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马铃薯细胞色素c还原酶14千道尔顿亚基的分子特征及线粒体导入途径

Molecular features and mitochondrial import pathway of the 14-kilodalton subunit of cytochrome c reductase from potato.

作者信息

Braun H P, Schmitz U K

机构信息

Institut für Genbiologische Forschung GmbH, Berlin, Germany.

出版信息

Plant Physiol. 1995 Apr;107(4):1217-23. doi: 10.1104/pp.107.4.1217.

Abstract

The cytochrome c reductase complexes from fungi and mammals both contain a 14-kD protein (yeast, 14.4 kD; bovine, 13.4 kD) that does not directly participate in electron transfer but possibly is indirectly involved in the function of the complex and has a role in assembly of the multimeric enzyme. A subunit of comparable size was identified for the bc1 complex of higher plants. The 14-kD protein from potato (Solanum tuberosum) was specifically separated from the isolated protein complex in the presence of 6 M urea and is, therefore, assumed to be a peripheral component. Direct sequence analysis of the proteins from potato and wheat (Triticum aestivum) and isolation of corresponding cDNA clones for the subunit from potato revealed clear similarity to the equivalent proteins from yeast and bovine. The wheat 14-kD protein seems to occur in two isoforms. The 14-kD protein from plants is very hydrophilic, has a characteristic charge distribution, and contains no potential membrane-spanning helices. In vitro import of the radiolabeled 14-kD protein from potato into isolated mitochondria depends on the membrane potential across the inner mitochondrial membrane. The protein seems to lack a cleavable mitochondrial presequence, because it is not processed upon translocation. Possible intramolecular regions involved in targeting of the 14-kD protein to plant mitochondria are discussed.

摘要

来自真菌和哺乳动物的细胞色素c还原酶复合物都含有一种14-kD蛋白(酵母为14.4 kD;牛为13.4 kD),该蛋白不直接参与电子传递,但可能间接参与复合物的功能,并在多聚体酶的组装中发挥作用。已鉴定出高等植物bc1复合物中存在大小相当的亚基。在6 M尿素存在的情况下,从马铃薯(Solanum tuberosum)中分离出了14-kD蛋白,并将其与分离出的蛋白复合物特异性分开,因此被认为是一种外周成分。对马铃薯和小麦(Triticum aestivum)中的蛋白进行直接序列分析,并分离出马铃薯该亚基的相应cDNA克隆,结果显示与酵母和牛中的等效蛋白有明显的相似性。小麦的14-kD蛋白似乎有两种同工型。植物中的14-kD蛋白非常亲水,具有独特的电荷分布,且不包含潜在的跨膜螺旋。将放射性标记的马铃薯14-kD蛋白体外导入分离的线粒体取决于线粒体内膜两侧的膜电位。该蛋白似乎缺乏可裂解的线粒体前导序列,因为它在转运时不会被加工。文中讨论了14-kD蛋白靶向植物线粒体可能涉及的分子内区域。

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