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I isolated gDNA, amplified 3 target genes via PCR, performed a PCR-clean up, diluted my pcr products, applied 1.5 ”l of my dilutions on a positively charged nylon membrane, UV-crosslinked, etc (everything according to the manual of DIG High Prime DNA labeling and Detection Starter Kit I, Roche). This worked fine for the pcr products after NBT/BCIP coloration: spot intensities decreased with increasing dilutions.
But: I wanted to do the same using gDNA (in comparison to the pcr products). I had 8 (very simple) dilutions. result: first 3 spots were visible and they had all the same intensity. Although I doubted it was a problem of dilution, I repeated the whole procedure with new dilutions, and again: pcr dilution row was fine whereas gDNA dilution row showed same intensities
any suggestions what the problem might be? I have no plausible explanation for this...
regards
