18 December 2015 4 1K Report

I've tried lentivirus but didn't get enough infected cells. An article (DOI:10.1172/jci78753) describes the following method: "B6 WT splenocytes were cultured in complete medium for 24 hours. The medium was then replaced with complete medium supplemented with Polybrene (Sigma-Aldrich) at a final concentration of 5 μg/ml, and the cells were infected with lentiviral particles carrying E2F7 or E2F8, or control vector for 3 days". But about 50% cells died after 48h of incubation in complete medium supplemented with 4,5,6 μg/ml Polybrene, more cells died in higher concentrations of Polybrene. Should I change the virus -containing medium after 24 hours and add fresh medium?  Is there any other method to stably overexpress mircoRNA in primary T cells?

Thanks in advance!

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