Primer
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Linden
Jun 14, 2015, 10:20:44 PM6/14/15
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Hey guys,
I am designing a 40 bp primer (it is for homologous recombination in yeast), but part of it also anneal at another part of the plasmid, just like the drawing attached. Could it be a big issue? I dont have another plasmid with this gene..
Thanks a lot!
Jeswin
Jun 14, 2015, 10:59:36 PM6/14/15
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What's the size difference between the target fragment and the unwanted larger fragment? You could run one PCR and isolate your target fragment. Then use that DNA as template for a second PCR amplification.
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Linden
Jun 15, 2015, 2:00:49 PM6/15/15
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Thanks, Phillyj
Maybe I could digest it out of the plasmid, run an agarose gel, purify and then amplify. Probably ok, right?
Jeswin
Jun 15, 2015, 2:29:45 PM6/15/15
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On Mon, Jun 15, 2015 at 2:00 PM, Linden <ff.lin...@gmail.com> wrote:
>
> Thanks, Phillyj
>
> Maybe I could digest it out of the plasmid, run an agarose gel, purify and then amplify. Probably ok, right?
>
I don't know if you want to digest the plasmid and then PCR. It might
>
> Thanks, Phillyj
>
> Maybe I could digest it out of the plasmid, run an agarose gel, purify and then amplify. Probably ok, right?
>
be easier to do PCR on the plasmid and then cut out the smaller
(Target) band. I am assuming that you get 2 bands with good
resolution. You may end up with a smear on the gel (after 1st PCR) so
then maybe a plasmid digest would help isolate the specific region you
want.
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Mega [Andreas Stuermer]
Jun 16, 2015, 4:01:29 AM6/16/15
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The short band may be amplified prefferably by the reaction?
Do you have the sequence of the entire thing?
Digestion is a good idea, if there is a restriction site inbetween....
Do you have the sequence of the entire thing?
Digestion is a good idea, if there is a restriction site inbetween....
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