ChIP: Difference between revisions

This protocol is in development.~ cmc 15:03, 21 August 2006 (EDT)

Overview

Replace this sentence with a brief description of the protocol and its goal.

Materials

11% Formaldehyde Solution

per 50 ml: (Final concentration)

• 14.9 ml of 37% Formaldehyde (11%)
  
• 1 ml of 5M NaCl (0.1M)
  
• 100 µl of 0.5 M EDTA, pH 8 (1 mM)
  
• 50 µl of 0.5 M EGTA, pH 8 (0.5 mM)
  
• 2.5 ml of 1M Hepes, pH 8 (50 mM)
  

2.5 M glycine (187.5 g/L)

• Dissolve glycine in water with constant stirring
  
• Don’t adjust pH
  

BSA/PBS Solution

per 100 mL:

• 10 mL of 10x PBS
  
• 500 mg of BSA
  
• 90 mL of H20
  

(good for at least a week)

Lysis Buffer 1 (LB1)

per 100 ml: (final concentration)

• 5 ml of 1M Hepes-KOH, pH 7.5 (50 mM)
  
• 2.8 ml of 5M NaCl (140 mM)
  
• 0.2 ml of 0.5M EDTA (1 mM)
  
• 10 ml of glycerol (10%)
  
• 5 ml of 10% NP-40 (0.5%)
  
• 0.25 ml of Triton X-100 (0.25%)
  

Lysis Buffer 2 (LB2)

per 100 ml: (final concentration)

• 4 ml of 5M NaCl (200 mM)
  
• 0.2 ml of 0.5M EDTA (1 mM)
  
• 0.1 ml of 0.5M EGTA (0.5 mM)
  
• 1.0 ml of 1M Tris pH 7.5 (10 mM)
  

Lysis Buffer 3 (LB3)

per 100 ml: (final concentration)

• 0.2 ml of 0.5M EDTA (1 mM)
  
• 0.1 ml of 0.5M EGTA (0.5 mM)
  
• 1.0 ml of 1M Tris-HCl, pH7.5 (10 mM)
  
• 2 mL of 5M NaCl (100 mM)
  
• 1 mL of 10% Na-Deoxycholate (0.1%)
  
• 500 mg of N-lauroyl sarcosine (0.5%)
  

Wash buffer (RIPA buffer)

per 100ml: (final concentration)

• 5ml of 1M Hepes, pH 7.6 (50 mM)
  
• 200µL of 0.5M EDTA (1 mM)
  
• 7 ml of 10% DOC (Na deoxycholate) (0.7%)
  
• 10 ml of 10% NP-40 (IPGEL) (1%)
  
• 10 ml of 5M LiCl or 2.12g powder (0.5 M)
  

Elution buffer

• 50mM Tris pH8
• 1mM EDTA
• 1% SDS

Procedure

I. Cell cross-linking

• Use 5x107 – 1x108 cells (70-80% confluency for adhesion cells of 8-12 15 cm2 plates or 175 cm2 flasks) for each ChIP reaction.
  

• Adherent cells:
  1. Add 1/10 volume of fresh 11% formaldehyde solution to plates.
  2. Swirl plates briefly and let them sit at RT for 10 min.
  3. Add 1/20 volume of 2.5 M glycine to plates to quench formaldehyde.
  4. Rinse cells twice with 5 ml 1X PBS. Harvest cells using silicon scraper.
  5. Spin cells at 4k for 10’ at 4°C.
  6. Transfer cells to 15ml conical tubes and spin 4k 10’ at 4°C.
  7. Flash freeze cells in liquid nitrogen and store pellets at –80 °C.
• Suspension cells:
  1. Add 1/10 volume of fresh 11% formaldehyde solution to flasks.
  2. Swirl flasks briefly and let them sit at RT for 20 min.
  3. Add 1/20 volume of 2.5 M glycine to flasks to quench formaldehyde.
  4. Spin cells at 2500rpm for 10’ at 4°C.
  5. Rinse cells with 100ml 1x PBS and spin cells at 2500rpm for 10’ at 4°C.
  6. Rinse cells with 10ml 1x PBS and transfer to 15ml conical tubes and spin 4k 10’ at 4°C.
  7. Flash freeze cells in liquid nitrogen and store pellets at –80 °C.

II. Preblock and binding of antibody to magnetic beads

• Keep beads on ice for all steps

1. wash 100 µL Dynal magnetic beads (per reaction) in 1 ml fresh BSA/PBS
2. collect the beads with magnet wash beads in 1.5 ml BSA/PBS 2 times, collect the beads with the magnet.
3. Add 6-10 µg of Ab + 250µL of PBS/BSA.
4. incubate 4 hr to O.N. on a rotating platform at 4∞C.
5. wash beads 3 times in 1.5 ml PBS/BSA.
6. Resuspend in 100µL PBS/BSA.

III. Cell Sonication

IV. Chromatin Immunoprecipitation

1. Add 100 µL Ab prebound Dynal magnetic beads from step III.
2. Rock 4∞C 6 hrs to O/N.

V. Washing, eluting, and reverse cross-linking

VI. RNase, Proteinase K

Notes

1. List troubleshooting tips here.
2. You can also link to FAQs/tips provided by other sources such as the manufacturer or other websites.
3. Anecdotal observations that might be of use to others can also be posted here.

Please sign your name to your note by adding ('''~~~~''') to the end of your tip.

References

• ChIP protocol, Young Lab

Contacts

• cmc
• odom