This is likely to be a very basic question - I am sorry for asking it but will do that anyway:)

We are trying to clone and sequence bacterial communities coming from different samples by using the same chemistry (well, mostly kits...) The total DNA concentration extracted from the samples is not predictive in any way of the number of clones growing on the plates. Moreover, some high-DNA samples produce notoriously low number of clones (blue-white screening) and have a poor sequencing success (16S rRNA) compared to other samples. What would be a plausible explanation for that (apart from a high contribution of non-bacterial DNA to the total sample DNA)?

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