Impact of Preservation Method and 16S rRNA Hypervariable Region on Gut Microbiota Profiling

Zigui Chen; Pak Chun Hui; Mamie Hui; Yun Kit Yeoh; Po Yee Wong; Martin C W Chan; Martin C S Wong; Siew C Ng; Francis K L Chan; Paul K S Chan

doi:10.1128/mSystems.00271-18

Impact of Preservation Method and 16S rRNA Hypervariable Region on Gut Microbiota Profiling

mSystems. 2019 Feb 26;4(1):e00271-18. doi: 10.1128/mSystems.00271-18. eCollection 2019 Jan-Feb.

Authors

Zigui Chen^{1

2}, Pak Chun Hui², Mamie Hui^{1

2}, Yun Kit Yeoh^{1

2}, Po Yee Wong², Martin C W Chan², Martin C S Wong^{1

3}, Siew C Ng^{1

4

5}, Francis K L Chan^{1

4}, Paul K S Chan^{1

2}

Affiliations

¹ Centre for Gut Microbiota Research, Faculty of Medicine, The Chinese University of Hong Kong, Hong Kong SAR, China.
² Department of Microbiology, Faculty of Medicine, The Chinese University of Hong Kong, Hong Kong SAR, China.
³ Jockey Club School of Public Health and Primary Care, Faculty of Medicine, The Chinese University of Hong Kong, Hong Kong SAR, China.
⁴ Department of Medicine and Therapeutics, Faculty of Medicine, The Chinese University of Hong Kong, Hong Kong SAR, China.
⁵ LKS Institute of Health Science, State Key Laboratory of Digestive Disease, Faculty of Medicine, The Chinese University of Hong Kong, Hong Kong SAR, China.

Abstract

Proper preservation of stool samples to minimize microbial community shifts and inactivate infectious agents is important for self-collected specimens requiring shipment to laboratories when cold chain transport is not feasible. In this study, we evaluated the performance of six preservation solutions (Norgen, OMNI, RNAlater, CURNA, HEMA, and Shield) for these aspects. Following storage of human stool samples with these preservatives at room temperature for 7 days, three hypervariable regions of the bacterial 16S rRNA gene (V1-V2, V3-V4, and V4) were amplicon sequenced. We found that samples collected in two preservatives, Norgen and OMNI, showed the least shift in community composition relative to -80°C standards compared with other storage conditions, and both efficiently inhibited the growth of aerobic and anaerobic bacteria. RNAlater did not prevent bacterial activity and exhibited relatively larger community shift. Although the effect of preservation solution was small compared to intersubject variation, notable changes in microbiota composition were observed, which could create biases in downstream data analysis. When community profiles inferred from different 16S rRNA gene hypervariable regions were compared, we found differential sensitivity of primer sets in identifying overall microbial community and certain bacterial taxa. For example, reads generated by the V4 primer pair showed a higher alpha diversity of the gut microbial community. The degenerate 27f-YM primer failed to detect the majority of Bifidobacteriales. Our data indicate that choice of preservation solution and 16S rRNA gene primer pair are critical determinants affecting gut microbiota profiling. IMPORTANCE Large-scale human microbiota studies require specimens collected from multiple sites and/or time points to maximize detection of the small effects in microbe-host interactions. However, batch biases caused by experimental protocols, such as sample collection, massively parallel sequencing, and bioinformatics analyses, remain critical and should be minimized. This work evaluated the effects of preservation solutions and bacterial 16S rRNA gene primer pairs in revealing human gut microbiota composition. Since notable changes in detecting bacterial composition and abundance were observed among choice of preservatives and primer pairs, a consistent methodology is essential in minimizing their effects to facilitate comparisons between data sets.

Keywords: 16S rRNA gene; amplicon sequencing; bacterial culture; gut microbiota; preservative.