為快速���、高效構建偽狂犬病病毒(pseudorabies virus��,PRV)糖蛋白E基因(gE)缺失病毒,基于CRISPR/Cas9基因編輯技術��,首先將pSpCas9(BB)-2A-GFP熒光質(zhì)粒轉(zhuǎn)染至VERO細胞和PK-15細胞�����,選出轉(zhuǎn)染效率較高的細胞系�,同時于http://crispr.mit.edu/網(wǎng)站設計并合成3個高評分的小導向RNA(small guide RNA�,sgRNA)����,通過噬斑形成試驗�,篩選出高效sgRNA。其次將篩選出的針對PRV gE基因的sgRNA轉(zhuǎn)染于PK-15細胞����,然后接種PRV-1病毒,經(jīng)過5 輪噬斑克隆純化獲得PRV-1-ΔgE���。結(jié)果顯示:VERO細胞比PK-15細胞具有更好的轉(zhuǎn)染效果���;gE-sgRNA1和gE-sgRNA2可作為針對gE基因的高效sgRNA;獲得了1株PRV gE基因缺失291 bp的病毒����,將其命名為PRV-1-ΔgE。研究表明�,CRISPR/Cas9基因編輯技術可作為一種高效編輯PRV-1缺失病毒基因的方法,同時也為后續(xù)快速應對PRV變異株研究提供了新思路�����。
Construction of PRV gE-deleted Strain Based on CRISPR/Cas9 Technology
In order to rapidly and effectively construct the gE-deleted strain of pseudorabies virus(PRV)���,the fluorescent plasmid of pSpCas9(BB)-2A-GFP was firstly transfected into VERO cells and PK-15 cells to select the cell lines with high efficiency. Meanwhile���,three small guide RNAs(sgRNAs)with high scores were designed and synthesized on http://crispr.mit.edu/ to select high-efficiency sgRNAs through plaque formation experiments. Then the selected sgRNA was transfected into PK-15 cells which subsequently were inoculated with PRV-1����,and finally PRV-1-ΔgE was obtained after five rounds of plaque clone purification. The results showed that VERO cells could be well transfected compared to PK-15 cells����;gE-sgRNA1 and gE-sgRNA2 could be used as the high-efficiency sgRNAs for gE gene;a strain of gE-deleted virus with a deletion of 291 bp was obtained and named as PRV-1-ΔgE. It was found that CRISPR/Cas9 gene editing technology could be used for effectively editing PRV-1 gene-deleted strain�����,which also provided new ideas to rapidly response to PRV variants in the future.
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