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Development and analysis of molecular methods for functional metagenomics of the human gut microbiome

by Kathy Lam

Institution: University of Waterloo
Year: 2016
Posted: 02/05/2017
Record ID: 2092765
Full text PDF: http://hdl.handle.net/10012/10330


Abstract

Interest in the human microbiome has risen quickly in recent years as the microbes that live in and on our body have been implicated in a growing number of human health and disease states. This interest has been supported by advances in DNA sequencing technology that have allowed us to obtain vast amounts of sequence data, and yet we have difficulty assigning function to many of the gene sequences obtained. As research on the role of these microorganisms continues, there will be an increased need for high-throughput methods that can provide knowledge of microbial gene function. Functional metagenomics is one such method, and it relies on first cloning environmental DNA to generate metagenomic libraries that are maintained in Escherichia coli and second, screening the cloned DNA for particular functions of interest. This powerful function-first method allows for the isolation of genes whose role may not have been predicted using DNA sequence homology. This thesis describes the analysis of techniques used in functional metagenomics research, as well as the development of new strategies to aid in functional screening of metagenomic libraries, particularly those constructed from gut-derived DNA. The work is divided into four data chapters that each explore a distinct aspect of the functional metagenomics approach. The first data chapter describes the evaluation of a pooled strategy for sequencing cosmid clones that were previously isolated in functional screens of metagenomic libraries. Ninety-two large-insert clones were pooled for Illumina-sequencing and the assembled sequence data were evaluated against reference sequence data that were obtained from individual barcoded Illumina sequencing of the same clones. The results indicated that a pooled strategy works well provided that sufficient sequencing depth is obtained and that pooled clones do not share sequence similarity to the extent that would be problematic for assembly of short reads that derive from those clones. The second data chapter is an exploration of possible causes for the known cloning bias of metagenomic libraries, by comparing environmental DNA before cloning to the DNA cloned in the final metagenomic library in E. coli. For a human gut metagenomic library, DNA was sampled and Illumina-sequenced at three different steps during the construction of the library. Analyses of the sequence data showed that there was indeed major bias in the final library, but that the bias was not due to fragmentation of the DNA during the cloning process as has been previously suggested; rather, the data were consistent with alternative hypotheses that suggest bias occurs after the DNA is introduced into E. coli, and analyses provide support for the hypothesis that spurious transcription of foreign DNA in E. coli may be contributing to the bias of libraries. Bias was also examined for a soil metagenomic library using 16S rRNA gene sequencing and though broad phylum-level biases were not as severe as observed for the human gut library, analyses revealed a bias in the…

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