I am currently working on fractionating mixed microbial DNA into individual species (which will be followed by DNA sequencing for identification). The mixed DNA was the product of several one-week intervals of a fermentation. Manufacturer's manual says each DGGE well should be loaded with 180-300 ng of DNA. Do we have to load a precise equal amount of mixed DNA of each fermentation interval into each gel well? thank you
Paul Rutland
Not really you are looking for band patterns and differences in patterns so as long as you load enough to see all of the bands that will be fine
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Mohamad Sufian So'aib
Yes, it makes sense since denaturing agent separate the mixed DNA into specific sequence regardless of the DNA amount. Thank you.
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