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作 者:曹玉玺[1] 赫晓霞[1] 付士红[1] 李浩[1] 梁国栋[1] 王环宇[1]
机构地区:[1]中国疾病预防控制中心病毒病预防控制所,北京102206
出 处:《中国媒介生物学及控制杂志》2016年第1期1-4,共4页Chinese Journal of Vector Biology and Control
基 金:国家科技重大专项课题(2013ZX10004-101)~~
摘 要:目的利用Taq Man实时荧光定量PCR技术,建立巴泰病毒(Batai virus,BATV)实时荧光定量PCR检测方法。方法根据Gen Bank发表的BATV基因序列资料分析结果,在其S片段编码非结构蛋白的基因区段设计BATV特异引物与探针,利用不同科、属的13株病毒核酸验证方法特异性,利用体外转录的定量RNA标准品建立基因拷贝数定量分析模型,重复实验检验方法的稳定性。结果引物与探针具有良好的特异性,定量分析模型的灵敏度为10拷贝/μl,同一样品重复检测循环阈值的变异系数均<2.50%。结论建立了一种特异、灵敏、高效的BATV一步法Taq Man实时荧光定量PCR检测方法,为今后该病毒的检测与研究工作提供技术手段。Objective To develop a rapid and sensitive detection method for Batai virus (BATV) based on TaqMan Real-time PCR. Methods Based on the BATV NS gene sequences of S segment published in GenBank, BATV specific primers and probe were designed. The specificity and stability of the system were evaluated. Quantitative standard curve of BATV TaqMan Real-time PCR was established. Results The specificity and stability test showed that the system is specific and the coefficient variables were all less than 2.50%. Quantitative standard curve based on the genomic copy was drawn, and the lowest detectable limit (LOD) of system is 10 copies/μl. Conclusion TaqMan Real-time PCR for BATV detection has been developed, which is more sensitive and more efficient than the general PCR.
分 类 号:R373.3[医药卫生—病原生物学]
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