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oxi2 突变体的重组分析及其在酿酒酵母中的翻译产物的初步分析。

Recombinational analysis of oxi2 mutants and preliminary analysis of their translation products in S. cerevisiae.

机构信息

Institute of Biochemistry and Biophysics, Polish Academy of Sciences, 36 Rakowiecka Street, 02-532, Warsaw, Poland.

出版信息

Curr Genet. 1983 Jun;7(3):225-33. doi: 10.1007/BF00434894.

Abstract

Genetic and biochemical studies were performed with mutants allocated to the mitochondrial oxi2 gene.Recombinational analysis of 19 oxi2 mutants was performed using α and a mutant strains derived from the same genetic background. The frequencies of wild-type recombinants in oxi2 (-) × oxi2 (-) crosses varied from 0.002 to 17%. The map of oxi2 mutations constructed on the basis of these frequencies shows many internal inconsistencies. In the course of rho (-) deletion mapping five classes of oxi2 mutations were distinguished. The results of deletion analysis are in agreement with those of recombinational mapping.The analysis of mitochondrial translation products by SDS-polyacrylamide electrophoresis of 20 oxi2 mutants shows that 17 of them are connected with conspicuous changes of 22 kd polypeptide band corresponding to subunit III of cytochrome oxidase. At least four of them carried instead of subunit III clearly visible significantly shorter polypeptides (12.8 to 20.1 kd). These were, most likely, shorter fragments of subunit III resulting from chain termination mutations. Colinearity was observed between the lenght of new polypeptides and the positions of the respective mutations on the recombinational map. These data confirm hat oxi2 encodes subunit III of cytochrome oxidase and suggest that translation of the oxi2 gene is in the direction from V303 to V273.

摘要

进行了遗传和生化研究,涉及分配给线粒体 oxi2 基因的突变体。使用来自相同遗传背景的α和 a 突变体菌株对 19 个 oxi2 突变体进行了重组分析。在 oxi2(-)×oxi2(-)杂交中,野生型重组体的频率从 0.002 到 17%不等。基于这些频率构建的 oxi2 突变图谱显示出许多内部不一致。在 rho(-)缺失作图过程中,区分了五类 oxi2 突变。缺失分析的结果与重组作图的结果一致。对 20 个 oxi2 突变体的线粒体翻译产物进行 SDS-聚丙烯酰胺电泳分析表明,其中 17 个与细胞色素氧化酶亚基 III 对应的 22 kd 多肽带的明显变化有关。其中至少有四个取代了亚基 III,明显可见明显较短的多肽(12.8 至 20.1 kd)。这些很可能是由于链终止突变导致的亚基 III 的较短片段。在新多肽的长度和重组图谱上各自突变的位置之间观察到了线性关系。这些数据证实 oxi2 编码细胞色素氧化酶的亚基 III,并表明 oxi2 基因的翻译方向是从 V303 到 V273。

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