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Immunoprecipitation of Acetylated Protein (or Peptides) with Anti-acetyl Lysine Agarose
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Immunoprecipitation Procedure
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1.
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Prepare beads: Gently resuspend the anti-acetyl lysine agarose beads and transfer the desired amount (typically 20–50 µl of bead slurry per sample) to a 1.5 mL vial.
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2.
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Wash beads:
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3.
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Incubate lysate: Add the prepared cell lysate (about 2 mg protein/50 µL beads) or digested crude peptide to the anti-acetyl lysine agarose beads and incubate on a rotor shaker at room temperature, for 120 minutes or 4oC overnight. (Increase the volume of the Agarose if a larger amount of crude protein sample is used).
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4.
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After incubation, wash the agarose beads with PBSt four times, through repeated centrifugation and aspiration. Finally wash with PBS to remove the Tween-20.
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Recovery of the Bound Acetylated Proteins
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For western blot:
Note: To detect acetylated lysine, it is recommended to use anti-acetyl lysine HRP conjugates (ICP0381). This avoids interference from IgG secondary antibodies.
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For Downstream Analysis:
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Note: do not use milk or milk products for blocking or for the solution, which may contain acetylated proteins.
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1.
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Pack a mini-column (as illustrated in the figure above):
Insert a small piece of glass wool at the bottom of a 5 mL pipette tip to act as a filter. Add 100 µL of anti-acetyl-lysine agarose slurry(equivalent to 50 µL bead volume) into the tip. Wash the beads sequentially as follows:
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2.
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Apply vacuum (optional): |
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3.
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Block the column:
Add 1 mL PBSt containing 1.5% BSA to the column and allow it to flow through naturally by gravity. |
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4.
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Load the sample: |
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5.
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Wash the column: Wash sequentially with:
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6.
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Elute the bound acetylated proteins/peptides: Elute with 120 µL of 0.5 M HCl. Discard the first 20 µL (void fraction), then collect 100 µL of the eluate. Freeze-dry or concentrate the eluted material for further analysis. If needed, neutralize the eluate with saturated Tris solution. |
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Note: do not use milk or milk products for blocking or for solution, which may contain acetylated proteins.
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