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编码反硝化副球菌亚硝酸还原酶的nir基因簇的转录调控涉及NNR和NirI,NirI是一种新型膜蛋白。

Transcription regulation of the nir gene cluster encoding nitrite reductase of Paracoccus denitrificans involves NNR and NirI, a novel type of membrane protein.

作者信息

Saunders N F, Houben E N, Koefoed S, de Weert S, Reijnders W N, Westerhoff H V, De Boer A P, Van Spanning R J

机构信息

Department of Molecular Cell Physiology, Faculty of Biology, BioCentrum Amsterdam, Vrije Universiteit, De Boelelaan 1087, NL-1081 HV Amsterdam, The Netherlands.

出版信息

Mol Microbiol. 1999 Oct;34(1):24-36. doi: 10.1046/j.1365-2958.1999.01563.x.

DOI:10.1046/j.1365-2958.1999.01563.x
PMID:10540283
Abstract

The nirIX gene cluster of Paracoccus denitrificans is located between the nir and nor gene clusters encoding nitrite and nitric oxide reductases respectively. The NirI sequence corresponds to that of a membrane-bound protein with six transmembrane helices, a large periplasmic domain and cysteine-rich cytoplasmic domains that resemble the binding sites of [4Fe-4S] clusters in many ferredoxin-like proteins. NirX is soluble and apparently located in the periplasm, as judged by the predicted signal sequence. NirI and NirX are homologues of NosR and NosX, proteins involved in regulation of the expression of the nos gene cluster encoding nitrous oxide reductase in Pseudomonas stutzeri and Sinorhizobium meliloti. Analysis of a NirI-deficient mutant strain revealed that NirI is involved in transcription activation of the nir gene cluster in response to oxygen limitation and the presence of N-oxides. The NirX-deficient mutant transiently accumulated nitrite in the growth medium, but it had a final growth yield similar to that of the wild type. Transcription of the nirIX gene cluster itself was controlled by NNR, a member of the family of FNR-like transcriptional activators. An NNR binding sequence is located in the middle of the intergenic region between the nirI and nirS genes with its centre located at position -41.5 relative to the transcription start sites of both genes. Attempts to complement the NirI mutation via cloning of the nirIX gene cluster on a broad-host-range vector were unsuccessful, the ability to express nitrite reductase being restored only when the nirIX gene cluster was reintegrated into the chromosome of the NirI-deficient mutant via homologous recombination in such a way that the wild-type nirI gene was present directly upstream of the nir operon.

摘要

反硝化副球菌的nirIX基因簇位于分别编码亚硝酸还原酶和一氧化氮还原酶的nir和nor基因簇之间。NirI序列对应于一种膜结合蛋白,该蛋白具有六个跨膜螺旋、一个大的周质结构域和富含半胱氨酸的细胞质结构域,这些结构域类似于许多铁氧化还原蛋白样蛋白质中[4Fe-4S]簇的结合位点。根据预测的信号序列判断,NirX是可溶的,显然位于周质中。NirI和NirX是NosR和NosX的同源物,NosR和NosX是参与调控斯氏假单胞菌和苜蓿中华根瘤菌中编码一氧化二氮还原酶的nos基因簇表达的蛋白质。对NirI缺陷突变菌株的分析表明,NirI参与了nir基因簇在氧限制和N-氧化物存在下的转录激活。NirX缺陷突变体在生长培养基中短暂积累亚硝酸盐,但其最终生长产量与野生型相似。nirIX基因簇本身的转录受FNR样转录激活因子家族成员NNR的控制。一个NNR结合序列位于nirI和nirS基因之间基因间区域的中间,其中心位于相对于两个基因转录起始位点的-41.5位置。试图通过在广泛宿主范围载体上克隆nirIX基因簇来互补NirI突变未成功,只有当nirIX基因簇通过同源重组重新整合到NirI缺陷突变体染色体中,使野生型nirI基因直接位于nir操纵子上游时,亚硝酸还原酶的表达能力才得以恢复。

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