I performed RNA isolation from B. subtilis (lysozyme combined with Trizol reagent method) and RNA samples were treated with DNase I. I had samples for running an agorose gel both before and after DNase I treatment. After running the gel we couldn't obtain any bands for DNA before DNase I treatment. Could you please help me for this, thanks in advance.
(gel picture is attached under files)
Chandru Subramani
Because you are isolating RNA, not DNA. Dnase treatment is to remove if there is any DNA contamination in the RNA samples. It is expected that DNA would be in low quantity as a contaminant. You may not see it on the agarose gel.
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