Caspases,Paracaspases, and Metacaspases Methods and Protocols

(Wang) #1
13


  1. Analyze a 10 μL aliquot from each fraction by SDS-PAGE. Pool
    the purest and most concentrated fractions. Proteins can be kept
    3–4 days at room temperature before proceeding to refolding.
    Optional: If higher protein concentration and purity are
    required, the following DEAE ion exchange purification proce-
    dure (steps 12– 16 ) is recommended. This procedure will help
    to remove some cleaved caspase-8.

  2. Pour 2 mL of DEAE Sephadex resin into an empty chroma-
    tography column (1.0 cm or less in diameter; e.g., Bio-Rad
    Econo-Pac 0.7 × 5.0-cm) and let the liquid drain by gravity
    flow. Rinse the resin twice with 5 bed volumes of Milli-Q water
    and then 5 bed volumes of urea buffer (DAY 6).

  3. Apply the pooled fractions containing caspase-8 (step 11) to
    the column and let drain.

  4. Wash the column with 5 bed volumes of urea buffer and let
    drain between each wash.

  5. Elute the protein with a step gradient of NaCl in urea buffer
    (0–400 mM; 10 fractions; 2 mL/fraction).

  6. Analyze a 10 μL aliquot from each fraction by SDS-PAGE.
    Pool the purest and most concentrated fractions. Proteins can
    be kept 3–4 days at room temperature before proceeding to
    refolding.


Note: Every step of this procedure is performed at room temperature.


  1. Centrifuge the pooled fractions from step 11 or step 16 in
    Subheading 3.1.2.2 for 15 min at 18,000 × g to remove insolu-
    ble proteins and residual resin. Transfer the supernatant to a
    dialysis tube (10,000 MWCO; prepared according to manufac-
    turer instructions) equilibrated in refolding buffer #1 (DAY 6).

  2. Dialyze overnight at room temperature against 1 L of refold-
    ing buffer #1. Stir buffer at low speed.

  3. The next day, dialyze for 5 h at room temperature against 1 L
    of refolding buffer #2. Stir buffer at low speed (DAY 7).

  4. Recover the dialyzed protein with a pipet.

  5. Centrifuge the protein solution for 30 min at 18,000 × g to
    remove any insoluble protein. Transfer the supernatant to a
    fresh tube.

  6. Determine the final protein concentration using a protein assay
    that is compatible with refolding buffer #2 (e.g., Pierce BCA
    protein assay). Use fresh refolding buffer #2 as a blank.
    Optional: Concentrate the caspase preparation using Millipore spin
    concentrators (10,000 MWCO).

  7. Active site titrate the caspase-8 according to Subheading 3.2.2.
    Assume a refolding yield of 5–10 % (see Note 17).


Refolding Full-Length
Caspase-8


Apoptotic Caspases Assays
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