Haynes Lab:Notebook/CRISPR Editing/2014/08/07: Difference between revisions

Revision as of 09:01, 7 August 2014

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08/07/2014

CRISPR on chromatin: transfections of g21, g22, g27 into Gal4EED/luc cells
Luc-mCh swap: building the donor sequence
SURVEYOR for C-on-C and mCherry

CRISPR on chromatin: transfections

gRNA21/Cas9, dox+
gRNA22/Cas9, dox+
gRNA27/Cas9, dox+
gRNA21/Cas9, dox-
gRNA22/Cas9, dox-
gRNA27/Cas9, dox-

On 8/05/14, cells were grown in 4 mL P/S-free medium to ~80% confluence in a 6-well plate, 3 with 1 μg/mL dox, 3 without dox

Luc-mCh swap: building the donor sequence

Designed nested PCR primers to gradually build homology arms onto mCherry. The resulting donor should...
- Place mCherry in-frame upstream of the luciferase gene
- Add an ATG start codon onto mCherry (we had to use KAH154 as a template, where mCherry has no start)
- Add a double stop (TAATAG) onto the end of mCherry
- Add 130 bp of homology with TK-luciferase to each end

SURVEYOR assay for C-on-C and mCherry

@@ Line 10: / Line 10: @@
 * CRISPR on chromatin: transfections of g21, g22, g27 into Gal4EED/luc cells
 * Luc-mCh swap: building the donor sequence
+* SURVEYOR for C-on-C and mCherry
@@ Line 33: / Line 34: @@
 ** Add a double stop (TAATAG) onto the end of mCherry
 ** Add 130 bp of homology with TK-luciferase to each end
+----
+'''SURVEYOR assay for C-on-C and mCherry'''

Haynes Lab:Notebook/CRISPR Editing/2014/08/07: Difference between revisions

Revision as of 09:01, 7 August 2014

08/07/2014

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