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甲苯处理的荚膜红假单胞菌及无细胞体系中色素结合蛋白的合成

Synthesis of pigment-binding protein in toluene-treated Rhodopseudomonas capsulata and in cell-free systems.

作者信息

Dierstein R

出版信息

Eur J Biochem. 1984 Feb 1;138(3):509-18. doi: 10.1111/j.1432-1033.1984.tb07945.x.

Abstract

Pigment-binding protein of the facultatively phototrophic bacterium Rhodospeudomonas capsulata could be selectively synthesized in toluene-treated cells as well as in homologous and heterologous cell-free translation systems by isolated polysomes. It is shown that the pigment-binding polypeptides of the light-harvesting complexes are encoded by messenger RNA of extreme longevity. The dependence of their synthesis on the concomitant synthesis of tetrapyrroles was demonstrated in the toluene-treated cells. The large Mr-28 000 polypeptide of the reaction center and the Mr-10 000 pigment-binding polypeptide of the light-harvesting complex II were found to be synthesized by free (water-soluble) polysomes without a cleavable 'leader' or 'signal' peptide [reviewed by W. Wickner (1979) Annu. Rev. Biochem. 48, 23-45]. The Mr-10 000 polypeptide, as synthesized in vitro, was studied in more detail. Unlike the membrane-assembled polypeptide in vivo it was insoluble in an organic solvent mixture (chloroform/methanol 1:1, v/v). After detergent denaturation in the presence of membrane isolated from the organism it became organic-solvent-soluble. Obviously the polypeptide could be induced to assume alternative conformations in which its apolar residues were either exposed to the solvent or buried within. These findings, in agreement with Wickner's hypothesis, indicate that the Mr-10 000 polypeptide may enter the lipid bilayer by a 'membrane-triggered' conformational change.

摘要

兼性光合细菌荚膜红假单胞菌的色素结合蛋白,可通过分离的多核糖体在经甲苯处理的细胞以及同源和异源无细胞翻译系统中选择性合成。结果表明,捕光复合物的色素结合多肽由寿命极长的信使RNA编码。在经甲苯处理的细胞中证实了它们的合成对四吡咯伴随合成的依赖性。发现反应中心的大Mr-28 000多肽和捕光复合物II的Mr-10 000色素结合多肽是由游离(水溶性)多核糖体合成的,没有可裂解的“前导”或“信号”肽[W. Wickner(1979年)《生物化学年度评论》48卷,23 - 45页综述]。对体外合成的Mr-10 000多肽进行了更详细的研究。与体内膜组装的多肽不同,它不溶于有机溶剂混合物(氯仿/甲醇1:1,v/v)。在存在从该生物体分离的膜的情况下经去污剂变性后,它变得可溶于有机溶剂。显然,该多肽可以被诱导呈现不同的构象,其中其非极性残基要么暴露于溶剂中,要么埋藏在内部。这些发现与Wickner的假设一致,表明Mr-10 000多肽可能通过“膜触发”的构象变化进入脂质双层。

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