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通过离子阱LCQ电喷雾电离质谱法评估人胰岛素原中的糖化位点。

Evaluation of the site(s) of glycation in human proinsulin by ion-trap LCQ electrospray ionization mass spectrometry.

作者信息

McKillop Aine M, Meade Angela, Flatt Peter R, O'Harte Finbarr P M

机构信息

School of Biomedical Sciences, University of Ulster, Northern Ireland BT52 1SA, Coleraine, UK.

出版信息

Regul Pept. 2003 May 15;113(1-3):1-8. doi: 10.1016/s0167-0115(02)00292-6.

DOI:10.1016/s0167-0115(02)00292-6
PMID:12686455
Abstract

The glycation of beta cell proteins is known to occur under hyperglycemic states. The site(s) of glycation in human proinsulin was investigated following exposure to a hyperglycemic environment under reducing conditions in vitro. Proinsulin and glycated proinsulin were separated by reversed-phase high-performance liquid chromatography (RP-HPLC) and identified using LCQ ion-trap electrospray ionization mass spectrometry. This revealed a major peak (>70% total) of monoglycated proinsulin (M(r) 9552.2 Da), a second peak (approximately 27%) of nonglycated proinsulin (M(r) 9389.8 Da), and a third minor peptide peak (approximately 3%) corresponding to diglycated proinsulin (M(r) 9717.9 Da). Following reduction of disulphide bridges with dithiothreitol, intact peptides were incubated with endoproteinase Glu-C to release nine daughter fragments for LC-MS analysis. This strategy revealed an N-terminal fragment of monoglycated proinsulin Phe(1)-Glu(13), which contained a single glucitol adduct (M(r) 1642.0 Da). A similar treatment of small amounts of purified diglycated proinsulin revealed a fragment with Phe(1)-Glu(13) linked by a disulphide bridge to Gln(70)-Glu(82) containing two glucitol adducts (M(r) 3292.7 Da). In summary, these studies indicate that the major site of glycation in proinsulin, like insulin, is the amino terminal Phe(1) residue. However, small amounts of diglycated proinsulin occur naturally, involving an additional site of glycation located between Gln(70) and Glu(82).

摘要

已知在高血糖状态下β细胞蛋白会发生糖基化。在体外还原条件下,将人胰岛素原暴露于高血糖环境后,对其糖基化位点进行了研究。通过反相高效液相色谱(RP-HPLC)分离胰岛素原和糖化胰岛素原,并使用LCQ离子阱电喷雾电离质谱进行鉴定。结果显示,单糖化胰岛素原(M(r) 9552.2 Da)有一个主峰(占总量的>70%),非糖化胰岛素原(M(r) 9389.8 Da)有第二个峰(约27%),以及对应双糖化胰岛素原(M(r) 9717.9 Da)的第三个小肽峰(约3%)。用二硫苏糖醇还原二硫键后,完整的肽段与内肽酶Glu-C孵育,释放出九个子代片段用于LC-MS分析。该策略揭示了单糖化胰岛素原Phe(1)-Glu(13)的N端片段,其含有一个单一的葡糖醇加合物(M(r) 1642.0 Da)。对少量纯化的双糖化胰岛素原进行类似处理,发现一个片段,其中Phe(1)-Glu(13)通过二硫键与含有两个葡糖醇加合物的Gln(70)-Glu(82)相连(M(r) 3292.7 Da)。总之,这些研究表明,胰岛素原中的主要糖基化位点与胰岛素一样,是氨基末端的Phe(1)残基。然而,少量的双糖化胰岛素原自然存在,涉及位于Gln(70)和Glu(82)之间的另一个糖基化位点。

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Rapid Non-Enzymatic Glycation of the Insulin Receptor under Hyperglycemic Conditions Inhibits Insulin Binding In Vitro: Implications for Insulin Resistance.高血糖条件下胰岛素受体的快速非酶糖基化抑制胰岛素结合体外:对胰岛素抵抗的影响。
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An insulin-like modular basis for the evolution of glucose transporters (GLUT) with implications for diabetes.胰岛素样模块基础是葡萄糖转运蛋白(GLUT)进化的基础,对糖尿病具有重要意义。
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