Master Protocol Details



Notes:	AM Bufer: 670 mM TrisHCl pH 8.8, 166 mM (NH4)2SO4, 20 mM MgCl2, 1.7 mg/ml BSA, 10 mM 2-mercaptoethanol (Add 2-mercaptoethanol to 10 mM just prior to use. Do not store with 2-mercaptoethanol in buffer.)
Expected Results:	Transgene (Reaction A) = primers flank CAG repeat so size will vary depending on CAG repeat number ({CAG repeat number x 3} + 221bp) Transgene (Reaction B) = 170 bp (primers do not flank CAG repeat)

Gel Image

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Gel Information:	Separated by gel electrophoresis on a 2.0% agarose gel.

Protocol Primers

Primer	5' Label	Sequence 5' --> 3'	3' Label	Primer Type
oIMR1594	-	CCG CTC AGG TTC TGC TTT TA	-	Transgene Forward
oIMR1596	-	TGG AAG GAC TTG AGG GAC TC	-	Transgene Reverse
oIMR6533	-	GGC TGA GGA AGC TGA GGA G	-	Transgene Reverse

Reaction/Components

Reaction Component	Volume (µl)	Final Concentration	Total Volume (µl)
ddH2O	5.14	-	5.14
10 X AM Buffer	1.20	1.09 X	1.20
25 mM MgCl2	0.96	2.18 mM	0.96
2.5 mM dNTP	0.96	0.22 mM	0.96
20 uM oIMR1594	0.24	0.44 uM	0.24
20 uM oIMR6533	0.24	0.44 uM	0.24
DMSO	1.20	-	1.20
5 U/ul Taq DNA Polymerase	0.06	0.03 U/ul	0.06
DNA	1.00	-	1.00

Cycling

Step #	Temp °C	Time	Note
1	94	3 min	-
2	94	30 sec	-
3	58	1 min	-
4	72	3 min	repeat steps 2-4 for 35 cycles
5	72	2 min	-
6	10	-	hold**

Reaction/Components

Reaction Component	Volume (µl)	Final Concentration	Total Volume (µl)
ddH2O	5.14	-	5.14
10 X AM Buffer	1.20	1.09 X	1.20
25 mM MgCl2	0.96	2.18 mM	0.96
2.5 mM dNTP	0.96	0.22 mM	0.96
20 uM oIMR1594	0.24	0.44 uM	0.24
20 uM oIMR1596	0.24	0.44 uM	0.24
DMSO	1.20	-	1.20
5 U/ul Taq DNA Polymerase	0.06	0.03 U/ul	0.06
DNA	1.00	-	1.00

This genotyping protocol is used for the following strains:

Genotyping resources and troubleshooting
This page contains guidelines, frequently asked questions, and helpful external links to genotyping and PCR resources.

Cycling

Step #	Temp °C	Time	Note
1	94	3 min	-
2	94	30 sec	-
3	55	1 min	-
4	72	1 min	repeat steps 2-4 for 35 cycles
5	72	2 min	-
6	10	-	hold**