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Large-scale expression in Escherichia coli and efficient purification of precursor and active caspase-7 by introduction of thrombin cleavage sites

机译:通过引入凝血酶裂解位点在大肠杆菌中大规模表达并有效纯化前体和活性caspase-7

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摘要

Caspases are a family of cysteine proteases that have critical roles in the apoptotic pathway. Caspase-7 is a well-known apoptotic effector that cleaves a variety of cellular substrates, and is known to be an important target in the treatment of many diseases. For efficient research, large amounts of the protein are required. However, it has been difficult to obtain sufficient quantities of either the precursor or active caspase-7 from Escherichia coli strain. In the present study, we constructed thrombin-activatable caspase-7 precursors by changing the auto-activation sites of the caspase-7 precursor into sequences susceptible to thrombin cleavage. These engineered precursors were highly expressed as soluble proteins in E. coli, and were easily purified by affinity chromatography (to levels of 10-15 mg per liter of E. coli culture), and were then readily activated by treatment with thrombin. In vitro cleavage assays and kinetic analyses revealed that the engineered active caspase-7 proteins had characteristics similar to those of wild-type caspase-7. This novel method is valuable for obtaining both precursor and active caspase-7, thereby contributing to the development of caspase-7-specific drugs to treat various diseases, including cancer and neurodegenerative conditions.
机译:胱天蛋白酶是半胱氨酸蛋白酶的家族,在凋亡途径中具有关键作用。 Caspase-7是一种众所周知的凋亡效应物,可裂解多种细胞底物,并且已知是治疗多种疾病的重要靶标。为了进行有效的研究,需要大量的蛋白质。但是,很难从大肠杆菌菌株中获得足够量的前体或活性胱天蛋白酶7。在本研究中,我们通过将caspase-7前体的自激活位点改变为易受凝血酶裂解的序列,构建了凝血酶可激活的caspase-7前体。这些工程化的前体在大肠杆菌中以可溶性蛋白的形式高表达,并易于通过亲和色谱法纯化(至每升大肠杆菌培养液10-15 mg的水平),然后通过凝血酶处理而易于活化。体外裂解测定和动力学分析表明,工程改造的活性caspase-7蛋白具有与野生型caspase-7相似的特征。这种新方法对于获得前体和活性caspase-7都很有价值,从而有助于开发caspase-7特异性药物来治疗各种疾病,包括癌症和神经退行性疾病。

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