Protocols
- Protocols
- Competent Cells Protocol
- hTERT-RPE serum starvation for synchronization
- Immunofluorescence Protocol
- hTERT-RPE serum starvation for synchronization
- Flow Cytometry Manuals
- Fork regression/restoration/footprinting
- SMARCAL1 DNA binding ATPase assays
- PI and BrdU Flow Cytometry Protocols
- Rong’s 293T suspension+mass spec
- Lysis with DNAse for all nuclear proteins including histones
- DNA Combing Protocol
- DNA fiber labeling
- Comet Assay
- Nascent ssDNA IF assay
- 53BP1 foci
- Retro/Lentivirus production
- PEI transfection of 293T cells
- siRNA transfection optimization
- Flag-His purification mammalian cells
- ATRflox cells Cre
- ATR kinase assay
- G2/M checkpoint assay
- Freezing/Thawing cells in Liquid Nitrogen
- RPA-ssDNA pull down
- GST protein purification from bacteria
- Bacterial expression/His purification
- HeLa siRNA/plasmid transfection
- Protein solubility test in E.coli
- Culture cells (300,000-400,000) on glass coverslip (6 well dish) for 24 hours prior to treatment with aphidicolin.
- Add 0.2 uM aphidicolin to treated wells and incubated at 37C for 24 hours.
Fixation and Permeabilization
- Aspirate off DMEM and rinse once in PBS. Aspirate off PBS.
- Thaw tube of 3% paraformaldehyde/2% sucrose fixative in water bath. Add 2ml paraformaldehyde/sucrose solution to each well of cells and incubated for 10 min at room temperature.
- Rinse 2 times with PBS, aspirated off. Add 0.5ml of cold Triton X-100 solution to each well and incubate 5 minutes on ice.
- Rinse well 4-5 times in PBS.
- Blocked with 5% BSA in PBS for 15 minutes at room temperature.
Immunostaining
- Spin antibodies down for 5 minutes at 13,000 rpm to remove debris (MAB 33802 mouse anti-53BP1, Sc-571 rabbit anti-Cyclin A).
- Place parafilm on top of lid of plate and made dilution of MAB33802 at 1:500 and Sc-571 at 1:200. Diluted antibodies in 3% BSA.
- If using small coverslips put 50ul (100ul for large coverslips) of antibody dilution onto parafilm and place coverslip onto the antibody solution with the cell side facing down.
- Incubated for 1 hour at 37C in humidity chamber to prevent drying out.
- Rinse twice in PBS for 2 minutes each wash.
- Repeat steps 6-9 with secondary antibody. Used Alexaflour 594 goat anti-mouse (red) at 1:500 and Alexaflour 488 goat anti-rabbit (green) and incubated for 30 minutes at 37C in humidity chamber.
- Wash with PBS 3 times.
- Label slides and place 5ul of Prolong Gold+DAPI mounting solution onto slide.
- Pull up coverslip out of well and dry the back with vacuum (non-cell side) and place cell side down onto slide containing Prolong.
- Gently push down with syringe tip to remove bubbles and then press gently with whatman paper.
- Store in slide holder at room temperature and let sit overnight.