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通过随机序列诱变确定的单纯疱疹病毒1型编码胸苷激酶假定核苷结合位点内允许的氨基酸替代[已修正]

Permissible amino acid substitutions within the putative nucleoside binding site of herpes simplex virus type 1 encoded thymidine kinase established by random sequence mutagenesis [corrected].

作者信息

Munir K M, French D C, Dube D K, Loeb L A

机构信息

Joseph Gottstein Memorial Cancer Research Laboratory, Department of Pathology, University of Washington, Seattle 98195.

出版信息

J Biol Chem. 1992 Apr 5;267(10):6584-9.

PMID:1313013
Abstract

We determined the essentiality of all amino acid replacements within an 11-codon sequence in the putative nucleoside-binding site of thymidine kinase encoded by herpes simplex virus type 1. This involved partial randomization of 11 codons in the gene to create a degenerate library, followed by genetic complementation using a tk- Escherichia coli strain and selection of unnatural active enzymes. We produced and tested 53,000 variants; of which 190 were found to be biologically active. Sequence analyses of functional variants revealed a high degree of flexibility in accommodating different types of amino acid substitutions in this region. However, no replacement was tolerated at proline-173, whereas tyrosine-172 could be replaced by only phenylalanine. To further define permissible substitutions at specified positions, we constructed a library with randomization at only four test codons. We produced and tested 600,000 variants; of which only 5 were active. Again proline-173 was conserved, and only tyrosine and phenylalanine were found at position 172. The identification of these conserved amino acids should provide important insights into the understanding of the structural basis of catalysis by this enzyme.

摘要

我们确定了单纯疱疹病毒1型编码的胸苷激酶假定核苷结合位点中11个密码子序列内所有氨基酸替换的必要性。这涉及对该基因中的11个密码子进行部分随机化以创建一个简并文库,随后使用tk-大肠杆菌菌株进行遗传互补并筛选非天然活性酶。我们产生并测试了53000个变体,其中190个被发现具有生物活性。对功能变体的序列分析表明,该区域在容纳不同类型氨基酸替换方面具有高度灵活性。然而,脯氨酸-173处不允许有任何替换,而酪氨酸-172只能被苯丙氨酸取代。为了进一步确定特定位置允许的替换,我们构建了一个仅在四个测试密码子处随机化的文库。我们产生并测试了600000个变体,其中只有5个具有活性。脯氨酸-173再次保守,并且在172位仅发现酪氨酸和苯丙氨酸。这些保守氨基酸的鉴定应为理解该酶催化的结构基础提供重要见解。

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