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具有W56R点突变的胞质溶胶合成亚基II(Cox2)前体在酵母线粒体中被正确加工,以挽救细胞色素氧化酶。

The cytosol-synthesized subunit II (Cox2) precursor with the point mutation W56R is correctly processed in yeast mitochondria to rescue cytochrome oxidase.

作者信息

Cruz-Torres Valentín, Vázquez-Acevedo Miriam, García-Villegas Rodolfo, Pérez-Martínez Xochitl, Mendoza-Hernández Guillermo, González-Halphen Diego

机构信息

Instituto de Fisiología Celular, Universidad Nacional Autónoma de México, México D.F., Mexico.

出版信息

Biochim Biophys Acta. 2012 Dec;1817(12):2128-39. doi: 10.1016/j.bbabio.2012.09.006. Epub 2012 Sep 15.

DOI:10.1016/j.bbabio.2012.09.006
PMID:22985601
Abstract

Deletion of the yeast mitochondrial gene COX2 encoding subunit 2 (Cox2) of cytochrome c oxidase (CcO) results in loss of respiration (Δcox2 strain). Supekova et al. (2010) [1] transformed a Δcox2 strain with a vector expressing Cox2 with a mitochondrial targeting sequence (MTS) and the point mutation W56R (Cox2(W56R)), restoring respiratory growth. Here, the CcO carrying the allotopically-expressed Cox2(W56R) was characterized. Yeast mitochondria from the wild-type (WT) and the Δcox2+Cox2(W56R) strains were subjected to Blue Native electrophoresis. In-gel activity of CcO and spectroscopic quantitation of cytochromes revealed that only 60% of CcO is present in the complemented strain, and that less CcO is found associated in supercomplexes as compared to WT. CcOs from the WT and the mutant exhibited similar subunit composition, although activity was 20-25% lower in the enzyme containing Cox2(W56R) than in the one with Cox2(WT). Tandem mass spectrometry confirmed that W(56) was substituted by R(56) in Cox2(W56R). In addition, Cox2(W56R) exhibited the same N-terminus than Cox2(WT), indicating that the MTS of Oxa1 and the leader sequence of 15 residues were removed from Cox2(W56R) during maturation. Thus, Cox2(W56R) is identical to Cox2(WT) except for the point mutation W56R. Mitochondrial Cox1 synthesis is strongly reduced in Δcox2 mutants, but the Cox2(W56R) complemented strain led to full restoration of Cox1 synthesis. We conclude that the cytosol-synthesized Cox2(W56R) follows a rate-limiting process of import, maturation or assembly that yields lower steady-state levels of CcO. Still, the allotopically-expressed Cox2(W56R) restores CcO activity and allows mitochondrial Cox1 synthesis to advance at WT levels.

摘要

酵母线粒体基因COX2的缺失导致呼吸作用丧失(Δcox2菌株),该基因编码细胞色素c氧化酶(CcO)的亚基2(Cox2)。苏佩科娃等人(2010年)[1]用一个表达带有线粒体靶向序列(MTS)和点突变W56R的Cox2(Cox2(W56R))的载体转化Δcox2菌株,恢复了呼吸生长。在此,对携带异位表达的Cox2(W56R)的CcO进行了表征。对野生型(WT)和Δcox2 + Cox2(W56R)菌株的酵母线粒体进行了蓝色非变性电泳。CcO的凝胶内活性和细胞色素的光谱定量分析表明,在互补菌株中仅存在60%的CcO,并且与WT相比,在超级复合物中发现的CcO较少。WT和突变体的CcO表现出相似的亚基组成,尽管含有Cox2(W56R)的酶的活性比含有Cox2(WT)的酶低20 - 25%。串联质谱证实,在Cox2(W56R)中W(56)被R(56)取代。此外,Cox2(W56R)与Cox2(WT)具有相同的N末端,表明在成熟过程中,Oxa1的MTS和15个残基的前导序列从Cox2(W56R)中被去除。因此,除了点突变W56R外,Cox2(W56R)与Cox2(WT)相同。在Δcox2突变体中,线粒体Cox1的合成强烈减少,但Cox2(W56R)互补菌株导致Cox1合成完全恢复。我们得出结论,胞质溶胶合成的Cox2(W56R)遵循一个限制速率的导入、成熟或组装过程,该过程产生较低的CcO稳态水平。尽管如此,异位表达的Cox2(W56R)恢复了CcO活性,并使线粒体Cox1合成以WT水平进行。

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