
vectors in Haiti, and recent expansion of different arboviruses in the Americas, I
hypothesize that arboviruses are circulating in Haiti and can be detected in and isolated
from plasma and other proper specimens taken from Haitians with symptoms consistent
with those of arbovirus infections.
The subsequent chapters in this dissertation address the above-mentioned
research aims.
26
Figure 1-1. The five major global respiratory conditions: Forum of International Respiratory Societies, 2013 [1]
Figure 1-2. Disease Burden of Influenza, CDC [1]
27
CHAPTER 2 COLLECTION OF VIABLE VIRUS AEROSOLS USING THE SKC BIOSAMPLER:
EVALUATION OF REVISED COLLECTION PROCEDURES
Introduction
To assess the true risk of respiratory viruses in small airborne particles (5µm),
an air sampling device is required that can collect particles from nanometer to
supermicrometer size range [50]. The commonly used bioaerosol samplers are
optimized for the collection of micrometer-sized particles like bacteria and fungal spores
[50]. These devices are thus inefficient in collecting nano-sized virus aerosols [38, 39].
For instance, several research groups previously attempted to use devices like the SKC
BioSampler (the current industry standard device), the AGI-30, a frit bubbler, or a
NIOSH two-stage cyclone for collection of virus aerosols [40-42]. Hogan et al. reported
the physical collection efficiency (i.e. the ability of a sampler to aspirate airborne
particles into its inlet, followed by removal of the particles from the airstream and their
subsequent transfer to a collection medium [51]) of bacteriophages MS2 (virus particle
diameter, d=27.5 nm) and T3 (d=45 nm) particles in the size range of 20 -100 nm to be
below 10%, and the collection efficiency of viable viruses was lower yet [40]. One
notable study by Lednicky and Loeb (2013) employed two different active air samplers:
a Sioutas Personal Cascade Impactor Sampler (PCIS) and an SKC BioSampler, to
detect and isolate airborne IFV from an apartment with two influenza patients [11].
Viable IFV was collected by both the devices located up to 3.7m away from one of the
sick occupants. PCIS, when placed 1.2 m away from one sick individual, collected a
range of particle sizes containing viable IFV but when the device was placed at
distances 2.1 and 3.7 m away from the patient, only fine to ultrafine (≤2.5 𝜇m) particles
yielded viable IFV [8]. Using a NIOSH two-stage cyclone or a BioSampler, Lindsley et
28
al. (2010) were able to isolate IFV from only two of twenty samples collected from
influenza patients [41]. Lindsley et al. (2015), in another study were able to isolate
viable IFV from cough particles (0.3 - 8 μm) collected from seven of total sixty-four
symptomatic test subjects [42]. However, the reported low collection efficiency of viable
viruses could be also due to virus inactivation during the collection process, which
reduces the validity of the data acquired, making accurate risk assessment even more
difficult [52]. Therefore, an improved system for efficient collection of viable (“live”) virus
particles is critical to assess the risk of airborne disease transmission.
In this study, a comparison was made of the performance of two SKC
BioSampler units for collection of viable virus aerosol in indoor settings, one operating
according to the manufacturer’s instructions and the other following revised operating
procedures.
Materials and Methods
Approval by an institutional review board (IRB) was not necessary for this study
because human subjects were not studied and could not be identified, and the sources
of the viruses detected could not be tracked.
Sampling Sites and Dates
Prior to air sample collection, approvals were obtained from the respective
building managers at the UF. Based on the availability of the sampling sites, eight (n =
08) paired air samples were collected from Health Professions/Nursing/Pharmacy
Complex (HPNP) classrooms and the Reitz Union cafeteria. Both buildings have their
own heating, ventilation and air conditioning (HVAC) systems. Paired samples were
collected at different times in 2016, using two BioSampler units operating at two
different collection air flow rates. The sampling strategy and operating parameters are
29
summarized in Table 2-1. Air samples were collected in typically empty classrooms
between class sessions, with few students occasionally present. However, many
students were present at the Reitz Union cafeteria during air sample collections.
Aerosol Collection System
For this study, the SKC BioSampler (SKC, Inc., Eighty Four, PA, USA, catalog#
225-9597) was used for active air sampling. The BioSampler is a type of impinger: an
air sampling device that collects airborne particles into a liquid collection medium by
means of impaction and diffusion (Figure 2-1). Impaction occurs when particles in the
air, in response to a tight turn in the air streamlines, depart from the streamlines due to
their inertia, and impact onto a collection surface or into a collection media (as in the
case of the BioSampler). Diffusion is the Brownian motion of smaller particles. A swirling
motion (centrifugal motion) of the collection medium in the BioSampler is created by
passing air through three 0.630 mm tangential nozzles. The swirling flow generates
fewer bubbles and thus helps to minimize reaerosolization of already collected particles
and damage to the collected microbial agents [53]
Two BioSampler units operating at two different flow rates were used for air
sampling on each day. Based on previous field and laboratory tests [45, 54-55;
unpublished data], where lower sampling rates (6-8 L/min) have resulted in increased
collection of airborne viruses using the BioSampler, a revised flow rate of 8 L/min was
chosen for this study. Flow rates of 12.5 L/min (manufacturer recommended) for 30
minutes and 8 L/min (revised flow rate) for approximately 47 min were used to sample
approximately 375 liters (0.375 m3) of air/sampler. The sampling units were placed
beneath an intake air vent, in areas of active air flow and at a height of 1-1.5 m from the
floor. As operating two BioSampler units at close proximity using two different flow rates
30
may affect virus aerosol collection of individual device, the two devices were separately
run in short intervals (30-45 min). The samplers were sterilized by autoclaving and filled
with 15 mL collection medium containing sterile phosphate buffered saline (PBS) and
0.5% w/v purified bovine serum albumin (BSA) fraction V (Life Technologies, Grand
Island, NY, USA) [11, 17]. To achieve the desired air flow rate, the devices were
attached to GAST vacuum pumps (oil-less, rotary vane-type vacuum pump; GAST
Manufacturing, Inc., catalog# 1532-101-G557X). The pumps were turned on and
warmed up by running them for five minutes prior to use. In-line vapor traps (SKC Inc.,
catalog# 225-22-01) were connected between the SKC BioSamplers and GAST pumps
in order to protect the pump from moisture. Prior to air sampling, the operating air flow
rate for each BioSampler was calibrated using a rotameter (a single-ball portable air
flowmeter; SKC, Inc. catalog# 320-440). During calibration, the rotameter was attached
to the inlet of the BioSampler and GAST pump was attached to its outlet. The operating
pressure of the pump, read from a built-in manometer, was adjusted using the pump
valve lever, until the desired air flow rate was indicated in the rotameter. After
calibration, the rotameter was detached from the BioSampler inlet and the rest of the
assembled unit (BioSampler- vapor trap-GAST pump) was used for collection of air
sample (Figure 2-1).
After completion of air sampling at each flow rate, the collection medium from
each unit was aseptically transferred into sterile 50mL conical polypropylene tubes,
placed in an insulated ice box and transported immediately to the laboratory. Air sample
collection media were stored in pairs from each collection day: one medium labeled
“SFR” was collected from the BioSampler operating at 12.5 L/min (manufacturer
31
recommended standard flow rate), and other medium labeled “RFR” collected from the
other BioSampler unit operating at an air flow rate of 8 L/min (revised flow rate). As
summarized in Tables 2-1 and 2-2, paired samples# 1, 2 and 3 were collected during
spring season; samples# 4, 5 & 6 collected in early fall and samples# 7 & 8 collected
after the Thanksgiving holiday in 2016 (exact dates given in Table 2-1). All the collected
samples were stored at -80°C until virus isolation was attempted in cell cultures.
Preparation of Cell Lines
To favor isolation of different human respiratory viruses, a variety of readily
available cell lines were used for virus isolation attempts. A549 (CCL-185), HeLa (CCL-
2), LLC-MK2 (CCL-7), MDCK NBL2 (CCL-34), MRC-5 (CCL-171), NCI-H292 (CRL-
1848), Vero E6 (CCL-81), and WI-38 (CCL-75) cells were obtained from the American
Type Culture Collection (Manassas, VA, USA). The cell lines were grown as
monolayers at 37°C and 5% CO2 in advanced Dulbecco's Modified Eagle's Medium
(aDMEM) (Invitrogen Corp., Carlsbad, CA, USA), supplemented with 2 mM L-Alanyl-L-
Glutamine (GlutaMAX, Invitrogen Corp.), 10% (v/v) low IgG, heat-inactivated gamma-
irradiated fetal bovine serum (HyClone, Logan, UT) and antibiotics [PSN; 50 μg/mL
penicillin, 50 μg/mL streptomycin, 100 μg/mL neomycin (Invitrogen Corp.) to inhibit
bacterial growth [56]. Prior to use, every cell line was treated with plasmocin for three
weeks to reduce the chance of mycoplasma contamination and verified free from
mycoplasma DNA by PCR [56].
Virus Isolation
Upon thawing on ice, aliquots of (~50 𝜇L) air sample collection medium (SFR and
RFR) were inoculated onto newly confluent monolayer of cells in 6-well plates.
Fungizone® Antimycotic (final concentration 0.125𝜇g/mL; Gibco, Catalog# 15290-018)
32
was incorporated into the cell growth medium, as needed, to inhibit fungal growth.
Serum free aDMEM supplemented with L-1-tosylamido-2-phenylethyl trypsin (final
concentration as appropriate for each cell line) was used to facilitate the isolation of IFV
and many other viruses. The inoculated cell lines in addition to negative controls were
incubated at 35°C with 5% CO2 and observed daily for virus-induced cytopathic effects
(CPE) for 26 days. Based on observation of characteristic CPE, spent cell growth media
and infected cells were collected at various time intervals, and tested for virus isolation
by antigen and genome based detection methods described below.
Rapid Detection of Influenza A and B Viruses
Cell cultures in serum-free media containing TPCK-trypsin that exhibited IFV-
induced CPE (IFV-induced CPE in MDCK cells includes granulation of the cytoplasm,
enlarged nuclei, round and refractile floating cells, followed by destruction of the cell
monolayer) typically were tested using a commercial solid phase ELISA (QuickVue
influenza A and B kit, Quidel Corp., San Diego, CA, USA) for rapid detection of
influenza A and B viruses.
GenMark Respiratory Viral Panel
A GenMark multiplex PCR eSensor XT-8 Respiratory Viral Panel (GenMark
Diagnostics, Inc., Carlsbad, CA) was used for respiratory virus detection and IFV
subtyping. This panel includes tests for common human respiratory viruses including
influenza A virus (with subtype determination); influenza B virus; respiratory syncytial
virus types A and B; parainfluenza virus types 1, 2, 3 and 4; human metapneumovirus,
human rhinovirus; adenovirus groups B, C and E; coronavirus types 229E, NL63, HKU1
and OC43. The panel does not include tests for bacterial or fungal pathogens. As
previously described, extracted nucleic acids from the spent cell-growth media were
33
used to perform a multiplex PCR/RT-PCR assay and the amplified DNA targets
analyzed by electrochemical detection [57]. After data acquisition and analysis, the
instrument generated an output: eSensor Respiratory Viral Panel Currents Report
(RUO). A current output of 3 nA (nanoamps) and above was considered positive
identification of a respiratory virus’ genomic nucleic acids.
Identification of Influenza Virus Types and Subtypes and Genomic Sequencing
After IFV were detected using the rapid ELISA test and RVP assay, RT-PCR
targeting specific gene sequences of IFV were performed for further confirmation. Viral
RNA (vRNA) was purified from spent cell growth media and RT-PCR performed using
primers as described in Table 2-3. Influenza virus A genomic segments [polymerase
genes PA, PB1 & PB2; hemagglutinin (HA); nucloecapsid (NP); neuraminidase (NA);
matrix proteins (M1 & M2); nuclear export protein (NEP) and nonstructural protein
1(NS1)] were sequenced following previously published methods [58-61].
Identification of Miscellaneous Respiratory Viruses
Human metapneumovirus, human parainfluenza virus types 1 and 4a, and
human coronavirus NL63 were identified by RT-PCR and sequencing of virus-specific
genes using previously published methods (Table 2-4; 62-65)
Results
Isolation and Identification of Viable Viruses in Aerosols Collected in Spring 2016 (April 4- 20)
Cell cultures were maintained for 26 days before being considered negative for
virus isolation. During this time, no CPE were observed in MDCK cells characteristic of
influenza virus infection. However, mixed cytopathic effects were observed after 21
days post infection (dpi) in LLC-MK2 and A549 cells inoculated with RFR air samples
34
but not in those inoculated with SFR air samples. Spent cell growth media and infected
cells from RFR inoculated cultures tested negative in GenMark RVP assays. However,
virus group/species specific RT-PCR and sequencing performed using vRNA extracted
from the same samples confirmed the presence of human metapneumovirus and
human parainfluenza virus 4a (collected April 8, 2016); human metapneumovirus and
human parainfluenza virus 1 (collected April 15, 2016) and human metapneumovirus,
human parainfluenza 4a and human coronavirus NL63 (collected April 20, 2016) (Table
2-2). The fact that GenMark RVP assays tested negative while sequencing results
identified viruses in the same samples may be due to one or more factors like: (a)
choice of primers used for PCR/RT-PCR step, (b) presence of sequence variants in the
viral targets, and/or (c) levels of virus in the specimen below the limit of detection for the
RVP assay. Probable failure of virus genome extraction and PCR/RT-PCR inhibition
may be ruled out since the internal control included in these samples (bacteriophage
MS2) was detected in the RVP assays.
Isolation and Identification of Viable Viruses in Aerosols Collected in Early Fall (August- September) 2016
No virus was isolated and detected from air samples collected from both
sampling sites (HPNP and the Reitz Union cafeteria) during early fall.
Isolation and Identification of Viable Viruses in Aerosols Collected after Thanksgiving (December) 2016
MDCK cells inoculated with any of the SFR and RFR air samples collected after
the Thanksgiving holiday did not show any IFV-induced CPE. However, VERO E6 and
LLC-MK2 cells inoculated with one of the air samples (RFR air sample collected
December 5, 2016) showed non-specific CPE 12 dpi, characterized by few floating dead
cells while the cells in the intact monolayer were darker and granular in appearance.
35
Cell spent growth media and cells from LLC-MK2 cultures tested positive for influenza
virus A using the GenMark RVP. Subsequent type and subtype specific RT-PCR
confirmed it to be influenza virus A subtype H1N1.
Sequence analyses of the influenza A H1N1 isolate revealed that it belonged to
HA subclade 6B.1 based on the criteria mentioned by the European Center for Disease
Prevention and Control [66]. GenBank accession numbers for the influenza
[A/Environment/Gainesville/12/2016(H1N1)] virus gene sequences are listed in Table
2-5. Deduced amino acid substitutions in the hemagglutinin (HA), neuraminidase (NA)
and matrix (M) proteins of our environmental isolate have been compared to those of
the 2015-16 northern hemisphere influenza A H1N1 vaccine strain, and available gene
sequences of clinical and environmental influenza A H1N1 strains detected in
Gainesville since 2013. As shown in Tables 2-6 to 2-8, when compared to the reference
vaccine H1N1 strain [A/California/07/2009(pdmH1N1)], there were changes in key
amino acid positions of the HA, NA and M proteins of our H1N1 isolate and other recent
isolates (clinical and environmental) from Gainesville.
Discussion
In this study, the performance of the SKC BioSampler operated using revised
operating procedures in collecting viable virus aerosols from various indoor locations at
UF was evaluated. Convenience samples were collected in 2016 during spring, early fall
and post-Thanksgiving period. Respiratory viruses were isolated from spring and post-
Thanksgiving air samples collected using a revised air flow rate but no virus was
isolated from samples collected following the manufacturer recommended air flow rate.
Influenza A H1N1 virus was isolated from only one air sample collected on
December 5, 2016. Viral genomic sequence analyses were performed using available
36
GenBank sequences of influenza A H1N1 strains detected in Gainesville from 2013 to
date. The reference strain used was influenza virus A/California/07/2009 (pdmH1N1),
which is defined as the pdm09 HA clade 1 and was used in the 2015-2016 northern
hemisphere flu vaccine. The influenza A virus isolated in this study
(A/Environment/Gainesville/12/2016(H1N1)] belonged to pandemic H1N1 2009 clade
6B.1. A shown in Tables 2-6 to 2-8, several amino acid substitutions over time became
fixed in the virus population possibly conferring some selective advantage to their
survival in human population. These include some of the signature amino acid
substitutions defining subgroup 6B (D97N, S185T and A256T in HA1; and E47K and
S124N in HA2) but also additional ones (P83S, K163Q, S203T, K283E and I321V in
HA1; E172K in HA2). The influenza A H1N1 strains detected in 2016 had few more
substitutions in HA1 (S84N, S162N and I216T) that might get fixed in the coming years.
Similar trends were also observed in NA and M amino acid sequences as shown in
Tables 2-7 & 2-8.
Sampling time and location play important roles in successful collection of virus
aerosols using any air sampler. Using the same revised air sampling flow rate for the
BioSampler, viable viruses were isolated during an influenza outbreak in April 2016 but
not during early fall season in 2016 when there was no ongoing influenza outbreak in
Gainesville. Influenza virus was again collected during a December sampling. Most of
the collections took place in empty classrooms, though two samples were also collected
in a crowded cafeteria at the Reitz Union. However, at the cafeteria, there were no
persons observed with obvious signs of respiratory ailments (i.e., no persons were seen
that were coughing or sneezing). More samplings during outbreaks of IFV and other
37
respiratory viruses at various locations and in the presence of sick individuals could
shed some more light as to the importance of emitting sources for viable virus aerosol
collection.
This study suggests that the revised collection procedures may work better for
collection of viable viruses in indoor settings. However, more studies need to be
performed to verify our findings and identify potential limiting factors for viable virus
collection using the BioSampler.
38
Figure 2-1. Schematic diagram of the SKC BioSampler (left) [image adapted from www.skcinc.com]; and the testing system installed at a sampling site (right).
39
Table 2-1. Air sample collection during 2016 using the BioSampler
Air sample# (in pairs)
Date & Location
RH & Temp. Flow rate (L/min)
Duration (min)
Volume of air sampled (m
3)
Sp
ring 1 4.8.16,
HPNP G101 42%, 22C 8a 30 240
43%, 20C 12.5b 30 375
2 4.15.16, HPNP SRA
44%, 24C 8 47 375
46%, 22C 12.5 30 375
3 04.20.16, HPNP G1404
42%, 21C 8 47 375
41%, 20C 12.5 30 375
Ea
rly F
all 4 08.29.16,
Reitz union cafeteria
43%, 22C 8 47 375
43%, 22C 12.5 30 375
5 08.31.16, HPNP G1404
48%, 24C 8 47 375
48%, 24C 12.5 30 375
6 09.06.16, Reitz union cafeteria
41%, 23C 8 47 375
41%, 23C 12.5 30 375
Po
st-
Tha
nksg
ivin
g 7 12.05.16,
HPNP G101 49%, 22C 30 47 375
49%, 22C 8 30 375
8 12.07.16, HPNP G114
48%, 23C 12.5 47 375
48%, 23C 8 30 375
a Revised air flow rate (RFR)
b Manufacturer recommended standard air flow rate (12.5 L/min) (SFR)
RH: Relative humidity Temp.: Temperature HPNP: Health Professions/Nursing/Pharmacy Complex; University of Florida G101, G114 and G1404: Ground floor room numbers; SRA: Student reception area
40
Table 2-2. Air sample cell culture
Sample#
Flow rate (L/min)
Cell lines Virus isolated & detected
MDCK (NBL2)
A549 MRC-5 LLC-MK2
VERO E6
HeLa NCI-H292
1 8a _ + _ + _ * _ hMPV, HPIV-4a 12.5b _ _ _ _ _ * _
2 8 _ + _ + _ * _ hMPV, HPIV-1 12.5 _ _ _ _ _ * _
3 8 _ + _ + _ * _ hMPV, HPIV-4a, HCoV-NL63
12.5 _ _ _ _ _ * _ 4 8 _ _ _ _ _ _ _
12.5 _ _ _ _ _ _ _ 5 8 _ _ _ _ _ _ _
12.5 _ _ _ _ _ _ _ 6 8 _ _ _ _ _ _ _
12.5 _ _ _ _ _ _ _ 7 8 _ _ _ + + _ _ Flu A H1N1
12.5 _ _ _ _ _ _ _ 8 8 _ _ _ _ _ _ _
12.5 _ _ _ _ _ _ _ a Revised air flow rate (RFR);
b Manufacturer recommended standard air flow rate (12.5 L/min) (SFR)
* Cell line not used hMPV, Human metapneumovirus; HPIV-1, Human parainfluenza virus type 1; HPIV-4a, Human parainfluenza virus type 4a; HCoV-NL63, Human coronavirus NL63; Flu A H1N1, Influenza A subtype H1N1
41
Table 2-3. Primers for the detection of and subtyping of influenza A virus.
Influenza virus Type/subtype
Gene fragment
Primer Sequence (5’ – 3’) Amplicon size (bp)
Reference
Influenza A All genes Uni12W AGCRAAAGCAGG [58]
A(H1N1)2009 HA-5’(H1) HKU-SWF GAGCTCAGTGTCATCATTTGAA 173 [59]
HKU-SWR TGCTGAGCTTTGGGTATGAA [59]
UFH1-JLR GGTTGAGCTTTGGGTATGAA J. Lednickya
NA-3’(N1) N1F401 GGAATGCAGAACCTTCTTCTTGAC 1073 [59]
NARUc ATATGGTCTCGTATTAGTAGAAACAAGGAGTTTTTT
[59]
All genes Uni R AGTAGAAACAAGG [58]
A(H3N2) HA-3’(H3) H3A1F3 TGCATCACTCCAAATGGAAGCATT 863 [59]
HARUc ATATCGTCTCGTATTAGTAGAAACAAGGGTGTTTT
[59]
NA-3’(N2) N2F387 CATGCGATCCTGACAAGTGTTATC 1082 [59]
NARUc ATATGGTCTCGTATTAGTAGAAACAAGGAGTTTTTT
[59]
aJ. Lednicky, unpublished.
42
Table 2-4. Primers for the detection of and subtyping of human metapneumovirus, human parainfluenza virus and human coronaviruses.
Pathogen Gene fragment Primer Sequence (5’ – 3’) Amplicon size (bp)
Ref.c
Meta -pneumovirus
Type A
Nucleoprotein (N) Fa: MPV01.2 AACCGTGTACTAAGTGATGCACTC 213 bp [62]
Ra: MPV02.2 CATTGTTTGACCGGCCCCATAA
Type B
Nucleoprotein (N) F: MV-Can-U918 AAGTCCAAAGGCAGGRCTGTTATC 75 bp
R: MV-Can-L992 CCTGAAGCATTRCCAAGAACAACAC
Parainfluenza virus
Type 1
Nucleoprotein (N) F: HPIV1-U82 TACTTTTGACACATTTAGTTCCAGGAG 86 bp [62]
R: HPIV1-L167 CGGTACTTCTTTGACCAGGTATAATTG
Type 2
Nucleoprotein (N) F: HPIV2-U908 GGACTTGGAACAAGATGGCCT 77 bp [62]
R: HPIV2-L984 AGCATGAGAGCYTTTAATTTCTGGA
Type 3
Nucleoprotein (N) F: HPIV3-U590 GCTTTCAGACAAGATGGAACAGTG 79 bp [62]
R: HPIV3-L668 GCATKATTGACCCAATCTGATCC
Type 4a
Fusion (F) F: Para4-F CATGGGTGTCAAAGGTTTATC 376 bp [63]
R: Para4-R TGCTGCTGTAACTTGTGCAGC
Type 4b
Fusion (F) F: Para4-F CATGGGTGTCAAAGGTTTATC 376 bp [63-64] R: Para4-R TGCTGCTGTAACTTGTGCAGC
Coronaviruses 229E, HKU1, NL63, and OC43
Polymerase Forward: Cor-FW ACWCARHTVAAYYTNAARTAYGC 251 bp [65]
Reverse: Cor-RV TCRCAYTTDGGRTARTCCCA
a F, forward
b R, reverse
c Ref, reference
43
Table 2-5. GenBank accession numbers for Influenza A virus gene sequences
A/environment/Gainesville/12/2016(H1N1) genome segment# GenBank#
1 Polymerase PB2 (PB2) gene KY681470.1 2 Polymerase PB1 (PB1) gene and nonfunctional PB1-F2 protein
(PB1-F2) gene KY681471.1
3 Polymerase PA (PA) and PA-X protein (PA-X) genes KY681472.1 4 Hemagglutinin (HA) gene KY681473.1 5 Nucleocapsid protein (NP) gene KY681474.1 6 Neuraminidase (NA) gene KY681475.1 7 Matrix protein 2 (M2) and matrix protein 1 (M1) genes KY681476.1 8 Nuclear export protein (NEP) and nonstructural protein 1 (NS1)
genes KY681477.1
Table 2-6. Amino acid changes in the deduced HA of H1N1 isolated December 05,
2016.
H1N1 strain Amino acid positions in HA1
36 83 84 97 137 149 162 163 185 203
California/07/2009a K P S D P I S K S S
Gainesville/10/2013 . S N N . . . Q T T
Gainesville/09/2013 . S N N . . . Q T T
Gainesville/08/2013 . S N N . . . Q T T
Gainesville/07/2014 . S . N S . . Q T T
Gainesville/06/2014 . S N N . . . Q T T
Gainesville/04/2014 . S N N . . . Q T T
Gainesville/03/2014 . S . N S . . Q T T
Gainesville/05/2014 . S . N . . . Q T T
ENV/Gainesville/01/2014e N S N N . . . Q T T
Gainesville/01/2015 . S . N . V . Q T T
ENV/Gainesville/08/2015e . S . N . V . Q T T
Gainesville/04/2016 . S N N . . N Q T T
Gainesville/03/2016 . S N N . . N Q T T
Gainesville/02/2016 . S N N . . N Q T T
Gainesville/01/2016 . S N N . . N Q T T
ENV/Gainesville/04/2016e . S N N . . N Q T T
ENV/Gainesville/03/2016e . S N N . . N Q T T
ENV/Gainesville/02/2016e . S N N . . N Q T T
ENV/Gainesville/01/2016e . S N N . . N Q T T
ENV/Gainesville/12/2016e . S N N . . N Q T T
44
Table 2-6. continued
H1N1 strain Amino acid positions in HA1
216 225 226 256 266 273 283 317 321
California/07/2009a I G R A I H K G I
Gainesville/10/2013 . . . T . . E R V
Gainesville/09/2013 . . . T . R E . V
Gainesville/08/2013 . . . T . . E R V
Gainesville/07/2014 . . . T . . E . V
Gainesville/06/2014 . . . T . R E . V
Gainesville/04/2014 . . . T . R E . V
Gainesville/03/2014 . . . T . . E . V
Gainesville/05/2014 . . . T . . E R V
ENV/Gainesville/01/2014e . . . T . . E R V
Gainesville/01/2015 . . . T . . E . V
ENV/Gainesville/08/2015e . . . T . . E . V
Gainesville/04/2016 T . . T . . E . V
Gainesville/03/2016 T . . T . . E . V
Gainesville/02/2016 T . . T . . E . V
Gainesville/01/2016 T . . T . . E . V
ENV/Gainesville/04/2016e T . . T V . E . V
ENV/Gainesville/03/2016e T . . T V . E . V
ENV/Gainesville/02/2016e T . . T V . E . V
ENV/Gainesville/01/2016e T . . T . . E . V
ENV/Gainesville/12/2016e T . . T . . E . V
45
Table 2-6. continued
H1N1 strain Amino acid positions in HA2
4 47 124 172
California/07/2009a G E S E
Gainesville/10/2013 R K N K
Gainesville/09/2013 . K N K
Gainesville/08/2013 R K N K
Gainesville/07/2014 R K N K
Gainesville/06/2014 . K N K
Gainesville/04/2014 R K N K
Gainesville/03/2014 R K N K
Gainesville/05/2014 R K N K
ENV/Gainesville/01/2014e R K N K
Gainesville/01/2015 . K N K
ENV/Gainesville/08/2015e . K N K
Gainesville/04/2016 . K N K
Gainesville/03/2016 . K N K
Gainesville/02/2016 . K N K
Gainesville/01/2016 . K N K
ENV/Gainesville/04/2016e . K N K
ENV/Gainesville/03/2016e . K N K
ENV/Gainesville/02/2016e . K N K
ENV/Gainesville/01/2016e . K N K
ENV/Gainesville/12/2016e . K N K a 2015-2016 vaccine strain, dot (.) in each column represents the same amino acid as in the vaccine
strain. All strains were isolated from humans unless otherwise specified. e Environmental isolate.
46
Table 2-7. Amino acid changes in the deduced NA of H1N1 isolated December 05, 2016.
H1N1 strain Amino acid positions in NA
13 20 34 40 44 48 82 86 117 200
California/07/2009a V A I L N T S A I N
Gainesville/08/2013 . T . . S . P . . S
Gainesville/09/2013 . T . . S . P . . S
Gainesville/10/2013 . T . . S . P . . S
Gainesville/07/2014 . . V . S . . . . S
Gainesville/06/2014 . . V . S . P . . S
Gainesville/04/2014 . . V . S . . . . S
Gainesville/03/2014 . . V . S . P . . S
Gainesville/05/2014 . T . . S . P . . S
ENV/Gainesville/01/2014e . . V . S . P . . S
Gainesville/01/2015 . . V I S . . V M S
ENV/Gainesville/08/2015e . . V I S . . V M S
Gainesville/04/2016 I . V I S . . . . S
Gainesville/03/2016 I . V I S . . . . S
Gainesville/02/2016 I . V I S . . . . S
Gainesville/01/2016 I . V I S . . . . S
ENV/Gainesville/04/2016e I . V I S A . . . S
ENV/Gainesville/03/2016e I . V I S A . . . S
ENV/Gainesville/02/2016e I . V I S A . . . S
ENV/Gainesville/01/2016e I . V I S . . . . S
ENV/Gainesville/12/2016e I . V I S . . . . S
47
Table 2-7. continued
H1N1 strain Amino acid positions in NA
241 248 264 265 270 314
California/07/2009a V N V K N I
Gainesville/08/2013 I D . . . .
Gainesville/09/2013 I D . . . .
Gainesville/10/2013 I D . . . .
Gainesville/07/2014 I D . . . .
Gainesville/06/2014 I D . . . .
Gainesville/04/2014 I D . . . .
Gainesville/03/2014 I D . . . .
Gainesville/05/2014 I D . . . .
ENV/Gainesville/01/2014e I D . . . .
Gainesville/01/2015 I D . . . .
ENV/Gainesville/08/2015e I D . . . .
Gainesville/04/2016 I D I . K M
Gainesville/03/2016 I D I . K M
Gainesville/02/2016 I D I . K M
Gainesville/01/2016 I D I R K M
ENV/Gainesville/04/2016e I D I . K M
ENV/Gainesville/03/2016e I D I . K M
ENV/Gainesville/02/2016e I D I . K M
ENV/Gainesville/01/2016e I D I . K M
ENV/Gainesville/12/2016e I D I . K M
48
Table 2-7. continued
H1N1 strain Amino acid positions in NA
321 351 369 386 397 432 469
California/07/2009a I Y N N N K K
Gainesville/08/2013 V F K . K . .
Gainesville/09/2013 V F K . K . .
Gainesville/10/2013 V F K . K . .
Gainesville/07/2014 V F K . K . .
Gainesville/06/2014 V F K . K . .
Gainesville/04/2014 V F K . K . .
Gainesville/03/2014 V F K . K . .
Gainesville/05/2014 V F K . K . .
ENV/Gainesville/01/2014e V F K . K . .
Gainesville/01/2015 V F K K . E .
ENV/Gainesville/08/2015e V F K K . E .
Gainesville/04/2016 V F K K . E .
Gainesville/03/2016 V F K K . E .
Gainesville/02/2016 V F K K . E .
Gainesville/01/2016 V F K K . E .
ENV/Gainesville/04/2016e V F K K . E .
ENV/Gainesville/03/2016e V F K K . E .
ENV/Gainesville/02/2016e V F K K . E .
ENV/Gainesville/01/2016e V F K K . E .
ENV/Gainesville/12/2016e V F K K . E N a 2015-2016 vaccine strain, dot (.) in each column represents the same amino acid as in the vaccine
strain. All strains were isolated from humans unless otherwise specified. e Environmental isolate.
49
Table 2-8. Amino acid changes in the deduced M proteins of H1N1 isolated December 05, 2016.
H1N1 strain M1 protein M2 protein
80 85 167 192 208 230 21 61
California/07/2009a V N T M Q K D R
Gainesville/10/2013 I N . V . R G .
Gainesville/09/2013 I N . V . R G .
Gainesville/08/2013 I N . V . R G .
Gainesville/07/2014 I N . V . R G .
Gainesville/06/2014 I N . V . R G .
Gainesville/04/2014 I N . V . R G .
Gainesville/03/2014 I N . V . R G .
Gainesville/05/2014 I N . V . R G .
Gainesville/01/2015 I N . V . R G .
ENV/Gainesville/08/2015e I N A V . R V .
Gainesville/04/2016 I N A V . R V .
Gainesville/03/2016 I N . V K R G .
Gainesville/02/2016 I N . V K R G .
Gainesville/01/2016 I N . V K R G .
ENV/Gainesville/04/2016e I N . V K R G .
ENV/Gainesville/03/2016e I N . V K R G .
ENV/Gainesville/02/2016e I N . V K R G .
ENV/Gainesville/01/2016e I N . V K R G .
ENV/Gainesville/12/2016e I N . V K R G K a 2015-2016 vaccine strain, dot (.) in each column represents the same amino acid as in the vaccine
strain. All strains were isolated from humans unless otherwise specified. e Environmental isolate.
50
CHAPTER 3 EVALUATION OF THE COLLECTION EFFICIENCY OF THE VIABLE VIRUS
AEROSOL SAMPLER IN A STUDENT HEALTH CARE CENTER
Introduction
The work detailed in this chapter was performed in collaboration with Maohua
Pan and C. Y. Wu. The virology aspects of the work were performed by Tania Bonny.
Airborne infectious agents in healthcare facilities pose risks to both patients and
employees. Nosocomial transmission of human influenza viruses is a major concern in
these healthcare facilities especially because immune-compromised patients that may
be present in those settings are at greater risk of getting infected and are more
vulnerable to the development of severe disease. As previously mentioned (Chapter 3),
transmission of influenza viruses from one person to another can occur in three routes:
direct contact of infectious secretions with mucus membranes of the upper respiratory
tract (URT), contact of virus-containing large droplet sprays with surfaces of the URT,
and inhalation of small aerosols and droplet nulcei [14, 23, 67]. A fourth route has been
shown in animal models: ocular infection, wherein airborne influenza viruses come into
contact with ocular surfaces [18]. The relative importance of each transmission route is
unknown and probably varies depending on virus strain, environmental conditions, etc.
[23]. Among them, the aerosol transmission mode is the most contentious one
especially with regard to: (a) economic reasons: expensive precautions would be
needed for implementation of appropriate infection control processes in health-care
settings, and (b) the fact that no clear evidence exists from which one can deduce from
lab experiment to real life and from animals to human beings [68]. If people can get
infected via aerosol transmission, N95 respirators rather than surgical masks will be
needed in addition to other interventions like increased air ventilation, isolation of
51
infected patients, and filtration system used for large droplets. Therefore, many efforts
are being expended to better understand the importance of the aerosol transmission
route of human influenza viruses. The same holds true for other human respiratory
viruses.
Previous air sampling studies for viruses were hindered by limitations in the air
sampling and detection methods available for airborne viruses (this dissertation,
Chapter 2). Samplers commonly used for virus sampling are designed for collecting
larger particles (those > 5 μm), such as fungal spores and bacteria, and are inefficient in
collecting nanoparticles (nanoparticles or nanomaterials are defined as substances with
at least one dimension that falls within 1-100 nm [69-70]). Furthermore, these samplers
were not designed to preserve the infectivity of the collected viruses. For example, the
commonly used SKC BioSampler has been shown to have less than 10% physical
collection efficiency for lab generated aerosols of MS2 bacteriophage [40] and less than
8.6% infectious collection efficiency for influenza H1N1 virus (2009) [46]. Polymerase
chain reaction (PCR) methods, which have been widely used for virus quantification,
provide a total count of the viral genomes (‘genome equivalents’), but do not
discriminate between genomes corresponding to viable vs non-viable viruses [71, 72].
These difficulties might account for the results of Lindsley et al. [41], wherein influenza
virus RNA was detected in 14 of the 30 test subjects yet infectious virus was isolated
from only 2. Therefore, it is hard to conclude whether the low infectious virus recovery
reported in the literature is meaningful or due to poor collection methodologies for
airborne viruses and/or inactivation of the viruses during the sampling process.
52
A recent study by Pan et al. introduced the “Viable virus aerosol sampler”
(VIVAS) [50]. The VIVAS uses a water-based condensation growth system [73], which
mimics what happens in human lungs on a cold day, targeting aerosolized particles
from 5 nm to more than 10 µm [73, 74]. Briefly, the system consists of eight parallel,
wet-walled growth tubes with four major components (Figure 3-1): the aerosol inlet,
conditioner, initiator and collector. The growth tubes operate on the same principle used
for the original water-based condensation particle counter (CPC) [74]. The conditioner
of each tube is held at 6C and serves to normalize the temperature and relative
humidity of the entering airflow [74]. The initiator is warmed to 45C to allow
condensation of the particles. Under these operating conditions, wettable particles enter
the conditioner at a total sample flow rate of 7-8 L/min. Through condensational growth,
particles as small as 5 nm amplify into droplets greater than 2µm in diameter [75]. The
outgoing flow is distributed among a set of 32 nozzles (0.66 mm diameter, 4
nozzles/growth tube, Figure 3-1) to minimize impaction stress and surface disruption.
The particles exit through the nozzles and gently impinge onto 1.5 mL of collection
medium contained in a 25 mm Petri dish.
In a previous study, VIVAS was used for the successful collection of laboratory-
generated virus aerosol, wherein the collection efficiency was more than 74% for viable
influenza H1N1 virus [46]. This high collection efficiency was attributed to the inherently
gentler impaction of the VIVAS, which preserves infectivity, as well as the high physical
collection efficiency due to the wide size range of airborne particles. For the work
described here, the efficiency of the VIVAS was evaluated for the collection of airborne
53
influenza and other respiratory viruses in a student health care center during the course
of a late onset influenza virus outbreak.
Materials and Methods
All procedures were reviewed and approved by the director of the student health
center. Approval by an institutional review board (IRB) was not necessary because
human subjects were not studied and could not be identified, and the sources of the
viruses detected could not be tracked.
Healthcare Facility
The healthcare facility of this work is the Student Health Care Center at UF
(Gainesville, Florida, USA). It is free-standing building that has its own heating,
ventilation, and air conditioning (HVAC) system. During the study, temperatures of the
indoor air were maintained at around 71°F (21.7°C) on the 1st floor and 73 °F (22.8°C)
on the 2nd floor, whereas the relative humidity ranged from 44% to 46% in both floors.
There were 4 – 6 air exchanges per hour.
Sampling Dates
Air samplings at the student health center were performed March 11, March 28
and April 8, 2016. During that time period, there was an outbreak of influenza in
Gainesville [76].
Aerosol Collection System
Ambient virus aerosol particles were collected using the VIVAS and an SKC
BioSampler. The collection system is schematically depicted in Figure 3-2. The VIVAS’
collection mechanism was previously described [77]; briefly, after passage through a
cool temperature condenser, the initiator (Figure 3-1) activates wettable particles as
small as 5 nm to form droplets greater than 2 µm in diameter. The enlarged particles are
54
subsequently directed through a set of 32 nozzles of 0.66-mm diameter for gentle
collection onto 1.5 mL of collection medium consisting of phosphate-buffered saline
(PBS) plus 0.5% (w/v) bovine serum albumin (BSA) fraction V in a 25 mm Petri dish in
the collector. The BioSampler is presently considered the reference air sampler for the
collection of aerosolized bacteria and fungi, and has been used in attempts to collect
virus aerosols, such as those described in [11, 78]. During its use, intake air is diverted
through three 0.63mm tangential nozzles above the collection medium, resulting in a
swirling airflow; this reduces impaction forces on particles that are deposited onto the
collection medium. The same collection medium for the VIVAS was used, but by
necessity the volume thereof in the BioSampler was 20mL. To avoid discrepancies of
virus concentration due to sampling location, the inlets of the VIVAS and the
BioSampler were bound together. Both the VIVAS and the BioSampler were operated at
a flow rate of 8 L/min, as this sampling rate was more effective for both air samplers for
the collection of virus aerosols and maintenance of the virus infectivity compared with
the standard flow rate of 12.5 L/min [43, 44]. To reduce noise, a Welch model 2014-B01
pump was used, and for further noise dampening, the pump was placed within a
covered box.
Air Sampler Placement
The layout of the study areas and their ceiling vents, and the air sampler
positions, are shown in Figure 3-3. The first sampling (March 11) was conducted in the
first floor lobby, near the student health care center receptionist’s desk. As the air was
sampled, it was observed that few people sat near the receptionist’s desk but many took
a drink at the fountain. During the second and third air samplings (March 28 and April
8), the air samplers were positioned within a waiting room on the second floor (Figure 3-
55
3). On both days, many patients exhibited signs of respiratory infection such as
coughing and sneezing. At both air sampling sites, the inlets of the air samplers were
set at a height of 1.2 m, oriented horizontal to the ground and facing the patients.
Negative control runs were also performed with a high-efficiency particulate air filter
installed at the inlet of the samplers. For each air sampler, a collection time of 60 min
was used to sample about 480 liters of air. Upon completion of air samplings, collection
medium in each sampler was aseptically transferred into sterile 50 mL conical
polypropylene tubes, transported in insulated ice box to the laboratory and stored at
-80C until further processing.
Virology Laboratory
Virology work was performed in the Lednicky biosafety level 2-enhanced
laboratory at the UF.
Air Sampler Collection Media Volume Reduction and Adjustment
To standardize volumes and obviate the need for large-scale cell cultures for
virus isolation attempts, air sampler collection media samples were concentrated using
Amicon Ultra-15 Centrifugal Filter Units with Ultracel-100 membranes with a molecular
weight cut-off of 100 kD (Millipore, Bedford, MA, USA) at 4000 × g for 20 minutes to a
volume of approximately 400m, the volumes adjusted to of 500 µm by addition of
collection medium, and the concentrate stored at −80°C until virus isolation in cell
cultures was attempted.
Cell Lines
For this pilot project, emphasis was on the isolation of influenza viruses and
genetic analyses thereof, but lesser efforts were nevertheless exerted to isolate other
56
common “culturable” human respiratory viruses to gain insights on the general utility of
the VIVAS for virus aerosols.
The term “culturable” refers to those viruses that can be isolated and propagated
using standard cell-lines/methods. In contrast, “non-culturable” respiratory viruses such
as Human coronavirus HKU1 can only be isolated and propagated in primary human
ciliated airway epithelial or similar complex and expensive cell systems. To favor
isolation of a wide variety of respiratory viruses, concentrated air sample collection
media was inoculated onto a variety of readily available (“standard”) cells lines. The
following cell lines, obtained from the American Type Culture Collection (ATCC), were
used for virus isolation attempts: A549 (CCL-185), HeLa (CCL-2), LLC-MK2 (CCL-7),
MDCK (CCL-34), MRC-5 (CCL-171), NCI-H292, and Vero E6 (CRL-1586). Common
human respiratory viruses that can be isolated using these cells are mentioned in Table
3-3. All the cell lines were propagated as monolayers at 37°C and 5% CO2 in Advanced
Dulbecco's Modified Eagle's Medium (aDMEM) or Eagle's Minimal Essential Medium
(EMEM) (Invitrogen, Carlsbad, CA, USA), as appropriate per cell line. Both aDMEM and
EMEM were supplemented with 2 mM L-Alanyl-L-Glutamine (GlutaMAX, Invitrogen,
Carlsbad, CA, USA.), antibiotics [PSN; 50 µg/ml penicillin, 50 µg/ml streptomycin, 100
µg/ml neomycin (Invitrogen, Carlsbad, CA, USA)], and 10% (v/v) low IgG, heat-
inactivated gamma-irradiated fetal bovine serum (HyClone, Logan, UT, USA). In
addition, EMEM was also supplemented with sodium pyruvate (Invitrogen Corp.) and
non-essential amino acids (Hyclone, Logan, UT, USA). Prior to the preparation of seed
stocks, each cell line was treated for 3 weeks with plasmocin and verified free of
mycoplasma DNA by PCR [79].
57
Cell Culture Media Formulations for Virus Isolation
Some respiratory viruses such as Influenza A viruses and various
paramyxoviruses are easiest to propagate in the presence of trypsin or similar protease
in the cell culture medium. However, FBS has a trypsin inhibitor, and cell lines vary in
their susceptibility to trypsin levels. Therefore, for the isolation and propagation of
viruses that require trypsin, FBS is typically omitted when possible and the
concentration of trypsin adjusted as needed per cell line. For this work, ten
combinations of cells and culture condition were used: Six cell lines in complete cell
growth medium plus serum (A549, HeLa, LLC-MK2, MDCK, MRC-5, NCI-H292, and
Vero E6), and four cell lines in serum-free media plus L-1-tosylamido-2-phenylethyl
chloromethyl ketone (TPCK)-treated mycoplasma- and extraneous virus-free trypsin
(Worthington Biochemical Company, Lakewood, NJ). TPCK-treated trypsin
concentrations were: 0.1 µg/ml for A549, LLC-MK2, and Vero cells, and 2.0 µg/ml for
MDCK cells.
Inoculation, Maintenance, and Observation of Cell Cultures
After thawing on ice, equal aliquots (~ 50 µl) of the archived concentrated air
sampler collection media were inoculated directly without pre-filtration onto newly
confluent cells in 6-well plates. Importantly, pre-filtration through a 0.45 µm pore-size, as
practiced by many to remove bacterial and fungal contaminants and particulates, was
not performed. This is because some human respiratory viruses are pleomorphic and/or
filamentous (such as wild-type human influenza A viruses), with lengths that exceed
0.45 µm, and these can be trapped by the filters. The inoculated cells were incubated
at 35°C, and observed daily for signs of virus-induced cytopathic effects (CPE), with re-
feeds performed every 3 days. Non-infected cells were maintained and re-fed in parallel
58
for comparison. Cells were maintained and observed for a total of 30 days before being
considered negative for virus isolation. In the event the virus that any of the cultures
were contaminated by yeast or filamentous fungi, amphotericin B (Fungizone,
Invitrogen) was available as a cell culture medium supplement, as needed.
Identification of Human Respiratory Viruses
Viruses were identified by cell tropism (Table 3-3), type of CPE they induced, use
of the GenMark Respiratory Virus Panel, solid phase ELISA for influenza A and B
viruses, group and/or virus species-specific PCR/RT-PCR, and sequencing of virus-
specific PCR amplicons or complete virus genomes.
GenMark Respiratory Virus Panel
The GenMark Dx multiplex PCR eSensor XT-8 Respiratory Viral Panel (eSensor
RVP; GenMark Diagnostics, Inc., Carlsbad, CA, USA) was used to screen spent cell
growth media for the genomic DNA or RNA of respiratory viruses according to the
manufacturer’s instructions. This detects the genomic material of influenza A virus
(including subtypes H1 and H3), influenza A virus 2009 H1N1, influenza B virus,
respiratory syncytial viruses A and B, parainfluenza viruses 1, 2, 3, and 4, human
metapneumovirus, adenoviruses B/E and C, coronaviruses (229E, -NL63, -HKU1,
-OC43), and human rhinoviruses A and B. Briefly, in the case of viral genomic RNA
(vRNA), the extracted nucleic acid is reverse transcribed and amplified using viral
specific primers with an RT‐PCR enzyme mix. The amplified DNA is converted to single‐
stranded DNA via exonuclease digestion and is combined with a signal buffer
containing ferrocene‐labeled signal probes that are specific for the different viral targets.
59
A signal in nanoAmperes (nA) is provided; signals higher than a threshold value is
considered positive.
Rapid Detection of Influenza A and B Viruses in Cell Cultures
A commercial solid phase ELISA test (QuickVue influenza A and B kit, Quidel
Corp., San Diego, CA, USA) was used following the manufacturer’s instructions to
quickly detect influenza virus in the spent media of cell cultures that exhibited typical
influenza virus-induced CPE (i.e., formation of visible changes in the appearance of the
nuclei of infected cells together with the formation of focal enlarged granular cells or
non-specific cell deterioration, followed by detachment of the swollen cells from the
growth surface) The ELISA test did not distinguish between influenza A virus types H1
and H3.
Identification of Influenza Virus Types and Subtypes and Genomic Sequencing
After detection of virus using the QuickVue influenza A and B kit and the
GenMark system, vRNA was purified from the virus particles in spent MDCK cell growth
media, and preliminary analyses performed by RT-PCR using the primers given in
Table 3-4 to establish virus type and subtype. Sequencing of influenza A virus genomic
segments 4 [hemagglutinin (HA) gene], 6 [neuraminidase (NA) gene], and 7 [matrix (M2
and M1) genes], and influenza B virus segments 4 [HA gene], 6 [NB glycoprotein (NB)
and NA genes], and 7 [matrix protein 1 (M1) and 2 (M2) genes] was accomplished
following previously [80, 81] described methods.
Identification of Respiratory Syncytial Virus Subtype A (RSV-A)
Both RSV subtypes A and B induce the formation of syncytia in LLC-MK2 and
Vero E6 cells, and to a lesser extent, in A549 cells. In general, the RSV-induced CPE
are first detected in LLC-MK2 cells, then in Vero E6, and lastly in A549 cells, regardless
60
of the presence or absence of trypsin. However, syncytia are generally observed earlier
in RSV-infected cell cultures in the presence of trypsin. Since many viruses induce the
formation of syncytia, confirmation through additional tests is required. The syncytium-
forming viruses were identified as RSV-A by analyses of vRNA purified 12 days post-
infection from virus particles in the spent-cell growth media of TPCK-containing LLC-
MK2 cells using the GenMark system, and by RT-PCR followed by sequencing of the
PCR amplicons. Weak 80-bp amplicons specific for RSV-A resulted when RT-PCR was
performed using forward primer RSA-U1137; 5’-AGATCAACTTCTGTCATCCAGCAA-3’
and reverse primer RSB-L1192 5’-GCACATCATAATTAGGAGTATCAAT-3’ [62], which
target the RSV-A nucleoprotein (N) gene but were optimized for older RSV-A strains,
suggesting these primers were not necessarily ideal for contemporary RSV-A strains in
the USA. To compensate for nucleotide changes in contemporary RSV-A strains in the
USA, the primers were slightly modified as: RSA-U1137-mod; 5’-
AGATCAACTTCTATCATCCAGCAA-3’ and RSB-L1192-mod: 5’-
AGCACATCATAATTAGGAGTGTCAAT-3’, and this improved RT-PCR detection,
resulting in the formation of robust 81-bp amplicons. The entire 81-bp amplicon
sequence was obtained by first re-amplifying a longer version (129 bp) with flanking
primers RSV-81 Forward: 5’-CAAGTTGAATGATACACTCAACAA-3’, and RSV-81
Reverse: 5’- AGAAACACATTAATAAGTTATGTG-3’, followed by sequencing to obtain
non-ambiguous reads of the internal 81-bp target sequence. In contrast, primers for the
detection of RSV-B [62] did not amplify a specific amplicon. Since short viral genomic
sequences are not very informative, a longer (660-bp) RSV-A genomic sequence
surrounding the 81-bp amplicon was therefore amplified and sequenced using primers
61
RSV-A NS2-N For: 5’-. CATGATGGGTTCTTAGAATGC-3’ and RSV-A NS2-N Rev: 5’-
CTGGAGCCACCTCTCCCATTTC-3’, and the 617-bp internal sequence thereof
determined.
Identification of Miscellaneous Respiratory Viruses
Adenovirus C (type 5), human parainfluenza viruses -2, -3, and -4a, and human
coronaviruses 229E and NL63, and human metapneumovirus were identified using the
GenMark system and by published PCR-based methods (Table 2-4; 62-65).
Results
Isolation and Identification of Viable Viruses in Aerosols Collected March 11, 2016
Viable human respiratory viruses were recovered by the VIVAS and the
BioSampler in each of three separate air sampling intervals performed on March 11, but
not in control runs performed with HEPA-filtered VIVAS and BioSampler air intakes
(Table 3-1). Cytopathic effects consistent with those caused by influenza viruses were
observed in MDCK cells beginning 6 days post-inoculation (p.i.), suggesting the
possibility that influenza A or B virus (or both) had been isolated (Figure 3-4).
Moreover, syncytia consistent with those expected for human respiratory syncytial virus
(RSV) were also observed in A549, LLC-MK2, and Vero cells regardless of trypsin
content but were much more pronounced and easiest to detect in the cells in serum-free
cell growth medium with added TPCK-trypsin. The syncytia became evident beginning 8
days post-inoculation of the LLC-MK2 cells with trypsin, and 10 days later in trypsin-free
LLC-MK2 cells. In contrast, no CPE were observed in mock-inoculated cells or in control
runs with HEPA-filtered samplers. Though the onset varied according to sampling
interval, in each case, the CPE were observed first in cells inoculated with collection
media from the VIVAS.
62
Solid-phase ELISA tests indicated that both influenza A and B viruses had been
isolated (Figure 3-5). Remarkably, RT-PCR indicated that influenza A subtypes H1 and
H3 had been isolated, as well as Victoria-lineage influenza B virus. Similarly, RSV-A
was identified in some of the cell cultures. The viruses detected per sampling interval
are listed in Table 3-1; GenBank accession #s for the influenza virus sequences are
listed in Table 3-5 and those of RSV-A in Table 3-6.
Whereas rare nucleotide sequence differences were noted between the influenza
H1N1 virus isolates, the genetic changes were silent, and the deduced HA, NA, and M1
and M2 amino acid sequences were conserved. These analyses revealed the H1N1
viruses belonged to HA subclade 6B.1 based on criteria mentioned in reference [82];
the results are presented in Table 3-7 relative to those of reference strains and other
recent local H1N1 viruses we isolated from humans or from other air samplings in other
studies. Amino acid substitutions were also evident in the NA protein (Table 3-8), and M
proteins (Table 3-9). Similar analyses performed as outlined in ref. [81] indicated that
the influenza H3N2 viruses belonged to HA clade subclade 3C.2a. These viruses have
amino acid changes at major immunogenic epitopes of the HA protein (Table 3-10) and
NA proteins (Table 3-11) relative to the vaccine strain. Finally, the influenza virus B
strains were all Victoria lineage (clade 1A) viruses, and as discussed in ref. [83], contain
amino acid substitutions N129D, V146I, and I117V.
The RSV-A sequences were alike for the four isolates, and were identical to
those reported for contemporary RSV-A in circulation in the USA.
63
Isolation and Identification of Viable Viruses Collected in Aerosols on March 28, 2016
A larger assortment of human respiratory viruses was isolated in air samplings
performed March 28, 2016 (Table 3-2). A GenMark read-out for one of the mixed
influenza A and B virus samples is shown in Figure 3-6. Examples of cell cultures
depicting virus-induced CPE are given in Figures 3-7 & 3-8. Sequencing of the
influenza viruses revealed that once again, H1N1 clade 6B.1, H3N2 clade 3C.2a, and
Victoria-lineage influenza B viruses had been isolated, as had been isolated during the
March 11, 2016 air samplings. The RSV-A sequences were identical to those of the
RSV-A sequences from March 11. As this project was originally designed to answer
whether influenza virus aerosols could be detected in the student healthcare center, the
other viruses were not sequenced after they were identified based on a combination of
diagnostic PCR or RT-PCR and GenMark analyses.
Isolation of Only One Type of Viable Virus from Aerosols on April 8, 2016.
Unlike the results of the first two air sampling studies, neither influenza viruses
nor RSV-A were isolated during the final air sampling studies at the student health care
center. Instead, only one cell culture was positive for human metapneumovirus subtype
A. Moreover, the virus was isolated from only one sample collected using the VIVAS
that had been inoculated onto LLC-MK2 cells in serum-free media with trypsin, and
required > 10 days incubation before CPE were formed in the infected cells.
Discussion
We evaluated the virus aerosol collection capabilities of a novel air sampler
(VIVAS) and a standard air sampler (BioSampler) in a student infirmary center during a
late onset influenza outbreak that spanned mid-February to early April, 2016. The
64
experiments were performed three times a day on three separate days. In the first
experiment (March 11, 2016), infectious influenza A H1N1 and H3N2 and influenza B
viruses and RSV were present in the collection media of the VIVAS in 3/3 air sampling
intervals, but not in all of the BioSampler samples (Table 3-1). In the second
experiment (March 28, 2016), influenza A and B viruses and RSV were collected by
both air samplers at each air sampling interval (Table 3-2), though it was noted that
influenza virus specific CPE were detected earlier in MDCK cells inoculated with VIVAS
collection media. No influenza viruses and RSV were collected in the third experiment
(April 8, 2016). Other human respiratory viruses were also collected in the second
experiment (Table 3-2), whereas human metapneumovirus was detected in one sample
collected using the VIVAS in the third experiment.
In previous studies, the VIVAS and similar devices were compared to the
BioSampler for the collection of virus-containing particles from below 100 nm to larger
than 10m [77, 84]. In those studies, the VIVAS outperformed the BioSampler at the
collection of lab-generated influenza virus and bacteriophage MS2 aerosols due to
gentle impaction and the amplification results [46, 76, 77]. Results from this study
indicates that the VIVAS is better than the BioSampler for the collection of virus
aerosols and preservation of virus viability than the BioSampler in the ambient
environment. Possible reasons might be: (1) the gentler impaction of the VIVAS is less
damaging to viruses during the collection process, and (2) the VIVAS has a higher
physical collection efficiency than the BioSampler for particles as small as 10 nm due to
the amplification results.
65
Apart from choice of a proper sampling location, the presence of an “emitting
source” favors successful detection of an agent being tested for. In our experiments, the
location chosen was a student infirmary, the agent was influenza A or B virus, and the
emitting source would be a person with an active respiratory infection who was
coughing and/or sneezing. Our findings were consistent with the previously mentioned
items, and information regarding the late onset influenza season of 2016 provided by
the State of Florida Department of Health [76] and reinforces the notion that successful
detection of virus aerosols favors location (i.e., virus aerosols should be highest at
enclosed sites with numerous sick persons) and timing of tests (i.e., the likelihood of
finding virus aerosols is higher during outbreaks of respiratory infection). For example,
in three sets of air samplings performed on three different days after the influenza
outbreak (Aug 19. and 26, and Sept. 9, 2016) at a small classroom one of the UF
engineering buildings (Black Hall), no viable respiratory viruses were isolated.
Various studies indicate that in temperate countries, influenza outbreaks typically
occur in the late fall or early winter, when it is cold and the humidity low [85, 86]. The
late onset influenza outbreak of 2016 occurred spanned February to about the
beginning of April. It is thus likely that influenza viruses were not collected April 8, as the
outbreak had been declared over, and few students sought medical treatment for
respiratory infections that day. In contrast, the influenza season was near peak levels
from March 6 – 12 [87], and influenza viruses were isolated in our air samplings on
March 11 and 28.
Viral genomic sequence analyses indicated that influenza H1N1 viruses were
from the pandemic H1N1 year 2009 lineage [A(H1N1)pdm09]. However, unlike
66
Influenza virus A/California/07/2009(pdmH1N1), which is defined as pdm09 HA clade 1,
and was used in the northern hemisphere influenza virus vaccines of 2015-2016, the
viruses isolated in this work were from pdm09 HA clade 6B.1. The signature amino acid
substitutions that define subgroup 6B viruses are D97N, S185T, and A256T in HA1, and
E47K S124N in HA2. Additional variations that had been observed in year 2016 include
S162K, D168N, K170E, R205K, A215G, E235D. As of February 2016, the
pdmH1N1(09) viruses in all European Union/European Economic Area countries had
additional substitutions K163Q, A256T and K283E in HA1 and E172K in HA2, and
newer strains also had P83S and I321V substitutions as well in HA1[88]. The situation
in North America was similar. Whereas various virus clusters emerged within clade 6B,
two dominant subclades, 6B.1 and 6B.2, were in wide circulation. Viruses in subclade
6B.1 have HA1 amino acid substitutions S84N, S162N (which results in the formation of
a new potential glycosylation motif at residues 162-164 of HA1), and I216T. Subclade
6B.2 viruses have HA1 amino acid substitutions V152T and V173I [88-90]. As shown in
Table 3-7, there were changes at key amino acid positions of the HA protein of the
H1N1 viruses of this work relative to the vaccine strain, and the same changes were
observed in H1N1 strains from the same time period that had been isolated from
humans. Importantly, changes also occurred in the amino acid sequence of the NA
protein (Table 3-8) and M protein (Table 3-9). Similarly, seven genetic groups based on
the HA gene have been defined for A(H3N2) viruses since 2009, and contemporary
H3N2 viruses belong to clade 3C, which has three subdivisions: 3C.1, 3C.2, and 3C.3.
The virus strain of the 2015-2016 northern hemisphere vaccine was
A/Texas/50/2012(H3N2), which is an HA subclade 3C.1 virus. Subclade 3C.2a viruses
67
have been dominant worldwide as of May 2016. The HA protein of 3C.2 contain amino
acid substitutions N145S in HA1 and D160N in HA2, whereas subclade 3C.2a contain
the following amino acid substitutions at the major antigenic epitopes of HA1: N144S
(resulting in loss of a potential glycosylation site), N145S, F159Y, K160T (in the majority
of viruses, resulting in the gain of a potential glycosylation site), N225D. Subclade
3C.2a viruses also contain (at other epitopes) L3I and Q311H in HA1, and D160N in
HA2 [81, 88]. The H3N2 viruses of this work were HA subclade 3C.2a (Table 3-10), and
also had amino acid changes in their NA protein (Table 3-11). Finally, the influenza B
viruses were Victoria-lineage, whereas the commonly used influenza trivalent vaccine of
2015 – 2016 had a Yamagata-lineage strain. Given that the UF has a highly-vaccinated
student and worker population, these findings raise the question whether some/most of
the influenza virus vaccines that had been used for the 2015-2016 season were not a
good match for the influenza viruses in circulation in early 2016 in Florida.
There are some limitations to this pilot study. First, the VIVAS and the
BioSampler were used to collect virus aerosols, but particle sizes were not determined.
It is well-known that respiratory viruses can be present in different-sized airborne
particles, and in particular, that influenza A virus can be detected in coughs and
exhalations. Some of the influenza viruses are found in particle sizes termed “fine”
particles, which stay airborne much longer than larger particles and can travel much
longer distances, though the importance of these in virus transmission remains
controversial [11, 71, 91, 92]. In this study, the VIVAS and the BioSampler were located
at least 2.0 m from seated patients, and viable (infectious) influenza A and B viruses
were isolated. Other respiratory viruses were also isolated, suggesting that patients
68
with other types of respiratory viruses also produce small particle aerosols that contain
infectious viruses. Future studies should consider particle size characterization for
better identification of the possible effects of exposure to virus and their deposition in
the respiratory tract. Second, only two locations at the healthcare facility were tested for
this study and the sample size is small. Further studies sampling more locations and
more times would be useful in quantifying the ability of the VIVAS in sampling different
kinds of infectious viruses compared with the BioSampler.
This study suggests that the VIVAS performs well for the collection of virus
aerosols and the preservation of virus viability. An additional benefit is that virus
aerosols are collected onto a small volume of collection medium, and that simplifies
downstream operations, including storage, transport, and virus isolation.
69
Figure 3-1. Schematic diagram of viable virus aerosol sampler (VIVAS): a) The entire VIVAS system with its individual components, b) A set of 32 distribution nozzles and c) impingement of droplets onto a collection medium in a Petri dish. [Figure adapted from Pan et al. (77)]
70
Figure 3-2. Schematic diagram of the testing system
71
Figure 3-3. Schematic layout of the student infirmary lobby. Top: first floor, bottom: second floor.
72
Figure 3-4. MDCK cells in serum-free cell culture medium plus trypsin. A) Non-infected (“mock-infected”) MDCK cells, 8 days post-seed; the cell monolayer is intact and crowded. B) MDCK cells inoculated with collection media from the VIVAS, sampling interval # 1, March 11, 2016. Numerous rounded floating dead cells and large emptied areas of the growing surface are visible. Images were taken at a magnification of 400X.
73
Figure 3-5. Solid-phase ELISA tests. A negative control reaction is shown in the left
panel, whereas influenza A and B antigens have been detected in cell culture media taken from MDCK cells inoculated with collection medium from VIVAS sampling interval # 2, March 11, 2016.
74
Figure 3-6. Representative GenMark RVP report of MDCK cells inoculated with collection medium from VIVAS sampling interval # 2, March 28, 2016. Positive detection of the genomic RNA of influenza pandemic 2009 H1, H3, and B viruses is shown. Other respiratory viruses were either not isolated, or were inhibited by influenza viruses (or out-competed by the influenza viruses) in these cells.
75
Figure 3-7. MRC-5 and A549 cells in serum-free cell culture medium plus trypsin. A)
Non-infected (“mock-infected”) MRC-5, 12 days post-seed; the cell monolayer is intact and crowded. MRC-5 cells inoculated with collection media from the B) BioSampler and C) VIVAS, sampling interval #3, March 28, 2016; 12 days post infection (pi). D) Non-infected (“mock-infected”) A549, 12 days post-seed. A549 cells inoculated with collection media from the E) BioSampler and F) VIVAS, sampling interval #3, March 28, 2016; 12 days pi. Images were taken at a magnification of 400X.
76
Figure 3-8. VERO E6 and LLC-MK2 cells in serum-free cell culture medium plus trypsin. A) Non-infected (“mock-infected”) VERO E6, 12 days post-seed; the cell monolayer is intact and crowded. VERO E6 cells inoculated with collection media from the B) BioSampler and C) VIVAS, sampling interval #1, March 28, 2016; 12 days post infection (pi). D) Non-infected (“mock-infected”) LLC-MK2, 12 days post-seed. LLC-MK2 cells inoculated with collection media from the E) BioSampler and F) VIVAS, sampling interval #2, March 28, 2016; 12 days pi. Images were taken at a magnification of 400X.
77
Table 3-1. Viable viruses in aerosols collected on March 11, 2016.
Virus isolated Sampling interval
HEPA filter
Air sampler Influenza A H1N1
Influenza A H3N2
Influenza B Victoria
RSV-A
1 - BioSampler +
- VIVAS + + + + 2 + BioSampler
+ VIVAS 3 - BioSampler +
- VIVAS + + + + 4 + BioSampler
+ VIVAS 5 - BioSampler +
- VIVAS + + + + 6 + BioSampler
+ VIVAS
Table 3-2. Viable viruses in aerosols collected on March 28, 2016.
Virus isolated Sampling interval
HEPA filter
Air sampler AdV CoV-229E CoV- NL63
IFV A H1N1
IFV A H3N2
1 - BioSampler + + + + - VIVAS + + + + 2 + BioSampler + VIVAS 3 - BioSampler + + + + + - VIVAS + + + + + 4 + BioSampler + VIVAS 5 - BioSampler + + + + - VIVAS + + + + + 6 + BioSampler + VIVAS
78
Table 3-2. continued
Virus isolated Sampling interval
HEPA filter
Air sampler IFV B HPIV-2 HPIV-3 HPIV-4a RSV-A
1 - BioSampler + + + +
- VIVAS + + + + +
2 + BioSampler
+ VIVAS
3 - BioSampler + + + +
- VIVAS + + + +
4 + BioSampler
+ VIVAS
5 - BioSampler + + + +
- VIVAS + + + +
6 + BioSampler
+ VIVAS
aAdV, adenovirus; CoV, coronavirus; IFV, Influenza virus; HPIV, human parainfluenza virus; RSV,
respiratory syncytial virus.
79
Table 3-3. Cell lines used for the isolation of common culturable human respiratory viruses.
Human Respiratory Virus
Cell lines MDCK (NBL2)
HeLa A549 MRC-5 VERO E6
LLC-MK2
Adenoviruses Some + ++a + + Coronavirus 229E ++ ++ ++ + Coronavirus NL63 +/-a + ++ Coronavirus OC43 ++ Influenza A and B viruses ++b Some + + Metapneumovirus + ++ Parainfluenzavirus 1 +/- + ++ Parainfluenzavirus 2 + +/- + ++ Parainfluenzavirus 3 + + + ++ Parainfluenzavirus 4a +/- +/- + ++ Parainfluenzavirus 4b + ++ Respiratory syncytial virus A + + +/- ++ ++ Respiratory syncytial virus B +/- ++ ++
Pic
orn
aviru
s g
roup Coxsackievirus A + +
Coxsackievirus B +/- ++ ++ + ++ ++
Echovirus + +/- ++ + ++ Enterovirus (most) ++ ++ + ++ Enterovirus 71 + ++ + ++ Enterovirus D68 ++ + +/- + Parechovirus ++ + Rhinovirus A, B + + ++ + +
a+/-; cell line supports replication of some virus strains.
b++; cell line supports virus replication.
80
Table 3-4. Primers for the detection of and subtyping of influenza A and B viruses. Influenza virus Type/subtype
Gene fragment
Primer Sequence (5’ – 3’) Amplicon size (bp)
Reference
Influenza A All genes Uni12W AGCRAAAGCAGG [58]
A(H1N1)2009
HA-5’(H1) HKU-SWF GAGCTCAGTGTCATC
ATTTGAA
173
[59]
HKU-SWR
TGCTGAGCTTTGGGTATGAA
[59]
UFH1-JLR GGTTGAGCTTTGGGTATGAA
J. Lednickya
NA-3’(N1) N1F401 GGAATGCAGAACCTT
CTTCTTGAC 1073
[59]
NARUc ATATGGTCTCGTATTAGTAGAAACAAGGAGTTTTTT
[59]
All genes Uni R AGTAGAAACAAGG [58]
A(H3N2)
HA-3’(H3) H3A1F3 TGCATCACTCCAAATG
GAAGCATT 863
[59]
HARUc ATATCGTCTCGTATTAGTAGAAACAAGGGTGTTTT
[59]
NA-3’(N2) N2F387 CATGCGATCCTGACA
AGTGTTATC 1082
[59]
NARUc ATATGGTCTCGTATTAGTAGAAACAAGGAGTTTTTT
[59]
B Victoria lineage
HA Bvf224 ACATACCCTCGGCAA
GAGTTTC 284
[59]
Bvr507 TGCTGTTTTGTTGTTGTCGTTTT
[59]
B Yamagata lineage
HA Byf226 ACACCTTCTGCGAAA
GCTTCA 388
[59]
Byr613 CATAGAGGTTCTTCATTTGGGTTT
[59]
aJ. Lednicky, unpublished.
81
Table 3-5. GenBank accession numbers for Influenza A and B virus sequences, March 11, 2016.
Virus GenBank accession numbers
Hemagglutinin gene
NB and/or Neuraminidase genes
Matrix genes
A/envr/GNVL/01/2016(H3N2) KX398081.1 KX398084.1 KX398087.1 A/envr/GNVL/02/2016(H3N2) KX398082.1 KX398085.1 KX398088.1 A/envr/GNVL/03/2016(H3N2) KX398083.1 KX398086.1 KX398089.1 A/envr/GNVL/01/2016(H1N1) KX398060.1 KX398064.1 KX398068.1 A/envr/GNVL/02/2016(H1N1) KX398061.1 KX398065.1 KX398069.1 A/envr/GNVL/03/2016(H1N1) KX398062.1 KX398066.1 KX398070.1 A/envr/GNVL/04/2016(H1N1) KX398063.1 KX398067.1 KX398071.1 B/envr/GNVL/01/2016 KX398072.1 KX398075.1 KX398078.1 B/envr/GNVL/02/2016 KX398073.1 KX398076.1 KX398079.1 B/envr/GNVL/03/2016 KX398074.1 KX398077.1 KX398080.1
Table 3-6. GenBank accession numbers for RSV-A NS2 and N gene partial cds
sequences.
Virus GenBank accession numbers
RSVA/Environmental Air/Gainesville/UF-1/2016 KX431988.1 RSVA/Environmental Air/Gainesville/UF-2/2016 KX431989.1 RSVA/Environmental Air/Gainesville/UF-3/2016 KX431990.1 RSVA/Environmental Air/Gainesville/UF-4/2016 KX431991.1
82
Table 3-7. Amino acid substitutions in the HA protein of H1N1 viruses from March 11, 2016.
H1N1 Clade Strain Isolation Source
Key amino acid positions in HA1
83 84 97 162
1 California/07/2009 Human P S D S 6 St. Petersburg/27/2011 Human S S D S 6A (subclade) HongKong/5659/2012 Human S S N S 6C (subclade) Massachusetts/10/2013 Human S S N S 6B (subclade) South Africa/3626/2013 Human S S S S 6B GNVL/08/2013 Human S S N S 6B GNVL/07/2014 Human S S N S 6B ENVR/GNVL/08/2015 Environment S S N S 6B ENVR/GNVL/12/2015 Environment S S N S 6B GNVL/01/2015 Human S S N S 6B.1 GNVL/01/2016 Human S N N N 6B.1 GNVL/02/2016 Human S N N N 6B.1 GNVL/03/2016 Human S N N N 6B.1 GNVL/04/2016 Human S N N N 6B.1 ENVR/GNVL/1/2016 Environment S N N N 6B.1 ENVR/GNVL/2/2016 Environment S N N N 6B.1 ENVR/GNVL/3/2016 Environment S N N N 6B.1 ENVR/GNVL/4/2016 Environment S N N N
83
Table 3-7. continued
H1N1 Clade Strain Isolation Source
Key amino acid positions in HA1
163 185 203 216
1 California/07/2009 Human K S S I 6 St. Petersburg/27/2011 Human K S T I 6A (subclade) HongKong/5659/2012 Human K T T I 6C (subclade) Massachusetts/10/2013 Human N S T I 6B (subclade) South Africa/3626/2013 Human Q T T I 6B GNVL/08/2013 Human Q T T I 6B GNVL/07/2014 Human Q T T I 6B ENVR/GNVL/08/2015 Environment Q T T I 6B ENVR/GNVL/12/2015 Environment Q T T I 6B GNVL/01/2015 Human Q T T I 6B.1 GNVL/01/2016 Human Q T T T 6B.1 GNVL/02/2016 Human Q T T T 6B.1 GNVL/03/2016 Human Q T T T 6B.1 GNVL/04/2016 Human Q T T T 6B.1 ENVR/GNVL/1/2016 Environment Q T T T 6B.1 ENVR/GNVL/2/2016 Environment Q T T T 6B.1 ENVR/GNVL/3/2016 Environment Q T T T 6B.1 ENVR/GNVL/4/2016 Environment Q T T T
84
Table 3-7. continued
H1N1 Clade Strain Isolation Source
Key amino acid positions in HA1
225 226 256 283
1 California/07/2009 Human G R A K 6 St. Petersburg/27/2011 Human G R A K 6A (subclade) HongKong/5659/2012 Human G R A K 6C (subclade) Massachusetts/10/2013 Human G R A E 6B (subclade) South Africa/3626/2013 Human G R T E 6B GNVL/08/2013 Human G R T E 6B GNVL/07/2014 Human G R T E 6B ENVR/GNVL/08/2015 Environment G R T E 6B ENVR/GNVL/12/2015 Environment G R T E 6B GNVL/01/2015 Human G R T E 6B.1 GNVL/01/2016 Human G R T E 6B.1 GNVL/02/2016 Human G R T E 6B.1 GNVL/03/2016 Human G R T E 6B.1 GNVL/04/2016 Human G R T E 6B.1 ENVR/GNVL/1/2016 Environment G R T E 6B.1 ENVR/GNVL/2/2016 Environment G R T E 6B.1 ENVR/GNVL/3/2016 Environment G R T E 6B.1 ENVR/GNVL/4/2016 Environment G R T E
Table 3-7. continued
H1N1 Clade Strain Isolation Source
Key amino acid positions in HA2
47 124 172
1 California/07/2009 Human E S E 6 St. Petersburg/27/2011 Human K S E 6A (subclade) HongKong/5659/2012 Human K N E 6C (subclade) Massachusetts/10/2013 Human K N K 6B (subclade) South Africa/3626/2013 Human K N K 6B GNVL/08/2013 Human K N K 6B GNVL/07/2014 Human K N K 6B ENVR/GNVL/08/2015 Environment K N K 6B ENVR/GNVL/12/2015 Environment K N K 6B GNVL/01/2015 Human K N K 6B.1 GNVL/01/2016 Human K N K 6B.1 GNVL/02/2016 Human K N K 6B.1 GNVL/03/2016 Human K N K 6B.1 GNVL/04/2016 Human K N K 6B.1 ENVR/GNVL/1/2016 Environment K N K 6B.1 ENVR/GNVL/2/2016 Environment K N K 6B.1 ENVR/GNVL/3/2016 Environment K N K 6B.1 ENVR/GNVL/4/2016 Environment K N K
85
Table 3-8. Amino acid changes in the deduced NA of H1N1 isolated March 11.
Strain Key amino acid positions in NA
13 19 20 34 40 44 82 86
California/07/2009 V M A I L N S A St. Petersburg/27/2011 V M A I L N S A HongKong/5659/2012 V A A I L N S A Massachusetts/10/2013 V M A I L S S A South Africa/3626/2013 V M A V L N S A GNVL/08/2013 V M T I L S P A GNVL/07/2014 V M A V L S S A ENVR/GNVL/08/2015 V M A V I S S V ENVR/GNVL/12/2015 V M A V I S S V GNVL/01/2015 V M A V I S S V GNVL/01/2016 I M A V I S S A GNVL/02/2016 I M A V I S S A GNVL/03/2016 I M A V I S S A GNVL/04/2016 I M A V I S S A ENVR/GNVL/1/2016 I M A V I S S A ENVR/GNVL/2/2016 I M A V I S S A ENVR/GNVL/3/2016 I M A V I S S A ENVR/GNVL/4/2016 I M A V I S S A
Table 3-8. continued
Strain Key amino acid positions in NA 106 117 126 200 241 248 264 265
California/07/2009 V I P N V N V K St. Petersburg/27/2011 I I P N I D V K HongKong/5659/2012 I I P N I D V K Massachusetts/10/2013 V I L S I D V K South Africa/3626/2013 V I P S I D V K GNVL/08/2013 V I P S I D V K GNVL/07/2014 V I P S I D V K ENVR/GNVL/08/2015 V M P S I D V K ENVR/GNVL/12/2015 V M P S I D V K GNVL/01/2015 V M P S I D V K GNVL/01/2016 V I P S I D I R GNVL/02/2016 V I P S I D I R GNVL/03/2016 V I P S I D I R GNVL/04/2016 V I P S I D I R ENVR/GNVL/1/2016 V I P S I D I R ENVR/GNVL/2/2016 V I P S I D I R ENVR/GNVL/3/2016 V I P S I D I R ENVR/GNVL/4/2016 V I P S I D I R
86
Table 3-8. continued
Strain Key amino acid positions in NA
270 314 321 369 386 397 432 451
California/07/2009 N I I N N N K D St. Petersburg/27/2011 N I I K N N K D HongKong/5659/2012 N I I K S N K G Massachusetts/10/2013 N I I K N N K D South Africa/3626/2013 N I V K N N K D GNVL/08/2013 N I V K N K K D GNVL/07/2014 N I V K K N K D ENVR/GNVL/08/2015 N I V K K N E D ENVR/GNVL/12/2015 N I V K K N E D GNVL/01/2015 N I V K K N E D GNVL/01/2016 K M V K K N E D GNVL/02/2016 K M V K K N E D GNVL/03/2016 K M V K K N E D GNVL/04/2016 K M V K K N E D ENVR/GNVL/1/2016 K M V K K N E D ENVR/GNVL/2/2016 K M V K K N E D ENVR/GNVL/3/2016 K M V K K N E D ENVR/GNVL/4/2016 K M V K K N E D
87
Table 3-9. Amino acid changes in the deduced M proteins of H1N1 from March 11,
2016.
H1N1 Clade Strain Isolation Source
M1 protein
80 85 167 192
1 California/07/2009 Human V N T M 6* St. Petersburg/27/2011 Human 6A (subclade) HongKong/5659/2012 Human I N T M 6C (subclade) Massachusetts/10/2013 Human I S T V 6B (subclade) South Africa/3626/2013 Human I N T V 6B GNVL/08/2013 Human I N T V 6B GNVL/07/2014 Human I N T V 6B ENVR/GNVL/08/2015 Environment I N A V 6B ENVR/GNVL/12/2015 Environment I N A V 6B GNVL/01/2015 Human I N A V 6B.1 GNVL/01/2016 Human I N T V 6B.1 GNVL/02/2016 Human I N T V 6B.1 GNVL/03/2016 Human I N T V 6B.1 GNVL/04/2016 Human I N T V 6B.1 ENVR/GNVL/1/2016 Environment I N T V 6B.1 ENVR/GNVL/2/2016 Environment I N T V 6B.1 ENVR/GNVL/3/2016 Environment I N T V 6B.1 ENVR/GNVL/4/2016 Environment I N T V
88
Table 3-9. continued
H1N1 Clade Strain Isolation Source
M1 protein M2 protein
208 230 21
1 California/07/2009 Human Q K D 6* St. Petersburg/27/2011 Human 6A (subclade)
HongKong/5659/2012 Human Q K D
6C (subclade)
Massachusetts/10/2013 Human Q R G
6B (subclade)
South Africa/3626/2013 Human Q R G
6B GNVL/08/2013 Human Q R G 6B GNVL/07/2014 Human Q R V 6B ENVR/GNVL/08/2015 Environment Q R V 6B ENVR/GNVL/12/2015 Environment Q R V 6B GNVL/01/2015 Human Q R V 6B.1 GNVL/01/2016 Human K R G 6B.1 GNVL/02/2016 Human K R G 6B.1 GNVL/03/2016 Human K R G 6B.1 GNVL/04/2016 Human K R G 6B.1 ENVR/GNVL/1/2016 Environment K R G 6B.1 ENVR/GNVL/2/2016 Environment K R G 6B.1 ENVR/GNVL/3/2016 Environment K R G 6B.1 ENVR/GNVL/4/2016 Environment K R G
89
Table 3-10. Amino acid sequences at HA major immunogenic epitopes A and B1 of influenza H3N2 viruses in Gainesville, Florida, March 11, 2016.
H3N2 Virus Strain Amino Acid Sequence of Epitope A (aa 121 – 132)
H3N2 Consensus sequencea
N N E S F N W T G V T Q
A/Texas/50/2012b N A/GNVL/01/2014C A A/GNVL/05/2014d A/GNVL/06/2014d A/GNVL/07/2014d A/GNVL/08/2014d A/GNVL/09/2014e A/CH/9715293/2013f A A/GNVL/01/2016g A/GNVL/02/2016g A/ENVR/GNVL/01/2016 A/ENVR/GNVL/02/2016 A/ENVR/GNVL/03/2016
Table 3-10. continued
H3N2 Virus Strain Amino Acid Sequence of Epitope A (aa 133 – 146)
H3N2 Consensus sequencea
N G T S A C K R R S N N S
A/Texas/50/2012b I A/GNVL/01/2014C I G S A/GNVL/05/2014d I S S A/GNVL/06/2014d I S S A/GNVL/07/2014d I S S A/GNVL/08/2014d I S S A/GNVL/09/2014e I S S A/CH/9715293/2013f S R G S A/GNVL/01/2016g I S S A/GNVL/02/2016g I S S A/ENVR/GNVL/01/2016 I S S A/ENVR/GNVL/02/2016 I S S
A/ENVR/GNVL/03/2016 I S S
90
Table 3-10. continued
H3N2 Virus Strain Amino Acid Sequence of Epitope B1 (aa 155 – 163)
H3N2 Consensus sequencea
T H L K F K Y P A
A/Texas/50/2012b N A/GNVL/01/2014C N A/GNVL/05/2014d N Y T A/GNVL/06/2014d N Y T A/GNVL/07/2014d N Y T A/GNVL/08/2014d N Y T A/GNVL/09/2014e N Y T A/CH/9715293/2013f N S A/GNVL/01/2016g N Y T A/GNVL/02/2016g N Y T A/ENVR/GNVL/01/2016 N Y T A/ENVR/GNVL/02/2016 N Y T
A/ENVR/GNVL/03/2016 N Y T aYamashita et al. [92]
bVirus in 2013 – 2014 and 2014 – 2015 vaccines, Northern Hemisphere; GenBank accession number
KC892952.1. cGenBank Accession number KJ439217.
dViruses in nasopharyngeal swabs collected November 2014.
eVirus in sputum collected in November 2014.
fVirus (A/Switzerland/9715293/2013) in 2015 -2016 vaccine, Northern Hemisphere; EPI_ISL_165829. gViruses in nasopharyngeal swabs collected March 2016 (identical sequences; A/GNVL/01/2016
deposited as GenBank # KX133410.1).
91
Table 3-11. Amino acid sequence differences in the NA of influenza H3N2 viruses, in Gainesville, Florida, March 11, 2016.
H3N2 Virus Strain Amino acid position in NA protein
H3N2 Consensus sequencea
58 65 79 150 197 221 245
A/Texas/50/2012b I I P H D E S A/GNVL/01/2014C M R A/GNVL/05/2014d V S R D A/GNVL/06/2014d V S R D A/GNVL/07/2014d V S R D A/GNVL/08/2014d V S R D A/GNVL/09/2014e V S R D A/CH/9715293/2013f R D A/GNVL/01/2016g R N D N A/GNVL/02/2016g R N D N A/ENVR/GNVL/01/2016 R N D N A/ENVR/GNVL/02/2016 R N D N A/ENVR/GNVL/03/2016 R N D N
Table 3-11. continued
H3N2 Virus Strain Amino acid position in NA protein
H3N2 Consensus sequencea
247 267 339 380 392 468
A/Texas/50/2012b S T D I I P A/GNVL/01/2014C G A/GNVL/05/2014d T A/GNVL/06/2014d T A/GNVL/07/2014d T A/GNVL/08/2014d T A/GNVL/09/2014e T A/CH/9715293/2013f T A/GNVL/01/2016g T K N V H A/GNVL/02/2016g T K N V H A/ENVR/GNVL/01/2016 T K N V H A/ENVR/GNVL/02/2016 T K N V H
A/ENVR/GNVL/03/2016 T K N V H aYamashita et al. [92].
bVirus in 2013 – 2014 and 2014 – 2015 vaccines, Northern Hemisphere; GenBank accession number
KC892952.1. cGenBank Accession number KJ439217.
dViruses in nasopharyngeal swabs collected November 2014.
eVirus in sputum collected in November 2014.
fVirus (A/Switzerland/9715293/2013) in 2015 -2016 vaccine, Northern Hemisphere; EPI_ISL_165829. gViruses in nasopharyngeal swabs collected March 2016 (GenBank# KX133410.1).
hNA amino acid sequence identical to that of A/GNVL/01/2016(H3N2).
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CHAPTER 4 ISOLATION AND IDENTIFICATION OF HUMAN CORONAVIRUS 229E FROM FREQUENTLY TOUCHED ENVIRONMENTAL SURFACES IN A CLASSROOM
Introduction
Acute respiratory illnesses (ARIs) comprise the most common illnesses affecting
humans, a significant proportion of which are caused by viruses [93]. The clinical
presentation can range from mild upper respiratory tract (URT) illness to severe lower
respiratory tract (LRT) involvement, manifested as pneumonia, bronchiolitis, croup and
exacerbations of asthma or wheezing [94]. According to the World Health Organization
(WHO), there are an estimated 450 million cases of pneumonia per year resulting in 4
million deaths, and approximately 200 million of these cases are caused by viruses [95].
The viruses most commonly implicated in ARIs are adenovirus, coronaviruses, human
metapneumovirus (hMPV), influenza A and B viruses, parainfluenza viruses types 1, 2,
3 and 4, rhinovirus and respiratory syncytial virus (RSV) [94, 96].
Human respiratory viruses can be transmitted from one person to another
through various routes of infection, as previously mentioned (Chapters 2 and 3). Indirect
contact transmission from fomites on contaminated surface has been reported to be
more significant in the spread of respiratory and other viral diseases than previously
thought [97, 98]. Most of the evidence investigating the role of contaminated
environmental surface in disease transmission comes from acute-care facilities [99].
“High-touch surfaces,” which are defined as surfaces frequently touched by healthcare
workers and patients, have a higher frequency of contamination than other sites [100-
103]. However, contact transmission through virus-containing fomites is not limited to
health care settings; it occurs in indoor and outdoor locations where both healthy and
diseased individuals share common space and facilities [45, 104]. At all these locales,
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symptomatic or asymptomatic individuals release virus particles through expiration and
respiratory maneuvers such as coughing and sneezing. The emitted virus particles
present in aerosols or attached to small particles can settle or are manually deposited
onto “high touch surfaces” and create opportunity for disease transmission. Moreover,
residual virus left behind on the surfaces by ineffective cleaning procedures can initiate
infection [105]. Thus, failure to comply with the cleaning regimen and use of suboptimal
concentrations of disinfectants has resulted in the survival of pathogens in health care
environmental surfaces [106, 107].
This study was designed to test whether viable respiratory viruses could be
isolated from high contact surfaces in a University classroom over several days during
the start of “influenza season” in November 2016, when students were observed
coughing and sneezing during classroom sessions.
Materials and Methods
Study Period and Site
Environmental surfaces were convenience-sampled once a day in the same
highly-utilized medium-sized classroom at a major university in Florida, USA, from 12-
26 November 2016. Samplings were performed between classroom sessions or on
week-ends, when students were not present in the classroom, and were typically taken
between 6-7 PM, as the classroom was cleaned Monday through Friday between 6:00
and 7:00 AM. The study period occurred during influenza season in Gainesville, Florida;
classes were in session during the testing period.
Ethics
The study was IRB exempt because (a) human subjects were not involved, (b)
environmental samples were taken at irregular times between classroom sessions, (c)
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students are not assigned seats at the classroom, and so therefore samples could not
be traced back to students.
Environmental Surfaces
High-touch environmental surfaces within a classroom were randomly selected
for sampling, except for the door handle, as there was only one door. The surfaces
chosen were: (a) seat backs made of hard polyvinylchloride, (b) formica desk tops, (c) a
wooden podium, and (d) a stainless-steel door handle. The daily cleaning regimen of
the classroom was provided by the cleaning staff upon inquiry. The desk tops, podium
and door handle were cleaned once in the morning, between 6–7 AM, using a
commercially available cleaning solution consisting of non-ionic surfactant (alcohol
ethoxylates) and an anionic surfactant (sodium xylene sulfonate).
Sample Collection
Swab samples were collected using flocked nylon swabs paired with Universal
Transport Medium (UTM) (Copan Diagnostics, Inc., Murrieta, CA, Cat#360C) as
previously described [45]. The UTM served as “virus transport medium” (VTM). Briefly,
for flat surfaces, flocked swabs, pre-moistened with sterile phosphate-buffered saline
and held at an angle of approximately 30 to the sampling surface, were moved across
a 25 cm2 area in 3 directions (horizontal, vertical and cross section) to ensure maximum
contact of the swab with the sampled surface. The door-knob handle was completely
swabbed. The swabs were then immediately inserted into the VTM and stored at -80C
until further processing.
Cell Cultures for Virus Isolation
Isolation of viruses was attempted in six different cell lines. These were:
American Type Culture Collection (ATCC, Manassas, VA) cell lines A549 (human lung
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adenocarcinoma epithelium; CCL-185), MDCK (NBL-2) (Madin Darby canine kidney
[Canis familiaris kidney epithelium], CCL-34), HeLa (human cervical adenocarcinoma
epithelium, CCL-2), LLC-MK2 (rhesus monkey kidney epithelium, CCL-7), VERO E6
(African green monkey kidney; CRL-1586) and MRC-5 (human lung fibroblast, CCL-
171). Cultures were propagated as monolayers in Gibco™ advanced Dulbecco's
Modified Eagle Medium (aDMEM) (Fisher Scientific, Cat#12491015) supplemented with
0.2 mM stabilized L-glutamine (L-alanyl-L-glutamine) (Gibco™ GlutaMAX, Fisher
Scientific, Cat# 35050-061), antibiotics [50 𝜇g/mL penicillin, 50 𝜇g/mL streptomycin, 100
𝜇g/mL neomycin (PSN, Fisher Scientific, Cat #15640055)] as previously described [11].
Based on prior tests performed by myself and the cumulative experience of the
Lednicky laboratory, the cell lines chosen support the isolation and propagation of many
common respiratory viruses (Table 3-3). Replicate sets of sub-confluent cell lines were
inoculated with aliquots of the collected material and one set incubated at 33˚C, the
other at 37°C, in humidified CO2 incubators. Two different incubation temperatures were
chosen to facilitate isolation of human respiratory viruses that preferentially grows better
at 37˚C than at 33˚C or vice versa. The inoculated cells were refed at three day intervals
with maintenance media and observed daily for formation virus-specific cytopathic
effects (CPE). The cells were observed for 21 days before being considered negative
for virus isolation. As some respiratory virus strains replicate and produce progeny in
the cells without causing easily observed CPE, the spent cell-growth media was
periodically tested using the GenMark RVP assay.
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GenMark RVP Assay
Respiratory virus detection and subtyping was performed using a GenMark
multiplex PCR eSensor XT-8 Respiratory Viral Panel (GenMark Diagnostics, Inc.,
Carlsbad, CA) following the manufacturer’s instructions. This panel includes tests for
influenza A virus (including subtype determination); influenza B virus; respiratory
syncytial virus types A and B; parainfluenza virus types 1, 2, 3 and 4; human
metapneumovirus, human rhinovirus; adenovirus groups B, C and E; human
coronavirus types 229E, NL63, HKU1 and OC43. As previously described, extracted
nucleic acids from the spent cell-growth media were used to perform a multiplex
PCR/RT-PCR assay and the amplified DNA targets analyzed by electrochemical
detection [57]. After data acquisition and analysis, the instrument generates an output:
eSensor Respiratory Viral Panel Currents Report (RUO).
Whole Genome Sequencing of CoV-229E
After all the cell-culture positive samples were confirmed to contain CoV-229E,
one isolate from (desk top on 23 November 2016) was sequenced using a gene walking
procedure as described [108]. The complete virus genome FASTA sequence from the
environmental CoV-229E isolate [deposited in GenBank under accession # KY996417]
was aligned and compared to whole genome CoV-229E sequences available at
GenBank using the NCBI BLAST program.
Assessment of CoV-229E Stability under Classroom Ambient Light, Temperature and Humidity Conditions
In a separate set of experiments that were prompted by our finding of Human
coronavirus 229E (CoV-229E) on classroom surfaces in this study, the survival of a
well-studied CoV-229E laboratory strain was assessed after its deposition onto three
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different coupons (stainless steel, hard plastic and glass) that were held under
controlled settings that simulated classroom ambient light cycle, temperature and
humidity conditions. A CoV-229E strain was obtained from the ATCC (catalog # VR-
740), propagated in MRC-5 cells, and the titer of the resulting virus stock preparation
obtained by plaque assay. As classrooms at the university are maintained at a
temperature of about 24°C and a relative humidity (RH) of 45 – 49% and a fluorescent
light cycle of 10 hrs off, 14 hrs on, the stability of CoV-229E VR-740 was assessed on
three different hard surfaces held at 24°C and approximately 50% RH with fluorescent
lights on for 14 hrs per day. Briefly, working in a biosafety cabinet, 20 µL aliquots (three
replicates/day, over a 7-day testing period) of tittered virus (2 x 104 plaque forming
units) were spotted and spread over the surface of sterile 1 cm2 hard plastic, glass, and
stainless steel coupons held in a sterile baking dish, and the coupons allowed to dry for
one hour. A controlled 50% RH environment was produced by placing each virus-
overlaid coupon into a sterile glass container with a saturated solution of magnesium
nitrate held in a separate compartment [109], and the glass container sealed with a
glass top. Virus survival was monitored for 7-days. Thus, there were 3 replicates for
each type of coupon for each test day [9 coupons/day] tested over 7 days, plus one
negative control for each coupon for each day [total = 12 coupons/day for days 0, 1 -7,
for a total of 96 coupons tested]. Briefly, virus was extruded off the different surfaces
and viable counts determined by plaque assay as: coupons were individually aseptically
immersed into separate sterile 50-mL polypropylene tubes containing 5 mL of aDMEM
without FBS. After an initial rehydration period of 15 minutes, three sterile 2-mm-
diameter glass beads were added to the tubes, and the tubes pulse-vortexed for 30
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seconds. Serial dilutions were prepared in cell growth medium and 1-ml aliquots
inoculated onto newly confluent monolayers of MRC-5 cells in 6-well plates. The
inoculum was removed after 3 hr and replaced with agarose overlays, and the plates
incubated at 37°C and 5% CO2 for 5 days. The monolayers were subsequently overlaid
with an agarose overlay containing vital stain, and incubated for 1 day. Plaques in the
monolayer were enumerated the following day (7 days post-infection). Triplicate
samples were processed for each time point.
Results
Six cell cultures inoculated with samples collected on four different days over an
11-day period displayed virus-induced cytopathic effects (CPE) consisting of cell
rounding, followed by clumping and detachment of the cells within 3-11 days post-
infection, whereas non-inoculated cells maintained in parallel retained a normal
phenotype (Figure 4-1). The CPE first appeared in cells incubated at 33˚C.
Viral genomic RNA extracted from cell lysates and virions in spent culture media
from the infected cells was identified as that of CoV-229E by the GenMark RVP system.
An example of a GenMark report for vRNA extracted from one of the isolates is given in
Figure 4-2. Of the 13 surfaces sampled over a 11-day period, 6 were positive for CoV-
229E (Table 4-1). Desk tops and the door knob were the most commonly contaminated
surfaces. Of note, the CoV-229E isolates formed lytic CPE in several cell lines and yet
replicated to high levels in LLC-MK2 cells without causing obvious CPE (Table 4-1).
Whole genome sequence comparison to available CoV-229E sequences at
GenBank revealed that an environmental CoV-229E isolate from our study was closely
related to a CoV-229E clinical isolate from the Netherlands (NL) in 2010 (GenBank
accession: JX503060.1). Deduced amino acid sequences of our environmental CoV-
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229E isolate’s: replicase 1ab, accessory, spike, envelope, membrane and nucleocapsid
proteins were almost identical to those of the 2010 NL isolates except for few
substitutions in the replicase 1ab (S686G, G763C, F992S, L1456V, T1623X, I3813T,
G4082R); spike (D213N, V603X); nucelocapsid (V46I) and accessory (V81X) proteins.
The complete genome sequence of CoV-229E/environment/Gainesville/1/2016 has
been deposited in the GenBank database (accession# KY996417).
In vitro tests indicated that after deposition onto glass, hard plastic, or stainless
steel for 7 days, there was an approximate reduction of the viable virus count by about
2.5 logs, yet a significant quantity of virus nevertheless remained infectious (Figure 4-3).
Discussion
Microbial contamination of ‘high-touch surfaces’ is common in both health care
and community settings [45, 111]. Some pathogens can survive for prolonged periods
on such surfaces and be transmitted to susceptible hosts [110-113]. Coronaviruses are
common causes of upper respiratory tract and enteric infections in healthy individuals
and often cause severe infections of the lower respiratory tract in patients with co-
morbidities [7, 97, 114]. CoV-229E, one of the four circulating strains of human
coronaviruses, has been implicated in lower respiratory tract involvement in young
infants [115-118], elderly individuals [119] and in immunocompromised patients [7, 114,
120, 121]. It is reported to be an important cause of nosocomial respiratory viral
infection in high-risk infants, with lower respiratory tract infections progressing to more
severe disease manifestations e.g. bronchitis, croup, bronchiolitis and pneumonia [122-
125]. In elderly individuals, CoV-229E infections are also frequent, including those with
underlying conditions [119]. Lower respiratory tract infections are a major cause of
hospitalizations and mortality in hematopoietic stem cell transplant patients and CoV-
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229E has been detected in increasing frequency in these patients [7, 120, 121]. It has
also been suggested as an autoimmune trigger in multiple sclerosis [114].
In this study, it was determined that infectious CoV-229E could be isolated from
“high touch surfaces” in a classroom where students were seen coughing and sneezing.
Others have reported detection of coronavirus genomic RNA on various inanimate
surfaces (e.g., telephones, doorknobs, computer mice, telephone handles, latex gloves
and sponges) in hospitals and apartment buildings [110, 126]. Taken together, these
findings seem counter-intuitive, as enveloped viruses are in general more susceptible to
various environmental stresses such as radiation, temperature, relative humidity than
non-enveloped viruses, mostly due to lipidic nature of their envelopes [127]. Upon
drying, virus infectivity is also reported to be affected by various environmental
conditions such as heat, moisture, pH, the type of surface, media composition and
component concentrations [128, 129]. The study of CoV-229E VR-740 survival
suggests that the virus can remain viable on different environmental surfaces (hard
plastic, glass and stainless steel) at ambient temperature (24ºC) and low relative
humidity condition (~50%) typical of an indoor environment, like a classroom, for at least
seven days at high titers. This is significant given that the minimum infective dose of
respiratory viruses can be very low [130]. Similar findings were made in studies of
transmissible gastroenteritis virus (TGEV) and mouse hepatitis virus (MHV) used as
surrogates to determine the effects of air temperature and relative humidity on the
survival of severe acute respiratory syndrome coronavirus (SARS-CoV) on stainless
steel [109], suggesting that other coronaviruses can remain infectious on environmental
surfaces for many days, and this may be a general property of CoVs.
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Of all the surfaces tested in the classroom, the isolation of infectious CoV-229E
from the door knob is probably of greatest significance: since it is constantly used, and
was thoroughly swabbed at each sampling, our finding suggests that there was frequent
deposition of the virus on the knob. From a public health perspective, a better choice
might be brass instead of stainless steel door handles, as brass has been reported to
be deleterious for CoV-229E, though quick inactivation on brass may not occur for other
viruses [131].
Given that the frequently touched surfaces in the classroom were cleaned every
morning, isolation of CoV-229E on several days during the sampling period could mean
frequent re-deposition of the virus on those surfaces and/or an ineffective daily cleaning
regimen. Alcohol ethoxylates (AE), the principal component of the cleaning solution
used on classroom surfaces, have previously been shown to have a bacteriostatic effect
on E. coli [132]. Another study assessed the efficacy of AE in reducing genomic loads of
common respiratory viruses on toys in daycare nurseries, though the effect on virus
viability was not investigated: in that study, a decrease in genomic loads of adeno-,
rhino- and respiratory syncytial viruses have been reported but the load of coronavirus,
the most prevalent virus group detected on toys, remained unchanged before and after
AE intervention [133]. Without investigating their effect on virus viability, it is hard to
conclude from our study whether use of AE with a short contact time was sufficient to
inactivate human respiratory viruses like CoV-229E or required more vigorous cleaning
of classroom surfaces involving frequent cleaning and longer contact time, especially
during respiratory infection outbreak periods.
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The study was limited to sampling few indoor surfaces from one classroom over
an 11-day period and was focused only on common human respiratory viruses. Using
RT-PCR, rhinovirus RNA was detected on the same surfaces, but viruses could not be
isolated in cell culture. Whole genome sequence analyses of the environmental CoV-
229E isolate in this study indicate it is genetically closely related to human CoV-229E
strains that are spatiotemporally widespread. Though one strain was identified by
sequencing of one isolate (only), and it is tempting to infer one person was the source, it
is possible that the same virus strain was circulating among the students and that the
virus detected over many days emanated from various sources (persons). A broader
study might include linking the virus to the person(s) shedding the virus. Also, further
study on the effects of commonly used cleaning and disinfecting solutions on CoV-229E
viability will help guide better cleaning and disinfection practices. Finally, air sampling
studies to detect virus aerosols performed together with surface environmental
samplings would be of interest.
As viable virus was isolated from high-contact surfaces, this study supports the
notion that contact transmission may be one route of infection for CoV-229E.
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Figure 4-1. Isolation of CoV-229E in VERO E6 and A549 cells at 33°C. A) Mock-infected VERO E6 cells, maintained in parallel with inoculated cells for 6 days. B) Advanced CPE in VERO E6, 6 days post infection (pi). C) Mock-infected A549 cells D) Advanced CPE in A549 cells, 6 days pi. Original images taken at a magnification of 400X.
104
Figure 4-2. eSensor Respiratory Viral Panel currents report for desk top7 (collected on 23 November 2016) inoculated cell culture sample. A signal value of 206 nA over a threshold value of 3 nA is significant and indicates that coronavirus 229E is the virus present in the sample.
105
Figure 4-3. Stability of CoV-229E on different hard surfaces over a 7-day observation period.
106
Table 4-1. Development of virus induced CPE in inoculated cell lines.
Sampling date
Surface tested Day Cell lines Respiratory virus identified by eSensor RVP
A549 MRC-5 LLC-MK2
VERO E6
11/12/16 Desk top1 Saturday -a - - - 11/13/16 Desk top2 Sunday - - - - 11/14/16 Desk top3 Monday - - - - 11/18/16 Desk top4 Friday +b + ?c + CoV-229E 11/19/16 Door knob Saturday - - - - 11/20/16 Desk top5 Sunday + + ? + CoV-229E 11/22/16 Podium Tuesday - - - - 11/22/16 Desk top6 Tuesday + + ? + CoV-229E 11/22/16 Door knob Tuesday + + ? + CoV-229E 11/22/16 Chair back Tuesday - - - - 11/23/16 Desk top7 Wednesday + + ? + CoV-229E 11/23/16 Door knob Wednesday + + ? + CoV-229E 11/23/16 Chair back Wednesday - - - - 11/24/16 Desk top8 Thursday - - - - 11/25/16 Door knob Friday - - - - 11/26/16 Chair back Friday - - - - a-, No CPE observed. b+, CPE observed. c?, No obvious CPE observed
107
CHAPTER 5 COMPLETE GENOME SEQUENCE OF ENTEROVIRUS D68 DETECTED IN
CLASSROOM AIR AND ON ENVIRONMENTAL SURFACES1
Introduction
Enterovirus D68 (EV-D68) (genus Enterovirus, family Picornaviridae) has
reemerged globally as an important human respiratory pathogen [134-136]. First
identified in 1962 [137], respiratory diseases due to EV-D68 were rarely reported until
the early 2000s [136, 138]. In 2014, EV-D68 caused an outbreak in the United States
that extended to early 2015 [136]. During the recent U.S. outbreaks, EV-68 mostly
affected children, causing clinical manifestations that ranged from mild respiratory
illness to severe respiratory distress requiring hospitalization [136, 139]. Alarmingly,
sporadic cases of nonpolio paralysis/acute flaccid myelitis associated with residual limb
weakness or other neurological deficits occurred during the recent American EV-D68
outbreaks [140-142]. At least three EV-D68 clades exist [136, 139, 142]; most recent
outbreak strains in the United States, including those that caused acute flaccid myelitis,
are from clade B1 [136, 139, 142]. Relatively few EV-D68 genomes have been fully
sequenced.
In this study, we amplified and sequenced the complete genome of enterovirus
D68 (EV-D68) that had been collected from classroom air using a filter-based air
sampling method and by swab sampling of environmental surfaces. Relatively high
Reprinted with permission from Lednicky JA, Bonny TS, Morris JG, Loeb JC. Complete genome sequence of enterovirus D68 detected in classroom air and on environmental surfaces. Genome Announcements. 2016 Jun 30;4(3]:e00579-16.
108
levels of EV-D68 genome equivalents were found per cubic meter of air by quantitative
real-time reverse transcription-PCR (RT-PCR).
Methods and Materials
The virus described here was detected in 4 of 6 air sampler filters and 12 of 16
desktops of a classroom in a university, on 8 September 2015, a few weeks after fall
season classes had started. To favor the detection of airborne virus, tests were
performed immediately after the day’s last classroom session, before airborne virus
would be removed in exhaust air by normal ventilation air exchanges. Active air
sampling was performed at 9 liters/min for 1 h to sample 0.540 m3 of breathing air using
a Sioutas Personal Cascade Impactor Sampler (PCIS) with polytetrafluoroethylene
filters, as described previously [11], and desktop swab samples immersed in UTM viral
transport medium (Copan Diagnostics, USA) [45]. cDNA synthesis from viral nucleic
acids extracted from filters [11] or swabs [45] was performed with avian myeloblastosis
virus (AMV) reverse transcriptase and random hexamers, and PCR was performed
using a panel of respiratory virus primers. Following identification of a specific virus,
quantitative real-time reverse transcription-PCR (RT- PCR) tests [143] was performed to
determine genomic equivalents of the identified virus/m3 in the air samples.
Results and Discussions
Quantitative real-time reverse transcription-PCR (RT- PCR) tests indicated
presence of 400 to 5,000 genomic equivalents of EV-D68/m3 in the air samples. Viral
RNA from the air sample with the highest concentration of virus was used for
sequencing [144], and the complete viral genome was designated EV-
D68/environment/Gainesville/1/2015. Phylogenetics indicate that the virus conforms to
109
EV-D68 clade B1. Attempts to isolate the virus in cell cultures [144] from material
extruded from filters or swab samples were unsuccessful due to rapid overgrowth of the
cells by reovirus and/or adenovirus also present in the samples.
The EV-D68/environment/Gainesville/1/2015 genome has 3 nucleotide (nt)
polymorphisms (C1817T, C3277A, and A4020G) that are present in the majority of EV-
D68 strains of the 2014 U.S. outbreak [139], and in EV-D68/Haiti/1/2014 (GenBank
accession no. KT266905.1) and EV-D68 MEX/DF/2014-InDRE2351 (GenBank
accession no. KT825142.1). For these, the resulting amino acid substitutions T860N
and S1108G at the cleavage sites of viral proteases P2A and P3C may affect their
cleavage efficiency and lead to increased virus replication [139]. As with our findings,
high levels of airborne enteroviruses were detected in a pediatric clinic [145], and this
may be a common finding in indoor settings with enterovirus-infected individuals. Our
work also suggests that young adults can produce airborne EV-D68 and raises the
question of whether airborne transmission is important for spreading the virus. The
complete genome sequence of EV-D68/environment/Gainesville/1/2015 has been
deposited in the GenBank database under the accession number KU509997.
110
CHAPTER 6 DETECTION OF ALPHACORONAVIRUS vRNA IN THE FECES OF BRAZILIAN FREE-
TAILED BATS (TADARIDA BRASILIENSIS) FROM A COLONY IN FLORIDA, USA2
Introduction
Bats (order Chiroptera, suborders Megachiroptera and Microchiroptera) are a
widely distributed group of mammals that comprise ~20% of all known mammalian
species [146]. They are reservoirs of many emerging and reemerging zoonotic viruses,
some of which are highly pathogenic in humans. The emerging viruses exert a
significant public health threat [147, 148] and include ebolaviruses, henipaviruses,
lyssaviruses and coronaviruses [149-154]. These are all viruses that can cause
infections through inhalation routes of exposure, and viruses such as Hendra, Nipah,
and SARS viruses cause severe respiratory infections in humans.
Coronaviruses, order Nidovirales, family Coronaviridae, subfamily Coronavirinae,
are enveloped positive-sense single-stranded RNA viruses. There are four CoV genera:
Alphacoronavirus, Betacoronavirus, Gammacoronavirus and Deltacoronavirus [155].
After it was found that SARS-CoV probably originated in bats [156, 157], a flurry of
investigations uncovered many more novel bat CoVs [158-171]. The recent description
of a bat CoV related to MERS-CoV in Mexican bats [172] emphasized the relevance of
investigating neotropical bats for CoVs.
Thirteen different species of insectivorous bats are found in Florida [173].
Brazilian free-tailed bats (Tadarida brasiliensis), also known as Mexican free-tailed bats,
are one of the most abundant species of bats found throughout Florida, except the
Reprinted with permission from Bonny TS, Driver JP, Paisie T, Salemi M, Morris JG, Shender LA, Smith L, Enloe C, Oxenrider K, Gore JA, Loeb JC, Wu C-Y, Lednicky JA. Detection of Alphacoronavirus vRNA in the Feces of Brazilian Free-Tailed Bats (Tadarida brasiliensis) from a Colony in Florida, USA. Diseases. 2017 Feb 27;5(1):7.
111
Florida Keys [173]. They roost in large colonies and, in Florida, they roost mostly in
man-made structures, including buildings and bridges [173]. Despite the abundance and
potential role of bats in disease transmission, viruses harbored by Florida bats remain
mostly underexplored. With human activity increasingly overlapping the habitats of bats,
the possibility of disease outbreaks resulting from spillover of bat CoVs cannot be ruled
out [174]. Although no human diseases caused by a bat CoV have been identified in
Florida, surveillance of CoVs in bat species is necessary to better predict and prevent
the next emergence of a CoV disease outbreak [174]. In this study, we investigated
whether CoV vRNA could be detected in the feces of Brazilian free-tailed bats in
Florida.
This study reports the detection of an alphacoronavirus RNA-dependent RNA
polymerase (RdRp) gene sequence in the feces of two of 19 different T. brasiliensis that
were capture/release bats that had been evaluated for overall health. The RdRp
sequence is similar but not identical to previously detected sequences in the feces of
two different species of bats (T. brasiliensis and Molossus molossus) in Brazil. In
common with the experience of others doing similar work, attempts to isolate the virus in
cell cultures were unsuccessful. We surmise that this and highly related
alphacoronavirus are carried by Brazilian free-tailed bats living in a wide eco-spatial
region. As various coronaviruses (CoVs) that affect humans emerged from bats, our
study raises the question whether CoVs such as the one detected in our work are yet-
to-be-detected pathogens of humans and animals other than bats.
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Materials and Methods
Collection and Processing of Bat Feces Samples
For this study, free-tailed bats were chosen for two reasons: (a) opportunity; the
bats were from a conservation site wherein the animals’ well-being is periodically
evaluated and bat fecal samples were available for evaluation; and (b) they are among
the most abundant bats often found roosting in buildings in Florida, and hence are most
likely to interact with humans. These bat species were identified and evaluated for
overall health by expert bat biologists of the Florida Fish and Wildlife Conservation
Commission (FWC). The FWC has no designated or required IACUC protocol; however
they follow the guidelines of American Society of Mammalogists for the capture and
handling bats [175]. Nineteen (n = 19) fecal samples were collected from
capture/release bats in Gilchrist County, 8 km southwest of Ft. White, Florida in May
2016. Following collection, the samples were immediately sent to a BSL2-enhanced
laboratory and stored at −80°C. Bat fecal pellets were homogenized to 10% (w/v)
suspensions in Gibco™ advanced Dulbecco’s Modified Eagle Medium (aDMEM) (Fisher
Scientific, Pittsburgh, PA, USA, Cat#12491015) supplemented with 0.2 mM L-alanyl-L-
glutamine (Gibco™ GlutaMAX, Fisher Scientific, Cat# 35050-061), antibiotics (50 μg/mL
penicillin, 50 μg/mL streptomycin, 100 μg/mL neomycin (PSN, Fisher Scientific, Cat
#15640055)) using Covidien Precision™ disposable tissue grinders (Fisher Scientific,
Cat# 06-434-1). The homogenates were cleared of debris by low-speed centrifugation
(5 min at 1500× g), and the supernatants filtered through 0.45 μm PVDF, sterile filters
(Fisher Scientific, Cat# 09-720-4) to remove bacteria and other particulates, and the
filtrates stored at −80°C until further use.
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Virus Isolation Attempts in Cell culture
American Type Culture Collection (ATCC, Manassas, VA, USA) cell lines VERO
E6 (African green monkey kidney; CRL-1586), A549 (human lung adenocarcinoma
epithelium; CCL-185), and Tb1 Lu (Tadarida brasiliensis lung epithelium; CCL-88) were
propagated as monolayers as previously described [11], and a newly confluent
monolayer of each of these three cell lines was inoculated with aliquots (75 μL) of the
filtered homogenates. The inoculated cells were incubated in a humidified 5% CO2
atmosphere at 35°C, and observed daily for virus-specific cytopathic effects (CPE).
Screening of Viral Nucleic Acids for Coronavirus RNA
Viral nucleic acids were extracted from both filtered homogenates and spent cell
media using the QIAamp viral RNA minikit (Qiagen, Germantown, MD, USA,
Cat#52904). CoV RNA screening was performed by reverse transcription-polymerase
chain reaction (RT-PCR) targeting conserved region of the RNA-dependent RNA
polymerase (RdRp) gene. Briefly, viral RNA was denatured at 65 °C for 5 min in the
presence of SUPERase-In RNase inhibitor (Invitrogen Corp., Carlsbad, CA, USA,
Cat#AM2694), cooled rapidly on ice and cDNA synthesis performed with Omniscript
Reverse Transcriptase (RT) (Qiagen, Cat# 205111) for 1 h at 37 °C using primer
CorTheoNL63R1 (5′-CCRTCATCAGANAGAATCATCAT-3′). PCR was performed using
One Taq DNA polymerase (New England BioLabs, Ipswich, MA, USA, Cat# M0480)
with primer pair CorTheoNL63F1 (5′-GGTTGGGAYTATCCYAANTGTGA-3′) and
CorTheoNL63R1. With an expected product size of 440 bp, PCR was performed as:
initial denaturation step (94°C for 2 min); followed by 40 cycles of 94°C (60 s), 48°C (60
s), 68°C (60 s), and a final extension step at 68°C for 5 min. PCR products were
visualized by gel electrophoresis in a 1.5% ethidium bromide-stained agarose gel.
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In preparation for sequencing, samples wherein a 440 bp PCR amplicon were
initially observed were re-amplified using high-fidelity polymerases. Briefly, cDNA was
produced using AccuScript High Fidelity Reverse Transcriptase (Agilent Technologies,
Inc., Santa Clara, CA, USA, Cat# 200820) in the presence of SUPERase-In RNase
inhibitor, and PCR was performed using Phusion Polymerase (New England BioLabs,
Cat# M0530S) with denaturation steps performed at 98°C. The re-amplified samples
were individually electrophoresed in a 1.5% ethidium bromide-stained agarose gel and
the 440 bp amplicon excised and purified using a Qiagen MinElute Gel Extraction kit
(Qiagen, Cat# 28604). The purified 440 bp PCR amplicons were then subjected to
Sanger Sequencing. Preliminary sequence analyses were performed with the NCBI
BLAST software.
Phylogenetic Analyses of the CoV RdRp Sequences
For phylogenetic analyses, all available RdRp CoV sequences were downloaded
from NCBI (http://www.ncbi.nlm.nih.gov/). The sequences were aligned using Clustal
Omega [176] and manually edited in Bioedit [177]. Phylogenetic signal was investigated
by likelihood mapping in the program TREE-PUZZLE [178] in order to assess the
phylogenetic signal in the sequence alignment and to remove the appropriate identical
sequences. The maximum likelihood tree was estimated using the best nucleotide
substitution model (TPM3 + I + G4) according to the results from IQ-TREE [179].
Bootstrapping (1000 replicates) was also performed using the IQ-TREE software. This
was done in order to statistically analyze branch support in the maximum likelihood tree.
The maximum likelihood tree was then manually edited in FigTree
(http://tree.bio.ed.ac.uk/software/figtree/) to display geographical locations of the
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sequences and to show branches with strong statistical support (bootstrap values
greater than 95%).
Results
Virus-induced CPE were not observed in cell cultures during a four-week
observation period, suggesting a virus(es) had not been isolated. However, CoVs do not
always cause easily discernable CPE in the cell lines used for this study, so for
additional evidence of virus isolation, RT-PCR tests were performed. Coronavirus RNAs
were also not detected by RT-PCR of spent cell culture media collected and tested by
RT-PCR every five days, and in RNA purified from the infected cells at the terminal
observation time-point (30 days post-infection). Attempts to isolate CoVs from the
inoculated cell lines were thus considered unsuccessful.
Out of 19 bat fecal samples, 440 bp amplicons corresponding to a conserved
region of the CoV RdRp gene were generated by RT-PCR from two filtered
homogenates (Figure 6-1). The sequence for both amplicons was identical and
submitted to GenBank (Accession: KX663833.1). Following BLAST analyses, the
consensus RdRp sequence was found to be highly similar but not identical to
alphacoronavirus RdRp sequences identified in Brazilian free-tailed bats and velvety
free-tailed bats (Molossus molossus) from southern Brazil [180]. The percentage of
nucleotide and amino acid sequence identity ranged from 94% to 96%.
Phylogenetic analyses suggest that the RdRp gene sequence that had been RT-
PCR-amplified from the feces of free-tailed bats in Florida clusters with RdRp gene
sequences that were from two different types of bats in Brazil (Figure 6-2).
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Discussion
Bats have been recognized as the natural reservoirs of a wide variety of viruses,
many of which are important human and animal pathogens. Special attention has been
paid to bat coronaviruses (BtCoVs) as the two emerging CoVs (SARS-CoV and MERS-
CoV) causing human disease outbreaks in recent years are suggested to have emerged
from bats [174]. It is plausible that other emerging BtCoVs may be able to cross the
species barrier and cause human disease [174].
In Florida, 13 different species of insectivorous bats reside, 12 of which are year-
round and only one species is seasonal [173]. Brazilian free-tailed bats are one of the
permanent residents. Considering the potential public health implications of bat species
living in close proximity to human inhabitants, the viruses harbored by these wide
varieties of bat species in Florida have largely been underexplored. To our knowledge,
this is the first report of alphacoronavirus vRNA detection in feces from presumably
healthy insectivorous bats in Florida. The high degree of sequence similarity of the
Florida BtCoV with that of a Brazilian BtCoV from two different bat species (T.
brasiliensis and M. molossus) [180] suggests that similar CoVs may be present in
different bat species and across geographically distant regions. Unlike the clade
containing the Brazilian and Florida free-tailed bat CoVs, most of the other RdRp
sequences cluster according to bat species, indicating that the viruses evolve according
to bat species (Figure 6-2). In the other bat coronavirus clades, geographical location
also appears to have an influence on the evolution of the viruses, but the clade with our
sequence of interest from Florida contains bat species from the families Molossidae and
Phyllostomidae. The similarity between our Florida BtCoV sequence and those of the
Brazilian BtCoVs could be an indicator of how bat BtCoVs in Florida will evolve. The
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branch length in the maximum likelihood tree implies that the Florida BtCoV is diverging
away from the Brazilian BtCoVs (Figure 6-2). The divergence of the Florida BtCoV could
indicate the beginning of a new clade based on geographical location and not bat
species. It is too early to infer other conclusions: Brazilian free-tailed bats are also found
in Mexico and in Texas, where they are called Mexican free-tailed bats. Unfortunately,
we were unable to find RdRp sequences for the BtCoVs of those bats in public
databases, and it is plausible that those bat populations found geographically closer to
Florida will harbor CoVs more similar to the one detected in this work.
Although restricted in sample number, location and the single bat species
investigated, this study suggests that surveillance and identification of CoVs in Florida
bats is worthy.
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Figure 6-1. Representative results of RT-PCR detection of alphacoronavirus vRNA in
Brazilian free-tailed bat feces (BF). Lane 1 (M), 100 bp MW markers; Lane 2 (+), HCoV-NL63 vRNA, positive control; Lane 3 (−), negative control; Lane 4, BF#1; Lane 5, BF#2; Lane 6, BF#3; Lane 7, BF#5; Lane 8, BF#6; Lane 9, BF#7; Lane 10, BF#17; Lane 11, BF# 18; Lane 12, BF#19. Virus-specific 440-bp PCR products amplified by PCR primers CorTheoNL63F1 and CorTheoNL63R1 are present in lanes 2, 6 (asterisk), and 10.
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Figure 6-2. Maximum likelihood tree based on the nucleotide sequences of partial RdRp gene of bat CoVs. In parenthesis are the bat species that make up the clade. Abbreviations: BtCoV, bat coronavirus; Rm-BtCoV, Rocky Mountain bat coronavirus. Red circle indicates strong statistical support (bootstrap >95%)
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CHAPTER 7 ISOLATION AND DETECTION OF ARBOVIRUSES AND HUMAN CORONAVIRUS
229E IN BLOOD COLLECTED FROM CHILDREN IN RURAL HAITI IN 2016
Introduction
Arthropod-borne viruses (arboviruses) are viruses that are transmitted to humans
by hematophagous arthropods such as mosquitoes, sandflies, biting midges and ticks
[181]. These viruses are maintained in transmission cycles between vertebrate hosts
and arthropod vectors [34]. Arboviral infections in humans can vary, ranging from
asymptomatic to fulminant fatal diseases. Clinical symptoms, when present, can be
categorized as systemic febrile illness, hemorrhagic fever and invasive neurological
disease [34]. At least 135 arboviruses have been implicated in human disease, the vast
majority of which are RNA viruses belonging to genera: Alphavirus, Flavivirus,
Orthobunyavirus, Nairovirus, Phlebovirus, Orbivirus, Vesiculovirus and Thogotovirus
[182, 183].
Mosquito-borne viruses are an emerging threat to human health and well-being
throughout the world [37]. The explosive spread of mosquito-borne viruses to new
geographical areas in the recent years has alarmed the public health community
worldwide. The continued presence of DENV, CHIKV, and ZIKV in endemic areas and
their expansion through the Americas place an estimated 3.9 billion people living in 120
different countries at risk [37]. DENV has been spreading across countries over the past
30 years and today an estimated 390 million people are infected annually [37]. In 2015-
2016, ZIKV infections swept across the Americas, resulting in more than 360,000
suspected cases [37]. CHIKV first emerged in the Americas in 2013 [184], with numbers
rising to 1.8 million suspected cases from 44 different countries and territories to date
[185]. With many more cases of these arboviral infections likely going undetected and/or
121
unreported, these numbers may just represent the tip of the iceberg. This escalating
burden of infections and potential spread of arboviruses to new geographic areas have
alarmed the public health community, resulting in a flurry of research to understand
arbovirus disease epidemiology, prevention and control [37]. As part of this ongoing
endeavor, researchers at UF have initiated projects to determine the causative agents
and incidence of arbovirus infections in Haiti and elsewhere in the Caribbean and in the
Americas.
Methods and Materials
Since July 2014, researchers at UF have been monitoring arboviral transmission
in rural Haiti, through collaboration with the school clinic associated with the
Christianville Foundation School, in the Gressier/Leogane region of Haiti, about 20
miles west of Port-au-Prince. The clinic serves four schools with approximately 1,250
students, from pre-kindergarten to grade 12 [186]. Following a protocol approved by the
University of Florida Institutional Review Board (IRB) and the Haitian National IRB,
diagnostic blood samples were routinely collected from children presenting with acute
undifferentiated febrile illness at the clinic. Written consent was obtained from
parents/guardians of all study participants. Between March and May 2016, blood
samples were obtained at the school clinic from a total of 111 school children who met
the criteria of acute undifferentiated febrile illness (i.e. febrile illness with no localizing
signs, as observed in patients with pneumonia, upper respiratory infections, urinary tract
infections) [187]. In this study, virus isolation and identification were attempted on
plasma derived from twenty-seven (n= 27) blood samples.
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Initial Screen of Plasma Samples for Zika-, Dengue- and Chikungunya Viruses
An initial screen for the presence of ZIKV, DENV and CHIKV vRNA in patient
plasma samples was performed by molecular methods. As previously described [13],
viral nucleic acids were first extracted from virions in the plasma samples using the
QIAamp viral RNA minikit (Qiagen, Cat#52904), then tested for the presence of ZIKV,
CHIKV and DENV types 1-4 using primers described by Faye et al. [188], Lanciotti et al.
[189], and Santiago et al. [190], respectively. Viral RNA that tested negative for the
vRNAs of ZIKV, CHIKV and DENV types 1-4 were further tested by RT-PCR using a
universal primer system for flaviviruses [191]. Virus isolation was concomitantly
attempted from all plasma samples that were found negative or borderline in these initial
RT-PCR tests. A variety of mammalian cell lines were used to cast a wide net and favor
the isolation of different viruses.
Virus Isolation in Cell Cultures
American Type Culture Collection (ATCC, Manassas, VA) cell lines A549 (human
lung adenocarcinoma epithelium; CCL-185), LLC-MK2 (rhesus monkey kidney
epithelium, CCL-7), VERO E6 (African green monkey kidney; CRL-1586) and MRC-5
(human lung fibroblast, CCL-171), WI-38 (human lung fibroblast, CCL-75), SK-N-BE(2)
(human neuroblastoma, CRL-2271) were propagated as monolayers in Gibco™
advanced Dulbecco's Modified Eagle Medium (aDMEM) (Fisher Scientific,
Cat#12491015) supplemented with 0.2 mM L-alanyl-L-glutamine (Gibco™ GlutaMAX,
Fisher Scientific, Cat# 35050-061), antibiotics [50 𝜇g/mL penicillin, 50 𝜇g/mL
streptomycin, 100 𝜇g/mL neomycin (PSN, Fisher Scientific, Cat #15640055)] and 10%
(v/v) low IgG, heat-inactivated gamma-irradiated fetal bovine serum (FBS) (HyClone,
Logan, UT) as previously described [13]. Aliquots of plasma samples (50 μL) from each
123
patient were inoculated onto sub-confluent cell lines and non-inoculated cells were
incubated in parallel with the inoculated ones at 37°C in a humidified CO2 incubator.
The cells were refed every 3 days with maintenance media and observed daily for
formation of virus-specific cytopathic effects (CPEs). The cells were observed for 26
days before being considered negative for virus isolation.
RT-PCR of vRNA Purified from Spent Cell Growth Media and Infected Cells
Viral nucleic acids were extracted from both spent cell growth media and infected
cells using QIAamp viral RNA minikit (Qiagen, Cat#52904). Standard RT-PCR for the
detection of ZIKV vRNA was performed as described by Balm et al. [192]. RT-PCR
using primers targeting specific regions of the CoV-229E matrix (M) and nucleocapsid
(N) genes were performed as previously described [193-195]. cDNA synthesis was
performed with Omniscript Reverse Transcriptase (RT) (Qiagen, Cat# 205111) in the
presence of SUPERase-In RNase inhibitor (Invitrogen Corp., Cat#AM2694) and One
Taq DNA polymerase (New England BioLabs, Cat# M0480) was used for PCR
amplification of cDNA. PCR amplicons were visualized by UV irradiation after size
separation through gel electrophoresis in a 1.5% ethidium bromide-stained agarose gel.
Purified vRNA samples extracted at various time intervals during cell culture
were also tested for the presence of DENV and ZIKV by real-time RT-PCR (rtRT-PCR)
using primers and probes described by Santiago et al. [190] and Faye et al. [188],
respectively.
Sequencing
Sequencing of ZIKV, DENV, CoV-229E genomes were performed using a
primer-walking approach and Sanger sequencing.
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GenMark RVP Assay
Respiratory virus detection and influenza virus subtyping were performed using a
GenMark multiplex PCR eSensor XT-8 Respiratory Viral Panel (GenMark Diagnostics,
Inc., Carlsbad, CA) following the manufacturer’s instructions. This panel includes tests
for influenza A virus (including subtype determination); influenza B virus; respiratory
syncytial virus types A and B; parainfluenza virus types 1, 2, 3 and 4; human
metapneumovirus, human rhinovirus; adenovirus groups B, C and E; human
coronavirus types 229E, NL63, HKU1 and OC43. As previously described, extracted
nucleic acids from the spent cell-growth media were used to perform a multiplex
PCR/RT-PCR assay and the amplified DNA targets analyzed by electrochemical
detection [57]. After data acquisition and analysis, the instrument generates an output:
eSensor Respiratory Viral Panel Currents Report (RUO).
Results
Twenty-seven (n= 27) plasma samples collected between March 3 and May 12,
2016 were inoculated onto several cell lines and few arboviruses and a human
respiratory virus were isolated and identified from the cell culture samples. The results
are summarized in Table 7-1.
Isolation and Identification of ZIKV in Plasma Sample Cell Culture
Some of the plasma sample inoculated LLC-MK2 and VERO E6 cells showed
CPE 17dpi, which were characteristic of ZIKV infection: prominent perinuclear vacuoles
in LLC-MK2 and VERO E6 cells, cell rounding and death with overall destruction of the
cell monolayer (Figure 7-1). CPE appeared earlier in inoculated LLC-MK2 than in VERO
E6 cells. Viral RNA extracted from the cell spent growth media and infected cells tested
positive for ZIKV by both conventional (Figure 7-5) and real-time RT-PCR.
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Isolation and Identification of DENV-3 in Plasma Sample Cell Culture
MRC-5 and VERO E6 cells inoculated with some plasma samples exhibited CPE
consistent with DENV infection. Diffuse cytopathic effects were observed in some of the
VERO E6 cell lines 26dpi and MRC-5 cells showing blebbing, cell rounding, followed by
destruction of the monolayer within 8dpi-13dpi. CPE in MRC-5 cells appeared earlier
than in VERO cells and were suggestive of DENV infection. Real-time RT-PCR using
extracted viral RNA from cell culture samples confirmed the presence of DENV type 3 in
the plasma samples (Fig 7-2; Table 7-1).
Co-infection of Plasma Cell Culture with ZIKV and DENV-4
A more intriguing pattern of CPE was observed in LLC-MK2 and VERO E6 cells
inoculated with plasma sample collected between April and May 2016. Within 4 days
post-inoculation, LLC-MK2 cells exhibited perinuclear vacuoles which appeared in
distinct clusters throughout the cell monolayer. As the CPE progression was followed
over the next few days, a diffuse cytopathic effect began to emerge and take over the
cell monolayer with the vacuoles gradually starting to diminish (Fig 7-3). By 8dpi, the
LLC-MK2 monolayer was almost destroyed. Similar pattern of CPE was also observed
in the inoculated VERO E6 cells (Fig 7-4). Real-time RT-PCR and sequencing results
confirmed that the cells were co-infected with two arboviruses: ZIKV and DENV-4.
Isolation and Identification of Human coronavirus 229E (CoV-229E)
Some cell cultures inoculated with one plasma sample (collected on March 8)
displayed CPEs that were distinct from what would be expected in cells infected with
alpha- and flaviviruses (Fig 7-6). The CPE observed were suggestive of those caused
usually by human respiratory viruses: vacuolation of cells, formation of syncytia,
followed by clumping and detachment of cells from the monolayer. The CPE were most
126
obvious in MRC-5 and VERO E6 cells and less apparent in LLC-MK2 cells. As some
respiratory virus strains replicate and produce progeny in the cells without causing
easily observed CPE, the spent cell-growth media from the inoculated cells was
periodically tested using molecular assay for the detection of possible viral agents. Viral
genomic RNA extracted from cell lysates and virions in spent culture media from three
inoculated cell lines (LLC-MK2, VERO E6 and MRC-5) were identified as CoV-229E by
the GenMark RVP system (Fig 7-7). GenMark RVP detection of CoV-229E was further
confirmed by RT-PCR assays using primers targeting specific regions of the CoV-229E
matrix (M) and nucleocapsid (N) genes and by sequencing of CoV-229E whole genome.
Discussion
Arboviral infections are believed to be prevalent in Haiti for many years. DENV,
first reported in 1976, is now considered endemic in Haiti [196]. ZIKV, an emerging
pathogen apparently introduced from French Polynesia and Easter Island in 2013-2014,
have reached Haiti and different parts of the Americas [197]. A previous study by the UF
researchers reported isolation of ZIKV from 3 children who were seen at a school clinic
in the Gressier region of Haiti in December 2014 [198]. Since DENV and ZIKV,
members of the Flaviviridae family, are both transmitted by Aedes mosquito vectors, co-
infection in human with ZIKV and DENV may not be surprising [199]. In fact,
researchers at UF have previously reported co-infection of ZIKV and DENV-2 in a
traveler returning from Haiti [200]. In the present study, ZIKV and DENV-3 were isolated
from different patient plasma cell cultures while many of the cell cultures (15 out of 27
samples tested) were co-infected with ZIKV and DENV-4. It is intriguing to observe the
diversity of arboviruses isolated from plasma samples collected just over a period of 3
months, suggesting more than one type of DENV and ZIKV may have been circulating
127
among Haitian population during that period. The CPE induced by ZIKV-DENV type 4
co-infection and its progression over time was also worth observing, where an earlier
appearance of ZIKV CPE was followed by DENV-4 CPE gradually taking over the cell
monolayer as time progressed. However, the dynamics of these two co-infecting viruses
in the patients remains unknown. In vitro studies have suggested that DENV antibodies
can enhance ZIKV infection [201]. Also, infections caused by these two flaviviruses are
often asymptomatic [197, 202]. When symptoms do occur, they tend to be quite similar.
Therefore, the impacts of co-infection of ZIKV-DENV type 4 in these patients remain to
be determined.
Except for one sample (Accession# 16-1-1480, collected May 11, 2016; positive
for DENV-3), all other plasma samples came out negative for ZIKV and DENV in the
initial RT-PCR based screening. As these viruses are most likely to be detected in blood
samples approximately 1 week after symptom onset [203], a low-level viremia at any
point during infection could lead to false negative RT-PCR results. For better diagnosis
and risk assessment, suspected arbovirus-containing human samples can be inoculated
onto susceptible cell lines which may allow for virus replication and subsequent
detection of viral RNA by RT-PCR [204].
In this study, CoV-229E was isolated from a single plasma sample cell culture.
The sample was obtained on March 8, from one of the 27 children with febrile illness but
with no apparent respiratory symptoms. No ZIKV or DENV was detected in this specific
plasma sample or in the inoculated cell cultures. Since the study was focused mainly on
arbovirus detection, blood samples were not collected from children exhibiting
respiratory symptoms. Isolation of CoV-229E from blood in one of these children was
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rather unexpected, and to our knowledge, has not been reported previously from Haiti.
CoV-229E is usually associated with respiratory diseases of varying severity ranging
from common cold to pneumonia [7]. Besides respiratory ailments, it has also been
implicated in neurological diseases in humans [205]. It is unclear if there were more
children infected with coronaviruses during that period and the impact of viremia in this
child with only febrile illness also remains unknown. A thorough investigation focusing
on respiratory infections among these children could shed some more light on the
dynamics of respiratory infections in a place where arboviral infections are also
prevalent.
This study was conducted on a limited number of plasma samples. It,
nevertheless, provided a learning opportunity to investigate the diversity of arboviruses
and concomitant presence of respiratory virus in rural Haiti. The findings reiterate the
importance of virus isolation using the appropriate cell lines and proper cell culture
techniques in diagnostic virology.
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Figure 7-1. Appearance of ZIKV-induced CPE in LLC-MK2 and VERO E6 cells. A) Normal LLC-MK2 cells. B) Perinuclear vacuolation of LLC-MK2 cells 17 days post infection (pi) at 37˚C. C) Normal VERO E6 cells. D) Vacuolation of VERO E6 cells and destruction of the monolayer 17 days post infection (pi) at 37˚C. All original images are at 400X magnification.
130
Figure 7-2. Appearance of DENV-induced CPE in VERO E6 and MRC-5 cells A) Normal VERO E6 cells. B) Diffuse cytopathic effects in VERO E6 cells 26 days post infection (pi) at 37˚C. C) Normal MRC-5 cells. D) Blebbing, cell rounding and destruction of MRC-5 monolayer 8 days post infection (pi) at 37˚C. All original images are at 400X magnification.
131
Figure 7-3. Appearance of CPE in LLC-MK2 cells induced by ZIKV-DENV co-infection. A) Normal LLC-MK2 cells; B), & C) Perinuclear vacuolation of LLC-MK2 cells 4 days post infection (pi) followed by; D) & E) diffuse cytopathic effects and destruction of monolayer 6 days pi and F) 8 days pi at 37˚C. All original images are at 400X magnification.
132
Figure 7-4. Appearance of CPE in VERO E6 cells induced by ZIKV-DENV co-infection. A) Normal VERO E6 cells. B) Vacuolation of VERO E6 cells 6 days post infection (pi) at 37˚C; followed by C) & D) diffuse cytopathic effects throughout the monolayer 8 days pi at 37˚C. All original images are at 400X magnification.
133
Figure 7-5. Representative results of RT-PCR detection of Zika virus in LLC-MK2 cells inoculated with patient plasma samples. From left to right: Lane 1, 100 bp MW markers; Lane 2, Zika virus positive control; Lane 3, negative control; Lane 4, Plasma sample#11 inoculated cells and Lane 5, Plasma sample#12 inoculated cells, both 17 days post infection (pi) at 37˚C. Virus-specific 192-bp PCR products amplified by Balm primers are present in lanes 2, 4 and 5.
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Figure 7-6. Appearance of VERO E6 and MRC-5 cells during cell culture. A) Normal VERO E6 cells. B) Cell clumps and destruction of VERO E6 monolayer 14 days post infection (pi) at 37˚C. C) Normal MRC-5 cells. D) Vacuolation and rounding of MRC-5 cells and destruction of the monolayer 14 days post infection (pi) at 37˚C. All original images are at 400X magnification.
135
Figure 7-7. Representative eSensor Respiratory Viral Panel currents report (RUO)
136
Table 7-1. Haiti plasma sample cell culture report
Sample accession#
Collection date
Cell lines Virus isolated & detected A549 MRC-5 WI-38 LLC-
MK2 VERO E6
SK-N-BE(2)
16-1-1582 03.03.16 * + * - + * DENV-3 16-1-1583 03.03.16 * + * - + * DENV-3 16-1-1584 03.04.16 * + * - + * DENV-3 16-1-1585 03.08.16 * + * + + * CoV-229E 16-1-1586 03.10.16 * + * - + * DENV-3 16-1-1587 03.10.16 * - * + + * ZIKV 16-1-1588 03.11.16 * - * + + * ZIKV 16-1-1580 04.04.16 * + * - + * DENV-3 16-1-1581 04.05.16 * + * - + * DENV-3 16-1-1543 04.06.16 - * - + + - ZIKV, DENV-4
16-1-1544 04.06.16 - * - + + - ZIKV, DENV-4
16-1-1545 04.06.16 - * - + + - ZIKV, DENV-4
16-1-1533 04.14.16 - * - + + - ZIKV, DENV-4
16-1-1534 04.15.16 - * - - - -
16-1-1537 04.15.16 - * - + + - ZIKV, DENV-4 16-1-1540 04.18.16 - * - + + - ZIKV, DENV-4 16-1-1542 04.20.16 - * - + + - ZIKV, DENV-4 16-1-1529 04.22.16 - * - + + - ZIKV, DENV-4 16-1-1530 04.25.16 - * - + + - ZIKV, DENV-4
137
Table 7-1. continued
Sample accession#
Collection date
Cell lines Virus isolated & detected A549 MRC-5 WI-38 LLC-
MK2 VERO E6
SK-N-BE(2)
16-1-1663 05.09.16 - * - + + - ZIKV, DENV-4 16-1-1487 05.10.16 - * - + + - ZIKV, DENV-4
16-1-1488 05.10.16 - * - + + - ZIKV, DENV-4 16-1-1489 05.10.16 - * - + + - ZIKV, DENV-4 16-1-1492 05.10.16 - * - + + - ZIKV, DENV-4 16-1-1479 05.11.16 * + * - + * DENV-3 16-1-1480 05.11.16 * + * - + * DENV-3 16-1-1483 05.12.16 - * - + + - ZIKV, DENV-4 * Cell line not used + CPE observed - CPE not observed DENV-3, Dengue virus type 3; CoV-229E, Coronavirus 229E; ZIKV, Zika virus; DENV-4, Dengue virus type 4
138
CHAPTER 8 CONCLUDING REMARKS
In this dissertation, attempts were made to detect, isolate and identify various
viruses, including human respiratory viruses, and arboviruses, from a variety of human
specimens and environmental samples. A combination of virus isolation in cell-culture
and PCR-based techniques were used to accomplish the tasks. This work was
performed in partial fulfillment of the requirements for the degree of doctor of philosophy
in public health, and to gain theoretical and practical knowledge in diagnostic and
applied virology for a career in public health microbiology. As shown in the body of work
presented here, the mating of cell-culture isolation of viruses with antigen and/or virus-
genome based detection methods can prove effective for virology-related health risk
assessments and surveillance. However, success depends on fine-tuning these
techniques relative to the virus in question. Starting from specimen/sample to virus
identification, every step requires careful consideration and planning regarding: (a)
choice of specimen/sample and manner of collection, (b) sample transport and storage,
(c) sample processing, (d) choice of appropriate cell-lines or primary cells for virus
isolation, and their maintenance, (e) use of proper optics for microscopy of virus-
infected cell cultures, and (f) antigenic and genome-based detection methods. Some
takeaway points and ideas for future research based on the findings of the body of work
presented in this dissertation are as follows:
As described in Chapter 1, the work undertaken in this dissertation had five
specific aims focusing on two broad categories of viruses: human respiratory viruses
and arboviruses. To advance our understanding of respiratory virus transmission and
investigate Florida bats as reservoirs of coronaviruses that might be potentially
139
pathogenic to humans, attempts were made to detect, isolate and identify these viruses
from aerosols, environmental surfaces and bat feces. For collection of viable virus
aerosols, three different air sampling devices were evaluated: a Sioutas Personal
Cascade Impactor Sampler (PCIS) with polytetrafluoroethylene filters, an SKC
BioSampler, and the VIVAS. Airborne viruses were successfully collected by all three
samplers, though their collection efficiencies and their abilities to retain virus infectivity
varied. For example, EV-D68 genome equivalents were detected from classroom air but
no viable EV-D68 was isolated in cell culture. It may be the case that the collected EV-
D68 genomes were inactivated by impaction onto the filters, though the collected
viruses may have been inactivated by drying as the sampled air was pulled through the
PCIS. When modified parameters (developed by our research group) were used instead
of standard operating procedures, the collection efficiency of the SKC BioSampler for
virus aerosols was improved but still considered sub-optimal. Nevertheless, viable
viruses were collected during air samplings performed during a late influenza outbreak
in spring and post-Thanksgiving 2016. Of the three different air sampling devices that
were tested under field conditions, the VIVAS out-performed the SKC BioSampler and
PCIS. To reduce the chances of collecting large expired/coughed/sneezed droplets, the
VIVAS was positioned at least 2 m away from seated patients during air sampling. And
indeed, viable (infectious) IFV and other respiratory viruses were isolated and identified
from these samples, suggesting that the patients’ respiratory actions produced small
aerosols containing infectious viruses.
However, as the VIVAS enlarges the size of the aerosol particles during
collection, the actual size of the collected particles in which viable viruses were present
140
was not determined. Future research could employ a particle sizer to characterize the
size distribution of the particles being collected prior to size amplification. This would
provide insights on the potential risk posed by the aerosols, especially with regard to
small particle aerosols that are breathed deep into the LRT, as deposition of respiratory
viruses therein can lead to pneumonia.
Viruses differ in their dimension and biophysical and external biochemical
properties. For example, non-enveloped viruses are usually hydrophilic, and enveloped
viruses hydrophobic. Apart from MS2 (a non-enveloped bacteriophage) and influenza A
H1N1 viruses (which are enveloped viruses), the collection efficiencies of the VIVAS for
other laboratory- generated aerosolized viruses are not known. It is important to find out
if the device works equally well for collecting hydrophilic (e.g. human adenovirus) and
other hydrophobic human respiratory viruses, and whether the collection media should
be adjusted so it is polar for hydrophilic and non-polar for hydrophobic viruses. As the
concentration of airborne viruses in ambient air is typically low, it would be informative
to test the collection efficiency of the VIVAS for different concentrations of various types
of aerosolized viruses.
Infections caused by many respiratory viruses can lead to severe disease
manifestations and complications, especially in children, elderly and the
immunocompromised. For instance, complications of the flu can include infections of the
ear (otitis media) and sinuses (sinusitis), pneumonia (caused by viral or secondary
bacterial infection), bronchitis, inflammation of the heart (myocarditis), brain
(encephalitis), muscle tissues (myositis, rhabdomyolysis), multi-organ failure (e.g.
respiratory and kidney failure), and exacerbation of chronic medical conditions like
141
asthma, congestive heart disease, or diabetes [206]. Since many of these complications
are life-threatening, it would be interesting to test the air facilities housing pediatric and
immunocompromised patients or in assisted living facilities for the elderly using the
VIVAS. If viable viruses are found in the ambient air using the VIVAS, and on high-touch
surfaces by surface sampling, additional infection control and prevention strategies
could be devised to help protect these groups of vulnerable populations from
preventable infections.
Detection of viable CoV-229E and the genomes of rhinovirus and EV-D68 on
classroom surfaces reinforces the notion that contact transmission may be a route of
transmission for these respiratory viruses in a classroom or similar setting. The high
degree of nucleotide sequence similarities of the environmental strains of CoV-229E
and EV-D68 to the clinical isolates suggests these viruses may have similar emitting
source(s). A broader study might include linking the virus to the person (s) shedding the
virus by simultaneous collection of clinical specimens from symptomatic individuals in
indoor settings and environmental samples from the same settings, followed by
attempts to isolate and identify human respiratory viruses from these specimens and
samples. The efficacy against common human respiratory viruses of alcohol ethoxylates
(AE), which had been used for cleaning of the classroom surfaces, was not investigated
in the studies presented in this dissertation. Given that the minimum infective dose of a
respiratory virus can be very low [130], it is worth performing independent evaluations of
commonly used cleaning and disinfecting agents against these common human
respiratory viruses.
142
The thirteen different bat species found in Florida, 12 of which are year-round
residents, may harbor viruses that can infect and cause illnesses in humans. In
particular, bats have been identified as natural hosts of coronaviruses that cause
severe/fatal infections in humans, and they are known to harbor other viruses such as
Rabies virus and paramyxoviruses that can also cause lethal infections in humans.
From a public health standpoint, a proactive approach should be taken with regards to
surveillance of Florida bats for potential human pathogens. In the study presented in
Chapter 6, alphacoronavirus RdRp gene sequence was detected in 2 out of 19 feces
specimens from presumably healthy Brazilian free-tailed bats in Florida. The high
degree of sequence similarity of the Florida BtCoV with that of a Brazilian BtCoV from
two different bat species (T. brasiliensis and M. molossus) [180] suggests that similar
CoVs may be present in different bat species and across geographically distant regions.
Future efforts at the identification/isolation of known or novel bat viruses should include
testing of different types of bat specimens and the use of primary bat cells (e.g. cells
from bat trachea, lungs, kidney, intestine etc.) for virus isolation.
Due to abundance of mosquito vectors, mosquito-borne infections are endemic in
Haiti. In the study described in Chapter 7, virus isolation and identification were
attempted on plasma derived from twenty-seven (n= 27) blood specimens collected
from children with undifferentiated febrile illnesses. Cell-cultures inoculated with 15 out
of 27 plasma specimens were co-infected with two arboviruses: ZIKV and DENV type 4.
Some other cell culture samples were positive only for ZIKV or DENV type 3.
Remarkably, CoV-229E was also isolated from a single plasma sample. The findings
suggest co-circulation of multiple arboviruses in Haiti during March-May 2016. In
143
addition, the isolation of CoV-229E from plasma serves as a reminder that multiple viral
agents cause febrile illnesses, and during an outbreak, undifferentiated fevers cannot
be assumed to have a common cause. Further investigations will shed more light on the
diversity of arboviral and respiratory virus infections among Haitians and also improve
understanding on the impacts of arbovirus co-infections in patients.
144
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BIOGRAPHICAL SKETCH
Tania was born in Bangladesh, grew up all over the country and spent several
years of her childhood in the Middle East. Travel had an enormous impact in her life and
continues to be so. Despite her strong desire to serve her country’s armed forces and
continue the family tradition, she gave that up for a more intellectually driven pursuit: to
become a microbiologist. She attended University of Dhaka, the oldest and renowned
institution of Bangladesh, and received her bachelor’s and master’s degrees in
microbiology. Right after post-graduation in 2010, she was appointed at her parent
department, Department of Microbiology, University of Dhaka, as a junior faculty
member. She had been involved in teaching and research back home until August
2013, when she got accepted into the One Health PhD Program at Environmental and
Global Health (EGH), University of Florida with Graduate School Preeminence Award.
At EGH, she was fortunate to receive training in virology under the mentorship of Dr.
John A. Lednicky. During her stay in “Lednicky Lab”, she was actively involved in
research on human respiratory viruses and arboviruses. She has presented several
posters on her research findings, authored or co-authored 3 published research articles
in peer reviewed journals and few more are in the pipeline for publication. She has
isolated and identified several human respiratory- and arboviruses from environmental
and clinical samples and forty-seven (47) viral genomic sequences identified through
her research have been published in GenBank.
During her stay at EGH, she was showered with love, affection and accolades
from her peers and faculty members. Tania received her PhD in Public Health from the
University of Florida in summer of 2017 and returned to Bangladesh to continue serving
at University Dhaka.