用待研基因shRNA慢病毒感染AGS细胞,3天后收集细胞,以600/孔接种6孔板,持续培养2周时间,待细胞形成单克隆后染色计数,结果显示,shRNA下调目的基因表达后,细胞单克隆数量显著减少,表明待研基因与AGS细胞克隆形成能力及增殖显著相关。
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