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脱氮副球菌GB17的亚硫酸盐脱氢酶、两种c型细胞色素和一种黄素蛋白的克隆与特性分析:亚硫酸盐脱氢酶在化能无机硫氧化中的重要作用

Cloning and characterization of sulfite dehydrogenase, two c-type cytochromes, and a flavoprotein of Paracoccus denitrificans GB17: essential role of sulfite dehydrogenase in lithotrophic sulfur oxidation.

作者信息

Wodara C, Bardischewsky F, Friedrich C G

机构信息

Lehrstuhl für Technische Mikrobiologie, Fachbereich Chemietechnik, Universität Dortmund, Germany.

出版信息

J Bacteriol. 1997 Aug;179(16):5014-23. doi: 10.1128/jb.179.16.5014-5023.1997.

Abstract

A 13-kb genomic region of Paracoccus dentrificans GB17 is involved in lithotrophic thiosulfate oxidation. Adjacent to the previously reported soxB gene (C. Wodara, S. Kostka, M. Egert, D. P. Kelly, and C. G. Friedrich, J. Bacteriol. 176:6188-6191, 1994), 3.7 kb were sequenced. Sequence analysis revealed four additional open reading frames, soxCDEF. soxC coded for a 430-amino-acid polypeptide with an Mr of 47,339 that included a putative signal peptide of 40 amino acids (Mr of 3,599) with a RR motif present in periplasmic proteins with complex redox centers. The mature soxC gene product exhibited high amino acid sequence similarity to the eukaryotic molybdoenzyme sulfite oxidase and to nitrate reductase. We constructed a mutant, GBsoxC delta, carrying an in-frame deletion in soxC which covered a region possibly coding for the molybdenum cofactor binding domain. GBsoxC delta was unable to grow lithoautotrophically with thiosulfate but grew well with nitrate as a nitrogen source or as an electron acceptor. Whole cells and cell extracts of mutant GBsoxC delta contained 10% of the thiosulfate-oxidizing activity of the wild type. Only a marginal rate of sulfite-dependent cytochrome c reduction was observed from cell extracts of mutant GBsoxC delta. These results demonstrated that sulfite dehydrogenase was essential for growth with thiosulfate of P. dentrificans GB17. soxD coded for a periplasmic diheme c-type cytochrome of 384 amino acids (Mr of 39,983) containing a putative signal peptide with an Mr of 2,363. soxE coded for a periplasmic monoheme c-type cytochrome of 236 amino acids (Mr of 25,926) containing a putative signal peptide with an Mr of 1,833. SoxD and SoxE were highly identical to c-type cytochromes of P. denitrificans and other organisms. soxF revealed an incomplete open reading frame coding for a peptide of 247 amino acids with a putative signal peptide (Mr of 2,629). The deduced amino acid sequence of soxF was 47% identical and 70% similar to the sequence of the flavoprotein of flavocytochrome c of Chromatium vinosum, suggesting the involvement of the flavoprotein in thiosulfate oxidation of P. denitrificans GB17.

摘要

嗜糖假单胞菌GB17的一个13kb基因组区域参与了硫代硫酸盐的无机营养氧化。在先前报道的soxB基因(C. Wodara、S. Kostka、M. Egert、D. P. Kelly和C. G. Friedrich,《细菌学杂志》176:6188 - 6191,1994年)附近,对3.7kb进行了测序。序列分析揭示了另外四个开放阅读框,即soxCDEF。soxC编码一个430个氨基酸的多肽,分子量为47339,其中包括一个40个氨基酸的推定信号肽(分子量为3599),在具有复杂氧化还原中心的周质蛋白中存在RR基序。成熟的soxC基因产物与真核钼酶亚硫酸盐氧化酶和硝酸还原酶具有高度的氨基酸序列相似性。我们构建了一个突变体GBsoxC delta,其soxC中存在一个框内缺失,该缺失覆盖了可能编码钼辅因子结合域的区域。GBsoxC delta不能利用硫代硫酸盐进行自养生长,但以硝酸盐作为氮源或电子受体时生长良好。突变体GBsoxC delta的全细胞和细胞提取物含有野生型硫代硫酸盐氧化活性的10%。从突变体GBsoxC delta的细胞提取物中仅观察到亚硫酸盐依赖的细胞色素c还原的极低速率。这些结果表明,亚硫酸盐脱氢酶对于嗜糖假单胞菌GB17利用硫代硫酸盐生长至关重要。soxD编码一个384个氨基酸的周质双血红素c型细胞色素(分子量为39983),含有一个推定信号肽,分子量为2363。soxE编码一个236个氨基酸的周质单血红素c型细胞色素(分子量为25926),含有一个推定信号肽,分子量为1833。SoxD和SoxE与反硝化假单胞菌和其他生物体的c型细胞色素高度相同。soxF揭示了一个不完整的开放阅读框,编码一个247个氨基酸的肽,带有一个推定信号肽(分子量为2629)。soxF推导的氨基酸序列与嗜硫红假单胞菌黄素细胞色素c的黄素蛋白序列有47%的同一性和70%的相似性,表明该黄素蛋白参与了嗜糖假单胞菌GB17的硫代硫酸盐氧化。

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