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Analyzing Gene Expression from Marine Microbial Communities using Environmental Transcriptomics

Analogous to metagenomics, environmental transcriptomics (metatranscriptomics) retrieves and sequences environmental mRNAs from a microbial assemblage without prior knowledge of what genes the community might be expressing. Thus it provides the most unbiased perspective on community gene expression...

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Autores principales: Poretsky, Rachel S., Gifford, Scott, Rinta-Kanto, Johanna, Vila-Costa, Maria, Moran, Mary Ann
Formato: Texto
Lenguaje:English
Publicado: MyJove Corporation 2009
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2789660/
https://www.ncbi.nlm.nih.gov/pubmed/19229184
http://dx.doi.org/10.3791/1086
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author Poretsky, Rachel S.
Gifford, Scott
Rinta-Kanto, Johanna
Vila-Costa, Maria
Moran, Mary Ann
author_facet Poretsky, Rachel S.
Gifford, Scott
Rinta-Kanto, Johanna
Vila-Costa, Maria
Moran, Mary Ann
author_sort Poretsky, Rachel S.
collection PubMed
description Analogous to metagenomics, environmental transcriptomics (metatranscriptomics) retrieves and sequences environmental mRNAs from a microbial assemblage without prior knowledge of what genes the community might be expressing. Thus it provides the most unbiased perspective on community gene expression in situ. Environmental transcriptomics protocols are technically difficult since prokaryotic mRNAs generally lack the poly(A) tails that make isolation of eukaryotic messages relatively straightforward (1) and because of the relatively short half lives of mRNAs (2). In addition, mRNAs are much less abundant than rRNAs in total RNA extracts, thus an rRNA background often overwhelms mRNA signals. However, techniques for overcoming some of these difficulties have recently been developed. A procedure for analyzing environmental transcriptomes by creating clone libraries using random primers to reverse-transcribe and amplify environmental mRNAs was recently described was successful in two different natural environments, but results were biased by selection of the random primers used to initiate cDNA synthesis (3). Advances in linear amplification of mRNA obviate the need for random primers in the amplification step and make it possible to use less starting material decreasing the collection and processing time of samples and thereby minimizing RNA degradation (4). In vitro transcription methods for amplifying mRNA involve polyadenylating the mRNA and incorporating a T7 promoter onto the 3 end of the transcript. Amplified RNA (aRNA) can then be converted to double stranded cDNA using random hexamers and directly sequenced by pyrosequencing (5). A first use of this method at Station ALOHA demonstrated its utility for characterizing microbial community gene expression (6).
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spelling pubmed-27896602011-07-21 Analyzing Gene Expression from Marine Microbial Communities using Environmental Transcriptomics Poretsky, Rachel S. Gifford, Scott Rinta-Kanto, Johanna Vila-Costa, Maria Moran, Mary Ann J Vis Exp Microbiology Analogous to metagenomics, environmental transcriptomics (metatranscriptomics) retrieves and sequences environmental mRNAs from a microbial assemblage without prior knowledge of what genes the community might be expressing. Thus it provides the most unbiased perspective on community gene expression in situ. Environmental transcriptomics protocols are technically difficult since prokaryotic mRNAs generally lack the poly(A) tails that make isolation of eukaryotic messages relatively straightforward (1) and because of the relatively short half lives of mRNAs (2). In addition, mRNAs are much less abundant than rRNAs in total RNA extracts, thus an rRNA background often overwhelms mRNA signals. However, techniques for overcoming some of these difficulties have recently been developed. A procedure for analyzing environmental transcriptomes by creating clone libraries using random primers to reverse-transcribe and amplify environmental mRNAs was recently described was successful in two different natural environments, but results were biased by selection of the random primers used to initiate cDNA synthesis (3). Advances in linear amplification of mRNA obviate the need for random primers in the amplification step and make it possible to use less starting material decreasing the collection and processing time of samples and thereby minimizing RNA degradation (4). In vitro transcription methods for amplifying mRNA involve polyadenylating the mRNA and incorporating a T7 promoter onto the 3 end of the transcript. Amplified RNA (aRNA) can then be converted to double stranded cDNA using random hexamers and directly sequenced by pyrosequencing (5). A first use of this method at Station ALOHA demonstrated its utility for characterizing microbial community gene expression (6). MyJove Corporation 2009-02-18 /pmc/articles/PMC2789660/ /pubmed/19229184 http://dx.doi.org/10.3791/1086 Text en Copyright © 2009, Journal of Visualized Experiments http://creativecommons.org/licenses/by/2.0/ 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 work is properly cited.
spellingShingle Microbiology
Poretsky, Rachel S.
Gifford, Scott
Rinta-Kanto, Johanna
Vila-Costa, Maria
Moran, Mary Ann
Analyzing Gene Expression from Marine Microbial Communities using Environmental Transcriptomics
title Analyzing Gene Expression from Marine Microbial Communities using Environmental Transcriptomics
title_full Analyzing Gene Expression from Marine Microbial Communities using Environmental Transcriptomics
title_fullStr Analyzing Gene Expression from Marine Microbial Communities using Environmental Transcriptomics
title_full_unstemmed Analyzing Gene Expression from Marine Microbial Communities using Environmental Transcriptomics
title_short Analyzing Gene Expression from Marine Microbial Communities using Environmental Transcriptomics
title_sort analyzing gene expression from marine microbial communities using environmental transcriptomics
topic Microbiology
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2789660/
https://www.ncbi.nlm.nih.gov/pubmed/19229184
http://dx.doi.org/10.3791/1086
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