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一种具有分裂细胞色素b的工程化细胞色素b6c1复合物能够支持荚膜红细菌的光合生长。

An engineered cytochrome b6c1 complex with a split cytochrome b is able to support photosynthetic growth of Rhodobacter capsulatus.

作者信息

Saribas A S, Mandaci S, Daldal F

机构信息

Department of Biology, Plant Science Institute, University of Pennsylvania, Philadelphia, Pennsylvania 19104, USA.

出版信息

J Bacteriol. 1999 Sep;181(17):5365-72. doi: 10.1128/JB.181.17.5365-5372.1999.

Abstract

The ubihydroquinone-cytochrome c oxidoreductase (or the cytochrome bc1 complex) from Rhodobacter capsulatus is composed of the Fe-S protein, cytochrome b, and cytochrome c1 subunits encoded by petA(fbcF), petB(fbcB), and petC(fbcC) genes organized as an operon. In the work reported here, petB(fbcB) was split genetically into two cistrons, petB6 and petBIV, which encoded two polypeptides corresponding to the four amino-terminal and four carboxyl-terminal transmembrane helices of cytochrome b, respectively. These polypeptides resembled the cytochrome b6 and su IV subunits of chloroplast cytochrome b6f complexes, and together with the unmodified subunits of the cytochrome bc1 complex, they formed a novel enzyme, named cytochrome b6c1 complex. This membrane-bound multisubunit complex was functional, and despite its smaller amount, it was able to support the photosynthetic growth of R. capsulatus. Upon further mutagenesis, a mutant overproducing it, due to a C-to-T transition at the second base of the second codon of petBIV, was obtained. Biochemical analyses, including electron paramagnetic spectroscopy, with this mutant revealed that the properties of the cytochrome b6c1 complex were similar to those of the cytochrome bc1 complex. In particular, it was highly sensitive to inhibitors of the cytochrome bc1 complex, including antimycin A, and the redox properties of its b- and c-type heme prosthetic groups were unchanged. However, the optical absorption spectrum of its cytochrome bL heme was modified in a way reminiscent of that of a cytochrome b6f complex. Based on the work described here and that with Rhodobacter sphaeroides (R. Kuras, M. Guergova-Kuras, and A. R. Crofts, Biochemistry 37:16280-16288, 1998), it appears that neither the inhibitor resistance nor the redox potential differences observed between the bacterial (or mitochondrial) cytochrome bc1 complexes and the chloroplast cytochrome b6f complexes are direct consequences of splitting cytochrome b into two separate polypeptides. The overall findings also illustrate the possible evolutionary relationships among various cytochrome bc oxidoreductases.

摘要

来自荚膜红细菌的泛醌 - 细胞色素c氧化还原酶(即细胞色素bc1复合物)由铁硫蛋白、细胞色素b和细胞色素c1亚基组成,这些亚基由组织成操纵子的petA(fbcF)、petB(fbcB)和petC(fbcC)基因编码。在本文报道的研究中,petB(fbcB)基因在遗传学上被拆分为两个顺反子,即petB6和petBIV,它们分别编码与细胞色素b的四个氨基末端和四个羧基末端跨膜螺旋相对应的两种多肽。这些多肽类似于叶绿体细胞色素b6f复合物的细胞色素b6和亚基IV,并且与细胞色素bc1复合物未修饰的亚基一起,形成了一种新型酶,称为细胞色素b6c1复合物。这种膜结合的多亚基复合物具有功能,尽管其含量较少,但它能够支持荚膜红细菌进行光合生长。通过进一步诱变,获得了一个由于petBIV第二个密码子的第二个碱基由C突变为T而导致该复合物过量产生的突变体。对该突变体进行的包括电子顺磁共振光谱在内的生化分析表明,细胞色素b6c1复合物的性质与细胞色素bc1复合物相似。特别是,它对细胞色素bc1复合物的抑制剂高度敏感,包括抗霉素A,并且其b型和c型血红素辅基的氧化还原性质未发生变化。然而,其细胞色素bL血红素的光吸收光谱发生了改变,这种改变方式让人联想到细胞色素b6f复合物的光谱。基于本文所述的研究以及对球形红细菌的研究(R.Kuras、M.Guergova - Kuras和A.R.Crofts,《生物化学》37:16280 - 16288,1998),似乎细菌(或线粒体)细胞色素bc1复合物与叶绿体细胞色素b6f复合物之间观察到的抑制剂抗性和氧化还原电位差异都不是将细胞色素b拆分为两个单独多肽的直接结果。总体研究结果也说明了各种细胞色素bc氧化还原酶之间可能的进化关系。

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