Modified RNA-seq method for microbial community and diversity analysis using rRNA in different types of environmental samples

RNA-seq-based SSU (small subunit) rRNA (ribosomal RNA) analysis has provided a better understanding of potentially active microbial community within environments. However, for RNA-seq library construction, high quantities of purified RNA are typically required. We propose a modified RNA-seq method f...

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Autores principales: Yan, Yong-Wei, Zou, Bin, Zhu, Ting, Hozzein, Wael N., Quan, Zhe-Xue
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2017
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5634646/
https://www.ncbi.nlm.nih.gov/pubmed/29016661
http://dx.doi.org/10.1371/journal.pone.0186161
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author Yan, Yong-Wei
Zou, Bin
Zhu, Ting
Hozzein, Wael N.
Quan, Zhe-Xue
author_facet Yan, Yong-Wei
Zou, Bin
Zhu, Ting
Hozzein, Wael N.
Quan, Zhe-Xue
author_sort Yan, Yong-Wei
collection PubMed
description RNA-seq-based SSU (small subunit) rRNA (ribosomal RNA) analysis has provided a better understanding of potentially active microbial community within environments. However, for RNA-seq library construction, high quantities of purified RNA are typically required. We propose a modified RNA-seq method for SSU rRNA-based microbial community analysis that depends on the direct ligation of a 5’ adaptor to RNA before reverse-transcription. The method requires only a low-input quantity of RNA (10–100 ng) and does not require a DNA removal step. The method was initially tested on three mock communities synthesized with enriched SSU rRNA of archaeal, bacterial and fungal isolates at different ratios, and was subsequently used for environmental samples of high or low biomass. For high-biomass salt-marsh sediments, enriched SSU rRNA and total nucleic acid-derived RNA-seq datasets revealed highly consistent community compositions for all of the SSU rRNA sequences, and as much as 46.4%-59.5% of 16S rRNA sequences were suitable for OTU (operational taxonomic unit)-based community and diversity analyses with complete coverage of V1-V2 regions. OTU-based community structures for the two datasets were also highly consistent with those determined by all of the 16S rRNA reads. For low-biomass samples, total nucleic acid-derived RNA-seq datasets were analyzed, and highly active bacterial taxa were also identified by the OTU-based method, notably including members of the previously underestimated genus Nitrospira and phylum Acidobacteria in tap water, members of the phylum Actinobacteria on a shower curtain, and members of the phylum Cyanobacteria on leaf surfaces. More than half of the bacterial 16S rRNA sequences covered the complete region of primer 8F, and non-coverage rates as high as 38.7% were obtained for phylum-unclassified sequences, providing many opportunities to identify novel bacterial taxa. This modified RNA-seq method will provide a better snapshot of diverse microbial communities, most notably by OTU-based analysis, even communities with low-biomass samples.
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spelling pubmed-56346462017-10-30 Modified RNA-seq method for microbial community and diversity analysis using rRNA in different types of environmental samples Yan, Yong-Wei Zou, Bin Zhu, Ting Hozzein, Wael N. Quan, Zhe-Xue PLoS One Research Article RNA-seq-based SSU (small subunit) rRNA (ribosomal RNA) analysis has provided a better understanding of potentially active microbial community within environments. However, for RNA-seq library construction, high quantities of purified RNA are typically required. We propose a modified RNA-seq method for SSU rRNA-based microbial community analysis that depends on the direct ligation of a 5’ adaptor to RNA before reverse-transcription. The method requires only a low-input quantity of RNA (10–100 ng) and does not require a DNA removal step. The method was initially tested on three mock communities synthesized with enriched SSU rRNA of archaeal, bacterial and fungal isolates at different ratios, and was subsequently used for environmental samples of high or low biomass. For high-biomass salt-marsh sediments, enriched SSU rRNA and total nucleic acid-derived RNA-seq datasets revealed highly consistent community compositions for all of the SSU rRNA sequences, and as much as 46.4%-59.5% of 16S rRNA sequences were suitable for OTU (operational taxonomic unit)-based community and diversity analyses with complete coverage of V1-V2 regions. OTU-based community structures for the two datasets were also highly consistent with those determined by all of the 16S rRNA reads. For low-biomass samples, total nucleic acid-derived RNA-seq datasets were analyzed, and highly active bacterial taxa were also identified by the OTU-based method, notably including members of the previously underestimated genus Nitrospira and phylum Acidobacteria in tap water, members of the phylum Actinobacteria on a shower curtain, and members of the phylum Cyanobacteria on leaf surfaces. More than half of the bacterial 16S rRNA sequences covered the complete region of primer 8F, and non-coverage rates as high as 38.7% were obtained for phylum-unclassified sequences, providing many opportunities to identify novel bacterial taxa. This modified RNA-seq method will provide a better snapshot of diverse microbial communities, most notably by OTU-based analysis, even communities with low-biomass samples. Public Library of Science 2017-10-10 /pmc/articles/PMC5634646/ /pubmed/29016661 http://dx.doi.org/10.1371/journal.pone.0186161 Text en © 2017 Yan 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 (http://creativecommons.org/licenses/by/4.0/) , which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
spellingShingle Research Article
Yan, Yong-Wei
Zou, Bin
Zhu, Ting
Hozzein, Wael N.
Quan, Zhe-Xue
Modified RNA-seq method for microbial community and diversity analysis using rRNA in different types of environmental samples
title Modified RNA-seq method for microbial community and diversity analysis using rRNA in different types of environmental samples
title_full Modified RNA-seq method for microbial community and diversity analysis using rRNA in different types of environmental samples
title_fullStr Modified RNA-seq method for microbial community and diversity analysis using rRNA in different types of environmental samples
title_full_unstemmed Modified RNA-seq method for microbial community and diversity analysis using rRNA in different types of environmental samples
title_short Modified RNA-seq method for microbial community and diversity analysis using rRNA in different types of environmental samples
title_sort modified rna-seq method for microbial community and diversity analysis using rrna in different types of environmental samples
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5634646/
https://www.ncbi.nlm.nih.gov/pubmed/29016661
http://dx.doi.org/10.1371/journal.pone.0186161
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