RNAlater stabilizing agent is normally used on fresh tissues. Available handbooks do not specify how I can use it on cultured cells that are meant to be used for RNA extraction. If I am going to perform a column RNA extraction, should I add it before cell lysis, or after finishing the whole extraction? And in what proportion? Thank you beforehand.
Thanks for your answer, Prabu.
I know it's not quite necessary, but I am going to be storing this RNA for some time and I can't turn it into cDNA to gain some stability, since I'm going to use it in gene expression analysis later, so, I was trying to fashion a way to add some stability for the storage and freezing.thaw cycles using the RNAlater.
Thanks, Maxim.
The alternatives that you proposed seem better to me than the RNAlater for this particular case.
Best regards.
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