I used NaCl extraction of DNA in genus Gammarus of Amphipoda. Though my concentration and 260/280 readings are really good, my 260/230 is very low.
Do I have contamination? If it's salt contamination, how can I treat it and purify it for PCR cheaply (my resources are very little sadly)?
Hi there,
High reading at 230nm is generally indicative of phenol and/or carbohydrate contamination of your DNA sample. DNA precipitation seems to be the cheapest for getting rid of these...
Hi Mr Katouzian
With salting out method you use ethanol at the last step, if the pellet was humid with ethanol you encounter this problem, take some time for ethanol evaporation and then use DNA pellet. unfortunately, I don’t have any suggestion for this problem. I hope you find a way for that.
Best.
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