胞内劳森氏菌lsaA基因克隆与序列分析  被引量:1

Cloning and sequence analysis of lsa A gene of Lawsonia intracellularis

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作  者:陈玉红[1] 郑新添[1] 李晓华[1] 戴爱玲[1] 

机构地区:[1]龙岩学院福建省预防兽医学与兽医生物技术重点试验室,福建龙岩364000

出  处:《福建畜牧兽医》2015年第6期18-20,共3页Fujian Journal of Animal Husbandry and Veterinary medicine

基  金:福建省教育厅A类项目(JA11247)资助

摘  要:目的:克隆并分析胞内劳森氏菌(Lawsonia intracellularis,LI)lsa A基因,为研究该基因提供基础。方法:根据已发表的LI基因组序列,设计2条引物,提取猪回肠黏膜的LI基因组,并用PCR技术扩增lsa A基因,将其克隆、测序,进行序列同源性、蛋白抗原性预测等分析。结果:扩增出与702 bp引物相符的基因片段,与Gen Bank的序列同源性为98.4%,该基因编码的蛋白预计具有良好的抗原性。结论:胞内劳森菌las A基因的成功克隆为增生性肠炎的防控提供研究基础。Objective: Cloning and sequence analysis of lsa A gene of Lawsonia intracellularis to lay the foundation for further study of the gene. Methods: 2 primers were designed to amplify Lawsonia intracellularis lsa A gene by PCR. Cloned and sequenced, the nucleotide sequence homology of this gene and protein antigenicity prediction analysis were carried out. Results: 702 bp PCR product in length were amplified, which have the sequence homology of 98.4% with that of published lsa A gene in Genbank. The protein lsa A encoded by lsa A gene is predicted to have good antigenicity by using DNAStar soft. Conclusion: The successful cloning of Lawsonia intracellularis lsa A gene lay the foundation for the prevention and control of proliferative enteritis.

关 键 词:胞内劳森氏菌 lsaA基因 序列分析 抗原预测 

分 类 号:S852.61[农业科学—基础兽医学]

 

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