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Computer-aided design of a catalyst for Edman degradation utilizing substrate-assisted catalysis

机译:利用底物辅助催化的埃德曼降解催化剂的计算机辅助设计

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摘要

Molecular biology has been revolutionized by the miniaturization and parallelization of DNA sequencing assays previously performed on bulk samples. Many of these technologies rely on biomolecular reagents to facilitate detection, synthesis, or labeling of samples. To aid in the construction of analogous experimental approaches for proteins and peptides, we have used computer-aided design to engineer an enzyme capable of catalyzing the cleavage step of the Edman degradation. We exploit the similarity between the sulfur nucleophile on the Edman reagent and the catalytic cysteine in a naturally occurring protease to adopt a substrate-assisted mechanism for achieving controlled, step-wise removal of N-terminal amino acids. The ability to expose amino acids iteratively at the N-terminus of peptides is a central requirement for protein sequencing techniques that utilize processive degradation of the peptide chain. While this can be easily accomplished using the chemical Edman degradation, achieving this activity enzymatically in aqueous solution removes the requirement for harsh acid catalysis, improving compatibility with low adsorption detection surfaces, such as those used in single molecule assays.
机译:先前对大样本进行的DNA测序分析的小型化和并行化已经彻底改变了分子生物学。这些技术中有许多依靠生物分子试剂来促进样品的检测,合成或标记。为了帮助构建蛋白质和多肽的类似实验方法,我们使用了计算机辅助设计来设计一种能够催化Edman降解的裂解步骤的酶。我们利用埃德曼试剂上的硫亲核试剂与天然存在的蛋白酶中的催化半胱氨酸之间的相似性,采用底物辅助机制来实现N末端氨基酸的受控,逐步去除。在肽的N端反复暴露氨基酸的能力是利用肽链进行性降解的蛋白质测序技术的核心要求。尽管可以使用化学Edman降解轻松实现此目的,但在水溶液中以酶促方式实现此活性消除了对苛刻酸催化的要求,从而提高了与低吸附检测表面(如单分子分析所用表面)的相容性。

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