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Host-derived fecal microRNAs can indicate gut microbiota healthiness and ability to induce inflammation

Disruption of intestine-microbiota symbiosis can result in chronic gut inflammation. We hypothesize that assessing the initial inflammatory potential of the microbiota in patients is essential and that host-derived miRNAs, which can be found in feces, could fulfill this function. We investigated whe...

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Autores principales: Viennois, Emilie, Chassaing, Benoit, Tahsin, Anika, Pujada, Adani, Wang, Lixin, Gewirtz, Andrew T., Merlin, Didier
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Ivyspring International Publisher 2019
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6599659/
https://www.ncbi.nlm.nih.gov/pubmed/31285778
http://dx.doi.org/10.7150/thno.35282
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author Viennois, Emilie
Chassaing, Benoit
Tahsin, Anika
Pujada, Adani
Wang, Lixin
Gewirtz, Andrew T.
Merlin, Didier
author_facet Viennois, Emilie
Chassaing, Benoit
Tahsin, Anika
Pujada, Adani
Wang, Lixin
Gewirtz, Andrew T.
Merlin, Didier
author_sort Viennois, Emilie
collection PubMed
description Disruption of intestine-microbiota symbiosis can result in chronic gut inflammation. We hypothesize that assessing the initial inflammatory potential of the microbiota in patients is essential and that host-derived miRNAs, which can be found in feces, could fulfill this function. We investigated whether the gut microbiota composition impacts the fecal miRNA profile and thereby indicates its ability to influence intestinal inflammation. Methods: We used high-throughput qPCR to compare fecal miRNA profile between germ-free and conventional mice. Conventionalization of germfree mice by various colitogenic and non-colitogenic microbiotas (IL10(-/-) and TLR5(-/-) associated microbiota) was performed. Results: We identified 12 fecal miRNAs impacted by the presence of a microbiota. Conventionalization of germfree mice by various colitogenic and non-colitogenic microbiotas associated with the development of intestinal inflammation (IL10(-/-) and TLR5(-/-) associated microbiota) yielded distinctively altered fecal miRNA profiles compared to that of mice receiving a “healthy” microbiota. Correlation analysis revealed the existence of interactions between the 12 abovementioned miRNAs and specific microbiota members. Conclusion: These results showed that fecal miRNA profile can be differentially and specifically impacted by microbiota composition, and that miRNA could importantly serve as markers of the colitogenic potential of the microbiota. This is particularly relevant to assess individual state of the microbiota in patients with dysbiosis-related disorders, such as IBD and potentially determine their ability to respond to therapeutics.
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spelling pubmed-65996592019-07-08 Host-derived fecal microRNAs can indicate gut microbiota healthiness and ability to induce inflammation Viennois, Emilie Chassaing, Benoit Tahsin, Anika Pujada, Adani Wang, Lixin Gewirtz, Andrew T. Merlin, Didier Theranostics Research Paper Disruption of intestine-microbiota symbiosis can result in chronic gut inflammation. We hypothesize that assessing the initial inflammatory potential of the microbiota in patients is essential and that host-derived miRNAs, which can be found in feces, could fulfill this function. We investigated whether the gut microbiota composition impacts the fecal miRNA profile and thereby indicates its ability to influence intestinal inflammation. Methods: We used high-throughput qPCR to compare fecal miRNA profile between germ-free and conventional mice. Conventionalization of germfree mice by various colitogenic and non-colitogenic microbiotas (IL10(-/-) and TLR5(-/-) associated microbiota) was performed. Results: We identified 12 fecal miRNAs impacted by the presence of a microbiota. Conventionalization of germfree mice by various colitogenic and non-colitogenic microbiotas associated with the development of intestinal inflammation (IL10(-/-) and TLR5(-/-) associated microbiota) yielded distinctively altered fecal miRNA profiles compared to that of mice receiving a “healthy” microbiota. Correlation analysis revealed the existence of interactions between the 12 abovementioned miRNAs and specific microbiota members. Conclusion: These results showed that fecal miRNA profile can be differentially and specifically impacted by microbiota composition, and that miRNA could importantly serve as markers of the colitogenic potential of the microbiota. This is particularly relevant to assess individual state of the microbiota in patients with dysbiosis-related disorders, such as IBD and potentially determine their ability to respond to therapeutics. Ivyspring International Publisher 2019-06-09 /pmc/articles/PMC6599659/ /pubmed/31285778 http://dx.doi.org/10.7150/thno.35282 Text en © Ivyspring International Publisher This is an open access article distributed under the terms of the Creative Commons Attribution (CC BY-NC) license (https://creativecommons.org/licenses/by-nc/4.0/). See http://ivyspring.com/terms for full terms and conditions.
spellingShingle Research Paper
Viennois, Emilie
Chassaing, Benoit
Tahsin, Anika
Pujada, Adani
Wang, Lixin
Gewirtz, Andrew T.
Merlin, Didier
Host-derived fecal microRNAs can indicate gut microbiota healthiness and ability to induce inflammation
title Host-derived fecal microRNAs can indicate gut microbiota healthiness and ability to induce inflammation
title_full Host-derived fecal microRNAs can indicate gut microbiota healthiness and ability to induce inflammation
title_fullStr Host-derived fecal microRNAs can indicate gut microbiota healthiness and ability to induce inflammation
title_full_unstemmed Host-derived fecal microRNAs can indicate gut microbiota healthiness and ability to induce inflammation
title_short Host-derived fecal microRNAs can indicate gut microbiota healthiness and ability to induce inflammation
title_sort host-derived fecal micrornas can indicate gut microbiota healthiness and ability to induce inflammation
topic Research Paper
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6599659/
https://www.ncbi.nlm.nih.gov/pubmed/31285778
http://dx.doi.org/10.7150/thno.35282
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