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细胞色素b6f亚基的膜结合。莱茵衣藻的 Rieske 铁硫蛋白是一种外在蛋白。

Membrane association of cytochrome b6f subunits. The Rieske iron-sulfur protein from Chlamydomonas reinhardtii is an extrinsic protein.

作者信息

Breyton C, de Vitry C, Popot J L

机构信息

Institut de Biologie Physico-Chimique, Centre National de la Recherche Scientifique URA 1187, Paris, France.

出版信息

J Biol Chem. 1994 Mar 11;269(10):7597-602.

PMID:8125983
Abstract

The mode of membrane attachment of five subunits from Chlamydomonas reinhardtii cytochrome b6f complex has been studied using biochemical approaches. Antisera specific for cytochrome f, cytochrome b6, the Rieske iron-sulfur protein, subunit IV, and a 4-kDa subunit (product of the petG gene) were used to quantify the degree of extraction of each of these polypeptides following various treatments. In contrast to the other four subunits, the Rieske protein was extracted to extents varying between 50 and 100% following two cycles of freezing and thawing in the presence of chaotropic agents (KSCN, urea, or NaI). The Rieske protein was not extracted by 2 M NaCl and was rather resistant to alkaline treatments, being extracted by 20 mM 3-(cyclohexylamino)propanesulfonic acid buffer only at pH > 11.5. The hydrodynamic behavior of the isolated Rieske protein was examined in the absence and presence of detergent by ultracentrifugation and by molecular sieving. The extracted protein bound neither to laurylmaltoside nor to C12E8 micelles. Its sedimentation coefficient (D20,w = 9.6 x 10(-11) m2 x s-1), diffusion coefficient (s20,w = 2S), an deduced molecular mass (20.0 +/- 1.7 kDa) are those expected for the monomeric protein. We conclude that the Rieske protein is extrinsic and therefore does not cross the membrane, although its association with the rest of the complex involves primarily hydrophobic interactions, and that the other four subunits analyzed are intrinsic.

摘要

利用生化方法研究了莱茵衣藻细胞色素b6f复合体五个亚基的膜附着模式。针对细胞色素f、细胞色素b6、 Rieske铁硫蛋白、亚基IV和一个4 kDa亚基(petG基因产物)的抗血清被用于量化在各种处理后这些多肽各自的提取程度。与其他四个亚基不同,在存在离液剂(硫氰酸钾、尿素或碘化钠)的情况下经过两轮冻融后,Rieske蛋白的提取率在50%至100%之间变化。Rieske蛋白不被2 M氯化钠提取,并且对碱性处理相当耐受,仅在pH > 11.5时被20 mM 3 -(环己基氨基)丙烷磺酸缓冲液提取。通过超速离心和分子筛法在有无去污剂的情况下检测了分离出的Rieske蛋白的流体动力学行为。提取的蛋白既不与月桂基麦芽糖苷结合,也不与C12E8胶束结合。其沉降系数(D20,w = 9.6 x 10(-11) m2 x s-1)、扩散系数(s20,w = 2S)以及推导的分子量(20.0 +/- 1.7 kDa)是单体蛋白所预期的值。我们得出结论,Rieske蛋白是外在的,因此不穿过膜,尽管它与复合体其他部分的结合主要涉及疏水相互作用,并且所分析的其他四个亚基是内在的。

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