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A gene-targeted approach to investigate the intestinal butyrate-producing bacterial community

dc.contributor.authorVital, Marius
dc.contributor.authorPenton, Christopher R
dc.contributor.authorWang, Qiong
dc.contributor.authorYoung, Vincent B
dc.contributor.authorAntonopoulos, Dion A
dc.contributor.authorSogin, Mitchell L
dc.contributor.authorMorrison, Hilary G
dc.contributor.authorRaffals, Laura
dc.contributor.authorChang, Eugene B
dc.contributor.authorHuffnagle, Gary B
dc.contributor.authorSchmidt, Thomas M
dc.contributor.authorCole, James R
dc.contributor.authorTiedje, James M
dc.date.accessioned2015-08-07T17:30:22Z
dc.date.available2015-08-07T17:30:22Z
dc.date.issued2013-03-04
dc.identifier.citationMicrobiome. 2013 Mar 04;1(1):8
dc.identifier.urihttps://hdl.handle.net/2027.42/112465en_US
dc.description.abstractAbstract Background Butyrate, which is produced by the human microbiome, is essential for a well-functioning colon. Bacteria that produce butyrate are phylogenetically diverse, which hinders their accurate detection based on conventional phylogenetic markers. As a result, reliable information on this important bacterial group is often lacking in microbiome research. Results In this study we describe a gene-targeted approach for 454 pyrotag sequencing and quantitative polymerase chain reaction for the final genes in the two primary bacterial butyrate synthesis pathways, butyryl-CoA:acetate CoA-transferase (but) and butyrate kinase (buk). We monitored the establishment and early succession of butyrate-producing communities in four patients with ulcerative colitis who underwent a colectomy with ileal pouch anal anastomosis and compared it with three control samples from healthy colons. All patients established an abundant butyrate-producing community (approximately 5% to 26% of the total community) in the pouch within the 2-month study, but patterns were distinctive among individuals. Only one patient harbored a community profile similar to the healthy controls, in which there was a predominance of but genes that are similar to reference genes from Acidaminococcus sp., Eubacterium sp., Faecalibacterium prausnitzii and Roseburia sp., and an almost complete absence of buk genes. Two patients were greatly enriched in buk genes similar to those of Clostridium butyricum and C. perfringens, whereas a fourth patient displayed abundant communities containing both genes. Most butyrate producers identified in previous studies were detected and the general patterns of taxa found were supported by 16S rRNA gene pyrotag analysis, but the gene-targeted approach provided more detail about the potential butyrate-producing members of the community. Conclusions The presented approach provides quantitative and genotypic insights into butyrate-producing communities and facilitates a more specific functional characterization of the intestinal microbiome. Furthermore, our analysis refines but and buk reference annotations found in central databases.
dc.titleA gene-targeted approach to investigate the intestinal butyrate-producing bacterial community
dc.typeArticleen_US
dc.description.bitstreamurlhttp://deepblue.lib.umich.edu/bitstream/2027.42/112465/1/40168_2012_Article_9.pdf
dc.identifier.doi10.1186/2049-2618-1-8en_US
dc.language.rfc3066en
dc.rights.holderVital et al; licensee BioMed Central Ltd.
dc.date.updated2015-08-07T17:30:23Z
dc.owningcollnameInterdisciplinary and Peer-Reviewed


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