I have cloned promotor of a gene upstream of luciferase gene. I have seen people using different cell lines in the papers for dual luciferase experiment.Can I just use hek cell line to see the effect of particular sequence in promotor of a gene(using wt and mutated plasmid). Why people transfect reporter construct in different cell line for this purpose.
In what tissues/cell types is your gene of interest expressed in vivo? It is typical to express the reporter construct in a cell line that normally expresses the gene of interest. For example, if you are studying a gene whose expression is restricted to neurons, maybe you should consider expressing the reporter gene in a neuronal cell line, not in HEK cells. Perhaps HEK cells do not express certain positive or negative regulators of transcription that are relevant to your gene. If your gene of interest is ubiquitously expressed then maybe HEK cells are okay.
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