Affiliation:
1. Department of Bioengineering, Nagaoka University of Technology, 1603-1 Kamitomioka, Nagaoka, Niigata 940-2188, Japan
2. Department of Applied Microbiology, Hoshi University, School of Pharmacy and Pharmaceutical Sciences, 2-4-41 Ebara, Shinagawa, Tokyo 142-8501, Japan
3. Department of Civil and Environmental Engineering, Tohoku Gakuin University, 1-13-1 Chuo, Tagajo, Miyagi 985-8537, Japan
Abstract
ABSTRACT
A Gram-positive polychlorinated-biphenyl (PCB) degrader,
Rhodococcus jostii
RHA1, degrades PCBs by cometabolism with biphenyl. A two-component BphS1T1 system encoded by
bphS1
and
bphT1
(formerly
bphS
and
bphT
) is responsible for the transcription induction of the five gene clusters,
bphAaAbAcAdC1B1
,
etbAa1Ab1CbphD1
,
etbAa2Ab2AcD2
,
etbAdbphB2
, and
etbD1
, which constitute multiple enzyme systems for biphenyl/PCB degradation. The
bphS2
and
bphT2
genes, which encode BphS2 and BphT2, virtually identical to BphS1 (92%) and BphT1 (97%), respectively, were characterized. BphS2T2 induced the activation of the
bphAa
promoter in a host,
Rhodococcus erythropolis
IAM1399, in the presence of a variety of aromatics, including benzene, toluene, ethylbenzene, xylenes, isopropylbenzene, and chlorinated benzenes, as effectively as BphS1T1. The substrate spectrum of BphS2T2 was the same as that of BphS1T1, except for biphenyl, which is a substrate only for BphS1T1. BphS2T2 activated transcription from the five promoters of biphenyl/PCB degradation enzyme gene clusters as effectively as BphS1T1. The targeted disruptions of the
bphS1
,
bphS2
,
bphT1
, and
bphT2
genes indicated that all these genes are involved in the growth of RHA1 on aromatic compounds. The hybrid system with
bphS1
and
bphT2
and that with
bphS2
and
bphT1
were constructed, and both systems conducted induced activation of the
bphAa
promoter, indicating cross-communication. These results indicated that RHA1 employs not only multiple enzyme systems, but also dual regulatory systems for biphenyl/PCB degradation. Comparison of the sequences, including
bphS2T2
, with the
bphS1T1
-containing sequences and the corresponding sequences in other rhodococcal degraders suggests that
bphS2T2
might have originated from
bphS1T1
.
Publisher
American Society for Microbiology
Subject
Molecular Biology,Microbiology
Cited by
31 articles.
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