Minor revision to V4 region SSU rRNA 806R gene primer greatly increases detection of SAR11 bacterioplankton

dc.contributor.author Apprill, Amy
dc.contributor.author McNally, Sean
dc.contributor.author Parsons, Rachel
dc.contributor.author Weber, Laura
dc.date.accessioned 2015-07-29T19:24:18Z
dc.date.available 2015-07-29T19:24:18Z
dc.date.issued 2015-06-04
dc.description Author Posting. © Inter-Research, 2015. This article is posted here by permission of Inter-Research for personal use, not for redistribution. The definitive version was published in Aquatic Microbial Ecology 75 (2015): 129-137, doi:10.3354/ame01753. en_US
dc.description.abstract High-throughput sequencing of small subunit ribosomal RNA (SSU rRNA) genes from marine environments is a widely applied method used to uncover the composition of microbial communities. We conducted an analysis of surface ocean waters with the commonly employed hypervariable 4 region SSU rRNA gene primers 515F and 806R, and found that bacteria belonging to the SAR11 clade of Alphaproteobacteria, a group typically making up 20 to 40% of the bacterioplankton in this environment, were greatly underrepresented and comprised <4% of the total community. Using the SILVA reference database, we found a single nucleotide mismatch to nearly all SAR11 subclades, and revised the 806R primer so that it increased the detection of SAR11 clade sequences in the database from 2.6 to 96.7%. We then compared the performance of the original and revised 806R primers in surface seawater samples, and found that SAR11 comprised 0.3 to 3.9% of sequences with the original primers and 17.5 to 30.5% of the sequences with the revised 806R primer. Furthermore, an investigation of seawater obtained from aquaria revealed that SAR11 sequences acquired with the revised 806R primer were more similar to natural cellular abundances of SAR11 detected using fluorescence in situ hybridization counts. Collectively, these results demonstrate that a minor adjustment to the 806R primer will greatly increase detection of the globally abundant SAR11 clade in marine and lake environments, and enable inclusion of this important bacterial lineage in experimental and environmental-based studies. en_US
dc.description.sponsorship This project was supported by NSF award OCE-1233612 to A.A. with contributions from BIOS Grant in aid award to S.McN. and NSF Oceanic Microbial Observatory OCE-0801991 subcontract to BIOS managed by R.P. en_US
dc.format.mimetype application/vnd.ms-excel
dc.format.mimetype application/pdf
dc.identifier.citation Aquatic Microbial Ecology 75 (2015): 129-137 en_US
dc.identifier.doi 10.3354/ame01753
dc.identifier.uri https://hdl.handle.net/1912/7426
dc.language.iso en_US en_US
dc.publisher Inter-Research en_US
dc.relation.uri https://doi.org/10.3354/ame01753
dc.subject SSU rRNA gene en_US
dc.subject 16S en_US
dc.subject SAR11 en_US
dc.subject Bacteria en_US
dc.subject Fluorescence in situ hybridization en_US
dc.subject FISH en_US
dc.title Minor revision to V4 region SSU rRNA 806R gene primer greatly increases detection of SAR11 bacterioplankton en_US
dc.type Article en_US
dspace.entity.type Publication
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relation.isAuthorOfPublication.latestForDiscovery 51d7f6bf-4019-4d91-8c08-418113454a1e
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