So this is a problem that has been inconsistent over the past year but has really become more prominent over the past few weeks - for practically every PCR I've run in order to genotype the mice we use for various genes, I will see faint product bands in the water control. Normally, I would contribute this to contamination, but instead of just seeing the same bands across all samples as you normally would if there's contamination, my samples will behave as 'normal', where either one or two bands will be present if the mouse being genotyped is heterozygous or homozygous for the gene of interest, or no band will be present at all if the mouse doesn't have the gene. If contamination is the issue, this shouldn't be the case, as I use the same water for the master mix and get varying results between the samples and the water control. My only other conclusions might be splash-over from other wells, although I tend to keep at least 1 well of space between my samples and the water control, or the formation of primer dimers, although those bands should be below 100bp, not at 200 or 300bp. Here is my typical method for preparing a PCR, in case anyone asks:

1. Prepare master mix - I do this separate from the DNA, and for the most recent PCR I replaced everything except for the primer aliquots I made a while ago

2. Add MM to pcr tubes - still separate from DNA, I follow the protocol I have for how much each sample should get

3. Add DNA to pcr tubes - I use new tips for each sample obviously, and know I'm not accidentally going into the wrong tubes and adding the wrong samples

4. Run the PCR

5. Add Loading Dye to PCR tubes

6. Load gel and run

Any thoughts? While the samples still show results that I would expect from a PCR done correctly, I don't trust them completely if the water control is acting like this, and obviously I need mice with specific genotypes for my experiments to work properly. Thanks for your help!

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