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Overview Hysigen provides an extensive array of shRNA reagents to furnish you with optimal tools for your RNAi experiments. We specialize in packaging all major virus types, including lentivirus, AAV, and adenovirus, across various titer scales, facilitating the delivery of your shRNAs into difficult-to-transfect cells. Key Advancements
Workflow 1. Cell preparation Cell resuscitation culture, using cells with fast proliferation rate, cells capable of forming good monoclonal clones, and cells with high cell transfection efficiency are the key factors for the success of the experiment, and it is recommended to meet the following conditions: ① Resuscitated cells should be passaged more than 3 times; ② Use cells with good clone formation as much as possible; ③ Passaging of cells 2 days before transfection; ④ Change the cell culture medium a single day before transfection; ⑤ Keep the cells at 50~85% confluence before transfection to keep the cells in the best proliferation state.
2. shRNA+SSR transfection (or transduction depends on the vector type ) ① Cell density is 70-85%. ② Mix shRNA plasmid+lipo and add to cells. ③ After incubation in (37ºC, 5% CO2) overnight. ④ Observe the expression rate of cellular GFP after 48 hours, the positive rate of GFP control should be more than 50%. Note: All the media used in the transfection process are antibiotic-free media, otherwise it will lead to cell death.
3. Transfection and drug screening After 48h of transfection, the cells are screened with Puromycin (Puro); after the cell confluence reaches 80%, the cells are passaged according to 1:2~1:3, and then continue to be cultured with drug screening for 1~2 weeks, then the construction of the interferon-stabilized transfected cell line can be completed. Technical Information RNA interference (RNAi) is the process of effectively silencing or inhibiting the expression of a target gene, which is achieved by degrading the corresponding mRNA of the target gene by double-stranded RNA (dsRNA).
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