首页> 美国卫生研究院文献>Journal of Bacteriology >Carboxyl-terminal processing of the cytoplasmic NAD-reducing hydrogenase of Alcaligenes eutrophus requires the hoxW gene product.
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Carboxyl-terminal processing of the cytoplasmic NAD-reducing hydrogenase of Alcaligenes eutrophus requires the hoxW gene product.

机译:嗜碱产碱杆菌胞质NAD还原氢酶的羧基末端加工需要hoxW基因产物。

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摘要

Two open reading frames (ORFs) were identified immediately downstream of the four structural genes for the soluble hydrogenase (SH) of Alcaligenes eutrophus H16. While a mutation in ORF2 had no obvious effect on hydrogen metabolism, an in-frame deletion in ORF1, subsequently designated hoxW, led to a complete loss of SH activity and hence a significant retardation of autotrophic growth on hydrogen. Hydrogen oxidation in the hoxW mutant was catalyzed by the second hydrogenase, a membrane-bound enzyme. Assembly of the four subunits of the SH was blocked in mutant cells, and HoxH, the hydrogen-activating subunit, accumulated as a precursor which was still capable of binding nickel. Protein sequencing revealed that HoxH isolated from the wild type terminates at His-464, whereas the C-terminal amino acid sequence of HoxH from the hoxW mutant is colinear with the deduced sequence. Processing of the HoxH precursor was restored in vitro by a cell extract containing HoxW. These results indicate that HoxW is a highly specific carboxyl-terminal protease which releases a 24-amino-acid peptide from HoxH prior to progression of subunit assembly.
机译:两个开放阅读框(ORF)被确定为在Alcaligenes eutrophus H16的可溶性氢化酶(SH)的四个结构基因的下游。虽然ORF2的突变对氢代谢没有明显影响,但ORF1的读框内缺失(后来称为hoxW)导致SH活性完全丧失,因此显着阻碍了氢的自养生长。 hoxW突变体中的氢氧化被第二种氢化酶(一种膜结合酶)催化。 SH的四个亚基的装配在突变细胞中被阻断,HoxH(氢激活亚基)作为前体积聚,仍然能够结合镍。蛋白质测序表明,从野生型中分离出的HoxH终止于His-464,而来自hoxW突变体的HoxH的C末端氨基酸序列与推导的序列共线。通过含有HoxW的细胞提取物在体外恢复了HoxH前体的加工。这些结果表明,HoxW是高度特异性的羧基末端蛋白酶,其在亚单位组装进行之前从HoxH释放出24个氨基酸的肽。

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