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Enhanced proteolytic cleavage of recombinant fusion proteins

机译:重组融合蛋白的增强蛋白水解切割

摘要

Disclosed are methods for increasing the yield of intact target proteins by cleaving fused polypeptides made by recombinant DNA techniques. The fused polypeptides are designed at the DNA level to have a preselected primary cleavage site in a pendant polypeptide fused to a protein of interest. Structural features of the fused polypeptide and cleavage reaction environment are controlled to favor cleavage by a preselected cleavage agent at the primary cleavage site over a second cleavage agent-sensitive amino acid sequence in the target protein. The cleavage reaction is terminated before completion when the ratio of intact target protein to truncated, cleaved target protein is optimized, and the remaining reaction mixture comprising uncleaved fused polypeptide is resubjected to the cleavage agent. The presence of charged organic molecules in the cleavage reaction mixture favors cleavage at the primary cleavage site. The endopeptidase used for cleavage may be immobilized on an insoluble support matrix.
机译:公开了通过切割重组DNA技术制备的融合多肽来增加完整靶蛋白产量的方法。在DNA水平上设计融合多肽,使其在与感兴趣蛋白质融合的侧链多肽中具有预先选择的初级切割位点。控制融合多肽的结构特征和裂解反应环境,以利于在靶蛋白中第二裂解剂敏感氨基酸序列上的一级裂解位点通过预选择的裂解剂进行裂解。当完整的靶蛋白与截短的,切割的靶蛋白的比例最优化时,切割反应在完成之前终止,并且将包含未切割的融合多肽的剩余反应混合物重新置于切割剂中。裂解反应混合物中带电荷的有机分子的存在有利于一级裂解位点的裂解。用于切割的内肽酶可以固定在不溶的支持基质上。

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