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鉴定视蛋白中被光活化的叠氮基[¹²⁵I]碘苯修饰的位点。

Identification of the sites in opsin modified by photoactivated azido[125I]iodobenzene.

作者信息

Davison M D, Findlay J B

出版信息

Biochem J. 1986 Jun 1;236(2):389-95. doi: 10.1042/bj2360389.

Abstract

Opsin labelled with photoactivated 1-azido-4-[125I]iodobenzene was proteolysed in situ with Staphylococcus aureus V8 proteinase to yield two radioactive membrane-bound fragments. These were separated, cleaved with CNBr and the resultant peptides sequenced in order to locate the radiolabelled residues. In the whole molecule, there was clear evidence for modification of at least 20 sites, identified as derivatives of cysteine, tryptophan, tyrosine, histidine and lysine residues. The probe primary reacted, therefore, with nucleophilic substituents. The positions of the modified sites relative to the confines of the phospholipid bilayer were consistent with all other studies on the disposition of the polypeptide chain. The location of these sites substantiated an earlier suggestion that not all the transmembrane segments should be regarded as continuous regular alpha-helices.

摘要

用光活化的1-叠氮基-4-[¹²⁵I]碘苯标记的视蛋白在原位用金黄色葡萄球菌V8蛋白酶进行蛋白水解,产生两个放射性膜结合片段。将这些片段分离,用溴化氰裂解,然后对所得肽段进行测序,以定位放射性标记的残基。在整个分子中,有明确证据表明至少有20个位点发生了修饰,这些位点被鉴定为半胱氨酸、色氨酸、酪氨酸、组氨酸和赖氨酸残基的衍生物。因此,该探针主要与亲核取代基发生反应。修饰位点相对于磷脂双层边界的位置与关于多肽链排列的所有其他研究一致。这些位点的定位证实了早期的一个观点,即并非所有跨膜片段都应被视为连续规则的α螺旋。

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