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大肠杆菌F18菌毛操纵子全基因克隆、表达及生物学活性
引用本文:张建军,朱国强.大肠杆菌F18菌毛操纵子全基因克隆、表达及生物学活性[J].微生物学报,2007,47(5):790-794.
作者姓名:张建军  朱国强
作者单位:扬州大学兽医学院,扬州,225009
基金项目:江苏省六大人才高峰基金;美国农业部USDA高新技术资助项目
摘    要:利用PCR技术以猪产肠毒素大肠杆菌F18标准菌株107/86和2134P基因组DNA为模板成功地扩增出编码F18ab和F18ac完整菌毛操纵子fed基因。将它们分别克隆入表达质粒载体pET-22b( ),结合酶切和核苷酸序列分析证明了PCR预期扩增产物的正确性。然后将克隆的重组载体DNA转化至大肠杆菌BL21(DE3),构建和筛选出分别含F18ab和F18ac完整fed基因的重组菌,经过IPTG诱导表达,在电镜下观察到上述两种重组菌能分别大量表达F18ab和F18ac菌毛。用热抽提法提纯其诱导表达的F18ab和F18ac菌毛,经SDS-PAGE电泳和考马斯亮蓝染色发现提纯后菌毛获单一分子量约为15kDa蛋白条带,免疫家兔后制备出高效价的兔抗血清,玻板凝集试验和Western blot结果表明:体外诱导表达的F18ab和F18ac菌毛具有和野生F18菌毛相同的抗原性。用表达F18ab和F18ac菌毛的上述2株重组菌分别进行小肠上皮细胞体外吸附试验和吸附抑制试验,结果表明:2株重组菌和野生菌株一样具有较强的粘附易感仔猪小肠上皮细胞的能力,而用表达F18ab和F18ac重组菌提纯的菌毛制备出兔抗血清都能有效地抑制上述重组菌或野生菌株对易感仔猪小肠上皮细胞的吸附结合。

关 键 词:产肠毒素大肠杆菌  F18菌毛  fed基因表达  生物活性
文章编号:0001-6209(2007)05-0790-05
收稿时间:2007/1/23 0:00:00
修稿时间:7/9/2007 12:00:00 AM

Cloning and expression of F18 fimbrial operon gene clusters from enterotoxigenic Escherichia coli and their bioactivity
ZHANG Jian-jun and ZHU Guo-qiang.Cloning and expression of F18 fimbrial operon gene clusters from enterotoxigenic Escherichia coli and their bioactivity[J].Acta Microbiologica Sinica,2007,47(5):790-794.
Authors:ZHANG Jian-jun and ZHU Guo-qiang
Institution:College of Veterinary Medicine; Yangzhou University; Yangzhou 225009; China;College of Veterinary Medicine; Yangzhou University; Yangzhou 225009; China
Abstract:The fed operon gene clusters with each size of 5.6kb,encoding the F18ab or F18ac fimbriae,was amplified respectively by high fidelity PCR using the genomic DNA templates from F18 fimbriae E. coli strains 107/86 or 2134P. The PCR products with the restriction enzyme sites at each end were digested and then cloned into the vector pET-22b( ),the recombinant plamids with the inserts of both type of fed gene clusters were constructed and screened,further confirmed by the means of combination with restriction endonuclease analysis and sequencing. The both types of fimbriae F18ab and F18ac were expressed efficiently in the E. coli BL21(DE3) after proper concentration of IPTG induction. Expressed fimbriae were revealed and comfirmed by transmissible electromicroscope observation. The both fimbriae F18ab and F18ac were isolated and purified from the recombinant E. coli,and only a single major band of protein with size of approximately 15kDa was visualized in Coomassie blue-stained gels after SDS-PAGE. The rabbits sera with high titer of anti-F18 fimbriae were detected after being immunized with the purified F18ab or F18ac fimbriae. The results of combination of agglutination assay with Western blotting showed that the sera directed against both fimbriae F18ab and F18ac reacted positively with the F18 fimbriae from both wild E. coli 107/86 and 2134P.Small intestine epithelial cells with F18 fimbriae receptors,which were from post-weaning piglets with the genotypes of FUT1 gene both M307~ GG and M307~ AG ,were prepared and tested for the adherence of E. coli expressing F18 fimbriae under the microscopic examination. Adhesion and adhesion inhibition test showed both of the recombinant E. coli expressing F18ab or F18ac fimbriae respectively could adhere to the jejunal epithelial cells in vitro as E. coli 107/86 and 2134p did. The both of anti-sera directed against fimbriae F18ab or F18ac respectively can efficiently inhibit the fimbriae-mediated post-weaning piglet jejunal epithelial cells adherence to both the recombinant E. coli (expressing F18ab or F18ac fimbriae) and wild type E. coli (107/86 and 2134P).
Keywords:Enterotoxigenic Escherichia coli  F18ab and F18ac fimbriae  fed operon gene cluster expression  biological activity
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