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Hi everyone,
I'm wondering if someone has an opinion/experience with that. Using Haloplex, considering the frequent occurence of restriction events in order to generate relatively small "sequencable" fragments from a whole genome, don't you run a high risk to actually CUT your mutated position (if they introduce a novel recognition site for the restriction enzymes)?
Wouldn't this completely obscure the aim for discovery mutational screening without prior knowledge of potential mutations?
Further, if the A but not the B allele of a heterozygous SNP is recognized by one of the restriction enzymes, wouldn't that also bias the allele-frequency of adjacent mutations on the same amplicon?
Best,
Max
I'm wondering if someone has an opinion/experience with that. Using Haloplex, considering the frequent occurence of restriction events in order to generate relatively small "sequencable" fragments from a whole genome, don't you run a high risk to actually CUT your mutated position (if they introduce a novel recognition site for the restriction enzymes)?
Wouldn't this completely obscure the aim for discovery mutational screening without prior knowledge of potential mutations?
Further, if the A but not the B allele of a heterozygous SNP is recognized by one of the restriction enzymes, wouldn't that also bias the allele-frequency of adjacent mutations on the same amplicon?
Best,
Max
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