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ATP合成酶复合体存在缺陷的线粒体突变体的核及线粒体回复突变体。

Nuclear and mitochondrial revertants of a mitochondrial mutant with a defect in the ATP synthetase complex.

作者信息

Hefta L J, Lewin A S, Daignan-Fornier B, Bolotin-Fukuhara M

出版信息

Mol Gen Genet. 1987 Apr;207(1):106-13. doi: 10.1007/BF00331497.

DOI:10.1007/BF00331497
PMID:2885722
Abstract

Yeast strain 990 carries a mutation mapping to the oli1 locus of the mitochondrial genome, the gene encoding ATPase subunit 9. DNA sequence analysis indicated a substitution of valine for alanine at residue 22 of the protein. The strain failed to grow on nonfermentable carbon sources such as glycerol at low temperature (20 degrees C). At 28 degrees C the strain grew on nonfermentable carbon sources and was resistant to the antibiotic oligomycin. ATPase activity in mitochondria isolated from 990 was reduced relative to the wild-type strain from which it was derived, but the residual activity was oligomycin resistant. Subunit 9 (the DCCD-binding proteolipid) from the mutant strain exhibited reduced mobility in SDS-polyacrylamide gels relative to the wild-type proteolipid. Ten revertant strains of 990 were analyzed. All restored the ability to grow on glycerol at 20 degrees C. Mitotic segregation data showed that eight of the ten revertants were attributable to mitochondrial genetic events and two were caused by nuclear events since they appeared to be recessive nuclear suppressors. These nuclear mutations retained partial resistance to oligomycin and did not alter the electrophoretic behavior of subunit 9 or any other ATPase subunit. When mitochondrial DNA from each of the revertant strains was hybridized with an oligonucleotide probe covering the oli1 mutation, seven of the mitochondrial revertants were found to be true revertants and one a second mutation at the site of the original 990 mutation. The oli1 gene from this strain contained a substitution of glycine for valine at residue 22. The proteolipid isolated from this strain had increased electrophoretic mobility relative to the wild-type proteolipid.

摘要

酵母菌株990携带一个定位在线粒体基因组oli1位点的突变,该基因编码ATP酶亚基9。DNA序列分析表明,该蛋白质第22位残基处的丙氨酸被缬氨酸取代。该菌株在低温(20摄氏度)下不能在甘油等非发酵碳源上生长。在28摄氏度时,该菌株能在非发酵碳源上生长,并且对抗生素寡霉素具有抗性。从990分离的线粒体中的ATP酶活性相对于其来源的野生型菌株有所降低,但残余活性对寡霉素具有抗性。与野生型蛋白脂质相比,突变菌株的亚基9(DCCD结合蛋白脂质)在SDS-聚丙烯酰胺凝胶中的迁移率降低。对990的10个回复菌株进行了分析。所有菌株都恢复了在20摄氏度下在甘油上生长的能力。有丝分裂分离数据表明,10个回复菌株中的8个归因于线粒体遗传事件,2个是由核事件引起的,因为它们似乎是隐性核抑制子。这些核突变保留了对寡霉素的部分抗性,并且没有改变亚基9或任何其他ATP酶亚基的电泳行为。当每个回复菌株的线粒体DNA与覆盖oli1突变的寡核苷酸探针杂交时,发现7个线粒体回复菌株是真正的回复菌株,1个是在原始990突变位点的第二次突变。该菌株的oli1基因在第22位残基处的缬氨酸被甘氨酸取代。从该菌株分离的蛋白脂质相对于野生型蛋白脂质具有增加的电泳迁移率。

相似文献

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Nuclear and mitochondrial revertants of a mitochondrial mutant with a defect in the ATP synthetase complex.ATP合成酶复合体存在缺陷的线粒体突变体的核及线粒体回复突变体。
Mol Gen Genet. 1987 Apr;207(1):106-13. doi: 10.1007/BF00331497.
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Amino acid substitutions in subunit 9 of the mitochondrial ATPase complex of Saccharomyces cerevisiae. Sequence analysis of a series of revertants of an oli1 mit- mutant carrying an amino acid substitution in the hydrophilic loop of subunit 9.酿酒酵母线粒体ATP酶复合体亚基9中的氨基酸替换。对oli1 mit-突变体一系列回复突变体的序列分析,该突变体在亚基9的亲水环中存在氨基酸替换。
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Amino acid substitutions in mitochondrial ATPase subunit 9 of Saccharomyces cerevisiae leading to oligomycin or venturicidin resistance.酿酒酵母线粒体ATP酶9亚基中的氨基酸替换导致对寡霉素或抗霉素A耐药。
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DNA sequence analysis of the oli1 gene reveals amino acid changes in mitochondrial ATPase subunit 9 from oligomycin-resistant mutants of Saccharomyces cerevisiae.对oli1基因的DNA序列分析揭示了酿酒酵母寡霉素抗性突变体线粒体ATP酶亚基9中的氨基酸变化。
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Biogenesis of mitochondria: DNA sequence analysis of mit- mutations in the mitochondrial oli1 gene coding for mitochondrial ATPase subunit 9 in Saccharomyces cerevisiae.线粒体的生物发生:酿酒酵母中编码线粒体ATP酶亚基9的线粒体oli1基因突变的DNA序列分析。
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Biogenesis of mitochondria: a mutation in the 5'-untranslated region of yeast mitochondrial oli1 mRNA leading to impairment in translation of subunit 9 of the mitochondrial ATPase complex.线粒体的生物发生:酵母线粒体oli1 mRNA 5'非翻译区的突变导致线粒体ATP酶复合体亚基9翻译受损。
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引用本文的文献

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RNA. 2000 Jul;6(7):937-51. doi: 10.1017/s1355838200991726.
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PET genes of Saccharomyces cerevisiae.酿酒酵母的PET基因。
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