影响酵母线粒体I族内含子bi2剪接和/或归巢活性的关键碱基取代。

T Szczepanek, K Jamoussi, J Lazowska
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引用次数: 16

摘要

来自相关酵母菌种的cyt b基因的第二个内含子(bi2)具有非常保守的序列,并且在野生型细胞中可以具有不同的功能。酿酒葡萄球菌内含子编码的蛋白质作为成熟酶促进内含子剪接,而同源的capensis内含子编码一种双功能蛋白,既作为成熟酶又作为归巢内切酶(I-ScaI)促进内含子移动。内含子bi2编码的蛋白属于一个大的基因家族,其特征是存在两个保守的LAGLIDADG基序(P1和P2)。在这项研究中,我们分析了酿酒葡萄球菌内含子bi2的一组剪接缺陷突变体,这些突变体携带影响成熟酶活性的非定向突变,以及一组引入由酿酒葡萄球菌内含子编码的双功能蛋白的定向错义突变。对这些突变的分析可以鉴定出保守的P1和P2基序中的残基,这些基序对剪接和归巢活性至关重要。此外,已经发现位于蛋白质c端部分的几个突变会影响这两种功能。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Critical base substitutions that affect the splicing and/or homing activities of the group I intron bi2 of yeast mitochondria.

The second intron (bi2) of the cyt b gene from related Saccharomyces species has an extraordinarily conserved sequence and can have different functions in wild-type cells. The protein encoded by the S. cerevisiae intron functions as a maturase to promote intron splicing, while the homologous S. capensis intron encodes a bifunctional protein that acts both as a maturase and as a homing endonuclease (I-ScaI) promoting intron mobility. The protein encoded by intron bi2 belongs to a large gene family characterized by the presence of two conserved LAGLIDADG motifs (P1 and P2). In this study, we analysed a set of splicing-deficient mutants of the S. cerevisiae intron bi2 that carry non-directed mutations affecting the maturase activity, and a set of directed missense mutations introduced into the bifunctional protein encoded by the S. capensis intron. Analysis of these mutations has allowed identification of the residues in the conserved P1 and P2 motifs which are crucial for splicing and homing activities. Moreover, several mutations which are located in the C-terminal part of the protein have been found to affect both functions.

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