I've faced a problem during my work.
In electrophoresis of ureC gene PCR product electrophoresis H pylori the the weight of gene band is 100bp more than the positive control weight while I observe a single sharp band in my electrophoresis.
Why the weight of my gene band is different from my positive control?
You might have thought about it but did you check the specificity of primers and the predicted product length?
Hi there,
UreC is around 1.4kb in size; A 0.1kb shift is not very easy to be sure of as apparent mobility of DNA fragments in agarose gel is dependent on parameters like quantity of DNA loaded, ionic strength of the samples. For instance if you run the same DNA sample with different concentrations of salt, the mobility will vary from one to an other. In conclusion, if you want to compare samples on agarose gel, make sure they have exactly the same contents in terms of composition and comparible DNA concentration.
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