Hi all,
I was wondering if there were other ways to determine the quality of a pcDNA3.1(+) plasmid? I have a plasmid that requires about 5x amount of total pcDNA to express my FLAG-tagged protein, compared to a plasmid containing the untagged protein. Could this be an issue of quality? I've already double checked the concentration.
Thank you!
Can run a gel and see how much is nicked supercoiled etc from batch to batch
The solution will depend on what level of protein expression you are looking to achieve. pCDNA has a CMV promoter and if your flag protein in under the CMV promoter it should be quite robust but if it is under the control of another gene and is acting as a reporter for that gene then this will dictate the quantity of DNA you use for transfection to get the desired result.
The quality of plasmids can be determined using an agarose gel electrophoresis experiment.
Please check the 260/280 absorbance ratio. If it is >1.9 - 2, you may have RNA present contributing to your quantitation, making it seem artificially higher than it is. The agarose gel suggestion is also a good one, especially if used with a marker of known DNA mass for comparison. Good Luck,
Ron
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