Haynes Lab:Notebook/CRISPR Editing/2016/09/02: Difference between revisions

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09/02/2016

qPCR of Luc14 31 and 34 treated ChIP samples

triplicate, IgG, FLAG, singlet inputs, technical triplicates, 313/311, GAPDH

Totally worked! Small error bars!

Started ChIPs on Gal4+puro and Gal4+dox g031 and g034

preclear with beads for 3 hours, nutation, 4deg

add FLAG beads

cut ends of tips to make wide bore

20ul beads/IP

wash 3x with TBS buffer

resuspend to original volume

add 20ul to empty tubes

put in magnet rack, remove TBS

add samples

add IgG to IgG samples

nutate overnight at 4deg

removed dox from Gal4+dox cells, expanded all cells to T-175s

@@ Line 24: / Line 24: @@
 :add IgG to IgG samples
 :nutate overnight at 4deg
+<br><br><br>
+removed dox from Gal4+dox cells, expanded all cells to T-175s
 <!-- ##### DO NOT edit below this line unless you know what you are doing. ##### -->

Haynes Lab:Notebook/CRISPR Editing/2016/09/02: Difference between revisions

Revision as of 20:23, 3 September 2016

09/02/2016

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