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Expression of Active Calf Chymosin in Aspergillus Niger

机译:活性小牛凝乳酶在黑曲霉中的表达

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摘要

Calf chymosin is an important protease used widely in the industry of food, medicine and plastics. We try use Aspergillus niger as a genetically engineered host to produce the heterologous protein. The prochymosin cDNA was cloned from the abomasum dells of unweaned calves by reverse transcription polymerase chain reaction (RT-PCR). The cloned fragment of 1100 bp in vector pUCm-T was then subcloned into an expression vector pyG1.2 containing the pyrG gene. The insert fragment was fused in frame with glucoamylase coding region under the control of A. niger glaA promoter. The recombined plasmid containing prochymosin cDNA transformed the M54, a pyrG gene auxotroph of Aspergillus niger. Three transformants was selected and they showed no obvious difference in expression and secretion of chymosin. The result of SDS-PAGE indicated that there was protein band of 36KD with the same molecular weight as chymosin. The milk coagulation test proved that the active chymosin had been expressed and secreted successfully by the recombinant A.niger. This study further emphasizes the potential importance of aspergillus niger as a useful host for the production of heterologous proteins with authentic biological properties.
机译:小牛凝乳酶是一种重要的蛋白酶,广泛用于食品,医药和塑料行业。我们尝试使用黑曲霉作为基因工程宿主来生产异源蛋白。通过逆转录聚合酶链反应(RT-PCR)从未断奶的小牛的厌恶小肠中克隆了凝乳酶原cDNA。然后将在载体pUCm-T中克隆的1100bp的片段亚克隆到含有pyrG基因的表达载体pyG1.2中。在A.niger glaA启动子的控制下,将插入片段与葡糖淀粉酶编码区框内融合。含有凝乳酶原cDNA的重组质粒转化了M54,一种黑曲霉的pyrG基因营养缺陷型。选择了三个转化子,它们在凝乳酶的表达和分泌上没有明显差异。 SDS-PAGE结果表明,存在一条与凝乳酶具有相同分子量的36KD蛋白条带。牛奶凝结试验证明,重组凝乳酶成功表达和分泌了活性凝乳酶。这项研究进一步强调了黑曲霉作为有用宿主生产具有真实生物学特性的异源蛋白质的潜在重要性。

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