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欧文氏杆菌甘露聚糖酶基因同源高效表达与缺失表达研究

Studis on the Homologous Expression and Truncated Expression of Mannanase Gene from Erwinia Carotovor

【作者】 李炫

【导师】 彭克勤; 刘正初;

【作者基本信息】 湖南农业大学 , 生物物理学, 2010, 硕士

【摘要】 草本纤维生物提取法是一种利用微生物分泌复合酶系降解草本纤维原料中的非纤维素物质而获得纯净天然纤维素纤维的方法,本室筛选和改造的欧文氏杆菌变异菌株CXJZ95-198和CXJZU120是迄今报道草本纤维提取效率最高的菌株,为了研究CXJZ95-198甘露聚糖酶基因的特点,提高CXJZU-120甘露聚糖酶表达水平,笔者进行了以下研究:利用生物信息学方法对欧文氏杆菌变异菌CXJZ95-198的甘露聚糖酶基因manA及其翻译产物进行了相似度比对,信号肽,跨膜区,系统进化树,二级结构和同源三维建模的分析、预测,结果表明manA核酸序列与其他来源的甘露聚糖酶基因序列相似度很低,翻译产物是胞外酶,N端前27AA可能为信号肽序列,根据三维结构预测结果设计引物,用PCR的方法分别扩增出manA 5’端截去0,81,111,141bp的四个甘露聚糖酶基因部分缺失片段,连接pET28a在E.coli BL21(DE3)中表达,结果证明,manA的翻译产物N端27个AA为信号肽序列,跨膜分泌时会被切割,N端27-37个AA缺失后对酶活无明显影响,N端37-47个AA缺失会引起酶活性丧失。将manA基因连接pEASY E1 express载体转入E.coli BL21(DE3)中,经透明圈,抗生素筛选后再将重组质粒从BL21(DE3)重组菌中提取出来,导入欧文氏杆菌变异菌株CXJZU-120中进行同源表达,用透明圈法发现CXJZU-120重组菌较原始菌在甘露聚糖酶筛选培养平板上产生的水解圈大2/3,培养25h后酶活测定结果表明,重组菌的甘露聚糖酶酶活较原始菌提高2.1倍。

【Abstract】 Bio-extraction of fiber from crops is a method using bacteria which producing series of enzymes to decompose hemicellulose of the crops.Two Erwinia carotovora CXJZ95-198 and CXJZU-120 have been isolated in this laboratory, which are reported as the most efficient deguming bacteria. In this study, the property of mannanase from CXJZ95-198,and the mannanase expression level on CXJZU-120 were investigated to promote their production, the results are as follows.manA, the mannanase gene of CXJZ95-198 has been analysed by bioinformatics method in homology alignment, signal peptide prediction, transmembrane region prediction, phylogenic tree foundation, second structure and crystal structure foundation. The results show that manA has low similarity in the alignment with other source of mannanase genes, and its translation product is extracellular. Signal peptides of 27AA from the N-terminal were found at the manA’s translation product. Four truncated mannanase genes were designed according to the homologous model, in which 0,81,111,141bp were deleted from the N-terminal respectively. N-truncated gene expression proved the 27aa aside the N terminal were signal peptide, and loss of the 37aa from the N terminal show little effect on mannanase activity. However, the enzyme will be inactivatied while the number of amino acid deltion was more than 47.The manA was cloned into plasmid pEASY El express and transferred into E.coli BL21 (DE3).The recombinant plasmids were extracted from the positive transformant, and transferred into Erwinia carotovor variant CXJZU-120. Measured by circle decomposing method, the mannanase expression level of the homologous recombinant was 2/3 higher than the original host CXJZU-120, and the promotion of mannanase activity is 2.1 times.

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