[蚓激酶基因在毕赤酵母中的克隆与表达]

[Cloning and expression of lumbrokinase gene in Pichia pastoris].

作者信息

Zhao Ming-ming, Li Ming, Han Zhen-lin, Wang Min, Du Lian-xiang

机构信息

Tianjin Key Laboratory of Industrial Microbiology, College of Biotechnology, Tianjin University of Science & Technology, Tianjin 300222, China.

出版信息

Wei Sheng Wu Xue Bao. 2006 Aug;46(4):581-5.

PMID:17037059

Abstract

Lumbrokinase gene F238 was amplified by RT-PCR from the total RNA of earthworm (Eisenia fetida). The gene including signal peptide sequence was inserted into pUCm-T vector to construct pUCm-T-F238. The product was sequenced. The GenBank accession number was DQ202401. Lumbrokinase F238 comprised 738bp and included an open reading frame that encoded a polypeptide of 245 amino acid residues, containing a signal peptide of 7 amino acid residues and a mature peptide of 238 amino acid residues. Both nucleotide and amino acid sequences homologies were 99% after the sequence was compared with Lumbricus rubellus F-III-2. There were two base pair mutations, which subsequently caused two amino acid mutations. The characteristics and structure of F238 was analysed and predicted with biology softwares and databases. The pl of F238 was 4.61. It had eleven Cysteines, which formed three disulfide bonds. Its secondary structure mainly consisted of beta-sheet. Lumbrokinase F238 had serine active center. It was a protease in trypsin family of serine protease superfamily. Lumbrokinase gene F238-m without signal peptide sequence was obtained by PCR using pUCm-T-F238 as template. The expression vector pPIC9-F238-m was constructed by inserting gene F238-m into yeast expression and secretion plasmid pPIC9. Plasmid pPIC9-F238-m was linearized with BgIII and then transformed into Pichia pastoris strain GS115 cell by electroporation method. Phenotypes of transformants were screened in MM and MD plates to ensure the integration of lumbrokinase gene F238-m into yeast chromosome DNA. Methanol was added to a final concentration of 0.5% for the expression of recombination protein every 24h to maintain induction. The result of SDS-PAGE showed that the molecular weight of the expression product was about 28 kDa, in correspondence with the theoretical molecular weight. After the induction of expression, the fibrinolytic activity of the supernatant was measured using artificial fibrin plates. Then the engineering strain of high activity was obtained, and the fibrinolytic activity was up to 100 U/mL.

摘要

通过RT-PCR从蚯蚓（赤子爱胜蚓）的总RNA中扩增出蚓激酶基因F238。将包含信号肽序列的该基因插入pUCm-T载体构建pUCm-T-F238。对产物进行测序。GenBank登录号为DQ202401。蚓激酶F238由738bp组成，包含一个开放阅读框，编码一个245个氨基酸残基的多肽，其中含有一个7个氨基酸残基的信号肽和一个238个氨基酸残基的成熟肽。将该序列与红蚯蚓F-III-2比较后，核苷酸和氨基酸序列同源性均为99%。存在两个碱基对突变，随后导致两个氨基酸突变。利用生物学软件和数据库对F238的特性和结构进行分析和预测。F238的等电点为4.61。它有11个半胱氨酸，形成三个二硫键。其二级结构主要由β-折叠组成。蚓激酶F238具有丝氨酸活性中心。它是丝氨酸蛋白酶超家族胰蛋白酶家族中的一种蛋白酶。以pUCm-T-F238为模板，通过PCR获得无信号肽序列的蚓激酶基因F238-m。将基因F238-m插入酵母表达分泌质粒pPIC9构建表达载体pPIC9-F238-m。用BgIII将质粒pPIC9-F238-m线性化，然后通过电穿孔法转化到毕赤酵母菌株GS115细胞中。在MM和MD平板上筛选转化子的表型，以确保蚓激酶基因F238-m整合到酵母染色体DNA中。每24小时添加甲醇至终浓度0.5%以维持重组蛋白的表达诱导。SDS-PAGE结果显示表达产物的分子量约为28 kDa，与理论分子量相符。诱导表达后，用人纤维蛋白平板测定上清液的纤溶活性。从而获得高活性工程菌株，纤溶活性高达100 U/mL。