Database Retrieval System V1.0

Name sreC
Function
anaerobic electron transport chain.
Definition sulfur reductase membrane anchor
AA seq
MNIKLWAWTIVFILIGGGIMFYGMSYNPLGWFQGFVSFTEPNDEPIPWGLLVIGYIFFGV IGTGVSTYNSLYELFNKNHKGKNPFDKIKLRNEWLAFAVLIPGWIMVFASTYKPAEALYI YLSFRDTSRIAWNGVLYALVGIGIIAEILALIGEKIKEEGKRGYLDRFLAWLSSKTSFEI PGLLKIVVDIDALIVGYAILAELILDANLGSVFGYLSTWVYEFGPFMSILLVVASFYAGI AMISFITPLYSWLRKPSVVSPPSAQPIATHSLGSGNVEPQEDNIMFKILARDGLLATISI GFLVLWWVWLTATNQETFPWAQLLLTGSWSLYFWIGLVLIGIIIPIALYSVAYKKESKGW LFASSIFALLGWFMLITIADVIPQAISWYYSVSPITPPGSTWAYELRSNFNGVSQFTQLP FAISQYDLVWFAGSALFLLGVYTLGVLLLPLEEEEKPKHVWIFK471
Structure
Reference
PMIDTitle & AuthorAbstractYear
012949162Membrane-bound hydrogenase and sulfur reductase of the hyperthermophilic and acidophilic archaeon Acidianus ambivalens. Laska S, Lottspeich F, Kletzin A. A sulfur reductase (SR) and a hydrogenase were purified from solubilized membrane fractions of anaerobically grown cells of the sulfur-dependent archaeon Acidianus ambivalens and the corresponding genes were sequenced. The SR reduced elemental sulfur with hydrogen as electron donor [45 U (mg protein)(-1)] in the presence of hydrogenase and either 2,3-dimethylnaphthoquinone (DMN) or cytochrome c in the enzyme assay. The SR could not be separated from the hydrogenase during purification without loss of activity, whereas the hydrogenase could be separated from the SR. The specific activity of the hydrogenase was 170 U (mg protein)(-1) with methyl viologen and 833 U (mg protein)(-1) with DMN as electron acceptors. Both holoenzymes showed molecular masses of 250 kDa. In SDS gels of active fractions, protein bands with apparent masses of 110 (SreA), 66 (HynL), 41 (HynS) and 29 kDa were present. Enriched hydrogenase fractions contained 14 micro mol Fe and 2 micromol Ni (g protein)(-1); in addition, 2.5 micromol Mo (g protein)(-1) was found in the membrane fraction. Two overlapping genomic cosmid clones were sequenced, encoding a five-gene SR cluster (sre) including the 110 kDa subunit gene (sreA), and a 12-gene hydrogenase cluster (hyn) including the large and small subunit genes and genes encoding proteins required for the maturation of NiFe hydrogenases. A phylogenetic analysis of the SR amino acid sequence revealed that the protein belonged to the DMSO reductase family of molybdoenzymes and that the family showed a novel clustering. A model of sulfur respiration in Acidianus developed from the biochemical results and the data of the amino acid sequence comparisons is discussed. 2003
124487535A comparative quantitative proteomic study identifies new proteins relevant for sulfur oxidation in the purple sulfur bacterium Allochromatium vinosum. Weissgerber T, Sylvester M, Kröninger L, Dahl C. In the present study, we compared the proteome response of Allochromatium vinosum when growing photoautotrophically in the presence of sulfide, thiosulfate, and elemental sulfur with the proteome response when the organism was growing photoheterotrophically on malate. Applying tandem mass tag analysis as well as two-dimensional (2D) PAGE, we detected 1,955 of the 3,302 predicted proteins by identification of at least two peptides (59.2%) and quantified 1,848 of the identified proteins. Altered relative protein amounts (≥1.5-fold) were observed for 385 proteins, corresponding to 20.8% of the quantified A. vinosum proteome. A significant number of the proteins exhibiting strongly enhanced relative protein levels in the presence of reduced sulfur compounds are well documented essential players during oxidative sulfur metabolism, e.g., the dissimilatory sulfite reductase DsrAB. Changes in protein levels generally matched those observed for the respective relative mRNA levels in a previous study and allowed identification of new genes/proteins participating in oxidative sulfur metabolism. One gene cluster (hyd; Alvin_2036-Alvin_2040) and one hypothetical protein (Alvin_2107) exhibiting strong responses on both the transcriptome and proteome levels were chosen for gene inactivation and phenotypic analyses of the respective mutant strains, which verified the importance of the so-called Isp hydrogenase supercomplex for efficient oxidation of sulfide and a crucial role of Alvin_2107 for the oxidation of sulfur stored in sulfur globules to sulfite. In addition, we analyzed the sulfur globule proteome and identified a new sulfur globule protein (SgpD; Alvin_2515). 2014

Laska S , Lottspeich F , Kletzin A . Membrane-bound hydrogenase and sulfur reductase of the hyperthermophilic and acidophilic archaeon Acidianus ambivalens[J]. Microbiology, 2003, 149(Pt 9):2357-2371.