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Deletion of the gene for subunit III leads to defective assembly of bacterial cytochrome oxidase.

机译:III亚基的基因缺失导致细菌细胞色素氧化酶的组装不良。

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摘要

COIII is one of the major subunits in the mitochondrial and a bacterial cytochrome c oxidase, cytochrome aa3. It does not contain any of the enzyme's redox-active metal centres and can be removed from the enzyme without major changes in its established functions. We have deleted the COIII gene from Paracoccus denitrificans. The mutant still expresses spectroscopically detectable enzyme almost as the wild-type, but its cytochrome c oxidase activity is much lower. From 50 to 80% of cytochrome a is reduced and its absorption maximum is 2-3 nm blue-shifted. The EPR signal of ferric cytochrome a is heterogeneous indicating the presence of multiple cytochrome a species. Proteolysis of the membrane-bound oxidase shows new cleavage sites both in COI and COII. DEAE-chromatography of solubilized enzyme yields fractions that contain a COI + COII complex and in addition haem-binding, free COI as well as free COII. The mutant phenotype can be complemented by introducing the COIII gene back to cells in a plasmid vector. We conclude that cytochrome oxidase assembles inefficiently in the absence of COIII and that this subunit may facilitate a late step in the assembly. The different oxidase species in the mutant represent either accumulating intermediates of the assembly pathway or dissociation products of a labile COI + COII complex and its conformational variants.
机译:COIII是线粒体中的主要亚基之一,是细菌细胞色素C氧化酶,细胞色素aa3。它不包含任何酶的氧化还原活性金属中心,可以从酶中去除,而无需改变其既定功能。我们已从反硝化副球菌中删除了COIII基因。该突变体仍几乎可以像野生型那样表达可光谱检测的酶,但其细胞色素c氧化酶活性要低得多。从50%到80%的细胞色素a被还原,其最大吸收为2-3 nm蓝移。铁细胞色素a的EPR信号异质,表明存在多种细胞色素a。膜结合氧化酶的蛋白水解在COI和COII中均显示新的切割位点。溶解的酶的DEAE色谱分离得到的馏分包含COI + COII复合物,以及血红素结合,游离COI和游离COII。可以通过将COIII基因导入质粒载体中的细胞来补充突变表型。我们得出的结论是,在没有COIII的情况下,细胞色素氧化酶组装效率不高,并且该亚基可能有助于组装的后期步骤。突变体中不同的氧化酶种类代表组装途径的中间体或不稳定的COI + COII复合物及其构象变体的解离产物。

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