首页> 美国卫生研究院文献>The Journal of Biological Chemistry >Cox25 Teams Up with Mss51 Ssc1 and Cox14 to Regulate Mitochondrial Cytochrome c Oxidase Subunit 1 Expression and Assembly in Saccharomyces cerevisiae
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Cox25 Teams Up with Mss51 Ssc1 and Cox14 to Regulate Mitochondrial Cytochrome c Oxidase Subunit 1 Expression and Assembly in Saccharomyces cerevisiae

机译:Cox25与Mss51Ssc1和Cox14合作调节酿酒酵母中的线粒体细胞色素c氧化酶亚基1的表达和装配。

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摘要

In the yeast Saccharomyces cerevisiae, mitochondrial cytochrome c oxidase (COX) biogenesis is translationally regulated. Mss51, a specific COX1 mRNA translational activator and Cox1 chaperone, drives the regulatory mechanism. During translation and post-translationally, newly synthesized Cox1 physically interacts with a complex of proteins involving Ssc1, Mss51, and Cox14, which eventually hand over Cox1 to the assembly pathway. This step is probably catalyzed by assembly chaperones such as Shy1 in a process coupled to the release of Ssc1-Mss51 from the complex. Impaired COX assembly results in the trapping of Mss51 in the complex, thus limiting its availability for COX1 mRNA translation. An exception is a null mutation in COX14 that does not affect Cox1 synthesis because the Mss51 trapping complexes become unstable, and Mss51 is readily available for translation. Here we present evidence showing that Cox25 is a new essential COX assembly factor that plays some roles similar to Cox14. A null mutation in COX25 by itself or in combination with other COX mutations does not affect Cox1 synthesis. Cox25 is an inner mitochondrial membrane intrinsic protein with a hydrophilic C terminus protruding into the matrix. Cox25 is an essential component of the complexes containing newly synthesized Cox1, Ssc1, Mss51, and Cox14. In addition, Cox25 is also found to interact with Shy1 and Cox5 in a complex that does not contain Mss51. These results suggest that once Ssc1-Mss51 are released from the Cox1 stabilization complex, Cox25 continues to interact with Cox14 and Cox1 to facilitate the formation of multisubunit COX assembly intermediates.
机译:在酵母酿酒酵母中,线粒体细胞色素C氧化酶(COX)的生物发生受到翻译调控。 Mss51,一种特定的COX1 mRNA翻译激活剂和Cox1伴侣,驱动调节机制。在翻译和翻译后过程中,新合成的Cox1与涉及Ssc1,Mss51和Cox14的蛋白质复合物发生物理相互作用,最终将Cox1移交给装配路径。此步骤可能由装配伴侣(例如Shy1)催化,该过程与从复合物中释放Ssc1-Mss51耦合。受损的COX装配导致复合物中Mss51的捕获,从而限制了它可用于COX1 mRNA翻译。一个例外是COX14中的无效突变,它不影响Cox1的合成,因为Mss51捕获复合物变得不稳定,并且Mss51易于翻译。在这里,我们提供的证据表明Cox25是一种新型的重要COX组装因子,其发挥的作用类似于Cox14。 COX25本身的无效突变或与其他COX突变组合的突变不会影响Cox1的合成。 Cox25是内部线粒体膜固有蛋白,具有亲水性C末端突出到基质中。 Cox25是包含新合成的Cox1,Ssc1,Mss51和Cox14的复合物的重要组成部分。此外,还发现Cox25在不包含Mss51的复合物中与Shy1和Cox5相互作用。这些结果表明,一旦从Cox1稳定复合物中释放Ssc1-Mss51,Cox25就会继续与Cox14和Cox1相互作用,以促进多亚基COX组装中间体的形成。

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