Vibratory reaction unit for the rapid analysis of proteins and glycochains.

Analytical Chemistry Insights Pub Date : 2007-09-17

Yukie Sasakura, Makoto Nogami, Noriko Kobayashi, Katsuhiro Kanda

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Abstract

A protein digestion system using immobilized enzymes for protein identification and glycochain analyses has been developed, and a vibration reaction unit for micro-scale sample convection on an enzyme-immobilized solid surface was constructed. BSA as a model substrate was digested by this unit, and was successfully identified by mass spectrometry (MS) analyses. Compared to the conventional liquid-phase digestion, the reaction unit increased the number of matched peptides from 9 to 26, protein score from 455 to 1247, and sequence coverage from 21% to 48%. Glycopeptidase F (NGF), an enzyme that cleaves N-glycans from glycoproteins, was also immobilized and used to remove the glycochains from human immunoglobulin G (IgG). Trypsin and NGF were immobilized on the same solid surface and used to remove glycochains from IgG in single-step. Glycochains were labeled with fluorescent reagent and analyzed by HPLC. Several peaks corresponding to the glycochains of IgG were detected. These results suggested that the single-step digestion system, by immobilized multiple enzymes (trypsin and NGF) would be effective for the rapid structural analysis of glycoproteins.

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用于快速分析蛋白质和糖链的振动反应单元。

建立了用于蛋白质鉴定和糖链分析的固定化酶蛋白质消化系统，并构建了用于微尺度样品在固定化酶固体表面对流的振动反应单元。BSA作为模型底物被该装置消化，并通过质谱(MS)分析成功鉴定。与传统液相消化相比，该反应单元将匹配肽数从9增加到26，蛋白质评分从455增加到1247，序列覆盖率从21%增加到48%。糖肽酶F (NGF)是一种从糖蛋白中切割n -聚糖的酶，也被固定化并用于从人免疫球蛋白G (IgG)中去除糖链。将胰蛋白酶和NGF固定在同一固体表面，用于一步去除IgG的糖链。用荧光试剂标记糖链，HPLC分析。检测到多个与IgG糖链对应的峰。这些结果表明，固定化多种酶(胰蛋白酶和NGF)的单步消化系统是快速分析糖蛋白结构的有效方法。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Analytical Chemistry Insights

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