DMS Chemical Footprinting of RNA
Notes:
RNA should be at 1 uM concentration (1 pmole/uL) There are 3 conditions (use a blank/background reaction for each condition).
Solutions
CE Buffer (10X)
- 1M Na Cacodylate (4.28 g into 20mL H2O) pH 7.4
- 5 mL of 1 M Na Cacodylate
- 100 uL of 0.5 M EDTA
- 44.9 mL H2O Sterile filter and allow vacuum to continue 5 mins. to allow for degassing.
1X CE Buffer
- 1 mL 10X CE
- 9 mL H2O
DMS Solution:
- 15 uL 100% ETOH
- 3 uL DMS
Quench Solution:
- 1.4 mL 2-beta-mercaptoethanol
- 0.5 mL 3 M Sodium Acetate (Ambion Buffer kit)
- 3.1 mL H2O
*Dilute RNA to 1 uM in 1x CE buffer
Conditions
Condition 1:
10 uL RNA (1 uM concentration) 2.5 uL 10x CE buffer 12.5 uL H2O
Condition 2:
10 uL RNA (1 uM concentration) 2.5 uL 10x CE buffer 1.25 uL 2 M KCl (Ambion Buffer kit) 11.25uL H2O
Condition 3:
10 uL RNA (1 uM concentration) 2.5 uL 10x CE buffer 1.25 uL 2 M KCl (Ambion Buffer kit) *1.25 uL 100 mM MgCl2 (diluted from 1M MgCl2 Ambion Buffer kit) 10 uL H2O *DO NOT ADD MgCl2 UNTIL READY TO INITIATE FOLDING.
Procedures
Folding Steps
Heat the 25 ul (Mg free) reaction mix at 90C for 3 mins. Take the sample out and let it cool to room temperature for about 10-15 mins-, after which give a quick spin on a table top centrifuge. Put the sample in a 50C heating block and let it equilibriate at 50C for 10 mins. Add MgCl2 (final Mg concentration 10 mM) to samples. Place sample in a 50C heating block for 15-30 mins. Take the sample out and put it in a heating block set at the folding temperature (25C or 37C). Incubate at the folding temperature for 1 hour. Initiate modification reaction (OH footprinting/DMS....etc.) at the same temperature used for folding (25C or 37C). Similarly, we prepare the unfolded sample in an identical way but skip the addition of MgCl2 at step 3.
DMS modification
To the 12.5 uL of folded RNA, add 0.5 uL of DMS solution Incubate for 2 minutes at 25C or 37C. Add 475 uL of quench solution (even to samples without DMS mod) Add 1 mL of 100% ETOH Freeze O/N at -80C Prepare RNA for RT
Reverse Transcription
Spin down samples at 14,000 RPM at 4C for 1 hour Remove supernatant Rinse with 100 uL of 70% ETOH Spin at 14,000 RPM at 4C for 0.5 hours Remove supernatant and dry pellet in speed-vac, medium heat for 3 mins.
RT Buffers
Annealing Buffer (50 mM Tris-CL, pH 8.3, 60 mM NaCl, and 10 mM DTT)
| Tris-Cl | 5 uL |
| NaCl | 1.1 uL |
| DTT | 10 uL |
| H2O | 83.9 uL |
| Total volume | 100 uL |
Reverse Transcription Mix
| 5x FS buffer | 4 uL per rx |
| 0.1 mM DTT | 1 uL per rx |
| RNase Out | 2 uL per rx |
| 10 mM dNTP mix | 2 uL per rx |
| *ddNTP 5 mM | 5 uL per rx |
| Superscript III enzyme | 1 uL per rx |
* Only use if doing a dideoxy sequencing reaction.
RT Reaction
Resuspend RNA pellet in 9 uL of annealing buffer Add 1 uL of cy5’ labeled primer at 10 uM Heat to 90C for 2 min. and slowly cool to 25C to allow primer to anneal. (1-1.5 hours) Note: Keep tubes in heat block and pull out whole block from heat. Use a thermometer to monitor the temp. Add 9 uL of reverse transcriptase mix Heat solution at 55C for 5 mins THEN add 1 uL of superscript III enzyme to each sample. Mix gently, briefly centrifuge, incubate at 55C for 10-15 mins.
Clean Up Sample
Add 2 uL of 2N NaOH Incubate at 95C for 3 mins. Add 2 uL of 2N HCl to neutralize Add 3 uL of 3 M Na-acetate Add 1 uL of 100 mM MgCl2 Add 90 uL of 100% ETOH Centrifuge at 14,000 RPM for 30 mins at 4C Remove supernatant Add 50 uL 70% ETOH Centrifuge at 14,000 RPM for 30 mins at 4C Dry pellet and re-suspend in 60 uL Sample Loading Solution (Beckman) Load 60 uL of sample in 96 well plate Add 1 uL of Ladder to each well Place drop of mineral oil on top and follow CEQ protocol
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