AGiR! for genomic integrity/cometassaydev

From Hackuarium
Jump to navigation Jump to search

This is the page where lab notes will be uploaded from runs of the cheek cell comet assay protocol...

CheekCellComet 2dec16slide2x10GFPb.jpg


Experiments

  • Cheek Cell comets

Conditions

  • tests of pbs vs saline
  • tests for optimal numbers of cells
  • tests of filtration vs gravity for eliminating big clumps of cells (1st attempt with lab 40micron filter run 8march2017, with Anna and Bastain)
  • tests for staining dyes
  • control conditions - negative control with no protease treatment, positive control with H2O2

Current 'best' protocol

1) isolate cells in saline solution (0.9% NaCl in water) after toothbrush collection - about 10ml solution Let biggest clumps settle away, and take remaining solution to pellet most cells (2ml eppi tube, 2k rpm, 2min), repeating until all solution is pelleted. Resuspend pellets and estimate cell concentration and quality under scope (can use hemocytometer for counting)

3) embed cells in 1% low melting point agarose (made up in standard saline solution)

- aiming for about 20,000 cells to be added to 100 microliters agarose (kept at 40oC)
- mix and put on clean microscope slide using a clean coverslip to flatten it in place.  (can flatten the cell suspension on top of a pre-made agarose base, if desired)

4) treat cell patches with first solutions: saline only, for test cases (3-5 replicates ideally); and H2O2 (0.01%) for positive control case.

5) equilibrate all cell patches with Proteinase K (PK) buffer (for 2ml: 40 microliters 0.5M Tris pH8, 400 microliters 0.5M EDTA, 1ml 5M NaCl, 20 microliters 1% Triton, 0.54ml H2O) x2 changes (drops of liquid, about 20-50 microliters depending on patch sizes)

6) treat cells with PK+ solution (final PK concentration at 0.5mg/ml: 5 microliters of 20mg/ml PK stock in 200 microliters PK buffer) keep at least one cell patch without this treatment as your negative control! RT incubation (watch under scope to see cells 'disappearing' leaving nucleoids - usually only about 20 minutes max)

7) as treatment seems sufficient, treat cell patches with 1X TBE pH9 (alkaline treatment) 2x 5 min

8) equilibrate all patches with normal 1X TBE 3x 2min

9) run the electrophoresis step: 12V 15 min (only 2 slides will fit easily in the gel box currently used in the lab, but other possibilities exist)

10) staining and imaging (most success with SYBR safe dye, diluted 1/10,000 in TBE for staining, and epifluor imaging, but hoping to assess alternatives that would form a nicely colored DNA 'comet tail' - neither Hemalum nor methylene blue seem very useful at all in this regard...)





Ideas for protocol improvement

More to come soon!!