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Expression and characterization of the prtV gene encoding a collagenase from Vibrio parahaemolyticus in Escherichia coli

机译:从大肠杆菌中编码胶原蛋白酶PRTV基因的PRTV基因的表达与表征

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Summary: The prtV gene, encoding a collagenase of Vibrio parahaemolyticus, was expressed in Escherichia coli and purified by affinity chromatography. The transformant E. coli BL21 (DE3) (pPRT2) secreted the recombinant PrtV, and the highest enzyme activity was detected in the culture supernatant after 5 h IPTG induction. The molecular mass of purified PrtV was 62 kDa as determined by gel filtration, which was similar to that obtained by SDS-PAGE (64 kDa). This suggested that PrtV was a monomer protein having no subunit structure. The isoelectric point of PrtV was 8·52. In addition, PrtV contained a 27 amino acid signal peptide, and the amino acid composition of the PrtV showed satisfactory agreement with that predicted from the DNA sequence. The optimum temperature and pH of PrtV were 40 °C and pH 7·5, respectively. The activity of PrtV was inhibited by chelators such as EDTA, EGTA and 1,10-phenanthroline; however, its activity was restored by the addition of various metal ions (Co2+, Mn2+, Ca2+, Cu2+, Ni2+and Zn2+), indicating that PrtV is a metalloprotease. PrtV degraded both type I collagen and synthetic substrate FALGPA well, showing that PrtV is indeed a collagenase.
机译:发明内容:在大肠杆菌中表达了编码vibrio parahaemolyticus的胶原酶PrTV基因,并通过亲和层析纯化。转化体大肠杆菌BL21(DE3)(DE3)(PPRT2)分泌重组PRTV,并在5小时IPTG诱导后在培养上清液中检测到最高酶活性。纯化PRTV的分子量为62kDa,如凝胶过滤测定,其类似于通过SDS-PAGE(64kDa)获得的。这表明PRTV是没有亚基结构的单体蛋白。 PRTV的等电点为8·52。此外,PRTV含有27个氨基酸信号肽,PRTV的氨基酸组成与从DNA序列预测的氨基酸组成表现出令人满意的协议。 PRTV的最佳温度和pH值分别为40℃和pH7·5。 PRTV的活性被螯合剂(如EDTA,EGTA和1,10-菲咯啉)抑制;然而,通过添加各种金属离子(CO 2 +,MN2 +,Ca 2+,Cu2 +,Ni2 +和Zn2 +)来恢复其活性,表明PRTV是金属蛋白酶。 PRTV均降解I型胶原蛋白和合成底物FalgPa,表明PRTV确实是胶原酶。

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