作者
Heather J. Galipeau,Alberto Caminero,Williams Turpin,Miriam Bermúdez-Brito,Alba Santiago,Josie Libertucci,Marco Constante,Juan A. Raygoza Garay,Gaston Rueda,Sarah Armstrong,Alex Clarizio,Michelle I. Smith,Michael G. Surette,Přemysl Berčík,Kenneth Croitoru,Elena F. Verdú,Paul L. Beck,Çharles N. Bernstein,Kenneth Croitoru,Leo Dieleman,Brian G. Feagan,Anne M. Griffiths,David S. Guttman,Kevan Jacobson,Gilaad G. Kaplan,Denis O. Krause,Karen Madsen,John K. Marshall,Paul Moayyedi,Mark J. Ropeleski,Ernest G. Seidman,Mark S. Silverberg,Scott B. Snapper,Andy Stadnyk,Hillary Steinhart,Michael G. Surette,Dan Turner,Thomas D. Walters,Bruce A. Vallance,Guy Aumais,Alain Bitton,Maria Cino,Jeff Critch,Lee A. Denson,Colette Deslandres,Wael El‐Matary,Hans Herfarth,Peter Higgins,Hien Q. Huynh,Jeff Hyams,David R. Mack,Jerry McGrath,Anthony Otley,Remo Panancionne
摘要
Background & Aims
Altered gut microbiota composition and function have been associated with inflammatory bowel diseases, including ulcerative colitis (UC), but the causality and mechanisms remain unknown. Methods
We applied 16S ribosomal RNA gene sequencing, shotgun metagenomic sequencing, in vitro functional assays, and gnotobiotic colonizations to define the microbial composition and function in fecal samples obtained from a cohort of healthy individuals at risk for inflammatory bowel diseases (pre-UC) who later developed UC (post-UC) and matched healthy control individuals (HCs). Results
Microbiota composition of post-UC samples was different from HC and pre-UC samples; however, functional analysis showed increased fecal proteolytic and elastase activity before UC onset. Metagenomics identified more than 22,000 gene families that were significantly different between HC, pre-UC, and post-UC samples. Of these, 237 related to proteases and peptidases, suggesting a bacterial component to the pre-UC proteolytic signature. Elastase activity inversely correlated with the relative abundance of Adlercreutzia and other potentially beneficial taxa and directly correlated with known proteolytic taxa, such as Bacteroides vulgatus. High elastase activity was confirmed in Bacteroides isolates from fecal samples. The bacterial contribution and functional significance of the proteolytic signature were investigated in germ-free adult mice and in dams colonized with HC, pre-UC, or post-UC microbiota. Mice colonized with or born from pre-UC–colonized dams developed higher fecal proteolytic activity and an inflammatory immune tone compared with HC-colonized mice. Conclusions
We have identified increased fecal proteolytic activity that precedes the clinical diagnosis of UC and associates with gut microbiota changes. This proteolytic signature may constitute a noninvasive biomarker of inflammation to monitor at-risk populations that can be targeted therapeutically with antiproteases.
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