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采用高效液相色谱法对人血清白蛋白及其他糖基化蛋白中与蛋白质(赖氨酸)结合的葡萄糖进行特异性定量分析。

Specific quantitation by HPLC of protein (lysine) bound glucose in human serum albumin and other glycosylated proteins.

作者信息

Schleicher E, Wieland O H

出版信息

J Clin Chem Clin Biochem. 1981 Feb;19(2):81-7. doi: 10.1515/cclm.1981.19.2.81.

Abstract

A specific and sensitive method for quantification of the fructose-lysine linkages present in non-enzymatically glycosylated albumin and other proteins is described. Protein is hydrolyzed for 18 h in 6 mol/l HCl at 95 degrees C to yield furosine (epsilon-N-(2-furoylmethyl)-L-lysine) known as a specific degradation product of fructose-lysine. Furosine is then separated on HPLC and quantified by its UV-absorbance against a prepared fructose-lysine standard. The method has been successfully used for the determination of glycosyl-albumin in diabetic patients starting from 100 microliter serum or less, as well as for various other proteins. Unlike the usually employed thiobarbituric acid assay the present procedure is truly specific for the detection of ketoamine linkages of glycosylated proteins.

摘要

本文描述了一种用于定量非酶糖基化白蛋白和其他蛋白质中果糖 - 赖氨酸键的特异性灵敏方法。蛋白质在95℃下于6mol/L盐酸中水解18小时,生成糠氨酸(ε - N -(2 - 糠酰甲基)-L - 赖氨酸),它是果糖 - 赖氨酸的一种特异性降解产物。然后通过高效液相色谱法分离糠氨酸,并根据其对制备的果糖 - 赖氨酸标准品的紫外吸光度进行定量。该方法已成功用于从100微升或更少血清中测定糖尿病患者的糖基化白蛋白,以及各种其他蛋白质。与通常采用的硫代巴比妥酸测定法不同,本方法对于检测糖基化蛋白质的酮胺键具有真正的特异性。

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