Haynes Lab:Notebook/CRISPR Editing/2015/05/22: Difference between revisions

05/22/2015

SYBR qPCR to determine plasmid counts for dilution experiment

Step 1: make two PCR tubes for each sample with the following volumes of water and gDNA for 2ng of gDNA per well

'	1rxn	x3.5 = 7ng
gDNA	x
water	to 4.5
Total	4.5	15.75

Tube label	Cell type	gRNA	ug DNA	ul lipo	rep	ng/µL	dilute 1:20	ul dilution	ul water
1	Gal4-EED	g034	0.5	3	1	81.058	4.0529	1.73	14.02
2	Gal4-EED	g034	0.5	3	2	86.697	4.33485	1.61	14.14
3	Gal4-EED	g034	0.5	5	1	23.89	1.1945	5.86	9.89
4	Gal4-EED	g034	0.5	5	2	24.767	1.23835	5.65	10.10
5	Gal4-EED	g034	1	3	1	85.32	4.266	1.64	14.11
6	Gal4-EED	g034	1	3	2	70.244	3.5122	1.99	13.76
7	Gal4-EED	g034	1	5	1	13.387	0.66935	10.46	5.29
8	Gal4-EED	g034	1	5	2	23.213	1.16065	6.03	9.72
9	water								15.75

Step 2: make primer master mixes. Will have to add 3.5x to each triplicate gDNA tube so can calculate mastermixes from that

8 samples, 2 tubes/sample, 1 tube for no template control, total of 17 tubes

'	1rxn	3.5/triplicate tube	17.7
primer	3	10.5	185.85
SYBR	7.5	26.25	464.625
Total	10.5	36.75	650.475

Step 3: mix gDNA and primer mixes

Add 36.75ul primer mix to each sample tube

Step 4: pipette plate

mix tubes immediately before pipetting, add 15 ul from each tube into 3 wells

'	1-3	4-6	7-9	10-12
A	__1 G__	__1 C__	blank-G	______
B	__2 G__	__2 C__	blank-C	______
C	__3 G__	__3 C__	______	______
D	__4 G__	__4 C__	______	______
E	__5 G__	__5 C__	______	______
F	__6 G__	__6 C__	______	______
G	__7 G__	__7 C__	______	______
H	__8 G__	__8 C__	______	______