CRISPR/Cas9-mediated genome editing can inhibit virus infection by targeting the conserved regions of the viral genomic DNA. Unexpectedly, we found previously that pseudorabies virus(PRV) could escape from CRISPR/Cas9...CRISPR/Cas9-mediated genome editing can inhibit virus infection by targeting the conserved regions of the viral genomic DNA. Unexpectedly, we found previously that pseudorabies virus(PRV) could escape from CRISPR/Cas9-mediated inhibition.In order to elucidate whether the escape of PRV from Cas9-mediated inhibition was due to cell deficiencies, such as genetic instability of sgRNA or Cas9 protein, the positive cells were passaged ten times, and PRV infection in the sgRNA-expressing cells was evaluated in the present study. The results showed that subculturing cells has no effect on Cas9-mediated cleavage of PRV. Different passages of PX459-PRV cells can stably express sgRNA to facilitate Cas9/sgRNA cleavage on the UL30 gene of PRV, resulting in a pronounced inhibition of PRV infection. Studies to elucidate the mechanism of PRV escape are currently in progress.展开更多
为建立鸭瘟病毒(DPV)快速、敏感的检测方法,本研究利用PCR技术扩增出DPV UL30基因中510bp的保守序列,并克隆到p MD18-T载体中作为标准品制作标准曲线,建立了DPV的SYBR Green I荧光定量PCR检测方法。该方法检测灵敏度可达5×101拷贝...为建立鸭瘟病毒(DPV)快速、敏感的检测方法,本研究利用PCR技术扩增出DPV UL30基因中510bp的保守序列,并克隆到p MD18-T载体中作为标准品制作标准曲线,建立了DPV的SYBR Green I荧光定量PCR检测方法。该方法检测灵敏度可达5×101拷贝,与鸭细小病毒、鸭圆环病毒、小鹅瘟病毒、鸭肝炎病毒、鸭H9亚型流感病毒和鸭副粘病毒均不发生交叉反应,具有良好的特异性和重复性。结果表明,建立的实时荧光定量PCR具有特异、敏感、快速、定量、重复性好等优点,可用于临床DPV的检测。展开更多
基金financially supported by the National Key Research and Development Program of China(No.2017YFD0500103)the Beijing Natural Science Foundation(No.5152023)+4 种基金the National Natural Science Foundation of China(No.31772747 and31272385)the Jilin Province Science and Technology Development Projects(20150204077NY)the Graduate Innovation Fund of Jilin Universitythe Program for Chang jiang Scholarsthe University Innovative Research Team(No.IRT1248)
文摘CRISPR/Cas9-mediated genome editing can inhibit virus infection by targeting the conserved regions of the viral genomic DNA. Unexpectedly, we found previously that pseudorabies virus(PRV) could escape from CRISPR/Cas9-mediated inhibition.In order to elucidate whether the escape of PRV from Cas9-mediated inhibition was due to cell deficiencies, such as genetic instability of sgRNA or Cas9 protein, the positive cells were passaged ten times, and PRV infection in the sgRNA-expressing cells was evaluated in the present study. The results showed that subculturing cells has no effect on Cas9-mediated cleavage of PRV. Different passages of PX459-PRV cells can stably express sgRNA to facilitate Cas9/sgRNA cleavage on the UL30 gene of PRV, resulting in a pronounced inhibition of PRV infection. Studies to elucidate the mechanism of PRV escape are currently in progress.
文摘为建立鸭瘟病毒(DPV)快速、敏感的检测方法,本研究利用PCR技术扩增出DPV UL30基因中510bp的保守序列,并克隆到p MD18-T载体中作为标准品制作标准曲线,建立了DPV的SYBR Green I荧光定量PCR检测方法。该方法检测灵敏度可达5×101拷贝,与鸭细小病毒、鸭圆环病毒、小鹅瘟病毒、鸭肝炎病毒、鸭H9亚型流感病毒和鸭副粘病毒均不发生交叉反应,具有良好的特异性和重复性。结果表明,建立的实时荧光定量PCR具有特异、敏感、快速、定量、重复性好等优点,可用于临床DPV的检测。