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Potential antifungal activity of Himalayan lichens: a methodological
assessment.
1Department of Botany
Pt. L.M.S. Government Post Graduate College,
Rishikesh(Dehradun),
Uttarakhand-249201, India
Himanshu Rai1, 2*, Roshni Khare1, 2, R.K. Gupta1, D.K. Upreti2, Priti Tiwari2
2Lichenology laboratory;
Plant Diversity, Systematics and Herbarium Division;,
CSIR-National Botanical research Institute,
Lucknow-226001, Uttar Pradesh, India
Lichen: Introduction
• Lichens, a symbiotic composite
of a fungus and a green or/ and
blue green algae
• Lichens are named based on the
fungal component, which plays
the primary role in determining
the lichens form.
• Lichens are among the most
tolerant organisms, capable of
inhabiting most of the terrestrial
habitats ranging from hot deserts
to alpine Antarctic habitats.
Parmelia sulcata
Lichens produce a wide array of both
Primary (intracellular) metabolites : amino acids,
polyols, carotenoids, polysaccharides, and
vitamins.
Secondary(extracellular) metabolites : Lichen
acids
Lichen Chemistry: Introduction
Lichen Secondary metabolites
Lichen secondary compounds are produced primarily by
the mycobiont.
Lichen secondary compounds are extracellular products
of relatively low molecular weight crystallized on the
hyphal cell walls of the cortex and/or medulla. .
Lichen secondary compounds are usually insoluble in
water and can be extracted into organic solvents.
Out of 800 secondary metabolites so far known from
lichens 650 are unique to them (82%).
Lichen Secondary metabolites: Major pathways
Lichen secondary metabolites are
derived from three chemical
pathways:
Shikimic acid pathway
•pulvinic acid derivatives (yellow
pigments)
Mevalonic acid pathway
•terpenes
Acetate-polymalonate pathway
•depsides, depsidones, usnic acid,
anthraquinones, xanthones,
aliphatic acids (majority of lichen
compounds)
Lichen Secondary compounds: Activities
LICHENS
Pulvinic acid
derivatives
Depsides,
Depsidones, Usnic
acid,
Anthraquinones,
Xanthones,
Aiphatic acids
Terpenes
Ecophysiological,
Immunostimulatory
and Enzyme
inhibitory
Objectives
Lichens from Uttarakhand have been studied taxonomically for past five decades (> 700 species known)
Lichens from Uttarakhand not have been screened for their biological activities (few reports).
A study was undertaken : To assess the antifungal activity of Himalayan lichens /
Lichens from Uttarakhand against some broad-spectrum plant pathogenic fungi.
To device an extraction protocol with maximum efficiency in terms of yield of secondary metabolites and screening assay for antifungal activity of lichen substances.
Experiment: Components
Lichens:
Four foliose lichen species:
Bulbothirx setschwanensis,
Everniastrum nepalense,
Heterodermia diademata,
Parmelaria thomsonii
collected from temperate
habitats of Pithoragarh
(1350-1760m), Uttarakhand
FUNGI:
Seven plant pathogenic
fungi :
Aspergillus flavus,
Aspergillus fumigatus
Alternaria alternata
Fusarium oxysporum
Fusarium solani
Fusarium roseum
Penicillium citrinum
Ketoconazole (positive control).
SOLVEN SYSTEM: .
Acetone,
Methanol Chloroform
Methodology: Procedure
2 Recovery
(Rotary evaporator )
3 Antifungal Assay
(Bauer-Kirby disc diffusion assay)
1 Extraction
(Soxhlet extractor)
Methodology: Soxhlet extraction
The solvent extraction was carried out at the specific boiling temperature of the solvents (acetone-56˚C, methanol-65˚C and chloroform -61.2˚C) for 48 hr for complete extraction of secondary compounds.
Methodology: Recovery
Rotary evaporation is a technique used to remove large volumes of volatile solvents from solutions. The rotary evaporator
rotates a flask containing the solution under a reduced pressure. The rotation spreads the solution out to form a thin film with a
greatly increased surface area speeding up the evaporation.
Lichen secondary metabolites were further recovered through gentle removal of solvents from lichen samples by evaporation using rotary evaporator (Büchi Rotavapor R-200TM).
Antifungal activity: Bauer-Kirby disc diffusion assay
Test solutions of lichen substances were prepared by dissolving recovered lichen substances in 10 ml of their respective solvents.
Experimental diffusion discs were prepared by loading five milliliters of lichen extract, 1 ml in each load on filter paper disks (6 mm in diameter), allowing the solvent to evaporate between each loading and leaving the lichen extracts on disk without the solvent.
All the three lichen extracts (i.e. acetone, methanol and chloroform) were loaded in this manner.
Loaded discs were planted on test plant pathogenic fungi culture plate in triplicate.
Commercially available synthetic antifungal drug Ketoconazole was used as positive control.
The plates were incubated for 5 days at 20°C to 25°C.
Growth was evaluated visually by comparing a particular plate with the negative control plates (having only plant pathogenic fungi).
Data Analysis: Multivariate study-PCA
Indirect gradient ordination method, principal component analysis (PCA) was used to summarise the effect of three solvent extracts of test lichens on test plant pathogenic fungi with reference to positive control Ketoconazole .
PCA was done on the basis of inhibition zone (mm) produced on test fungi colonies, utilizing correlation ma-trix, using multivar option in PAST 2.09.
Results: Extraction efficiency
15%
12%
15%
12%
The extraction process resulted in 10-15% efficiency in yield of secondary metabolites.
Results: Differential Antifungal activity
Preeti Tiwari, Himanshu Rai, Dalip Kumar Upreti, Suman Trivedi, Preeti Shukla
(2011).Assessment of antifungal activity of some Himalayan foliose lichens against
plant pathogenic fungi. American Journal of Plant Sciences, 2:841-846.
Preeti Tiwari, Himanshu Rai, Dalip Kumar Upreti, Suman Trivedi, Preeti Shukla
(2011).Assessment of antifungal activity of some Himalayan foliose lichens against plant
pathogenic fungi. American Journal of Plant Sciences, 2:841-846.
Results of comparative antifungal screening of the different solvent extracts (A = Acetone, M = Methanol, and Cl = Chloroform) of Himalayan foliose lichens and commercially available fungicide Ketoconazole(K), against selected plant pathogenic fungi (AF = Aspergillus flavus, Alt = Alternaria alternata, AFU = Aspergillus fumigatus, FUR = Fusarium roseum, FUS = Fusarium soloni, FOX = Fusarium oxysporum, and PC = Penicilium citrinum). Reported values are in Arithmetic mean ± Standard error.
Results: Principal Component Analysis
PCA Biplots of selected lichen
(a) = Bulbothrix setschwanensis,
(b) = Parmelaria thomsonii,
(c) = Heterodermia dia-demata
(d) = Everniastrum nepalense)
extracts (A = Acetone,
M = Methanol,
Cl = Chloroform)
and commercially available fungicide Ketoconazole(K) on different plant pathogenic fungi.
Preeti Tiwari, Himanshu Rai, Dalip Kumar Upreti, Suman Trivedi, Preeti Shukla (2011).Assessment of antifungal activity of some Himalayan
foliose lichens against plant pathogenic fungi. American Journal of Plant Sciences, 2:841-846.
PCA analysis required four components (axis) to account for 100% variance in dataset for all the four lichenized fungi. The first two components (axis) of PCA explained maximum variation
PCA biplots concluded that though positive control Ketoconazole showed higher degree of antifungal activity against some of the plant pathogenic fungi (Alternaria alternata, Aspergillus flavus, Aspergillus fumigatus and Penicillium citrinum), the lichen extracts acetone and methanol extracts of lichens were comparatively more effective against some broad spectrum plant pathogenic fungi (Fusarium oxysporum, F. solani, F. roseum)
Conclusions
The better performance of lichenic extracts against commercially available antifungal Ketoconazole against some (Fusarium roseum, Fusarium solani and Fusarium oxysporum) plant pathogenic fungi suggests their superior potentials as fungicides.
The selective antifungal effect of acetone and methanol extracts of test lichens over chloroform extracts can be attributed to the presence of different constituent secondary metabolites in lichen thalli .
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