1. Metagenomics (Environmental Genomics, Ecogenomics, Community Genomics) Dr. Bhavesh Patel Principal V.P. and R.P.T.P. Science College Vallabh Vidyanagar, Gujarat (bhavesh1968@rediffmail.com)

2. Life on earth Thought to be ~3.8 billion years old. For the first 1.5 billion years it was all aquatic microbes. Less then 2% bacteria are presently cultured in the laboratory (an estimate) “ great plate count anomaly”- the discrepancy between plate count and DMC. Size and diversity (8,00,000insect spp is known and 7000 bacterial spp. )

3. The early attempt A.V.Leeuwenhoek -16 th century Spallanzani - 18 th century L.Pasteur - 19 th century Were the first to use meat broth or similar infusion for bacterial culture. However, the drawback was that the broth contains mixture of bacteria.

4. Robert Koch Was the first to use potato slices as a solid surface to give colonies on its surface. However, he soon realize that only a limited number of organism grew on potato. This was probably the first recognition of unculturability “In vitro”.

5. What is Unculturability? “Unculturability means the organisms are unable to grow in laboratory otherwise these organisms are very well growing rather flourishing in one or other natural environment.”

6. Reasons for Unculturability “In Vitro” High nutrient content Absence of required nutrient Toxic substance produced by other bacteria Some bacteria may depend on other for growth Environmental conditions are not suitable Disruption of bacterial cytokine networks

7. Cultivating Unculturables-Early attempts Enriched and Enrichment cultivation Media with low nutrients Modifying the cultural conditions:- Carbon dioxide and oxygen conc. Long incubation Addition of humic acid etc. Simulation of natural environment Gel micro droplets

8. Culture independent approach Metagenomics The term was first used in 1998 by Handelsman in the University of Wisconsin. It can be appropriately defined as “ the application of modern genomics techniques to the study of communities of microbial organisms directly in their natural environments, bypassing the need for isolation and lab cultivation of individual species.”

9. Environmental Libraries Various environmental samples were used to construct metagenomic libraries Small inserts with 2-15 Kb in plasmid vector Large inserts with40-130 Kb in cosmid, fosmid or Bacterial Artificial Chromosome (BAC) vector

10. Metagenomic DNA Plasmid libraryCosmid or BAC library Activity or sequence based screening Single gene product- Biocatalyst Multiple gene product- Bioactive compound Sequencing and characterization

11. Biocatalyst and Bioactive compound isolated from metagenomic libraries Product Vector Sample AgaraseCosmidSoil Alcohol oxidoreductasePlasmidSoil AmidaseCosmidSoil AmylaseCosmid,BACSoil CellulaseCosmidSoil ChitinaseLambda-ZAP Marine water DNaseBACSoil EsterasePlasmidSoil Lipase PlasmidSoil IndirubinBACSoil TurbomycinBACSoil ViolaceinCosmidSoil

12. THANK YOU Thank you for your time and attention Thank you for your participation!!! Any question?