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叶绿体翻译的膜蛋白在体内的加工。浮萍中快速合成的32000道尔顿防护蛋白及其前体的分析。

Processing of a chloroplast-translated membrane protein in vivo. Analysis of the rapidly synthesized 32 000-dalton shield protein and its precursor in Spirodela oligorrhiza.

作者信息

Reisfeld A, Mattoo A K, Edelman M

出版信息

Eur J Biochem. 1982 May;124(1):125-9. doi: 10.1111/j.1432-1033.1982.tb05914.x.

Abstract

The 32 000-dalton (Da) shield protein regulating electron transport in Spirodela oligorrhiza is an integral chloroplast membrane polypeptide. It is rapidly synthesized, constituting a major chloroplast-translation product in vivo. Following in vitro translation of spirodela chloroplast RNA in a wheat germ system, a 33 500-Da polypeptide is produced. Synthesis of a 33 500-Da protein, associated with the chloroplast membrane, is also seen in vivo, within 2 min of pulse-labeling spirodela with radioactive amino acids. Comparative analyses among these polypeptides reveal: (a) all three are deficient in lysine residues; (b) the two 33 500-Da species have indistinguishable partial proteolytic digestion patterns while that for the 32 000-Da protein differs only slightly from them; (c) radioactivity from the 33 500-Da polypeptide is rapidly chased in vivo into the 32 000-Da protein, even in the presence of protein synthesis inhibitors. These results show the 33 500-Da proteins synthesized in vitro and in vivo to be the precursor form of the 32 000-Da shield protein in spirodela, with processing commencing only after completion of the precursor polypeptide chain and insertion into the membrane.

摘要

在少根紫萍中调节电子传递的32000道尔顿(Da)屏蔽蛋白是一种叶绿体膜整合多肽。它合成迅速,是体内叶绿体翻译的主要产物。在小麦胚芽系统中对少根紫萍叶绿体RNA进行体外翻译后,产生了一种33500道尔顿的多肽。在用放射性氨基酸脉冲标记少根紫萍后2分钟内,在体内也能看到与叶绿体膜相关的33500道尔顿蛋白质的合成。对这些多肽的比较分析表明:(a)这三种多肽都缺乏赖氨酸残基;(b)两种33500道尔顿的多肽具有难以区分的部分蛋白水解消化模式,而32000道尔顿蛋白质的模式与它们只有轻微差异;(c)即使存在蛋白质合成抑制剂,33500道尔顿多肽的放射性在体内也会迅速追踪到32000道尔顿的蛋白质中。这些结果表明,在体外和体内合成的33500道尔顿蛋白质是少根紫萍中32000道尔顿屏蔽蛋白的前体形式,加工仅在完整的前体多肽链合成并插入膜后开始。

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