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Functional Genomics for Drosophila
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Chromatin immunoprecipitation (ChIP) protocol from Drosophila embryos

Overview

Target DNA binding protein that has been cross-linked to chromatin (which has been sheared) will be purified using antibodies raised against the specific target protein. Staphylococcus aureus cells (SAC) will be used to purify antibody/chromatin complex via protein A expressed on the bacterial cell surface. Protein A coupled to a support could be used but SAC is cheaper and it has a higher binding capacity than the equivalent amount of protein A beads that are commercially available.

Fixed chromatin solution will be precleared with SAC to remove non-specific binding of components before addition of antibody to the chromatin solution. After sufficient time for antibody/chromatin interaction this complex is purified using a fresh batch of SAC. The antibody/chromatin/SAC complex is washed and the antibody/chromatin complex is eluted using a SDS/low salt buffer. RNAase is added to remove any RNA and the cross linking is reversed by heating. Following an ethanol precipitation, protein is removed using proteinase K treatment and phenol/chloroform extraction. After another ethanol precipitation, a solution containing enriched DNA fragments (which were bound by the target protein) is produced.

This protocol was developed by Rob White's laboratory. This is a modification of the Farnham laboratory mouse protocol (http://genomecenter.ucdavis.edu/farnham/farnham/).

Unless otherwise stated, all centrifugations are at full speed in a standard microfuge.

Equipment and reagents

*See solutions and reagents

Solutions and reagents

Dialysis buffer

Reagent stock concentration Working concentration required Amount required / 50 ml
500mM EDTA.Na2, pH 8 2 mM 200 µl
1M Tris.HCl, pH 8 50 mM 2.5 ml
Sarkosyl* 0.2% 100 mg
Water   Make to 50 ml

This buffer should be made up the day before as the detergents take a while to dissolve. Heating at 37 °C helps.
*Omit for monoclonal antibodies.

10 x PBS; pH 7.4

Make to a total volume of 1 litre

PBS/SDS/BME solution

Reagent stock concentration Working concentration required Amount required / 10 ml
10X PBS 1X 1 ml
10% SDS 3% 3 ml
beta-mercaptoethanol 10% 1 ml
Water   Make to 10 ml

Nuclear lysis buffer

Autoclave without SDS and then add appropriate amount of SDS from 10% stock.

Protease inhibitors:

Protease inhibitor Stock concentration Working concentration Amount required per ml Comments
Aprotinin 2.2 mg/ml 3.3 µg/ml 1.5 µl Dissolve in water, store at 4 °C.
Leupeptin 10 mg/ml 10 µg/ml 1 µl Dissolve in water, store at 4 °C.
Pepstatin 2 mg/ml 4 µg/ml 2 µl Dissolve in methanol, store at -20 °C. Heat to 48 °C to dissolve before storage.
AEBSF, hydrochloride* 100 mM 1 mM 10 µl Dissolve 100 mg in 4.18 ml water, store at 4 °C. This is a non-toxic alternative to PMSF

*4-(-2-Aminoethyl) benzenesulfonlyfluoride, HCl

IP Dilution Buffer

Reagent stock concentration Working concentration required Amount required / 50ml
10% SDS 0.01% 50 µl
20% Triton X-100 1.1% 2.75 ml
500 mM EDTA.Na2, pH 8 1.2 mM 120 µl
1M Tris.HCl, pH 8 16.7 mM 835 µl
4M NaCl 167 mM 2.09 ml
Water   Make to 50 ml

IP wash buffer

Reagent stock concentration Working concentrationrequired Amount required / 50ml
1M Tris.HCl, pH 9* 100 mM 5 ml
1M LiCl 500 mM 25 ml
10% Nonidet P40 (NP40) 1% 5 ml
Deoxycholic acid 1% 0.5 g
Water   Make to 50 ml

This buffer should be made up the day before because the detergents take a while to dissolve. Heating at 37 °C helps.
*pH 8 for monoclonal antibodies

IP Elution buffer

Reagent stock concentration Working concentration required Amount required / 50ml
1M NaHCO3 50 mM 2.5 ml
10% SDS 1% 5 ml
Water   Make to 50 ml

TE buffer

Reagent stock concentration Working concentration required Amount required / 50ml
1M Tris.HCl, pH 8 10 mM 0.5 ml
500mM EDTA.Na2, pH 8 1 mM 100 µl
Water   Make to 50 ml

5X PK Buffer

Reagent stock concentration Working concentration required Amount required / 50ml
1M Tris.HCl, pH 7.5 50 mM 2.5 ml
500mM EDTA.Na2, pH 8 25 mM 2.5 ml
10% SDS 1.25% 6.25 ml
Water   Make to 50 ml

Protocol

Preparation of Staphylococcus aureus cells (SAC):

  1. Resuspend Zymed Protein A reagent in 10 ml water.
  2. Centrifuge at 5000 rpm (4400 x g) for 5 minutes at 4 °C in 15 ml Falcon tubes (or equivalent) in the Sigma 4K10 bench top centrifuge.
  3. Discard supernatant and resuspend pellet in 10 ml dialysis buffer.
  4. Repeat steps 2 and 3.
  5. Repeat step 2, discard supernatant and resuspend in 3ml PBS/SDS/BME solution. Aliquot into 6 microfuge tubes and boil in water bath for 30 minutes.
  6. Centrifuge for 5 minutes at room temperature.
  7. Discard supernatant and resuspend in 1 ml Dialysis Buffer.
  8. Repeat steps 6 and 7.
  9. Discard supernatant and resuspend pellets in final volume of 4 ml Dialysis Buffer.
  10. Store as 100 µl aliquots at -20 °C.

Chromatin immunopurification procedure:

Day 1
  1. Thaw out 100 µl aliquot of SAC and add 20 µl Bovine Serum Albumin to preblock SAC.
  2. Incubate overnight at 4 °C on a roller (3 hours is fine).
Day 2
  1. Centrifuge blocked SAC for 1 minute, discard supernant and resuspend in 100 µl of 1X dialysis buffer. Add 1ml of Dialysis Buffer and invert to mix.
  2. Repeat step 13.
  3. Centrifuge for 1 minute, discard supernatant and resuspend in 100 µl of Dialysis Buffer. Store on ice until required.
  4. To preclear chromatin, thaw out chromatin aliquot and add 15 µl blocked SAC to each chromatin aliquot. Rotate on roller at 4 °C for 15 minutes.
  5. Centrifuge for 1 minute and transfer supernatant to fresh tube.
  6. Repeat step 17 and transfer supernatant to fresh tube.
  7. To fresh tube add chromatin (for Heat Shock Factor experiments we used 20-25 µl) to a total volume of 100 µl (use nuclear lysis buffer to make the volume up). Add 200 µl IP Dilution Buffer. Add serum (for Heat Shock Factor (HSF) we used 1 µl of pre-immune or anti-HSF antiserum). Incubate overnight at 4 °C on roller.
  8. Set up a fresh aliquot of SAC and block overnight, as per steps 11 to 12.
Day 3
  1. For monoclonal antibodies only, add 1 µg of an appropiate secondary antibody that binds to Protein A and incubate for an additional hour at 4 °C on roller. Only omit this step when working with a polyclonal antibody that binds to Protein A.
  2. Process overnight blocked SAC, as per steps 13 to 15.
  3. Add 10 µl SAC (from step 22) to each IP reaction. Rotate for 15 minutes at room temperature.
  4. Centrifuge for 1 minute, remove supernatant and discard. Pulse spin, then remove remaining residual fluid. Resuspend pellet in 200 µl Dialysis Buffer using pipette tip. Add 1 ml Dialysis Buffer and invert to mix.
  5. Incubate on roller at room temperature for 3 minutes.
  6. Repeat steps 24-25 once.
  7. Centrifuge for 1 minute, remove supernatant and discard. Pulse spin, then remove the remaining residual fluid. Resuspend pellet in 200 µl IP Wash Buffer using pipette tip. Add 1 ml IP Wash Buffer and invert to mix.
  8. Incubate on roller at room temperature for 3 minutes.
  9. Repeat steps 27-28 three times.
  10. Centrifuge for 1 minute, remove supernatant and discard.
  11. Resuspend pellet in 150 µl IP Elution Buffer and vortex at setting 3 for 15 minutes at room temperature.
  12. Centrifuge for 1 minute and transfer supernatant to fresh tube.
  13. Repeat step 31.
  14. Centrifuge for 1 minute and pool supernatant with that of step 32. Centrifuge for 5 minutes and transfer to fresh tube.
  15. Add 1 µl RNase (stock 10 mg/ml, in water) and 22.5 µl 4M NaCl (final concentration 0.3M). Incubate samples at 67 °C for 4-5 hours to reverse cross-linking.
  16. Cool for 1-2 minutes on ice. Add 812 µl ice-cold ethanol, mix by inversion and store at -20 °C overnight.
Day 4
  1. Centrifuge at 4 °C for 20 minutes and remove supernatant.
  2. Pulse spin and remove remaining residual fluid.
  3. Air dry for 1 hour.
  4. Resuspend pellet (quite large and white) in 100 µl TE.
  5. Add 25 µl 5X PK buffer and 1.5 µl proteinase K. Incubate at 45 °C for 2 hours.
  6. Add 175 µl TE to each sample. Add 300 µl phenol/chloroform/isoAmyl alcohol and vortex to mix.
  7. Centrifuge for 1 minute and carefully remove upper aqueous layer to fresh tube.
  8. Add 300 µl chloroform and centrifuge for 1 minute. Carefully remove upper aqueous layer to fresh tube.
  9. Add 37.5 µl 4M NaCl, 10 µg (0.5 µl) glycogen, and 750µl ethanol (ice-cold). Store overnight at -20 °C.

Please note, instead of perfoming steps 42 to 48, it is possible to purify the genomic DNA using a QIAquick PCR purification kit (Qiagen; Cat. No. 28104), as per the manufacturers instructions. Elution is either performed with water, when the material is to be used for a microarray experiments, or else, the Qiagen supplied elution buffer can be used, e.g., when performing a quality control test. This modification to the method increases yield; hence reducing the background signal after hybridisation for both standard and quality control extractions.

Day 5
  1. Centrifuge at 4 °C for 20 minutes and remove supernatant.
  2. Pulse spin and remove remaining residual fluid.
  3. Air dry pellet (small and white) for 1 hour and resuspend pellet in 30 µl water. Store at -20 °C.

Version 1.2. R. Auburn. (10-08-2006)