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Efficient inhibition of African swine fever virus replication by CRISPR/Cas9 targeting of the viral p30 gene (CP204L)

机译:通过针对病毒p30基因的CRISPR / Cas9靶向有效抑制非洲猪瘟病毒复制(CP204L)

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African swine fever is a devastating viral disease of domestic and wild pigs against which no vaccine or therapy is available. Therefore, we applied the CRISPR (clustered regularly interspaced short palindromic repeats) – Cas9 nuclease system to target the double-stranded DNA genome of African swine fever virus (ASFV). To this end, a permissive wild boar lung (WSL) cell line was modified by stable transfection with a plasmid encoding Cas9 and a guide RNA targeting codons 71 to 78 of the phosphoprotein p30 gene (CP204L) of ASFV. Due to targeted Cas9 cleavage of the virus genome, plaque formation of ASFV was completely abrogated and virus yields were reduced by four orders of magnitude. The specificity of these effects could be demonstrated by using a natural ASFV isolate and escape mutants possessing nucleotide exchanges within the target sequence, which were not inhibited in the Cas9-expressing cell line. Growth of the cell line was not affected by transgene expression which, as well as virus inhibition, proved to be stable over at least 50 passages. Thus, CRISPR-Cas9 mediated targeting of the ASFV p30 gene is a valid strategy to convey resistance against ASF infection, which may also be applied in its natural animal host.
机译:非洲猪瘟是家畜和野猪的致命病毒性疾病,尚无针对其的疫苗或疗法。因此,我们应用了CRISPR(聚类的规则间隔的短回文重复序列)-Cas9核酸酶系统来靶向非洲猪瘟病毒(ASFV)的双链DNA基因组。为此,通过用编码Cas9的质粒和靶向ASFV的磷蛋白p30基因(CP204L)的71至78位密码子的引导RNA稳定转染来修饰许可的野猪肺(WSL)细胞系。由于病毒基因组的靶向Cas9裂解,ASFV的噬菌斑形成被完全消除,病毒产量降低了四个数量级。这些作用的特异性可以通过使用天然的ASFV分离物和逃逸突变体来证明,这些突变体在靶序列内具有核苷酸交换,而在表达Cas9的细胞系中没有被抑制。细胞系的生长不受转基因表达的影响,转基因表达以及病毒抑制作用被证明在至少50次传代中是稳定的。因此,CRISPR-Cas9介导的针对ASFV p30基因的靶向是传达抵抗ASF感染的有效策略,也可应用于其天然动物宿主中。

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