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[14C]氰酸钾对牛γ-II-晶状体蛋白的氨甲酰化位点。

Site of carbamoylation of bovine gamma-II-crystallin by potassium [14C]cyanate.

作者信息

Martin S, Harding J J

机构信息

Nuffield Laboratory of Ophthalmology, University of Oxford, U.K.

出版信息

Biochem J. 1989 Sep 15;262(3):909-15. doi: 10.1042/bj2620909.

Abstract

One possible route to cataract formation may be via the carbamoylation of lens proteins due to increased concentrations of cyanate in the body resulting from uraemia associated with renal failure and with severe diarrhoea. Carbamoylation of gamma-II-crystallin, which is found in the lens core, could alter the surface charge network of the molecules, resulting in aggregation, increased light-scattering and hence cataract. We have attempted to locate the site(s) of carbamoylation in gamma-II-crystallin. gamma-II-Crystallin was isolated by gel chromatography and ion-exchange chromatography. gamma-II-Crystallin was then carbamoylated by incubation with potassium [14C]cyanate, followed by citraconylation and digestion with trypsin to give peptides that were separated by high-resolution ion-exchange chromatography. The amino acid compositions of the radioactive peptides were compared with the expected peptide composition for gamma-II-crystallin. The radioactive peptide compositions, which agreed with the theoretical peptides, all matched with the N-terminal region of gamma-II-crystallin and had in common the presence of the N-terminal glycine residue. It appears that the alpha-amino group of the N-terminal glycine was the main site of carbamoylation. This site forms part of the charge network on the surface of gamma-II-crystallin.

摘要

白内障形成的一条可能途径可能是由于肾衰竭和严重腹泻相关的尿毒症导致体内氰酸盐浓度增加,从而使晶状体蛋白发生氨甲酰化。晶状体核心中存在的γ-II-晶状体蛋白的氨甲酰化可能会改变分子的表面电荷网络,导致聚集、光散射增加,进而形成白内障。我们试图确定γ-II-晶状体蛋白中氨甲酰化的位点。通过凝胶色谱和离子交换色谱分离出γ-II-晶状体蛋白。然后将γ-II-晶状体蛋白与[14C]氰酸钾一起孵育进行氨甲酰化,接着进行柠康酰化并经胰蛋白酶消化得到肽段,这些肽段通过高分辨率离子交换色谱进行分离。将放射性肽段的氨基酸组成与γ-II-晶状体蛋白预期的肽段组成进行比较。与理论肽段相符的放射性肽段组成均与γ-II-晶状体蛋白的N端区域匹配,并且都共同存在N端甘氨酸残基。看来N端甘氨酸的α-氨基是氨甲酰化的主要位点。该位点构成了γ-II-晶状体蛋白表面电荷网络的一部分。

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本文引用的文献

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Cyanate effects on the lens in vitro.
Invest Ophthalmol. 1973 Jul;12(7):544-7.

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