Affiliation:
1. Fachbereich Biologie, Universität Konstanz, D-78457 Konstanz,1 and
2. Max-Planck-Institut für Terrestrische Mikrobiologie, D-35043 Marburg,2 Germany
Abstract
ABSTRACT
A dissimilatory sulfite reductase (DSR) was purified from the anaerobic, taurine-degrading bacterium
Bilophila wadsworthia
RZATAU to apparent homogeneity. The enzyme is involved in energy conservation by reducing sulfite, which is formed during the degradation of taurine as an electron acceptor, to sulfide. According to its UV-visible absorption spectrum with maxima at 392, 410, 583, and 630 nm, the enzyme belongs to the desulfoviridin type of DSRs. The sulfite reductase was isolated as an α
2
β
2
γ
n
(
n
≥ 2) multimer with a native size of 285 kDa as determined by gel filtration. We have sequenced the genes encoding the α and β subunits (
dsrA
and
dsrB
, respectively), which probably constitute one operon.
dsrA
and
dsrB
encode polypeptides of 49 (α) and 54 kDa (β) which show significant similarities to the homologous subunits of other DSRs. The
dsrB
gene product of
B. wadsworthia
is apparently a fusion protein of
dsrB
and
dsrD
. This indicates a possible functional role of DsrD in DSR function because of its presence as a fusion protein as an integral part of the DSR holoenzyme in
B. wadsworthia
. A phylogenetic analysis using the available Dsr sequences revealed that
B. wadsworthia
grouped with its closest 16S rDNA relative
Desulfovibrio desulfuricans
Essex 6.
Publisher
American Society for Microbiology
Subject
Molecular Biology,Microbiology
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