Real-time PCR quantification and diversity analysis of the functional genes aprA and dsrA of sulfate-reducing prokaryotes in marine sediments of the Peru continental margin and the Black Sea

Blazejak, Anna; Schippers, Axel

dc.identifier.uri	http://dx.doi.org/10.15488/464
dc.identifier.uri	http://www.repo.uni-hannover.de/handle/123456789/487
dc.contributor.author	Blazejak, Anna
dc.contributor.author	Schippers, Axel
dc.date.accessioned	2016-08-30T10:20:24Z
dc.date.available	2016-08-30T10:20:24Z
dc.date.issued	2011
dc.identifier.citation	Blazejak, Anna; Schippers, Axel: Real-time PCR quantification and diversity analysis of the functional genes aprA and dsrA of sulfate-reducing prokaryotes in marine sediments of the Peru continental margin and the Black Sea. In: Frontiers in Microbiology 2 (2011), 253. DOI: http://dx.doi.org/10.3389/fmicb.2011.00253
dc.description.abstract	Sulfate-reducing prokaryotes (SRP) are ubiquitous and quantitatively important members in many ecosystems, especially in marine sediments. However their abundance and diversity in subsurface marine sediments is poorly understood. In this study, the abundance and diversity of the functional genes for the enzymes adenosine 5'-phosphosulfate reductase (aprA) and dissimilatory sulfite reductase (dsrA) of SRP in marine sediments of the Peru continental margin and the Black Sea were analyzed, including samples from the deep biosphere (ODP site 1227). For aprA quantification a Q-PCR assay was designed and evaluated. Depth profiles of the aprA and dsrA copy numbers were almost equal for all sites. Gene copy numbers decreased concomitantly with depth from around 10(8)/g sediment close to the sediment surface to less than 10(5)/g sediment at 5 mbsf. The 16S rRNA gene copy numbers of total bacteria were much higher than those of the functional genes at all sediment depths and used to calculate the proportion of SRP to the total Bacteria. The aprA and dsrA copy numbers comprised in average 0.5-1% of the 16S rRNA gene copy numbers of total bacteria in the sediments up to a depth of ca. 40 mbsf. In the zone without detectable sulfate in the pore water from about 40-121 mbsf (Peru margin ODP site 1227), only dsrA (but not aprA) was detected with copy numbers of less than 10(4)/g sediment, comprising ca. 14% of the 16S rRNA gene copy numbers of total bacteria. In this zone, sulfate might be provided for SRP by anaerobic sulfide oxidation. Clone libraries of aprA showed that all isolated sequences originate from SRP showing a close relationship to aprA of characterized species or form a new cluster with only distant relation to aprA of isolated SRP. For dsrA a high diversity was detected, even up to 121 m sediment depth in the deep biosphere.	eng
dc.description.sponsorship	DFG/IODP/ODP/SCHI 535/5
dc.language.iso	eng
dc.publisher	Lausanne : Frontiers Research Foundation
dc.relation.ispartofseries	Frontiers in Microbiology 2 (2011)
dc.rights	CC BY-NC 3.0 Unported
dc.rights.uri	https://creativecommons.org/licenses/by-nc/3.0/
dc.subject	deep biosphere	eng
dc.subject	real-time pcr	eng
dc.subject	subsurface	eng
dc.subject	odp	eng
dc.subject	sulfate-reducing prokaryotes	eng
dc.subject	apra	eng
dc.subject	dsra	eng
dc.subject.ddc	500 \| Naturwissenschaften	ger
dc.title	Real-time PCR quantification and diversity analysis of the functional genes aprA and dsrA of sulfate-reducing prokaryotes in marine sediments of the Peru continental margin and the Black Sea
dc.type	Article
dc.type	Text
dc.relation.issn	1664-302X
dc.relation.doi	http://dx.doi.org/10.3389/fmicb.2011.00253
dc.bibliographicCitation.volume	2
dc.bibliographicCitation.firstPage	253
dc.description.version	publishedVersion
tib.accessRights	frei zug�nglich