固定化蛋白酶水解后蛋白质的组成分析。

Journal of applied biochemistry Pub Date : 1984-08-01
F C Church, H E Swaisgood, G L Catignani
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引用次数: 0

摘要

将蛋白酶K、羧肽酶A和B、氨基肽酶M、肠粘膜外肽酶和脯氨酸酶固定在衍生化的多孔玻璃微珠上,研究了蛋白质的总酶水解。结合使用固定化酶和酸水解来评估蛋白质质量,将比单独使用酸水解提供更准确的化学评分。天然蛋白底物(β -乳球蛋白和胰岛素)的酶水解产物的氨基酸分析产生了92%的理论值和103%的标准酸水解物观察值。这些结果表明,与传统的酸水解方法相比,使用固定化蛋白酶的组合可以在18-24小时内基本实现蛋白质底物的全水解。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Compositional analysis of proteins following hydrolysis by immobilized proteases.

Pronase, proteinase K, carboxypeptidases A and B, aminopeptidase M, intestinal mucosa exopeptidases and prolidase, immobilized to derivatized controlled-pore glass beads, were used in a study of total enzymic hydrolysis of proteins. The combined use of immobilized enzymatic and acid hydrolysis, for assessment of protein quality, will give a more accurate chemical score than that afforded by acid hydrolysis alone. Amino acid analysis of enzymic hydrolysates of native protein substrates (beta-lactoglobulin and insulin) yielded 92% of the theoretical values and 103% of the values observed for standard acid hydrolysates. These results suggest that using a combination of immobilized proteases in concert gives essentially total hydrolysis of protein substrates in a time period (18-24 h) comparable to conventional acid hydrolysis methods.

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