pentadecamer library post in-fusion 4-19-13
2014-08-29azim58 - pentadecamer library post in-fusion 4-19-13
4-19-13
Finished ethanol precipitation after the in-fusion.
Ran 1 uL of each sample out onto a gel.
see
"F:\kurt\storage\CIM Research Folder\DR\2013\4-19-13\electroeluted
library\gel of electroeluted library 4-19-13.svg"
This is a gel of the electroeluted library after ethanol precipitation,
an in-fusion reaction, and another ethanol precipitation.
Estimated percent recovery from original cDNA synthesis amount to the
cDNA now after an electroelution, ethanol precipitation, in-fusion, and
another ethanol precipitation.
132*"ng"/(2133*"ng")*100.0 = 6.19%
see 4-10-13 experiment for the gel of the original cDNA which was used to
determine the 2133 ng amount.
1 = 4T1 cDNA created from random pentadecamers (13.2 ng/uL)
2 = Positive control eluted (2.7 kb PUC19 and 2 kb control insert) (0.17
ng/uL)
3 = Positive control (2.7 kb PUC19 and 2 kb control insert) (5.97 ng/uL)
4 = Negative Control (2.7 kb pSMART2IFD) (0.46 ng/uL)
- Electroporation
How do they do it in the SMARTer In-Fusion directional manual?
They just transform their full 10 uL In-fusion reaction without
quantitating anything.
How do I usually do it?
I use 10 pg to 100 ng.
Let's say I use 1 uL which uses 13.2 ng of DNA. How many colonies would I
have if I assumed a 5e6 cfu/ug transformation efficiency
5e6*"cfu"/"ug"*1*"ug"/(1000*"ng")*13.2*"ng" = 66,000 cfu
1e8 cfu -> 1.32e6 cfu
I'll just try an electroporation using 2 uL of the solution I have and
see what kind of transformation efficiency I get.