Molecular Bead Shaving : A newprocedure for magnetic readoutbiosensors

Harisha Ramachandraiah

Degree project in applied biotechnology, Master of Science (2 years), 2010Examensarbete i tillämpad bioteknik 30 hp till masterexamen, 2010Biology Education Centre and Department of Genetics and Pathology, Molecular Medicine, UppsalaUniversitySupervisors: Associate Professor Dr.Mats Nilsson and Dr.David Herthnek

Table of contents

Abbreviations

Summary

1.0 Introduction.............................................................................................................. 3

1.1 Biosensors................................................................................................................. 3

1.2 Magnetic particle based biosensors.......................................................................... 4

1.2.1 SQUID.................................................................................................................. 5

1.3 Nucleic acid based sensors and enzymes................................................................. 5

1.4 DNA Ligase............................................................................................................. 6

1.5 Restriction Enzymes................................................................................................. 6

1.6 Padlock probes and Rolling circle replication.......................................................... 7

1.7 Volume- amplified magnetic nanobead detection assay.......................................... 8

1.8 Molecular bead shaving........................................................................................... 10

1.8.1 Concept of the project and approach.................................................................... 10

1.9 Aim of the project.................................................................................................... 13

2.0 Results...................................................................................................................... 14

2.1 Initial optimization of RCA primer and restriction oligonucleotides concentrations for the

preparation of Dreadlock probes..................................................................................... 14

2.2 Background signal reduction.................................................................................... 14

2.2.1 Heat treatment of captured RCA primers............................................................... 15

2.2.1.2 Preheat treatment coupling and post hybridization ligation................................ 16

2.2.2 Pre-restriction digestion before RCA to reduce background signal....................... 16

2.3 Selection of suitable enzyme for molecular bead shaving........................................ 17

2.4 Determination of optimum restriction digestion time............................................... 18

2.5 Effect of salt on release of digested blobs from dreadlock probes............................ 18

2.6 Finding the optimum post restriction digestion incubation time............................... 19

2.7 Effect of heat and incubation time after salt treatment............................................. 20

2.8 Blocking of beads to avoid non specific binding of RCA primers............................ 20

2.9 Comparison of signals between 100 nM RO and 10 nM RO..................................... 21

2.10 Comparison between Dynabeads®MyOneTM Streptavidin C-1 and T-1 magnetic beads

with respect to signal........................................................................................................ 22

2.11 Theoretical calculation............................................................................................. 22

3.0 Discussion.................................................................................................................. 23

4.0 Materials and Methods.............................................................................................. 26

4.1 Oligonucleotides........................................................................................................ 26

4.2 Padlock probes hybridization and ligation................................................................ 27

4.3 Capturing of RCA primers to beads.......................................................................... 27

4.4 RCA on magnetic beads............................................................................................ 27

4.5 C2CA and monomerization....................................................................................... 27

4.6 Molecular bead shaving of DNA coils...................................................................... 28

4.7 Blocking of beads surface.......................................................................................... 28

4.8 Labeling of RCA coils............................................................................................... 28

4.9 Microfluidic quantification, image acquisition and analysis..................................... 28

5. Acknowledgment......................................................................................................... 30

6. References.................................................................................................................... 31

1

Abbreviations

AMP Adenosine mono-phosphate

ATP Adenosine tri-phosphate

BSA Bovine serum albumin

C2CA Circle-to-circle amplification

DNA Deoxy-ribonucleic acid

dNTPs Deoxy-nucleotide tri-phosphate

ELISA Enzyme linked immunosorbent assay

HRCA Hyper-branched rolling circle amplification

MBS Molecular bead shaving

NAD Nicotinamide adenine dinucleotide

OLA Oligonucleotide ligation assay

PCR Polymerase chain reaction

PNK Polynucleotide kinase

RCA Rolling circle amplification

RCP Rolling circle product

RGB Red-green-blue

RNA Ribonucleic acid

RO Restriction oligonucleotides

SMD Single molecule detection

SSD Salmon sperm DNA

S/N Signal to noise ratio

SNPs Single nucleotide polymorphism

SQUID Superconducting quantum interference device

TIFF Tagged image file format

VAM-NDA Volume- amplified magnetic nanobead detection assay

2

Summary

In diagnostics the detection of the causative agent or biomarkers is the most important step

before any treatment. A number of new biosensors have been developed for early stage

detection of many diseases, but magnetic particle based biosensors have received

considerable attention because of their unique properties of physical, chemical and biological

stability.

This project focuses mainly on the proof of principle and development of a new procedure

called “Molecular Bead Shaving” (MBS) for both magnetic and optical readout for detection

of DNA. To perform MBS, molecular tools such as padlock probes and rolling circle

amplification (RCA) were employed to synthesize DNA coils (Blobs) on the magnetic beads

to produce a probe. A target DNA-specific padlock was amplified and monomerized by

circle-to-circle amplification (C2CA) and used along with a specific enzyme to release the

DNA coils from the beads.

For the optical readout, micron-sized particles were used and the released blobs were labelled

with fluorescent oligonucleotides and visualized by confocal microscopy. For magnetic

readout the change in Brownian relaxation behaviour of magnetic nanobeads induced by a

change in hydrodynamic bead volume was measured using Superconducting Quantum

Interference Device magnetometers. More specifically, when beads contain DNA coils, the

hydrodynamic bead volume will be increased and by cutting off the DNA coils using

amplified target DNA and restriction enzyme the hydrodynamic bead volume will decrease.

This change in hydrodynamic bead volume induces a change in Brownian relaxation

frequency upon magnetization which is measured by Superconducting Quantum Interference

Device (SQUID).

We have successfully demonstrated the principle of MBS for optical readout and have begun

the work to translate this procedure for magnetic readout.

3

1.0 Introduction

Keeping good health is one of the biggest concerns for human civilization. Efforts towards

developing drugs are ongoing at an ever higher pace, but before treatment a suitable

diagnostic method is necessary to identify the disease. In spite of the extensive research and

medical revolutions we still lack the potential to efficiently combat various diseases. Many

times the failure to treat a disease is related to the improper or late diagnosis of the disease.

So it is imperative to identify the cause of disease at an early stage. In clinical diagnostics and

biomedical research the detection of biomolecules is most insistent. An ideal diagnostic

method should be reliable, robust, flexible, convenient, sensitive, high throughput, highly

selective, affordable, portable [52], and should be reliable at different places such as the

battle field, hospitals, post office, doctor’s office, food markets and even at home [11].

Apparently, the growing technological advancement in biomarker detection, quantification,

imaging and single molecule detection at low concentration, plays a vital role to detect the

infectious agents selectively.

Many conventional techniques like PCR, immunological techniques like radioactive

immunoassay (RIA) and enzyme linked immunosorbent assay (ELISA), fluorescence based

assay, culture and colony counting approaches are powerful, but they are laborious, time-

consuming and may require bulky instruments [42] [6]. In this context, biosensors are more

reliable, robust may allow label free detection and are expected to reach implications in

medicine, point-of-care clinical diagnostics, genomic and proteomic research [21].

1.1 Biosensors

According to the International Union of Pure and Applied Chemistry (IUPAC), a biosensor is

defined as a device, which provides quantitative analytical information using a bio-

recognition element when coupled to a signal transduction system [10]. A typical biosensor

consists of signal transduction and bio-recognition elements. Usually, nucleic acids, protein,

carbohydrates, lipids and whole cells are used as the bio-recognition elements, of which

nucleic acids and proteins are being widely used in this post genomic era [44]. There is a

wide range of transduction system including mechanical, potentiometric, thermal, optical,

magnetic, electrochemical and piezoelectric that are in use today. These versatile tools have

great applicability in both the academy and industry, specifically in the areas which

encompass diagnostics, environmental monitoring, life science and drug discovery.

A majority of available diagnostic methods requires some kind of fluorescent, luminescent,

radiometric or colorimetric readout to detect the biomolecules of interest (targets), levying

limitation of additional time, false positive results (due to unspecific interactions) and costs.

Especially, fluorescent tags are being widely used in many biological applications, but have

disadvantages of low intensity, self-absorption, photo bleaching, self- fluorescence and

thermal fluctuations [44]. To some extent quantum dots, the fluorescent semiconductor nano

crystals exhibit high quantum yield and overcome some of these problems related to

fluorescence. They also exhibit a tuneable emission profile, but the difficulty in synthesis of

quantum dots and high costs limit its application [44]. To overcome some of the limitations

4

posed by previously mentioned methods, a variety of label-free bio-sensing platforms were

developed based on optical and non-optical detection methods such as Surface Plasmon

Resonance, bilayer interferometer, cantilever detection systems, label-free intrinsic imaging,

acoustic detection systems and magnetic detection systems [37]. Consequently, more than

6000 articles and 1100 patents issued or pending have been published between 1998 and

2004 [56].

1.2 Magnetic particle based biosensors

In 1986, Dynal Biotech introduced functionalized magnetic microparticles for the separation

of desired molecules from an arbitrary solution. Today such particles are used for bio-

separation, cell sorting and as direct labels to detect molecules [42].

Usually, these magnetic nanoparticles are single magnetic domains made up of Fe3O4, Fe2O3

or CrO2 either dispersed in polymer matrix or in silica [4] and are super paramagnetic. Due to

the super paramagnetic properties the magnetic particles spontaneously flip upon

magnetization and randomize the magnetization directions at room temperature, avoiding

agglomeration [5].

Magnetic particles are widely used in bio-sensing platforms because of their unique

properties of physical, chemical and biological stability. They facilitate sensitive

measurement in body fluids such as blood, serum, plasma, urine, saliva cerebral spinal fluid

and urine, because these fluids virtually not exhibit magnetic background [21]. Furthermore,

their magnetic properties are stable over time and easy surface fuctionalization of magentic

beads with a plethora of biological and chemical surface coatings, which simplifies the

binding of specific biomolecules. Last but not least, the size of the particles can be tailored

from micron-to-nano scale, thus increasing surface to volume ratio [20].

In 1949 pioneering work by Neel et al. [5] showed the importance of single magnetic

particles and relaxation events. Later in 1974 Dreyer et al. used magnetic particles to label

biomolecules [5]. Many methods were developed for detection of magnetic labels either

directly or indirectly. In 1996, Kriz et al. demonstrated the magnetic bead assay for the first

time, by using induction coils to measure the change in magnetic permeability of specific

binding events in a Maxwell bridge setup [8]. In the same year, it was shown that

piezoresistive cantilevers could be used to measure the change in specific binding of

functionalized beads to the biomolecules [20]. Several magnetic based biosensors were

developed such as Hall effect biosensors [8], anisotropic magnetoresistance biosensors, giant

magnetoresistance biosensors, tunnelling magnetoresistance biosensors [5],

magnetoimpedence biosensors, fluxgate biosensors and Magnetic signature based biosensors

[5].

5

1.2.1 SQUID

Superconducting Quantum Interference Device (SQUID) is a device which detects extremely

weak changes in the magnetic field of an applied magnetic flux. SQUID uses a

superconducting coil that contains Josephson junctions, which measures the decay in

remanence of magnetized nanoparticles. When an external magnetic field is applied to the

super paramagnetic particles they line up along the field lines and when the field is removed

they remained aligned for a short period before randomizing again. This decay in self-

magnetization is defined as remanence.

Biofunctionalized super paramagnetic nanoparticles increases in the hydrodynamic volume,

when binding to the target. When these particles are magnetized and demagnetized by an

external field, they undergo two types of relaxation; the Neel’s relaxation and Brownian

relaxation. Brownian relaxation depends on the hydrodynamic volume of the nanoparticles.

Compared to the target-bound particles, the unbound particles rapidly relax the Brownian

rotation and do not contribute to the overall signal. By measuring the difference in remanence

of samples using SQUID, it is possible to deduce the amount of surface bound particle [48].

The magnetic susceptibility measured by the SQUID is given by equation (1) [31].

(1)

ω is the angular frequency of the applied magnetic field, Hac is the amplitude of the applied

magnetic field, m(ω) is the complex magnetization, χ0 and χ∞ are the high and low frequency

susceptibility respectively. τ is the characteristic relaxation time. The Neel’s relaxation and

Brownian relaxation time is given by τN (2) and τ

B (3) respectively.

Vp is the nanoparticle volume, k is the Boltzman constant, T is temperature in Kelvin, τ0 is

microscopic relaxation time, K is magnetic anisotropic constant, Vb is the volume of the bead

and η is the viscosity of the solution.

1.3 Nucleic acid based sensors and enzymes

A major discovery of the 20th Century was the discovery of the double stranded DNA

structure by Watson and Crick in 1953 [54]. The unique properties of specific base pairing

between two DNA strands, and sequence variations within and between species provide a

unique tool for diagnostics [40]. Relying on the hybridization principle many techniques

emerged of which immunoassays like Immuno-RCA [46], Immuno-PCR [45], Biobarcodes

[40], Proximity ligation assay [49] and Aptamers [33] are widely in use today.

Apart from nucleic acids, enzymes are also used in the bio-sensing platform. Combination of

oligonucleotides and enzymes are utilized to facilitate a wide range of bio-sensing

applications. Enzymes such as polymerases, ligases and restriction enzymes are being widely

used and will be described below.

6

1.4 DNA Ligase

DNA ligase catalyzes the phosphodiester bond formation between 5’-phosphate and 3’-OH

group of nucleotides [28]. This end-joining event is necessary for DNA repair, replication

and recombination. Ligation is a three step process involving adenylation, deadenylation and

nick closure. During adenylation the adenosine mono-phosphate (AMP) group is transferred

from ATP or NAD to the catalytic site, followed by deadenylation where AMP is transferred

to the 5’- phosphate at the nick through a pyrophosphate linkage. Finally, forming of the

phosphodiester bond between 3’-OH and 5’-phosphate group is done by releasing AMP [55].

The high fidelity of ligase enabled ligase-based technologies such as Oligo Ligation Assay

(OLA) [53], Ligase mediated target amplification, Ligation detection reaction and universal

arrays, and ligation based sequencing [51].

1.5 Restriction enzymes

Restriction endonucleases is a group of deoxyribonucleases, which recognizes nucleotide

sequences specifically and cuts double stranded DNA, either forming blunt ends or sticky

ends depending on the type of enzymes used. They are widely used in gene cloning,

identification of single nucleotide polymorphisms (SNPs), genomic DNA digestion etc.

At certain specific reaction conditions some restriction enzymes shows relaxed, sequence

specificities called Star activity. Reaction conditions such as non-optimal buffer, high

glycerol concentration, presence of organic solvents, substitution of Mg2+

with other divalent

cations [Mn2+

, Cu2+

, Zn2+

], high enzyme concentration and prolonged reaction time will

contribute to the star activity [18][19]. In this study we used four different restriction

enzymes (Table 1).

Table 1: Restriction enzymes used in this study Name of

Enzymes

Recognition Site Preferred

buffer

Optimal

temp

Inactivation temp

and time

Ref

MscI

5’…TGGCCA…3’

3’…ACCGGT…5’

NEBuffer 4

37 oC

65oC for 20 min

and at salt

concentrations

> 150 mM.

[16]

ScaI

5’…AGTACT…3’

3’…TGCTGA…5’

NEBuffer 3 37 oC 80o for 20 min [14]

ScaI-HF™ 5’…AGTACT…3’

3’…TGCTGA…5’

NEBuffer 4 37 oC 65oC for 20 min [17]

AluI 5’...AGCT...3’

3’...TCGA...5’

NEBuffer 4 37 oC 65oC for 20 min [15]

7

1.6 Padlock probes and Rolling circle replication

Padlock probes are the extension of Oligonucleotide Ligation Assay (OLA) [53], which relies

on a pair of independent oligonucleotide probes. Upon adjacent hybridization to a target

sequence, they are joined by the action of ligase and the can be amplified by PCR. By

contrast, the padlock probe is a linear single stranded oligonucleotide typically consisting of

70-90 nucleotides; it consists of a linker sequence that may carry a detection tag flanked by

two different segments complimentary to the target DNA or RNA [35, 34]. On proper

hybridization to the target sequence the 3’-OH and the added 5’-Phosphate terminal end of

the probe segments are brought in close proximity and by the action of ligase they are

converted into circularized probe (see Figure 1). The inability of ligase to covalently join

mismatching oligonucleotides, especially at the 3’-terminus, guarantees the selectivity by

distinguishing between similar sequences variants [53]. Some of the major advantages of

these probes are; the dual recognition target complimentary segments of probes, providing

high specificity and excellent sensitivity, circularization traps the probes by catenation to the

target sequence, resisting extreme stringent washes [35]. It has been demonstrated that the

padlock probes can detect single nucleotide variation in situ [36].

Figure 1: Schematic representation of nucleic acid target recognition using padlock probes. The ends of

padlock probe hybridized to specific matching nucleic acid is covalently joined by the action of ligase to form

circularized probe target complex, which can be amplified and detected.

In 1990s, two independent researchers showed that a circularized DNA molecule can be used

as a template for DNA replication by DNA polymerase in a RCA reaction [1, 12]. Later,

circularized padlock probes were used as template for RCA [43]. Researchers at Yale

University School of Medicine demonstrated isothermal exponential hyper branched RCA

[HRCA] by employing the highly processive φ29 DNA polymerase, which has a strong 3’-5’

strand displacement exonuclease activity [29,30] and showed that the visualization of

individual rolling circle products (RCP) was possible by hybridizing short fluorescent

detection probes to the tandem repeated sequence of the RCP. In an isothermal RCA single-

stranded DNA concatamers will be generated and in solution spontaneously collapse into

8

sub-micron sized DNA coils (blobs), the size of which depends on the replication time (RCA

time).

Usually padlock probes are produced synthetically by phosphoroamidite chemistry, and is

limited by the length and high cost. Comparatively, longer and cheaper padlock probes can be

synthesized using PCR and shown to have three-fold greater signal in in situ analysis [9] even

though it resulted in lower yield than chemical synthesis. Recently, it has been shown that by

using padlock probes and RCA it is possible to detect microRNA [50] and in situ detection of

individual transcripts [7].

A highly controlled amplification of reacted padlock probes was demonstrated by Circle-to-

Circle amplification (C2CA) [13]. C2CA is a three-step process initiated by RCA of

circularized probes, followed by monomerization of concatemeric amplification products and

another cycle of circularization and RCA reaction. After three cycles of C2CA a billion-fold

amplification is possible but the reaction is completely depending on the RCA time and

number of cycles. The reaction kinetics is represented by nc: where c is the number of cycles

and n is the number of monomer produced during RCA reaction per cycle [13].

Advancing technological development in microscopy and fluorescence based technology

makes it possible to visualize and measure single molecule responses. In contrast to the

golden standard for nucleic acid, quantitative real-time PCR, single molecule detection

(SMD) provides better precision and more accurate measurement [23]. RCP are the true

single molecule amplified signal, containing 1000 tandem repeats of a 100-mer DNA circle

after one hour polymerization [22]. Hybridization of fluorescent-labelled oligonucleotides

(detection probes) to RCP makes them to appear as a bright spot under confocal microscope

due to confined cluster of fluorophore. In 2006 Jarvius et al reported a novel approach of

homogenous detection and enumeration of labelled blobs by pumping them through a

microfluidic chamber, fabricated using thermoplastic injection moulding and visualized under

confocal microscope [24, 25], where each Blobs visible as a bright spot compared to the

background fluorophore. Multiplexing was made possible by tagging different RCP with

different fluorescent tagged detection oligos [23].

1.7 Volume- amplified magnetic nanobead detection assay [VAM-NDA]

In 2001 Connolly and St. Pierre theoretically proposed a biosensor based on Brownian

relaxation frequency of magnetic beads. Later, the same principle was employed by others

and demonstrated antibody-antigen binding activity [48]. By combining the DNA technology

with nano-diagnostic technology Stromberg et al developed [38] a novel nucleic acid

detection assay. In this assay the magnetic nanoparticles are biofunctionalized with single-

stranded covalently conjugated oligonucleotide detection probes, which contains a sequence

that complementary to the tandem repeating sequences of the RCP. In the presence of RCP in

the test sample, the bio-functionalized magnetic beads cluster together with the RCP by

sequence specific hybridization and increases the hydrodynamic volume of the beads, which

essentially corresponds to the size of the blobs, thus the Brownian relaxation frequency of

magnetic beads was considerably lowered, which was measured by SQUID magnetometer at

9

37oC. However, no changes in the magnetic frequency spectrum can be seen in the absence of

RCA coils in the test sample (see Figure 2) [38]. The positive samples has essentially exhibit

two different frequencies High frequency peak (HFP) and low frequency peak (LFP) in the

imaginary part of the complex magnetisation spectrum. Using this HFP and LFP peak

discrimination between the negative and positive samples can be done, which is referred as

“turn-off” or “turn-on” detection. ”Turn-on” detection is possible by using 40 nm sized beads

but only turn off detection is possible with larger beads [32].

Figure 2: Schematic illustration of the VAM-NDA. In positive samples the padlock probe recognise target

single stranded DNA molecule (grey lines) and the ends of the padlock probes (light blue lines) hybridized to

the target DNA molcules and joined by the action of ligase. Circularized probes obtained after ligation are

amplified by RCA for a specified period. The produced RCP is detected by the addtion of biofunctionalized

nanoparticle that contains a detection sequence, which are complementary to the RCP repeating motifs. Upon

this, binding of biofunctionalized beads to the RCP exhibits Brownian relaxation behavior measured by SQUID

magnetometer. In negative sample no change in the magnetic spectrum can be observed, where as in positive

samples the magnetic spectrum decreases.

A limit of detection of 4 pM target DNA was reported in this method [38], and showed that

an excess of genomic background material in the test sample will not affect the detection

sensitivity. A increasing in temperature significantly increases the bead incorporation

kinetics, but immobilization kinetics is limited by diffusion of coil and also depends on bead

size [38, 32]. Multiplexing was reported by incorporating different sized (40 nm, 130 nm and

250 nm) specific biofunctionalized beads for each kind of targets [39]. However, there are

several problem associated with this procedure such as enhanced kinetics and increase

amplification signal [32].

No circularization

No Ligation

No RCA

m’’

log(f)

Positive sample Negative sample

10

1.8 Molecular bead shaving

In this study we would like to modify the VAM-NDA method by developing a new principle

called “Molecular bead shaving”.

1.8.1 Concept of the project

Instead of having covalently conjugated detection probes on the nanobeads as previously

described in VAM-NDA [38], RCA primers were covalently conjugated to the nanoparticles

and blobs will be synthesized by employing Padlock probes and RCA. These Blobs-on-bead

complexes were named “Dreadlock probes”, which will be used as the reporter molecule (see

Figure 3a).

Specific target DNA identified by using specific padlock probes was amplified by using

C2CA. Furthermore, RCP obtained after C2CA were monomerized. These monomers, which

contain a sequence complementary to a Dreadlock root sequence, are used as restriction

oligos (RO) and together with a specific restriction enzyme can cut off the blobs from the

Dreadlock probes and release them into solution. This process of cutting off the Blobs from

the bead surface is referred as to “Molecular bead shaving” (MBS). The loss of Blobs from

the Dreadlock probes reduces the hydrodynamic volume of the beads and shifts the Brownian

relaxation frequency from low to high, which can be measured by a SQUID magnetometer.

This change in magnetic frequency spectrum from low to high is easier to interpret than

measuring the reduction of the frequency spectrum from high to low as described in VAM-

NDA [38]. If the target DNA is not present in the test sample, there will not be any restriction

oligos synthesised for restriction digestion of Dreadlock probes, and thus no changes in the

Brownian relaxation frequency will be observed. By developing this new principle of

molecular bead shaving a better sensitivity can be achieved. In an ideal case, we expect each

monomer formed after C2CA and final monomerization will potentially release every

synthesized blob from the Dreadlock probes, thus increasing the sensitivity, and amplifying

the signal. The disadvantage of this method is the presence of non-biofunctionalized beads,

which constitute part of the background signal. Since, the SQUID magnetometer

measurement takes around 2.5 hour per sample, which is a limiting factor when large

numbers of samples were used; thus, we modified our approach for optical readout instead of

magnetic readout as explained below.

11

Figure 3a: Schematic illustration of the Molecular bead shaving concept. (A) Preparation of Dreadlock

probes: The DNA coils (Blobs) syntheized onto the nanoparticles that conatins covalently conjuagted RCA

primer, by emlpoying padlock probes and RCA. (B) In positive samples the padlock probe recognizes the target

single stranded DNA molecule (grey lines) and the ends of the padlock probes (light blue lines) hybridized to

the target DNA molcules and joined by the action of ligase, and these circularized probes were amplified by

C2CA and finally monomerized. These monomer have a sequence that are complementary to the dreadlock root

(yellow line). Together with suitable enzyme release the blob from the dreadlock probes and reduces the

hydrodynamic bead volume that induces a change in Brownian relaxation frequency, that is measured by

SQUID. (C) In the absence of target DNA molecule, no monomers were produced, thus no change in the

magnetic spectrum will be observed.

Approach

To investigate the principle of Molecular bead shaving, Dreadlock probes were synthesized

on streptavidin coated micron-sized beads using biotinylated RCA primers instead of

biofunctionalized nanobeads as explained in the concept. After restriction digestion of

dreadlock probes, the blobs will be released from the bead surface and labeled with the

fluorescently tagged oligonucleotides that are complementary to the tandem repeat sequence

of blobs. Furthermore, homogenous detection and enumeration of the labelled blobs was

achieved by pumping the sample through the microfluidic chamber and visualized under

confocal microscope. In the absence of target DNA in the original sample no blobs will be

RCA

C2CA

Monomerization No monomerization

No circularization

No Ligation

No RCA

No C2CA

B).Positive sample C).Negative sample

m’’

log(f)

A). Preparation of Dreadlock probes

Restriction enzyme

12

released from the Dreadlock probes and no fluorescent signal can be observed (see Figure

3b). Dreadlock probes without added RO were used as negative control in all the

experiments.

Figure 3b: Schematic illustration of the Molecular bead shaving appraoch. (A) Preparation of Dreadlock

probes: The blobs are syntheized onto the streptavidin coated micron-sized beads by capturing biotinylayed

RCA primers using padlock probes and RCA. (B) In positive samples the padlock probe recognizes the target

single stranded DNA molecule (grey lines) and the ends of the padlock probes (light blue lines) hybridized to

the target DNA molcules and joined by the action of ligase. Reacted probes are amplified by C2CA and finally

monomerized. These monomer have a sequence that are complementary to the dreadlock root (yellow line).

Together with suitable enzyme releases the blobs from the dreadlock probes. The released blobs were labelled

with the fluorescent tagged oligonucleotides that are complementary to the tandem repeat sequence of RCP.

Furthermore, homogenous detection and enumeration of the labelled blobs was achieved by pumping the sample

through the microfluidic chamber and visualized under confocal microscope. (C) In the absence of target DNA

in the original sample no blobs will be seen.

RCA

C2CA

Monomerization No monomerization

No circularization

No Ligation

No RCA

No C2CA

No Signals

A).Preparation of Dreadlock probes B).Positive sample C).Negative sample

13

1.9 Aim of the present study

The principle aim of this project work is to develop a new magnetic biosensor principle

called Molecular bead shaving, a potential platform for rapid and low cost magnetic nano

diagnostic assay.

To set up and test the concept of Molecular bead shaving onto micron-sized beads for

optical readout.

Translation of the MBS procedure for biofunctionalized nanometer sized beads for

magnetic readout.

o To optimize covalent conjugation of oligos onto to the nanobeads.

o Separation of non-biofunctionalized beads, which constitute part of the

background signal.

14

2.0 Results

2.1 Initial optimization of RCA primer and restriction oligonucleotides concentrations for the

preparation of dreadlock probes

To test the principle of molecular bead shaving our first aim was to obtain an optimum

coverage of blobs onto the streptavidin-coated beads. This was necessary in order to have a

good dynamic range. Since the amount of dreadlock probe synthesis depends on the number

of biotinylated RCA primers coupled onto the beads, we started our investigation by

determining the optimal concentration of RCA primers required to produce dreadlock probes

and restriction oligos required for restriction digestion to cleave blobs from the dreadlock

complex. Three different concentration of RCA primers (10 pM, 100 pM and 1 nM) and two

different concentration of restriction oligos (RO) 10nM and 1µM were used. In the following

experiments synthetic oligos, which have same polarity as their C2CA monomerized products

were used as a restriction oligos.

Figure 4: Determination of optimal concentration of RCA primers and restriction oligos. 1 nM, 100 pM

and 10 pM represent three different concentrations of RCA primers. X axis represents the concentration of RO

and Y axis represents the number of Blobs counted under confocal microscope respectively. The Negative

samples contain no restriction oligonucleotides.

As shown in Figure 4 increasing the concentration of RCA primers, resulted in high signal

with low standard deviation, but equally increased signals were seen in negative samples (no

added RO). Thus the signal to noise ratio (S/N) was drastically reduced, where S/N ratio is

the number of blobs counted in positive samples divided by number of blobs counted in the

negative samples

2.2 Background signal reduction

It was hypothesized that the cause for background signal could be due to nonspecific binding

of RCA primers to the beads surface or it could be due to the complementary binding of RCA

primer to itself and others due to its palindromic nature as shown in Figure 5. We also

suspected that the reduction in S/N could be due to star activity of the ScaI enzyme.

1

10

100

1000

10000

100000

neg 10nM 1µM

Nu

mb

er

of

cou

nte

d B

lob

s(l

og 1

0)

Concentration of Restriction oligos

10pM

100pM

1nM

15

5' TTTTTTTTTTTTTTTTTTTTAATTACCAGTACTCGACAACATTGGCGTGACTCAAAGGCTCAC 3’

3' ACTCGGAAACTCAGTGCGGTTACAACAGCTCATGACGATTAATTTTTTTTTTTTTTTTTTTT 5’

Figure 5: Schematic representation of streptavidin coated magnetic beads coupled to RCA primers. RCA

primer self-annealing sites are marked in red.

2.2.1 Heat treatment of captured RCA primers

To test the proposed hypothesis of non-specific binding of RCA primers onto the bead

surface, an experiment was performed in which beads coupled with RCA primes with pre-

hybridized circularized padlock probes were heated at different temperatures for 10 min

before RCA, presuming that the heat treatment might reduce the non-specific binding of the

RCA primers to beads surface.

Figure 6: Preheat treatment coupling and post ligation. Padlock probes were hybridized with RCA primers

and ligated; thereafter these RCA primers were coupled onto to the beads and heated at different temperatures

before RCA for 10 minutes.

The results shown in Figure 6 demonstrate that the background signal linearly decreased with

increase in temperature. The value at 55oC may be an experimental error and the signals tend

to disappear at higher temperatures of 75oC and 85

oC.

0

500

1000

1500

2000

2500

3000

3500

4000

noheat 55 65 75 85

Nu

mb

er o

f c

ou

nte

d B

lob

s

Temperature (oC)

neg

100nM RO

16

2.2.1.2 Preheat treatment coupling and Post hybridization ligation

In this experiment, the beads initially coupled only with RCA primers were heated at

different temperature for 10 minutes and washed with 1X B&Wtw buffer, after which the

hybridization and ligation of padlock probes were carried out.

A B

Figure 7: Preheat treatment coupling and Post ligation. (A) Number of amplified signals (B) Signal to noise

ratio in the experiment.

As shown in the Figure 7A the number of blobs drastically diminished with the increase in

temperature, but at higher temperatures (65oC and 75

oC) the background signal was reduced

significantly with proportional decrease in positive signals. Figure 7B shows an increase in

the S/N ratio with the increase in temperature.

2.2.2 Pre-restriction digestion before RCA to reduce background signal

To test the hypothesis of complementary binding of RCA primers forming itself and others

causing background signal, an experiment was performed in which RCA primers coupled

onto the beads were treated with ScaI to digest the dimers of RCA primers. After restriction

digestion the beads were washed with 1X B&Wtw buffer followed by RCA and MBS.

1

10

100

1000

10000

100000

RT 55 65 75

Nu

mb

er

of

cou

nte

d B

lob

s(l

og 1

0)

Temperature (oC)

neg

100nM RO

1

10

100

1000

RT 55 65 75

S/N

Temperature (oC)

17

Figure 8: Pre-restriction digestion of RCA primers. Number of amplified single blobs

As seen in Figure 8 there is no difference in the signal between the pre-restriction digestion

and normal sample. From this result it is clear that complementary sequence of RCA primers

might not be responsible for causing the background signal.

2.3 Selection of suitable enzyme for Molecular bead shaving

After several experiments with ScaI the background signals did not reduce. So we tested a

High Fidelity ScaI-HF and MscI enzymes for molecular bead shaving. In this experiment we

used three different enzymes ScaI, MscI and ScaI-HF respectively.

A B

Figure 9: Finding a right enzyme for molecular bead shaving (A) Number of amplifed signals obtained after

restriction digestion with three enzymes (B) Signal to noise ratio in the experiment.

From the above results it is evident that Sca1-HF is not suitable for molecular bead shaving.

Even though the S/N ratio of MscI is higher than the ScaI, the numbers of blobs in the

positive sample are proportionally lower. However, here afterwards we used MscI enzyme

for rest of our experiments unless mentioned.

1

10

100

1000

10000

neg 100 nM RO

Nu

mb

er o

f co

un

ted

Blo

bs

(lo

g1

0)

Concentration of Restriction oligos

Pre ScaI digestion

No pre ScaI digestion

1

10

100

1000

10000

neg 100nM RO

Nu

mb

er o

d c

ou

nte

d B

lob

s

(lo

g1

0)

concentration of RO

ScaI-HF

MscI

ScaI

0

5

10

15

20

25

ScaI-HF MscI ScaI

S/N

Enzymes

18

2.4 Determination of optimum Restriction digestion time

When MscI was used for the restriction digestion, we observed a low background signal and

also the numbers of counted blobs in the positive samples were too low when compared to

the theoretical amount of blobs. Therefore, to increase the signal, we investigated the

optimum time required by the enzymes to cut the blobs from dreadlock probes, by digesting

the samples at different incubation periods at 37oC.

A B

Figure 10: Restriction Digestion time study (A) Dreadlock probes were treated with Mscl and digested at

different incubation periods at 37 0C (B) Signal to noise ratio in the experiment.

The results above show that the signals increased linearly with the incubation time and seem

to saturate after 30 minutes. From Figure 10B it was evident that the S/N increased with

increasing in the incubation time. This suggests an incubation time of 30 minutes is quite

sufficient. Hereafter we used 30 minutes restriction digestion time for rest of the experiments

unless mentioned.

2.5 Effect of salt on release of digested blobs from Dreadlock probes

It was suspected that the low signals in the positive samples could be due to non-specific

adsorption of cleaved blobs onto the surface of beads, caused by van der Waals force or by

electrostatic interaction between beads surface and blobs. Therefore, in order to reduce these

interactions and to increase the signals, an experiment was performed in which 1% (v/v)

Tween20 and a high concentration of salt was added to the restriction digested samples.

1

10

100

1000

10000

1 3 10 30 60

Nu

mb

er

of

cou

nte

d B

lob

s(l

og 1

0)

Time (minutes)

neg

100nM RO

1

10

100

1 3 10 30 60

S/N

Time (minutes)

19

A B

Figure 11: Effect of salt on release of digested blobs. (A) Number of amplified signals, after the addition of

1% (v/v) Tween20 and with varying concentration of NaCl to the restriction digested samples (B) Signal to

noise ratio in the experiment.

Figure 11 (A and B) shows that the signals increased linearly with the increasing

concentration of salt, thereby increasing the S/N ratio. This results suggest that salt is

necessary to release the blobs from the dreadlock probes. However, the values at 1 M NaCl in

both the panels might be an experimental error. Hereafter, 2 M NaCl and 1% Tween20 was

added to the restriction digested dreadlock probe samples unless mentioned.

2.6 Finding the optimum post restriction digestion incubation time

Addition of salt appeared to increase the S/N ratio. However, to further increase the S/N ratio,

the salt treated restriction digested dreadlock probes were incubated at 650C for different

interval time, presuming that increase in temperature with sufficient incubation time could

probably enhance the kinetics of blob release from the dreadlock probes and might yield

better S/N ratios.

A B

Figure 12: To determine the optimum post-restriction digested incubation time (A) Number of amplified signals, after the heat treatment of restriction digested dreadlock probes (B) Signal to noise ratio in the

1

10

100

1000

10000

100000

0 0.5 1 2

Nu

mb

er o

f co

un

ted

Blo

bs

Concentration of NaCl (M)

neg

pos

0

10

20

30

40

50

60

0 0.5 1 2

S/N

Concentration of NaCl (M)

1

10

100

1000

10000

100000

normal 0 10 30 60

Nu

mb

er o

f co

un

ted

Blo

bs

(log

10)

Time (minutes)

neg

pos

0

10

20

30

40

50

60

normal 0 10 30 60

S/N

Time (minutes)

20

experiment. Normal in the panel (A) represents the sample without addition of any salt and also not heated, 0

minute in both the panels represent sample with no salt added but heated at 65oC.

As shown in the Figure 12A the signal increased linearly with respect to the incubation time,

but as shown in the panel (B) the S/N ratio decreased over incubation time.

2.7 Effect of heat and incubation time after salt treatment

It was suspected from the previous experiment that heating the samples at 65oC for an hour

would cause subsequent unspecific release of blobs from the dreadlock probes thus

decreasing the S/N ratio. Therefore, to investigate the effect of heat and incubation time, in

this experiment the temperature was further increased from 65oC to 75

oC and incubated for

15 min instead of one hour incubation.

Figure 13 Effects of heat and incubation time Samples after restriction digestion were heated at two different

temperatures 65oC and 75oC respectively. A negative control without the enzyme was also included in this

experiment.

The above result in Figure 13 shows that, at temperature of 75 0C the background signal

increased and supports our theory of breakage of streptavidin and biotin interactions.

2.8 Blocking of beads to avoid non specific binding of RCA primers

From our previous experimental results it was evident that addition of salt is necessary to

reduce the electrostatic interaction between beads. Therefore, to reduce the non-specific

interaction of blobs to the surface and binding of RCA primers, we used blocking agents such

as 2% dry milk and Salmon Sperm DNA (SSD) to block the bead surface.

1

10

100

1000

10000

100000

+ + + - - 75 ºC

- - - + + 65 ºC

- + + + + Mscl

- - + - + 100

nM_RO

Nu

mb

er

of

cou

nte

d b

lob

s(l

og 1

0)

21

Figure 14: Blocking of bead surface. To reduce non-specific binding of blobs and RCA primers, blocking was

carried out as described in the material and methods.

As seen in Figure 14 blocking of bead surface did not sufficiently decreases the S/N ratio.

2.9 Comparison of signals between 100 nM RO and 10nM RO

In order to measure the sensitivity of the molecular bead shaving, two different

concentrations of RO for digestion of blob-on-beads complex were used and the differences

in signal were measured.

Figure 15: Signal comparison between 100 nM and 10 nM RO respectively. Restriction digestion was

performed at two different concentrations to RO to find the difference in signal. STD and SHTD represent salt

treated dreadlock probes and salt and heat treated dreadlock probes respectively.

Initially, it was shown in the Figure 4 that no signal can be observed at the 10nM RO

concentration. However, the addition of salt and heat, the S/N ratio was increased and signals

tend to appear at the 10nM RO concentration Figure 15. This sets a new limit of detection for

molecular bead shaving, but the S/N is comparatively lower than that of 100 nM RO treated

samples.

1

10

100

1000

10000

100000

- - - - + + 2% milk

- - + + - - SSD

- + - + - + 100 nM RO

Nu

mb

er

of

cou

nte

d B

lob

s(l

og 1

0)

1

10

100

1000

10000

100000

Nu

mb

er o

f co

un

ted

Blo

bs

neg

pos

22

2.10 Comparison between Dynabeads®MyOneTM Streptavidin C-1 and T-1 magnetic beads

with respect to signal

It was suggested that by using C-1 beads a better coverage of RCA primers and non-specific

binding of released blobs might be possible. In this experiment C-1 beads were compared

with T-1 beads C-1 Beads have a hydrophilic surface, whereas T-1 Beads have a hydrophobic

surface. Two different enzymes MscI and ScaI were tested at the same time.

A B

Figure 16: Signal comparisons between C1 and T1 Beads. (A) Number of amplified signal from MscI

digested Dreadlock probes. (B) Number of amplified signals from ScaI restriction digested dreadlock probes.

SD represents no salt and heat treated and SAHT represents salt and heat treated samples respectively.

From these results in Figure 16 it can be easily seen that the S/N ratio is much lower in C-1

beads compared to T-1 beads.

2.11 Theoretical calculation

Name of Oligo Concentration Volume Moles Number of Oligos (moles X Avogadro number)

Capture Oligo 500pM 1µl 5E-16 3.01E+08

RO 100nM 10µl 1E-12 6.02E+11

Therefore, Number of RO to required to release the blobs from dreadlock probes

= Number of RO/Number of Blobs in dreadlock probes

=6.02E+11/3E+8= 2000

Note: To obtain 1picomoles of RO from C2CA protocol requries 10attomoles of target oligos

1

10

100

1000

10000

100000

Nu

mb

er o

f c

ou

nte

d B

lob

s

(lo

g1

0)

1

10

100

1000

10000

100000

T1

C1

23

3.0 Discussion

The main purpose of this project was to investigate the principle of Molecular bead shaving,

which is a novel procedure for magnetic readout.

As a “Proof of principle” for Molecular bead shaving. Our investigation started with finding

the optimum amount of blobs that can be synthesised on the beads. Such a high coverage of

blobs was necessary to obtain a good dynamic range, while the background was expected to

be reduced. We showed that the optimum amount of RCA primer required for a good

coverage was around 6 per bead and above this amount the beads tend to aggregate after

RCA. Aggregation of beads might be due to cross linking or chain entanglement of RCA

products [38, 41] and was found to be irreversible after vortexing. The signals increased with

an increasing concentration of the RCA primer, with an equal increase in the background

signal. However, before proceeding to further experiments, at this point it was imperative to

have a steady background to set a threshold and to limit the sensitivity.

Initially, we hypothesised that the background problem might be due to nonspecific

adsorption of RCA primers onto the bead surface or it could be due to complementary

binding of RCA primers to itself and others or it could be due to star activity of the restriction

enzyme. We tested our hypotheses by performing several experiments, which included

removal of any non-specific adsorbed RCA primers, by heat treating the beads coupled with

RCA primers and ligated padlock probes. This resulted, a significant reduction in the

background signal. Subsequently, incubation at higher temperatures reduced the positive

signals. But above 75oC the signals completely disappeared as shown in Figure 6. This could

be due to slipping off circularized padlock probes from the template RCA primers, which

depends on the Tm of the padlock probes. To avoid such problem of slipping off circularized

padlock probes another experiment was conducted in which the beads were coupled only

with RCA primers were heated at different temperatures. After washing, the padlock probes

were ligated on RCA primers, and interestingly it showed a drastic reduction in the

background signal, but equally decreased the positive signals as well. This heat-treatment

experiment supported our hypothesis that the RCA primers were non-specific adsorbed onto

the bead surface thus constitute the background problem. Since this heat treatment step was

laborious and MscI seemed to solve the background problem, this protocol was put on hold

and there was no time to revisit.

To validate our theory of complementary binding of RCA primers which constitute

background problems, the RCA primer-coupled onto the beads initially was treated with

restriction enzyme. Unfortunately, the experimental results did not support our hypothesis

and also the theory of star activity of enzyme was disapproved (data not shown).

In this investigation three different Restriction enzymes Scal, ScaI-HF and Msc1 were tested

for molecular bead shaving. A very low S/N was observed with ScaI-HF treated sample.

Even though the S/N ratio of MscI treated dreadlock probes showed a higher S/N, the

numbers of blobs in the positive were very less compared to the ScaI treated samples. Our

observation suggested the NEBuffer 3 facilitates non specific drop off of blobs, which was

24

not observed in NEBuffer 4 (data not shown). Further, the time required by Msc1 to release

the blobs from the dreadlock probes was determined by digesting the dreadlock probes at

different time intervals at 37oC. The results suggested that 30 minutes incubation was quite

sufficient to obtain a good signal and above this incubation time the signal might saturate

(Figure 10).

In comparison to the theoretically calculated values the signals obtained in the positive

sample was very low. We suspected that even after restriction digestion of dreadlock probes,

the blobs cleaved from the deadlock probes were not freely released into the solution, rather

they remain attached to the bead surface. This sticking of blobs to the bead surface could be

due to Van der Waals or electrostatic interactions between them. Interestingly, when

restriction digested samples were treated with 1% (v/v) Tween20 and 2 M NaCl Figure 11, a

significant 3.5 times increase in S/N ratio was observed, and this result suggested that the

electrostatic interaction between the beads and blobs could be reduced by adding high

concentrations of salt and non-ionic surfactants. Our experiments directed to increase the S/N

ratio by heat treatment did not yield fruitful results. However, incubating the samples for

longer time at higher temperature increased the signals in positive samples, but also a slight

increase in the background signal was observed. Thus, the S/N ratio was reduced linearly

with respect to incubation time. From these results it was suspected that the reduction in S/N

ratio is most likely due to breakage of streptavidin and biotin interactions or it could be due to

leakage of streptavidin from the beads [3]. To investigate the effect of heat causing

background signal and to reduce the incubation time, we further heated the previously salt

treated restriction digested sample at 75oC for 15 minutes, this experimental results support

the fact that increase in background signal could be due to breakage of streptavidin and biotin

interactions or it could be due to leakage of streptavidin from the beads.

Non-specific binding is a common problem associated with hybridization assays and factors

like hydrophobicity of the monolayer and electrostatic interaction could be responsible for the

nonspecific binding [20]. To reduce the nonspecific binding we blocked the beads using

blocking agents like BSA, dry milk and SSD. Here we expected to have a better signal with

less background. But from the experiment we found out that this was not the case and there

was no change in the signal. We also investigated two different types of beads, C-1 and T-1,

having different surface properties, to increase the coverage and to reduce the S/N ratio. As

shown in Figure 16, T-1 beads were better than C-1 beads for our experiments due to the

higher S/N ratios.

According to our theoretical calculation it has been estimated that roughly 2000 RO were

required to release a blob from the dreadlock probes. It suggests that a very high

concentration of restriction oligos is required to drive the reaction. Requirement of high

concentration of RO suggests that the digestion process is limited by diffusion of RO or

restriction enzymes. At low concentration of RO very few will diffuse through the dreadlock

probes and hybridizes with the dreadlock root thus limiting the restriction digestion, this

could probably be the reason for low sensitivity, which was also hinted by the need of more

time for restriction digestion.

25

With this method originally developed for magnetic readout, a detection limit of one

attomole of target DNA sequence was achieved by using synthetic RO Figure 15, but it is

interesting to see how the C2CA derived monomers affects the detection sensitivity.

However, we envisage that better sensitivity might be possible by translating this method to

biofunctionalized nanobeads, that might give less sterical problems and have better kinetics,

but the drawback of that bead entrapment by the blobs has to be considered.

In conclusion, we have partly achieved our aim, and showed that as a proof of principle the

Molecular bead shaving method was successfully developed for optical readout. Further, we

would like to translate this molecular bead shaving procedure to the magnetic readout.

Translation of this principle for nanobeads might offer possibilities to design a new

generation, point-of-care diagnostic devices.

26

4.0 Materials and Methods:

4.1 Oligonucleotides

The oligonucleotide sequences used for this study are listed in Table 1. 1µM padlock probe

were 5’ phosphorylated enzymatically by 0.1U/µl T4 PNK (Fermentas) in 1X manufacture’s

Buffer A and 1mM ATP for 30 min at 37oC, followed by inactivation at 65

oC for 20 min.

Name DNA sequence 5’-3’ Kind of

Oligonucleotide

Modific

ations

Manufactur

ers

Snag_Dreadlocklock1

Snag_Root_MscI_EC

Snag_Root_ScaI_EC

B2_CO_EC

B2_SW_EC_ny

BNL_DO_EC1RCA

B2_AluIprimer

BNL_AluI_RO

Snag_Primer_Scal_

Biotin

Snag_Primer_MscI_Bi

otin

ACGCCAATGTTGTCGGTGGATATTG

TCTTACACGATTGCAGACCTGGTGT

GAGCCTTTGAGTC

TACCTTTGCTCATTGACGTGTATGCA

GCTCCTCAGTATTTGTTGTCGTGGCC

AGATAATCTTTGGAAGGGAGTAAAG

TTAA

TACCTTTGCTCATTGACGTGTATGCA

GCTCCTCAGTATTTGTTGTCGAGTAC

TGGTAATTTTTGGAAGGGAGTAAAG

TTAA

CTCTCTCTCTCGTGCCAGCAGCCGCG

GTAATACGGAGGGTGCAAGCGTTA

TAACGCTTGCACCCTCCGTATTACCG

CGGCTGCTGGCACGGAGTTAGCCGG

TGCTTCTTCTGCGGGTAACGTCAATG

AGCAAAGGTATTAACTTTACTCCCTT

CC

GTGGATAGTGTCTTACACGAUUUU

TACTGAGGAGCTGCATACAC

GTGTATGCAGCTCCTCAGTA

TTTTTTTTTTTTTTTTTTTTAATTACC

AGTACTCGACAACATTGGCGTGACT

CAAAGGCTCAC

TTTTTTTTTTTTTTTTTTTTGATTATC

TGGCCACGACAACATTGGCGTGACT

CAAAGGCTCAC

Padlock probe

Padlock probe

Padlock probe

Capture Oligo

Sandwich probe

Detection Oligo

Primer

Restriction Oligo

RCA-Primer

RCA-Primer

_

_

_

5’-

Biotin

_

5’-Cy3

_

_

_

5’-

Biotin

5’-

Biotin

Integrated

DNA

Technology

”

”

Biomers

Biomers

Integrated

DNA

Technology

”

”

”

”

Note: a) Poly (T) tail at the 5’ of RCA primers acts as a spacers.

http://130.238.210.194/oligos/showoligo.php?showid=10537http://130.238.210.194/oligos/showoligo.php?showid=10538

27

4.2 Padlock probes hybridization and ligation

Padlock probe hybridization and ligation was carried out in a single reaction containing 10

nM padlock probes, 0.25 U/µl AmpLigase (Epicenter Biotechnologies) 1 X AmpLigase

buffer [20 mM Tris-HCl (pH 8.3), 25 mM KCl, 10 mM MgCl, 0.25 mM NAD, 0.01% (v/v)

Triton® X-100], sterile filtered (stf) 0.2 µg/µl BSA (New England BioLabs) and 500 pM of

RCA Primers and the reaction mixture was incubated at 55oC for 10 min.

4.3 Capturing of RCA primers to beads

A bead suspension of 5 µl (5*107 beads) Dynabeads® MyOneTM Streptavidin T1

(Invitrogen) beads were washed using the same initial bead volume with 1X B&Wtw buffer

(10 mM Tris-HCl [pH 7.5], 5 mM EDTA, 0.1 % [v/v] Tween20, and 1M NaCl) Beads were

trapped along one side of the tube by using permanent magnet and the storage buffer is

removed. After removing the magnet 1 X B&Wtw buffer was added along the wall of the

tubes and vortex to resuspend the beads, this washing procedure repeated for three times.

Coupling of RCA primers was carried out by adding 20 µl of ligated Padlock probes solution

to the washed beads followed by incubation for 5 min at room temperature with rotation. The

beads were washed with 1X B&Wtw buffer two times to remove non captured RCA primers.

4.4 RCA on magnetic beads

RCA reaction was performed on the RCA primers coupled beads by adding the solution

containing 0.1 U/µl of φ29 DNA Polymerase (Fermentas) 1X φ29 buffer (33 mM Tris-acetate

[pH 7.9 at 37oC], 10 mM Mg-acetate, 66 mM K-acetate, 0.1% [v/v] Tween20, 1 mM DTT),

(stf) 0.2µg/µl BSA and 125µM dNTPs in a total volume of 20µl, followed by incubation at

37oC for 20 min. The polymerization reaction was terminated by inactivating the DNA

polymerase at 65oC for 5 min.

4.5 C2CA and Monomerization

Preparation of DNA Circle for C2CA reaction was carried out slight differently from padlock

probe hybridization and ligation. 500 nM synthetic E.coli Sandwich probes (B2_SW_EC_ny)

acts as template (which are complementary to both the capture oligo and the padlock probes),

100 nM Padlock probes, 50 nM capture oligo (B2_CO_EC) were added to the reaction

mixture containing 0.25 U/µl AmpLigase in 1X AmpLigase buffer and (stf) 0.2 µg/µl BSA

and incubated at 55oC for 10 min. Coupling of capture oligo and RCA reaction was

performed as before with an excess of 0.1U/µl of φ29 DNA Polymerase. The RCP were

monomerized by adding 120 nM of replication oligo (BNL_ALU_RO) complementary to the

replication sequence in the RCP products together with 120 mU/µl of Alul in 1 X φ29

polymerase buffer and 0.2 µg/µl BSA. Addition was made in 5 µl to an initial 20 µl RCA

solution, final volume 25 µl, followed by incubation for 10 min at 37oC, and inactivation at

65oC for 10 min. Further, the monomerized solution separated from the magnetic beads. And

28

the monomerized RCR product were religated and amplified in the same reaction containing

(stf) 0.2 µg/µl BSA, 0.67 mM ATP, 14 mU/µl T4 DNA Ligase, 60 mU/µl φ29 DNA

polymerase, 100µM dNTPs in 1 X φ29 polymerase Buffer, addition were made in 10 µl to an

initial 25 µl monomerized solution and the final volume 35µl, followed by incubation for

37oC for 20 min and the enzyme is inactivated at 65

oC for 5 min. The second RCA Products

were monomerized by adding 120 nm of replication oligo (B2_ ALU primer) complementary

to the replication sequence for the second RCR products together with 55 mU/µl of Alul in 1

X φ29 polymerase buffer and 0.2 µg/µl BSA, addition was made in 5µl to the above solution

to total volume 40 µl, incubated 37oC for 10 min, followed by enzyme inactivation at 65

oC

for 10 min. These monomerized RCP were used as target molecules for the Reporter

Dreadlock Probes for Molecular bead shaving.

4.6 Molecular bead shaving of DNA coils

After performing RCA on beads, the beads are washed twice as before using 1X B&Wtw

buffer. Releasing of DNA coils from the dreadlock probes was performed by adding 100 nM

restriction oligo or C2CA amplified monomers (that recognise the complementary sequence

present at the root of the DNA coil) with 0.08 U/µl of Mscl or Scal (New England Biolabs)

depending upon the Oligos used, in the manufactures 1X NEBuffer 3 or 4 respectively, in a

total volume of 50 µl, followed by incubation at 37oC for 30 min. After vortexing for 30 sec,

2 M NaCl with 1% (v/v) Tween20 added and incubated for 1 hour at 65oC. The beads were

separated from the released coils by using a permanent magnet.

4.7 Blocking of beads surface

A bead suspension of 5 µl were washed using the same initial bead volume with 1X saline

sodium citrate (SSC) buffer (150mM NaCl, 15 mM sodium citrate) and 100 mg/ml of SSD

was added and incubated for 1 hour with rotation. After incubation the beads was washed

with 1X SSC buffer three times and RCA was performed as explained above. Blocking of

beads with milk was carried similarly expect SSD, 2% dry milk dissolved in 1X PBS was

added.

4.8 Labeling of RCA coils

The solution of released RCA coils obtained after molecular bead shaving was mixed with

the labeling mixture containing 5 nM Cy3 labeled detection oligos, (stf) 20 mM EDTA, (stf)

20mM Tris-Hcl (pH 8.0), 0.1% (v/v) Tween20 (stf) and 1 M NaCl (stf) in a total final volume

of 100 µl and incubate at 70oC for 2 min, and 55

oC for 15 min.

4.9 Microfluidic quantification, image acquisition and analysis

The homogenous solution of labelled blobs was pumped at a flow rate of 5 µl/min through a

custom made microfluidic channel (200 x 40µm cross section) using syringe pump (PHD-

2000, Harvard Instruments, USA). The microfluidic setup was placed onto the confocal

microscope (LSM 5 META, Zeiss, Germany) the microscope focus was set to the centre of

microfluidic channel and the pinhole was set to 300 µm, 40X objective used for detecting the

labeled blobs. The microscope operated in line scan mode with scanning path perpendicular

29

to liquid flow direction and 30,000 line scans of 512 pixels were recorded with pixel time of

1.6 µs [51].

The Images were stored as 24 bit RGB TIFF files and analyzed using dedicated software

written in MATLAB 7.0. A threshold of 40% was set and objects between 2 pixels and 10

pixels retained and the rest were removed from the list. The signal intensity subsequently

calculated were used to produce a dot plot and the collective signals in dot plots were

partitioned by defined gates and the number of objects calculated as an average of 10%

brightest objects to avoid out-of- focus objects [26].

30

5.0 Acknowledgement

This project was carried out at Rudbeck laboratory at Uppsala University. I would like to

thank Professor Mats Nilsson for providing me an opportunity to carry out my Master degree

project.

I am wholeheartedly thankful to Dr. David Herthnek, whose encouragement, guidance,

excellent supervision and support throughout the project, enabled me to understand how to

and how not to conduct experiments. I was motivated by the scientific discussion, which we

had during my thesis work, which helped to me think critically. And I appreciate his patience

and support.

I would also like to thank Mattis Strömberg and Teresa Zardan Gomez de la Torre for

introducing me to the DynoMag instruments and for the useful discussion. I thank Rongqin

ke for showing me the fabrication of microfluidic channels. And also I thank Anja Mezger

and Anna Engström for the useful discussions.

I express my gratitude to professor Staffan Svärd for his support and guidance throughout my

master degree and for his generosity.

I am thankful to all those whoever I met during this project work.

I owe my gratitude to my friends Sagar S Manoli, Naveen Kumar GC, Chetan Nagaraja and

Sanjith Kallipati for providing me the financial help and support, without which it would

have been difficult.

I am thankful to my Parents and Sisters for everything.

31

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