机构地区: 广东药学院基础学院广东省生物活性药物研究重点实验室
出 处: 《生物技术通报》 2010年第4期150-155,共6页
摘 要: 构建家蝇天蚕素-人溶菌酶(Mdc-hly)融合基因,实现Mdc-hly基因在大肠杆菌中的表达。通过RT-PCR分别扩增出家蝇天蚕素和人溶菌酶的成熟肽基因序列,再利用Gene-SOEing技术构建融合基因,将融合基因克隆至pET32a表达载体,转化E.coli BL21(DE3),经IPTG诱导得到高效表达,融合蛋白分子量约为38kD。Western blotting杂交证实了表达蛋白的抗原活性。成功构建了融合其因并进行了原核表达,为进一步的生物活性研究打下基础。 The DNA fragment encoding the mature peptide of Musca domestica cecropin and human lysozyme were obtained by RT-PCR. The Mdc-hly gene was constructed in a Mdc-linker-hly format with the standard 15-amino acid linker (Gly4Ser)3 by Gene-SOEing,and the final full length product was cloned into the pET-32a vector for protein expression in Escherichia coli strain BL21(DE3). The expression fusion protein Mdc-hly-Trx were about 38 kD and Western blotting analysis confirmed that the 38 kD protein was the fusion protein,because it was specifically recognized by mouse anti-His monoclonal antibody. The fusion gene Mdc-hly was successfully constructed and expressed,the results of which could provide foundation for further study of its biological activity.
领 域: [生物学]