G418筛选稳定表达细胞系PROTOCOL
1.G418的配制: 取1g G418溶于1ml 1M的HEPES液中,加蒸馏水至10ml,过滤消毒,4度保存。2.细胞培养:取待测培养细胞,制备成细胞悬液,按等量接种入多孔培养板中,培养6小时左右开始加药。3.制备筛选培养基:在100ug/ml~1000ug/ml范围内确定几个梯度,比如先做个100ug/ml、400ug/ml、800ug/ml、1000ug/ml,按梯度浓度用培养基稀释G418制成筛选培养基。4.加G418筛选: 吸除培养孔中培养基,PBS洗涤一次,每孔中加入不同浓度的筛选培养基。5.换液:根据培养基的颜色和细胞生长情况,每3~5天更换一次筛选培养基。方法同4。6.确定最佳筛选浓度:在筛选10~14天内能够杀死所有细胞的最小G418浓度即为最佳筛选浓度。在第一轮就筛选出最佳G418浓度的可能性不大,最有可能的是出现这种情况:用某一浓度G418的量在筛选14天后还不能杀死细胞,而用下一个梯度的 G418的量在1......阅读全文
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Protocol-for-Trichl...
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Yale-Immunofluorescence-Protocol
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Immunofluorescence-Microscopy-Protocol
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Immunofluorescence-Microscopy-Protocol
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Adhesion-Assay-Protocol
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RNA-Isolation-Protocol
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Intracellular-Staining-Protocol
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Basic-ELISA-Protocol
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Urea-Lysis-Protocol
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Cytotoxicity-Assays-Protocol
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Silver-Staining-Protocol
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