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作 者:柯晓煜[1,2] 丁红晖[3] 郭燕[3] 陈明发[1] 林永[1] 夏幼辰[1] 孙潺[1] 杨东亮[1] 吴珺[1]
机构地区:[1]华中科技大学同济医学院附属协和医院感染科 [2]同济医学院附属同济医院急诊科,武汉430030 [3]同济医学院附属同济医院临床免疫研究室
出 处:《肝脏》2012年第11期775-778,共4页Chinese Hepatology
基 金:国际科技合作与交流专项(2011DFA31030);国家自然科学基金资助项目(81001313);中国博士后科学基金资助项目(20090460949)
摘 要:目的优化扩增武汉地区HCV1b型患者HCV非结构蛋白3(NS3)的cDNA,并进行测序。方法从患者血清中提取HCVRNA,采用型特异性引物扩增分型法检测HCV患者基因分型。设计3对外侧引物和3对内侧引物,采用套式PCR技术(方案一)分别扩增HCV1b型患者的HCVNS33个区段,然后用3对内侧引物进行测序。为了优化NS3扩增和测序效果和减少操作繁琐,对引物进行改进,设计1对外侧引物和1对内侧引物,采用改进的套式PCR技术(方案二)直接扩增HCV1b型患者的HCVNS3区,然后用3个正向引物和1个逆向引物进行测序。结果改进的套式PCR技术(方案二)与套式PCR技术(方案一)相比,操作较为简单,而且扩增效率增高,扩增效果较好。结论采用改进的套式PCR技术(方案二)扩增和测序HCVNS3区更迅速、有效、实用。Objective To optimize the amplification and sequencing of non structural protein 3 (NS3) gene in patients infected with hepatitis C virus (HCV) genotype lb. Methods The genotyping after extracting HCV RNA from the serum was detected with type specific primers assay. After designing three pairs of outside primers and three pairs of inner primers, HCV NS3 (HCV genotype 1b) were amplified by a nested PCR assay (option Ⅰ) with above primers and sequenced. In order to optimize effects of NS3 amplification and sequencing and to reduce the complicated operation, we improved the new nested PCR assay (option Ⅱ) and redesigned the primers, including a pair of outside primers and a pair of inner primers. We amplified directly HCV NS3 (HCV genotype 1b) with improved nested PCR assay and sequenced NS3 with three forward primers and a reverse primer. Results Compared to the original nested PCR assay (option Ⅰ), the improved nested PCR assay (option Ⅱ) is simpler in operation and of higher efficiency. Conclusion The improved nested PCR assay (option Ⅱ) is more effective and practical for amplification and sequencing of HCV NS3.
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