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

Gorzelak, Monika A.; Gill, S K; Tasnim, Nishat; Zahra, Ahmadi-Vand; Jay, Michael N.; Gibson, Deanna L.

doi:10.1371/journal.pone.0134802

Cited by 248 publications

(254 citation statements)

References 35 publications

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“…In general, our findings agree with those from many of the previous studies considering the impact of the collection method and short-term storage at room temperature in predominantly Western populations (6)(7)(8)(9)(10)(11)(12)(13)(14)(15)(16)(17)(18)(19)(20)(21)(22)(23). In general, FOBT cards or Whatman FTA cards, which have feces smeared on the card itself that then dries, have been found to be relatively stable at room temperature and similar to immediately frozen samples without preservatives (6,10,15,21,22).…”

Section: Figsupporting

confidence: 90%

“…The impact of the type of fecal sample collection method on microbial data has been considered in a number of previous studies (6)(7)(8)(9)(10)(11)(12)(13)(14)(15)(16)(17)(18)(19)(20)(21)(22)(23). However, the majority of these studies were conducted in North American or European populations near academic or clinical laboratories and typically included only a small number of methods.…”

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Comparison of Fecal Collection Methods for Microbiota Studies in Bangladesh

Vogtmann

Chen

Kibriya

et al. 2017

Appl Environ Microbiol

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To our knowledge, fecal microbiota collection methods have not been evaluated in low-and middle-income countries. Therefore, we evaluated five different fecal sample collection methods for technical reproducibility, stability, and accuracy within the Health Effects of Arsenic Longitudinal Study (HEALS) in Bangladesh. Fifty participants from the HEALS provided fecal samples in the clinic which were aliquoted into no solution, 95% ethanol, RNAlater, postdevelopment fecal occult blood test (FOBT) cards, and fecal immunochemical test (FIT) tubes. Half of the aliquots were frozen immediately at Ϫ80°C (day 0) and the remaining samples were left at ambient temperature for 96 h and then frozen (day 4). Intraclass correlation coefficients (ICC) were calculated for the relative abundances of the top three phyla, for two alpha diversity measures, and for four beta diversity measures. The duplicate samples had relatively high ICCs for technical reproducibility at day 0 and day 4 (range, 0.79 to 0.99). The FOBT card and samples preserved in RNAlater and 95% ethanol had the highest ICCs for stability over 4 days. The FIT tube had lower stability measures overall. In comparison to the "gold standard" method using immediately frozen fecal samples with no solution, the ICCs for many of the microbial metrics were low, but the rank order appeared to be preserved as seen by the Spearman correlation. The FOBT cards, 95% ethanol, and RNAlater were effective fecal preservatives. These fecal collection methods are optimal for future cohort studies, particularly in low-and middle-income countries. IMPORTANCEThe collection of fecal samples in prospective cohort studies is essential to provide the opportunity to study the effect of the human microbiota on numerous health conditions. However, these collection methods have not been adequately tested in low-and middle-income countries. We present estimates of technical reproducibility, stability at ambient temperature for 4 days, and accuracy comparing a "gold standard" for fecal samples in no solution, 95% ethanol, RNAlater, postdevelopment fecal occult blood test cards, and fecal immunochemical test tubes in a study conducted in Bangladesh. Fecal occult blood test cards and fecal samples stored in 95% ethanol or RNAlater adequately preserve fecal samples in this setting. Therefore, new studies in low-and middle-income countries should include collection of fecal samples using fecal occult blood test cards, 95% ethanol, or RNAlater for prospective cohort studies.

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Section: Figsupporting

confidence: 90%

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confidence: 99%

Comparison of Fecal Collection Methods for Microbiota Studies in Bangladesh

Vogtmann

Chen

Kibriya

et al. 2017

Appl Environ Microbiol

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“…Investigators in a number of previous studies have assessed different collection methods for fecal samples and the impact of leaving a sample at room temperature on the fecal microbiome (10,(18)(19)(20)(21)(22)(23)(24)(25)(26)(27)(28)(29)(30)(31)(32)(33). The FOBT card, or a similar Whatman FTA card (GE Healthcare Life Sciences, Pittsburgh, Pennsylvania), has been tested in a few studies (10,21,26,32).…”

Section: Discussionmentioning

confidence: 99%

“…RNAlater has also been tested in a number of studies (10, 20-24, 26, 30, 32), but the results varied. The majority of studies concluded that RNAlater was an acceptable preservative for microbial analyses of fecal samples (10,22,23,26,30), although in some studies, researchers detected decreased alpha diversity (20,21,30), decreased DNA purity or yields (21,24), or lower stability at room temperature for longer periods (33) compared with immediately frozen fecal samples. Storage of fecal samples in 70% ethanol does not appear to be suitable for microbiome analyses (10), but 95% ethanol has been previously observed to adequately preserve fecal samples (23,33).…”

Section: Discussionmentioning

confidence: 99%

Comparison of Collection Methods for Fecal Samples in Microbiome Studies

Chen²,

et al. 2016

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Prospective cohort studies are needed to assess the relationship between the fecal microbiome and human health and disease. To evaluate fecal collection methods, we determined technical reproducibility, stability at ambient temperature, and accuracy of 5 fecal collection methods (no additive, 95% ethanol, RNAlater Stabilization Solution, fecal occult blood test cards, and fecal immunochemical test tubes). Fifty-two healthy volunteers provided fecal samples at the Mayo Clinic in Rochester, Minnesota, in 2014. One set from each sample collection method was frozen immediately, and a second set was incubated at room temperature for 96 hours and then frozen. Intraclass correlation coefficients (ICCs) were calculated for the relative abundance of 3 phyla, 2 alpha diversity metrics, and 4 beta diversity metrics. Technical reproducibility was high, with ICCs for duplicate fecal samples between 0.64 and 1.00. Stability for most methods was generally high, although the ICCs were below 0.60 for 95% ethanol in metrics that were more sensitive to relative abundance. When compared with fecal samples that were frozen immediately, the ICCs were below 0.60 for the metrics that were sensitive to relative abundance; however, the remaining 2 alpha diversity and 3 beta diversity metrics were all relatively accurate, with ICCs above 0.60. In conclusion, all fecal sample collection methods appear relatively reproducible, stable, and accurate. Future studies could use these collection methods for microbiome analyses. feces; microbiota; specimen collection Abbreviations: FIT, fecal immunochemical test, FOBT, fecal occult blood test, ICC, intraclass correlation coefficient, OTU, operational taxonomic unit.

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“…Some of the studies, such as the study conducted by Zhu et al (15), used patients with no history of antibiotics, probiotics, proton pump inhibitors, and histamine receptor antagonists within 3 mo before examining the fecal microbiota; however, others did not consider all of these precautions. In addition, the collection and processing of fecal samples have been shown to produce large variances and inaccuracies in the interpretation of the taxa present in the microbiota (48), which may be a contributing factor to the conflicting data found in NAFLD microbiome studies. Even so, all of these studies have evaluated the association, and well-designed studies are needed to unravel any causal relation between the gut microbes and NAFLD.…”

Section: Introductionmentioning

confidence: 99%

Nonalcoholic Fatty Liver Disease, the Gut Microbiome, and Diet

Mokhtari

Gibson

Hekmatdoost

2017

Advances in Nutrition

133

100

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Nonalcoholic fatty liver disease (NAFLD) is the most common liver disorder in the world, yet the pathogenesis of the disease is not well elucidated. Due to the close anatomic and functional association between the intestinal lumen and the liver through the portal system, it is speculated that the gut microbiome may play a pivotal role in the pathogenesis of NAFLD. Furthermore, diet, which can modulate the gut microbiome and several metabolic pathways involved in NAFLD development, shows a potential tripartite relation between the gut, diet, and the liver. In this review, we summarize the current evidence that supports the association between NAFLD, the gut microbiome, and the role of diet. Adv Nutr 2017;8:240-52.

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

Cited by 248 publications

References 35 publications

Comparison of Fecal Collection Methods for Microbiota Studies in Bangladesh

Comparison of Fecal Collection Methods for Microbiota Studies in Bangladesh

Comparison of Collection Methods for Fecal Samples in Microbiome Studies

Nonalcoholic Fatty Liver Disease, the Gut Microbiome, and Diet

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