MNase Digestion
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- injecting the rats with sodium pentobarbitol
- transcardial perfusion 100ml/2min Saline nitride heparine for each rat
- transcardial perfusion with 400ml/4min 1% phospahte buffered paraformaldehyde
- Dissect rat adrenal gland and put in PBS on ice and tranfer to the lab
- Separate medulla in PBS (the tissues were in PBS around 60 min)
- 4 medullas in Dounce homogenizer in 1ml PBS,
- Quenching by adding with 1/20 of stock Glycine (2.5M), final concentration is 125mM
- homogenize the tissues and let the tube sit for 5 min at RT
- Spinning down the cells at 16000rcf, supernatant is removed
- The cell pellet is resuspended in 1ml Nucleus Isolation Buffer (NIB) (10mM HEPES at pH 7.8, 2mM MgoAc2, 0.3M sucrose, 2mM CaCl2, 1%Triton-X) let the tube sit for 10 min at RT
- Spinning down the cells at 1000rcf, supernatant is removed
- resuspend the cells in 1ml NIB
- Spinning down the cells at 1000rcf, supernatant is removed
- resuspending the cells in 500 µl in NIB
- prewarm the cells ar 37°C form 1 min
- Prepare 2 MNase digestion reaction (total volume 250µl each), MNase stock concentration : 20U/µl diluted to 2 U/µl
- 1: add 5µl of 2U/µl to get 10U, 10min, RT
- 2: add 2.5µl of 20U/µl to get 50U, 10min, RT
- Stop the reaction with 10 µl EDTA(500mM), the final concentration was 20mM
- Add 6.25µl of 20%SDS (final concentration 0.5%)
- Adding 2.5µl of Proteinase K 20mg/µl) (final concentration 0.2 µg/l)
- Incubate at first 55 C for 1-2 hours and then overnight at 65 C
- add 2.4µl RNAse (final concentration 50µg/ml) for 20min at 37° C
- DNA Purification with just Phenol:cholorophorm:isoamyl and Ethanol precipitation