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AGOROSE GEL PROBLEM

Discussion of all aspects of biological molecules, biochemical processes and laboratory procedures in the field.

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AGOROSE GEL PROBLEM

Postby biolog35 » Mon Aug 18, 2008 11:46 am

ı have really interesting problem.ı digested my plasmid DNA(2.5ug).To control digestion ı loaded 5 ul rxn mixture into well and ı see an excellent band.After checkıng dıgestıon ı dephosphorylated plasmıd DNA and loaded all mıxture into another weel but ı could not see any band :( ı could not understand reason.any idea? please
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Postby Cat » Tue Aug 19, 2008 2:19 pm

You need to purify your DNA prior to running your gel. Salts and other impurities can interfere with the electrophoresis.
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Re:

Postby canalon » Tue Aug 19, 2008 5:09 pm

Cat wrote:You need to purify your DNA prior to running your gel. Salts and other impurities can interfere with the electrophoresis.

:shock: Never heard that. I use electrophoresis to purify DNA...

As for the original question. Besides contamination of reagents by DNAse (it happened to someone I knew), there is no reason the DNA should disappear. The question is how much DNA in "all the mixture"? And did you had a purification step between the digestion and the dephosphorylation. If something went wrong at that step, that might explain your problems
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