Affiliation:
1. Lehrstuhl für Mikrobiologie, Universität Karlsruhe, D-76128 Karlsruhe, Germany
Abstract
ABSTRACT
The synthesis of a functional nitrous oxide reductase requires an assembly apparatus for the insertion of the prosthetic copper. Part of the system is encoded by maturation genes located in
Pseudomonas stutzeri
immediately downstream of the structural gene for the enzyme. We have studied the transcriptional organization and regulation of this region and found a
nosDFYL tatE
operon structure. In addition to a putative ABC transporter, consisting of NosD, NosF, and NosY, the operon encodes a Cu chaperone, NosL, and a component of the Tat translocon, TatE. The
nosD
operon was activated in response to anaerobiosis and nitrate denitrification. The membrane-bound regulator NosR was required for operon expression; in addition, DnrD, a regulator of the Crp-Fnr family, enhanced expression under anaerobic conditions. This establishes a likely signal transduction sequence of NO → DnrD →
nosR
/NosR →
nosD
operon. DnrD-dependent expression was also observed for the
nnrS
operon (located immediately downstream of the
nosD
operon), which encodes a putative heme-Cu protein (NnrS) and a member of the short-chain dehydrogenase family (ORF247). The NosF protein, encoded within the
nosD
operon, exhibits sequence similarity to ABC-type ATPases. It was fused to the
Escherichia coli
maltose-binding protein and overexpressed in soluble form. The fusion protein was purified and shown to have ATPase activity. NosF is the first maturation factor for which a catalytic function has been demonstrated in vitro.
Publisher
American Society for Microbiology
Subject
Molecular Biology,Microbiology
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