I did CTAB for DNA extraction and I got good DNA IN BOTH side (Quantity and Quality) but I had RNA in my gel. I wanted to add RNAse after that and when I add it my DNA were degraded.
Could you please tell me if you had this experience or if you have some tips share it with me.
When should I add RNAse in the CTAB protocol for Streptomyces DNA extraction
More Golsa Nayeb Ghanbar Hosseini's questions See All
Similar questions and discussions