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Methods for Improving Human Gut Microbiome Data by Reducing Variability through Sample Processing and Storage of Stool

Gut microbiome community analysis is used to understand many diseases like inflammatory bowel disease, obesity, and diabetes. Sampling methods are an important consideration for human microbiome research, yet are not emphasized in many studies. In this study, we demonstrate that the preparation, han...

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Autores principales: Gorzelak, Monika A., Gill, Sandeep K., Tasnim, Nishat, Ahmadi-Vand, Zahra, Jay, Michael, Gibson, Deanna L.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2015
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4529225/
https://www.ncbi.nlm.nih.gov/pubmed/26252519
http://dx.doi.org/10.1371/journal.pone.0134802
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author Gorzelak, Monika A.
Gill, Sandeep K.
Tasnim, Nishat
Ahmadi-Vand, Zahra
Jay, Michael
Gibson, Deanna L.
author_facet Gorzelak, Monika A.
Gill, Sandeep K.
Tasnim, Nishat
Ahmadi-Vand, Zahra
Jay, Michael
Gibson, Deanna L.
author_sort Gorzelak, Monika A.
collection PubMed
description Gut microbiome community analysis is used to understand many diseases like inflammatory bowel disease, obesity, and diabetes. Sampling methods are an important consideration for human microbiome research, yet are not emphasized in many studies. In this study, we demonstrate that the preparation, handling, and storage of human faeces are critical processes that alter the outcomes of downstream DNA-based bacterial community analyses via qPCR. We found that stool subsampling resulted in large variability of gut microbiome data due to different microenvironments harbouring various taxa within an individual stool. However, we reduced intra-sample variability by homogenizing the entire stool sample in liquid nitrogen and subsampling from the resulting crushed powder prior to DNA extraction. We experimentally determined that the bacterial taxa varied with room temperature storage beyond 15 minutes and beyond three days storage in a domestic frost-free freezer. While freeze thawing only had an effect on bacterial taxa abundance beyond four cycles, the use of samples stored in RNAlater should be avoided as overall DNA yields were reduced as well as the detection of bacterial taxa. Overall we provide solutions for processing and storing human stool samples that reduce variability of microbiome data. We recommend that stool is frozen within 15 minutes of being defecated, stored in a domestic frost-free freezer for less than three days, and homogenized prior to DNA extraction. Adoption of these simple protocols will have a significant and positive impact on future human microbiome research.
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spelling pubmed-45292252015-08-12 Methods for Improving Human Gut Microbiome Data by Reducing Variability through Sample Processing and Storage of Stool Gorzelak, Monika A. Gill, Sandeep K. Tasnim, Nishat Ahmadi-Vand, Zahra Jay, Michael Gibson, Deanna L. PLoS One Research Article Gut microbiome community analysis is used to understand many diseases like inflammatory bowel disease, obesity, and diabetes. Sampling methods are an important consideration for human microbiome research, yet are not emphasized in many studies. In this study, we demonstrate that the preparation, handling, and storage of human faeces are critical processes that alter the outcomes of downstream DNA-based bacterial community analyses via qPCR. We found that stool subsampling resulted in large variability of gut microbiome data due to different microenvironments harbouring various taxa within an individual stool. However, we reduced intra-sample variability by homogenizing the entire stool sample in liquid nitrogen and subsampling from the resulting crushed powder prior to DNA extraction. We experimentally determined that the bacterial taxa varied with room temperature storage beyond 15 minutes and beyond three days storage in a domestic frost-free freezer. While freeze thawing only had an effect on bacterial taxa abundance beyond four cycles, the use of samples stored in RNAlater should be avoided as overall DNA yields were reduced as well as the detection of bacterial taxa. Overall we provide solutions for processing and storing human stool samples that reduce variability of microbiome data. We recommend that stool is frozen within 15 minutes of being defecated, stored in a domestic frost-free freezer for less than three days, and homogenized prior to DNA extraction. Adoption of these simple protocols will have a significant and positive impact on future human microbiome research. Public Library of Science 2015-08-07 /pmc/articles/PMC4529225/ /pubmed/26252519 http://dx.doi.org/10.1371/journal.pone.0134802 Text en © 2015 Gorzelak et al http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Gorzelak, Monika A.
Gill, Sandeep K.
Tasnim, Nishat
Ahmadi-Vand, Zahra
Jay, Michael
Gibson, Deanna L.
Methods for Improving Human Gut Microbiome Data by Reducing Variability through Sample Processing and Storage of Stool
title Methods for Improving Human Gut Microbiome Data by Reducing Variability through Sample Processing and Storage of Stool
title_full Methods for Improving Human Gut Microbiome Data by Reducing Variability through Sample Processing and Storage of Stool
title_fullStr Methods for Improving Human Gut Microbiome Data by Reducing Variability through Sample Processing and Storage of Stool
title_full_unstemmed Methods for Improving Human Gut Microbiome Data by Reducing Variability through Sample Processing and Storage of Stool
title_short Methods for Improving Human Gut Microbiome Data by Reducing Variability through Sample Processing and Storage of Stool
title_sort methods for improving human gut microbiome data by reducing variability through sample processing and storage of stool
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4529225/
https://www.ncbi.nlm.nih.gov/pubmed/26252519
http://dx.doi.org/10.1371/journal.pone.0134802
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