Host Interferon-Stimulated Gene 20 Inhibits Pseudorabies Virus Proliferation

Host interferon-stimulated gene 20(ISG20)exerts antiviral effects on viruses by degrading viral RNA or by enhancing IFN signaling.Here,we examined the role of ISG20 during pseudorabies virus(PRV)proliferation.We found that ISG20 modulates PRV replication by enhancing IFN signaling.Further,ISG20 expression was upregulated following PRV infection and poly(I:C)treatment.Ectopic expression of ISG20 inhibited PRV proliferation in PK15 cells,whereas knockdown of ISG20 promoted PRV proliferation.In addition,ISG20 expression upregulated IFN-βexpression and enhanced IFN downstream signaling during PRV infection.Notably,PRV UL24 suppressed the transcription of ISG20,thus antagonizing its antiviral effect.Further domain mapping analysis showed that the N terminus(amino acids 1-90)of UL24 was responsible for the inhibition of ISG20 transcription.Collectively,these findings characterize the role of ISG20 in suppressing PRV replication and increase the understanding of host-PRV interplay.

基于CRISPR/Cas9系统Ⅰ型干扰素受体亚单位1基因敲除的Caco-2细胞系的构建

目的利用成簇规律间隔短回文重复序列(clustered regularly interspaced short palinmic repeats,CRISPR)/CRISPR相关蛋白9(CRISPR-associated protein 9,Cas9)系统在人结肠腺癌细胞Caco-2中敲除Ⅰ型干扰素受体亚单位1(interferon alpha/beta receptor subunit 1,IFNAR1)基因,构建IFNAR1基因敲除Caco-2细胞系。方法利用CRISPR/Cas9技术设计特异性识别IFNAR1基因外显子区的sgRNA(single guide RNA)序列,构建LentiCRISPRv2-IFNAR1-sgRNA重组质粒,慢病毒包装后感染Caco-2细胞,嘌呤霉素抗性筛选,有限稀释法培养单克隆细胞系。通过靶基因测序和Western blot法验证IFNAR1基因敲除情况;通过加入外源性IFNβ检测IFNAR1基因敲除细胞CXC趋化因子配体10(CXC chemokine ligand 10,CXCL10)和干扰素刺激基因20(interferon-stimulatd gene 20,ISG20)mRNA水平。结果质粒LentiCRISPRv2-IFNAR1-sgRNA测序结果显示插入位置均位于BsmBⅠ酶切黏性末端。共获得2株IFNAR1基因敲除单克隆细胞株,测序结果显示Caco-2-IFNAR1-KO1的IFNAR1第6个外显子发生5 bp缺失,Caco-2-IFNAR1-KO2的第7个外显子发生18 bp缺失,同时有1 bp增加。与野生型Caco-2细胞相比,Caco-2-IFNAR1-KO1和Caco-2-IFNAR1-KO2细胞IFNAR1蛋白未见表达。相比于0 ng/mL IFNβ,在50 ng/mL外源IFNβ刺激下,Caco-2-IFNAR1-KO1和Caco-2-IFNAR1-KO2细胞CXCL10基因mRNA水平(t分别为0.566和1.268,P>0.05)和ISG20基因mRNA水平(t分别为1.522和1.733,P>0.05)均无明显升高;与野生型Caco-2细胞相比,在50 ng/mL外源IFNβ刺激下,Caco-2-IFNAR1-KO1和Caco-2-IFNAR1-KO2细胞CXCL10基因mRNA水平(t分别为6.763和6.777,P<0.05)和ISG20基因mRNA水平(t分别为5.664和5.653,P<0.05)均显著降低。结论利用CRISPR/Cas9技术成功获得了IFNAR1基因敲除的Caco-2细胞株,该细胞系依赖Ⅰ型IFN受体(interferon alpha/beta receptor,IFNAR)激活的下游分子被明显抑制,为进一步探讨病毒感染Caco-2细胞后的天然免疫反应及复制包装机制提供了有力的工具。