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用于内蛋白酶特异性完整亚位点图谱分析的淬灭荧光底物的部分混合肽库。

Portion-mixing peptide libraries of quenched fluorogenic substrates for complete subsite mapping of endoprotease specificity.

作者信息

Meldal M, Svendsen I, Breddam K, Auzanneau F I

机构信息

Department of Chemistry, Carlsberg Laboratory, Valby-Copenhagen, Denmark.

出版信息

Proc Natl Acad Sci U S A. 1994 Apr 12;91(8):3314-8. doi: 10.1073/pnas.91.8.3314.

Abstract

A solid-phase assay for the complete subsite mapping of the active site of endoproteases has been developed. A library of resin-bound protease substrates was synthesized both on kieselguhr-supported polyamide resin and on a polyethylene glycol-poly-(N,N-dimethylacrylamide) copolymer type of resin that allows proteases to diffuse into the interior and perform their catalytic activity. Anthranilic acid and 3-nitrotyrosine were used as an efficient donor-acceptor pair for the resonance energy transfer. The synthesis was performed in a manual library generator that allows simple wet mixing of the beads and parallel washing procedures. After treatment with subtilisin Carlsberg, fluorescing beads were collected and subjected to peptide sequencing, affording the preferred sequences, their cleavage bond, and a semiquantitative estimation of the turnover. A statistical distribution of preferred amino acids was obtained for each subsite. The result was compared with data from kinetic studies in solution.

摘要

已开发出一种用于对内肽酶活性位点进行完整亚位点图谱绘制的固相分析方法。在硅藻土负载的聚酰胺树脂以及聚乙二醇 - 聚(N,N - 二甲基丙烯酰胺)共聚物类型的树脂上合成了树脂结合的蛋白酶底物文库,这种树脂能使蛋白酶扩散到内部并发挥其催化活性。邻氨基苯甲酸和3 - 硝基酪氨酸被用作共振能量转移的有效供体 - 受体对。合成在手动文库生成器中进行,该生成器允许对珠子进行简单的湿法混合和平行洗涤程序。用枯草杆菌蛋白酶卡尔伯格处理后,收集发出荧光的珠子并进行肽测序,得到优选序列、它们的切割键以及周转率的半定量估计。获得了每个亚位点优选氨基酸的统计分布。将结果与溶液中动力学研究的数据进行了比较。

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Multiple column peptide synthesis, Part 2 (1, 2).多柱肽合成,第2部分(1, 2)。
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