I am experiencing a contamination problem in my DNA extracts. I did DNA extraction from water samples using phenol/chloroform. However, I do get a shoulder/high peak at 230 nm whereas there is a slight peak at 260 nm when measured with Nanodrop. My 230:260:280 ratio is more like this: 1.6:0.8:0.5.
I adapted my fieldwork sampling protocol from Foote et al. (2012). Based on the literature search, and similar problems people have experienced, I do think that the high peak at 230 nm is due to some salt contamination along with residual ethanol. I am in the midst of troubleshooting, but I am not sure how to fix this problem. There are people suggesting to use ether (to remove organic solvents) or to dialyse the probe if salt is the contaminant. Also, during PCR some additional reagents can be used, such as BSA and/or glycerol to prevent any potential inhibitors getting amplified.
Any suggestions on how to carry out? I would like to have purified DNA before troubleshooting with PCR step, ideally.
http://www.plosone.org/article/info%3Adoi%2F10.1371%2Fjournal.pone.0041781