首页> 外文期刊>Journal of Protein Chemistry >Analysis of the disulfide bonding pattern between domain sequences of recombinant prochymosin solubilized from inclusion bodies.
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Analysis of the disulfide bonding pattern between domain sequences of recombinant prochymosin solubilized from inclusion bodies.

机译:从包涵体中溶解的重组凝乳酶原的结构域序列之间的二硫键模式分析。

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摘要

Prochymosin contains three disulfide bonds linking Cys45 to Cys50, Cys206 to Cys210, and Cys250 to Cys283. To analyze the disulfide bonding pattern between domain sequences in the recombinant prochymosin molecule solubilized from inclusion bodies by 8 M urea (designated as solubilized prochymosin), a simple peptide mapping method was established. This process consists of thiol alkylation, cleavage with cyanogen bromide, diagonal electrophoresis on polyacrylamide gel, and N-terminal sequencing. By using this procedure it was found that Cys45 and Cys50 located in the N-terminal domain are not mispaired with the cysteine residues, located in the C-terminal domain, in the solubilized wild-type prochymosin and its mutants. This result implies that Cys45 and Cys50, the partners of a native disulfide, are restricted in some ordered structures existing in inclusion bodies and remaining after solubilization. These native structural elements act as folding nuclei to initiate and facilitate correct refolding. The strategy of preserving the native-like structures including native disulfide in the solubilized inclusion bodies to enhance renaturation efficiency may be applicable to other recombinant proteins.
机译:胰凝乳蛋白酶包含三个将Cys45连接到Cys50,Cys206连接到Cys210和Cys250连接到Cys283的二硫键。为了分析由8 M尿素(称为溶解的胰凝乳蛋白酶)从包涵体中溶解的重组胰凝乳蛋白酶分子中域序列之间的二硫键键合模式,建立了一种简单的肽图分析方法。此过程包括硫醇烷基化,溴化氰裂解,聚丙烯酰胺凝胶上的对角电泳和N端测序。通过使用该程序,发现在溶解的野生型胰凝乳蛋白酶及其突变体中,位于N-末端结构域的Cys45和Cys50未与位于C-末端结构域的半胱氨酸残基错配。该结果暗示天然二硫键的伴侣Cys45和Cys50受包涵体中存在并溶解后保留的某些有序结构的限制。这些天然结构元件充当折叠核,以启动并促进正确的重新折叠。在溶解的包涵体中保留包括天然二硫键在内的天然样结构以提高复性效率的策略可能适用于其他重组蛋白。

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