GoTaq PCR Genotyping

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Revision as of 16:21, 10 August 2010 by Kalefish (Talk | contribs) (Created page with '==Materials(100uM)== *GoTaq Master Mix *Primer Mix: Add 10uL of forward and reverse primer, 20uL total, into 1mL of dH20. *Reaction Mixture: 25uL GoTaq Mix, 10uL of Primer Mix, ...')

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Materials(100uM)

GoTaq Master Mix
Primer Mix: Add 10uL of forward and reverse primer, 20uL total, into 1mL of dH20.
Reaction Mixture: 25uL GoTaq Mix, 10uL of Primer Mix, 14uL Nuclease-Free Water, and 1uL of template
Gel: 0.3g Agarose to 30mL of TAE, microwave until dissolved and add 1uL of EtBr.

Procedure

Prepare gel 30 minutes before PCR is finished.
Prepare Reaction Mixture, adding 13x all materials except for the template.
Add this mixture to each PCR tube.
Label and add each template to the corresponding PCR tube.
Run PCR under genotyping>inoki (~1 hour)
Load samples in gel and run on 30V (horizontally.)

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