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Molecular cloning and characterization of protein disulfide isomerase of Brugia malayi a human lymphatic filarial parasite

机译:人淋巴丝虫疟原虫马来亚蛋白的二硫键异构酶的分子克隆与表征

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摘要

Lymphatic filariasis results in an altered lymphatic system and the abnormal enlargement of body parts, causing pain, serious disability and social stigma. Effective vaccines are still not available nowadays, drugs against the disease is required. Protein disulfide isomerase (PDI) is an essential catalyst of the endoplasmic reticulum which is involved in folding and chaperone activities in different biological systems. Here, we report the enzymatic characterization of a Brugia malayi Protein disulfide isomerase (BmPDI), which was expressed and purified from Escherichia coli BL21 (DE3). Western blotting analysis showed the recombinant BmPDI could be recognized by anti-BmPDI Rabbit serum. The rBmPDI exhibited an optimum activity at pH 8 and 40 °C. The enzyme was inhibited by aurin and PDI inhibitor. Recombinant BmPDI showed interaction with recombinant Brugia malayi calreticulin (rBmCRT). The three-dimensional model for BmPDI and BmCRT was generated by homology modelling. A total of 25 hydrogen bonds were found to be formed between two interfaces. There are 259 non-bonded contacts present in the BmPDI-BmCRT complex and 12 salt bridges were formed in the interaction.
机译:淋巴丝虫病导致淋巴系统改变,身体部位异常增大,引起疼痛,严重的残疾和社会污名。如今仍无法获得有效的疫苗,需要针对这种疾病的药物。蛋白质二硫键异构酶(PDI)是内质网的重要催化剂,内质网参与不同生物系统中的折叠和分子伴侣活性。在这里,我们报告了马来布鲁氏菌蛋白二硫键异构酶(BmPDI)的酶促表征,该酶从大肠杆菌BL21(DE3)表达和纯化。 Western印迹分析表明,重组BmPDI可被兔抗BmPDI血清识别。 rBmPDI在pH 8和40°C下表现出最佳活性。该酶被aurin和PDI抑制剂抑制。重组BmPDI显示出与重组马来西亚马来酸钙网蛋白(rBmCRT)的相互作用。通过同源性建模生成了BmPDI和BmCRT的三维模型。发现在两个界面之间总共形成了25个氢键。 BmPDI-BmCRT复合物中存在259个非键接触,并且在相互作用中形成了12个盐桥。

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