BCR 2.0 Cloning Progress 07/01

pEXPR 1-pLac:mKate-2

pEXPR TRE:Syk-pTet:RFP-TEVp

pEXPR TRE:Syk-pTet:RFP-tTEVp

Notes

all three tTEV constructs are correct. TEV #3 is correct

tube name	Constants Definition	2-log ladder	pEXPR 1-pLac:mKate-2	pEXPR 1-pLac:mKate-2	pEXPR 1-pLac:mKate-2	pEXPR 1-pLac:mKate-2	pEXPR 1-pLac:mKate-2	pEXPR 1-pLac:mKate-2	pEXPR 1-pLac:mKate-2	pEXPR TRE:Syk-pTet:RFP-tTEV	pEXPR TRE:Syk-pTet:RFP-tTEV	pEXPR TRE:Syk-pTet:RFP-tTEV	pEXPR TRE:Syk-pTet:RFP-TEV	2-log ladder	pEXPR TRE:Syk-pTet:RFP-TEV	pEXPR TRE:Syk-pTet:RFP-TEV	pEXPR TRE:Syk-pTet:RFP-TEV
Tube Number			1/1	1/2	1/3	2/1	2/2	2/3	1/2	B1	B2	B3	C1		C2	C3	C2
gel lane	0	1/1	1/2	1/3	1/4	1/5	1/6	1/7	1/8	1/9	1/10	1/11	1/12	NaN	2/1	2/2	2/3
DNA mass desired (ng)	500	500	500	500	500	500	500	500	500	500	500	500	500	500	500	500	500
total volume(ul)	20	20	20	20	20	20	20	20	20	20	20	20	20	20	20	20	20
DNA concentration (ng/ul)			332.8	253.5	358.6			360.9	253.5	245.9	294.3	280.5	338.5		213.9	254.8	213.9
Enzyme Name			NheI	NheI	NheI	NheI	NheI	NheI	undigested	PvuII	PvuII	PvuII	PvuII		PvuII	PvuII	undigested
Buffer Name			2.1	2.1	2.1	2.1	2.1	2.1	water	3.1	3.1	3.1	3.1		3.1	3.1	water
gel/lane	0	1/1	1/2	1/3	1/4	1/5	1/6	1/7	1/8	1/9	1/10	1/11	1/12	NaN	2/1	2/2	2/3
DNA volume		#DIV/0!	1.50	1.97	1.39	#DIV/0!	#DIV/0!	1.39	1.97	2.03	1.70	1.78	1.48	#DIV/0!	2.34	1.96	2.34
buffer volume	2	2	2	2	2	2	2	2	2	2	2	2	2	2	2	2	2
enzyme volume	1	1	1	1	1	1	1	1	1	1	1	1	1	1	1	1	1
strip tube #		1/1	1/2	1/3	1/4	1/5	1/6	1/7	1/8	1/9	1/10	1/11	1/12	2/1	2/2	2/3	2/4
water volume	17.0	#DIV/0!	15.5	15.0	15.6	#DIV/0!	#DIV/0!	15.6	15.0	15.0	15.3	15.2	15.5	#DIV/0!	14.7	15.0	14.7
gel/lane	0	1/1	1/2	1/3	1/4	1/5	1/6	1/7	1/8	1/9	1/10	1/11	1/12	NaN	2/1	2/2	2/3
loading dye	4	4	4	4	4	4	4	4	4	4	4	4	4	4	4	4	4
results			good	bad, pZDonor	good	bad pick	bad pick	bad		good	good	good	???		contaminated	good
notes

SDM

SDM 2,3, and 4/5 were run.

4/5 resulted from a mislabelling issue in which one sample is referred to by both numbers 4 and 5. This is one sample, not two, and no other samples are titled SDM 4 or SDM 5.

PCR Conditions:

SDM2 - Correcting CD79B Point Mutation from PCR - QuickChange Mutagenesis Q5 protocol 5 min elongation time, 70C annealing temperature

SDM3 - Correcting CD79B Point Mutation from PCR (Same as above, different protocol) - Golden Gate Mutagenesis Q5 protocol 5 min elongation time, 67C annealing temperature

LR

hEF1a:CymR

hEF1a-CuO:mKate

CMV5-Cuo:mKate

(pDEST_Seq4-Seq5)

Child pages

BCR 2.0 Cloning Progress 07/01

SDM

LR