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Frequently Asked Questions

What roles do positive and negative controls play in RNAi experiments, and how should I select?

Positive controls: These are verified siRNAs targeting housekeeping or reporter genes (e.g., GAPDH, ACTB, GFP/EGFP). They are used to assess the feasibility of the entire experimental system (transfection, RNA extraction, QC, etc.). We provide effective siRNA positive controls targeting GAPDH, ACTB, GFP/EGFP.

Negative controls: These are non-specific siRNAs used to demonstrate the specificity of siRNA effects. They can be universal or scrambled sequences based on requirements.


Should the results of negative controls be the same across different groups? What if there is significant deviation?
What should I do if the silencing effect is not satisfactory?
Why is no fluorescence observed after transfection?
Why is there a lot of cell death after transfection?
Why is there low efficiency of cell transfection?
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