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首页> 外文期刊>ACS Omega >Investigating the Deoxyribonuclease Activity of CRM197 with Site-Directed Mutagenesis
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Investigating the Deoxyribonuclease Activity of CRM197 with Site-Directed Mutagenesis

机译:用定点诱变研究CRM197的脱氧核糖核酸酶活性

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The protein cross-reactive material 197 (CRM197) is known to catalyze the hydrolytic cleavage of DNA (DNase activity). A suspected metal-binding site (S109, T111, and E112) and suspected DNA-binding motif (T89, K90, and V91) were predicted within the CRM197 protein X-ray crystal structure (4AE0) using METSITE and DNABindProt, respectively. Between these two predicted sites is a groove (K103, E116, T120, E122, F123, and R126) that may assist in DNase activity. Alanine scanning was performed at these sites to determine which amino acids might be important for DNase activity. These mutations individually or in combination either maintained or increased the overall DNase activity compared to the unmodified CRM197. Mutation at the suspected metal-binding site showed similar fluctuations to the overall DNase activity whether the DNase assays were run with Mg2+ and Ca2+ or Mn2+. However, many of the mutations within the suspected DNA-binding motif saw significant differences depending on which metal was used. Only some of the improvements in DNase activity could be attributed to improved folding of the mutants compared to the unmodified CRM197. This study should provide a basis for further mutagenesis studies to remove the DNase activity of CRM197.
机译:已知蛋白交叉反应材料197(CRM197)催化DNA的水解切割(DNase活性)。分别使用METSITE和DNABindProt在CRM197蛋白X射线晶体结构(4AE0)中预测了可疑的金属结合位点(S109,T111和E112)和可疑的DNA结合基序(T89,K90和V91)。在这两个预测的位点之间是一个凹槽(K103,E116,T120,E122,F123和R126),可有助于DNase的活性。在这些位点进行了丙氨酸扫描,以确定哪些氨基酸可能对DNase活性很重要。与未修饰的CRM197相比,这些突变单独或组合保持或增加了总DNA酶活性。无论使用Mg2 +和Ca2 +或Mn2 +进行DNase分析,在可疑金属结合位点的突变都显示出与总DNase活性相似的波动。但是,根据所使用的金属,可疑的DNA结合基序中的许多突变都存在显着差异。与未修饰的CRM197相比,DNase活性的某些改善只能归因于突变体折叠的改善。该研究应为进一步诱变研究以去除CRM197的DNase活性提供基础。

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