Microbial drivers of DMSO reduction and DMS-dependent methanogenesis in saltmarsh sediments

Author:

Tebbe Dennis Alexander1ORCID,Gruender Charlotte2,Dlugosch Leon1,Lõhmus Kertu3,Rolfes Sönke1,Könneke Martin1,Chen Yin2ORCID,Engelen Bert1,Schäfer Hendrik2ORCID

Affiliation:

1. Institute for Chemistry and Biology of the Marine Environment, University of Oldenburg , Carl-von-Ossietzky-Str. 9-11, 26129 Oldenburg, Germany

2. School of Life Sciences, University of Warwick , CV4 7AL Coventry, UK

3. Institute of Biology and Environmental Sciences, University of Oldenburg , Carl-von-Ossietzky-Str. 9-11, 26129 Oldenburg, Germany

Abstract

Abstract Saltmarshes are highly productive environments, exhibiting high abundances of organosulfur compounds. Dimethylsulfoniopropionate (DMSP) is produced in large quantities by algae, plants, and bacteria and is a potential precursor for dimethylsulfoxide (DMSO) and dimethylsulfide (DMS). DMSO serves as electron acceptor for anaerobic respiration leading to DMS formation, which is either emitted or can be degraded by methylotrophic prokaryotes. Major products of these reactions are trace gases with positive (CO2, CH4) or negative (DMS) radiative forcing with contrasting effects on the global climate. Here, we investigated organic sulfur cycling in saltmarsh sediments and followed DMSO reduction in anoxic batch experiments. Compared to previous measurements from marine waters, DMSO concentrations in the saltmarsh sediments were up to ~300 fold higher. In batch experiments, DMSO was reduced to DMS and subsequently consumed with concomitant CH4 production. Changes in prokaryotic communities and DMSO reductase gene counts indicated a dominance of organisms containing the Dms-type DMSO reductases (e.g., Desulfobulbales, Enterobacterales). In contrast, when sulfate reduction was inhibited by molybdate, Tor-type DMSO reductases (e.g., Rhodobacterales) increased. Vibrionales increased in relative abundance in both treatments, and metagenome assembled genomes (MAGs) affiliated to Vibrio had all genes encoding the subunits of DMSO reductases. Molar conversion ratios of <1.3 CH4 per added DMSO were accompanied by a predominance of the methylotrophic methanogens Methanosarcinales. Enrichment of mtsDH genes, encoding for DMS methyl transferases in metagenomes of batch incubations indicate their role in DMS-dependent methanogenesis. MAGs affiliated to Methanolobus carried the complete set of genes encoding for the enzymes in methylotrophic methanogenesis.

Funder

Hanse-Wissenschaftskolleg Institute for Advanced Studies in Delmenhorst, Germany

Deutsche Forschungsgemeinschaft

RCUK | Engineering and Physical Sciences Research Council

RCUK | Biotechnology and Biological Sciences Research Council

Publisher

Oxford University Press (OUP)

Subject

Ecology, Evolution, Behavior and Systematics,Microbiology

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