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利用结构同源蛋白支架对聚酮合成酶样酶进行合理设计。

Rational design of a scytalone dehydratase-like enzyme using a structurally homologous protein scaffold.

作者信息

Nixon A E, Firestine S M, Salinas F G, Benkovic S J

机构信息

152 Davey Laboratory, Department of Chemistry, Pennsylvania State University, University Park, PA 16802-6300, USA.

出版信息

Proc Natl Acad Sci U S A. 1999 Mar 30;96(7):3568-71. doi: 10.1073/pnas.96.7.3568.

Abstract

The generation of enzymes to catalyze specific reactions is one of the more challenging problems facing protein engineers. Structural similarities between the enzyme scytalone dehydratase with nuclear transport factor 2 (NTF2) suggested the potential for NTF2 to be re-engineered into a scytalone dehydratase-like enzyme. We introduced four key catalytic residues into NTF2 to create a scytalone dehydratase-like active site. A C-terminal helix found in scytalone dehydratase but absent in NTF2 also was added. Mutant NTF2 proteins were tested for catalytic activity by using a spectroscopic assay. One of the engineered enzymes exhibited catalytic activity with minimal kcat and Km values of 0.125 min-1 and 800 microM, respectively. This level of catalytic activity represents minimally a 150-fold improvement in activity over the background rate for substrate dehydration and a dramatic step forward from the catalytically inert parent NTF2. This work represents one of the few examples of converting a protein scaffold into an enzyme, outside those arising from the induction of catalytic activity into antibodies.

摘要

生成能够催化特定反应的酶是蛋白质工程师面临的更具挑战性的问题之一。酶促黑素脱水酶与核转运因子2(NTF2)之间的结构相似性表明,NTF2有可能被重新设计成一种类似促黑素脱水酶的酶。我们将四个关键催化残基引入NTF2,以创建一个类似促黑素脱水酶的活性位点。还添加了一个在促黑素脱水酶中发现但在NTF2中不存在的C端螺旋。通过光谱分析测试突变型NTF2蛋白的催化活性。其中一种工程酶表现出催化活性,其最小催化常数(kcat)和米氏常数(Km)分别为0.125 min-1和800 microM。这种催化活性水平相对于底物脱水的背景速率而言,活性至少提高了150倍,并且相对于无催化活性的亲本NTF2而言向前迈出了巨大的一步。这项工作代表了将蛋白质支架转化为酶的少数例子之一,这不同于通过诱导抗体产生催化活性而产生的例子。

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