Zirus, Inc., 1384 Buford Business Boulevard, Suite 700, Buford, GA, 30518, USA,
Mol Biotechnol. 2014 May;56(5):429-37. doi: 10.1007/s12033-013-9730-0.
We have employed gene-trap insertional mutagenesis to identify candidate genes whose disruption confer phenotypic resistance to lytic infection, in independent studies using 12 distinct viruses and several different cell lines. Analysis of >2,000 virus-resistant clones revealed >1,000 candidate host genes, approximately 20 % of which were disrupted in clones surviving separate infections with 2-6 viruses. Interestingly, there were 83 instances in which the insertional mutagenesis vector disrupted transcripts encoding H/ACA-class and C/D-class small nucleolar RNAs (SNORAs and SNORDs, respectively). Of these, 79 SNORAs and SNORDs reside within introns of 29 genes (predominantly protein-coding), while 4 appear to be independent transcription units. siRNA studies targeting candidate SNORA/Ds provided independent confirmation of their roles in infection when tested against cowpox virus, Dengue Fever virus, influenza A virus, human rhinovirus 16, herpes simplex virus 2, or respiratory syncytial virus. Significantly, eight of the nine SNORA/Ds targeted with siRNAs enhanced cellular resistance to multiple viruses suggesting widespread involvement of SNORA/Ds in virus-host interactions and/or virus-induced cell death.
我们采用基因陷阱插入突变技术,在使用 12 种不同病毒和几种不同细胞系的独立研究中,鉴定出能导致细胞对裂解性感染产生表型抗性的候选基因。对超过 2000 个病毒抗性克隆的分析显示出超过 1000 个候选宿主基因,其中约 20%的基因在分别感染 2-6 种病毒的克隆中被破坏。有趣的是,有 83 个实例中,插入诱变载体破坏了编码 H/ACA 类和 C/D 类小核仁 RNA(SNORAs 和 SNORDs,分别)的转录本。其中,79 个 SNORAs 和 SNORDs 位于 29 个基因(主要是编码蛋白)的内含子中,而 4 个似乎是独立的转录单元。针对候选 SNORA/D 的 siRNA 研究在针对牛痘病毒、登革热病毒、甲型流感病毒、人鼻病毒 16、单纯疱疹病毒 2 或呼吸道合胞病毒进行测试时,提供了它们在感染中的作用的独立证实。重要的是,用 siRNA 靶向的 9 个 SNORA/D 中的 8 个增强了细胞对多种病毒的抗性,这表明 SNORA/D 广泛参与病毒-宿主相互作用和/或病毒诱导的细胞死亡。