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家蝇幼虫抗菌肽天蚕素基因的克隆及其在大肠杆菌中融合表达

Cloning of the antibacterial peptide cecropin gene of Musca domestica larvae and its fusion expression in Escherichia coli

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收录情况: ◇ 统计源期刊 ◇ 北大核心 ◇ CSCD-C

机构: [1]Department of Laboratory,The Second Affiliated Hospital,Guangzhou University of TCM (Guangdong Pro— vincial Hospital of TCM),Guangzhou 510120,China [2]School of Pre-clinical Medicine,Guangdong College of Pharmacy, Guangzhou 510224,China [3]Department of Pathogenic Biology,Guangdong Medical Co llege, Zhanjiang 524023,China
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关键词: Musca domestica cecropin antibacterial peptide gene cloning fusion expression

摘要:
In the present study, the total RNA was extracted from three instar larvae of Musca domestica, the cDNA sequence encoding the ORF of cecropins was amplified by RT-PCR, and the target fragment was further sequenced after being cloned into T vector pUCm-T. Then, the cDNA sequence of the mature cecropins was amplified by PCR with recombinant plasmid pUCm-T/cecropin as template, the N-terminal rare codon GGA of E. coli was changed to the favorable codon GGC,and a Asn codon AAC was added in front of the stop coden TAA in the C- terminus. This mutant gene designated as mCecropin was then ligated with the fusion expression vector pGEX-4T-1. After restriction analysis and DNA sequencing, the positive recombinant plasmid pGEX-4T-1/mCecropin was transformed to different strains of E. coli cells and the fusion protein was expressed after IPTG induction. The fusion protein was assayed by SDS-PAGE and the E. coli BL21(DE3) cell was chosen as the host cell for the expression of the fusion protein. The expressed fusion protein GST-mCecropin was purified by GSTrap affinity coloum and the GST marker was then cleaved by thrombin. In this way, the fusion protein mCecropin with antibacterial activity was obtained after purification with HiTrap benzamidine column.

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第一作者机构: [1]Department of Laboratory,The Second Affiliated Hospital,Guangzhou University of TCM (Guangdong Pro— vincial Hospital of TCM),Guangzhou 510120,China
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