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Caspases,Paracaspases, and Metacaspases Methods and Protocols

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  1. After extensive washing with PBS, monospecifi c antibody is
    eluted with fi ve 0.5 ml aliquots of 0.1 M glycine-HCl buffer
    (pH 2.3) and immediately neutralized with 0.5 ml of 1 M
    Tris–HCl (pH 8.0).

  2. Measure absorbance at 280 nm in each fraction and calculate
    IgG concentration in mg/ml using formulae A280 × 0.714.

  3. Exchange buffer to PBS using PD-10 column equilibrated
    with PBS or dialyze against PBS. Store in small aliquots at
    −80 °C.


Cleavage-site-directed antibody (h14Y178) is prepared by immu-

nizing rabbits with synthetic hexapeptide CGYIAY, in which

GYIAY corresponds to the C-terminal end of p20 cleaved by

KLK7. h14Y178 can be purifi ed using above described procedure

for h14D146.

It is important to distinguish zymogen from the active form of

caspase-14, since proteolytic activation is a critical event for physi-

ological action of caspase-14. Here we describe two kinds of ELISA

quantifi cation assays using H99 antibody directed to the large

subunit of human caspase-14 (to measure total caspase-14) and

cleavage- site-directed antibody, h14D146 (to measure active

caspase- 14). We used in-house monoclonal anti-caspase-14 anti-

body, clone 3, as an immobilized antibody that showed the highest

sensitivity in the ELISA system. However, commercially available

mouse monoclonal antibody to caspase-14 can also be used.


  1. Immobilize 1 μg/ml of anti-caspase-14 (clone 3 or commer-
    cially available monoclonal antibody) in PBS by overnight
    incubation in a 96-well plate.

  2. Tap off the solution from the plate.

  3. Block by adding 200 μl/well of ImmunoBlock diluted with
    PBS and incubate for 1 h at room temperature.

  4. Tap off the solution from the plate and wash each well with
    200 μl of PBS containing 0.1 % Tween 20 (PBST).

  5. Add 100 μl samples (cell extracts) and incubate at 37 °C for
    1 h. Use recombinant procaspase-14 as a standard to quantify
    total caspase-14. Use revC14 as a standard to quantify active
    caspase-14.

  6. Wash the wells three times with 200 μl of PBST.

  7. For measurement of total caspase-14, add 2 μg/ml of H99
    antibody in 1:20 diluted ImmunoBlock and incubate for 1 h at
    37 °C. The active form of caspase-14 is measured in a similar
    way using h14D146 as a primary antibody instead of H99.


3.5.2 Cleavage-Site-
Directed Antibody
(h14Y178)


3.6 ELISA Assays
for Caspase-14


Mami Yamamoto-Tanaka and Toshihiko Hibino

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