Difference between revisions of "GoTaq PCR Genotyping"

Latest revision as of 14:50, 6 December 2010

GoTaq Master Mix
Primer Mix (from 100uM Primer Stocks): Add 10uL of forward and reverse primer, 20uL total, into 980uL of dH20 to make a 1uM solution.
Reaction Mixture: 25uL GoTaq Mix, 10uL of Primer Mix, 15uL of template. If doing several samples make a master mix of primer mix + template (25 uL GOTaq + 10 uL Primer Mix)x # of Samples + 1
Gel: 0.3g Agarose to 30mL of TAE, microwave until dissolved and add 1uL of EtBr.

@@ Line 1: / Line 1: @@
-==Materials(100uM)==
+==Materials==
 *GoTaq Master Mix
-*Primer Mix: Add 10uL of forward and reverse primer, 20uL total, into 1mL of dH20.
+*Primer Mix (from 100uM Primer Stocks): Add 10uL of forward and reverse primer, 20uL total, into 980uL of dH20 to make a 1uM solution.
-*Reaction Mixture: 25uL GoTaq Mix, 10uL of Primer Mix, 14uL Nuclease-Free Water, and 1uL of template
+*Reaction Mixture: 25uL GoTaq Mix, 10uL of Primer Mix, 15uL of template.  If doing several samples make a master mix of primer mix + template (25 uL GOTaq + 10 uL Primer Mix)x # of Samples + 1
 *Gel: 0.3g Agarose to 30mL of TAE, microwave until dissolved and add 1uL of EtBr.
@@ Line 12: / Line 12: @@
 *Add this mixture to each PCR tube.
 *Label and add each template to the corresponding PCR tube.
-*Run PCR under genotyping>inoki (~1 hour)
+*Run PCR under appropriate [[Genotyping Program]]
-*Load samples in gel and run on 30V (horizontally.)
+*Load samples in gel and run on 130V (horizontally.)
+[[Category:Mouse Work]]
+[[Category:PCR]]
+[[Category:Genotyping]]