Binding Kinetics of CD137 Antibody

Example 7

Jurkat cells (i.e., an immortalized human T lymphocyte cell line) characterized by stable, over-expression of hCD137 were plated at 20,000 cells/well and stained with a titration of primary murine anti-CD137 antibody BBK2 (BBK2-mlgG1) for 4 hours at 4° C. Secondary anti-mouse AF488 stain, at a constant amount, was added for 30 minutes at 4° C. After washing, plates were run on a flow cytometer and binding of BBK2-mlgG1 (and the negative control, i.e., mlgG1) was determined based on geometric mean fluorescence intensity in the AF488 channel. Results from these assays are provided in FIGS. 1A and B.

As shown in FIGS. 1A and 1B, the murine BBK2 antibody binds to human T cells (i.e. CD137-expressing Jurkat cells), with an EC₅₀=35 pM.

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US10434185B2. Compositions and methods for the depletion of CD137+ cells (2019-10-08). Magenta Therapeutics, Inc. [US]. Inventors: Adam Hartigan [US], Anthony Boitano [US], Michael Cooke [US], Megan D. Hoban [US], Rahul Palchaudhuri [US].

Patent 2019

Anti antibody Antibody Assays Cd137 Cell line Cells Figs Fluorescence Human Jurkat cells Murine Stain T cells Titration

Top 5 similar protocols

Variable analysis

independent variables

Titration of primary murine anti-CD137 antibody BBK2 (BBK2-mIgG1)

dependent variables

Binding of BBK2-mIgG1 (and the negative control, i.e., mIgG1) based on geometric mean fluorescence intensity in the AF488 channel

control variables

Jurkat cells (i.e., an immortalized human T lymphocyte cell line) characterized by stable, over-expression of hCD137 were plated at 20,000 cells/well
Secondary anti-mouse AF488 stain, at a constant amount, was added for 30 minutes at 4° C

controls

Negative control: mIgG1

Annotations

Based on most similar protocols

Use Jurkat cells (immortalized human T lymphocyte cell line) overexpressing human CD137 as the cell line for the binding assay (Protocol 1, Protocol 2, Protocol 3, Protocol 4, Protocol 5).

Stain the cells with a titration of primary murine anti-CD137 antibody BBK2 (BBK2-mIgG1) for 4 hours at 4°C (Protocol 1).

Add a constant amount of secondary anti-mouse AF488 stain for 30 minutes at 4°C (Protocol 1).

Wash the cells and analyze binding of BBK2-mIgG1 (and the negative control mIgG1) by measuring the geometric mean fluorescence intensity in the AF488 channel using flow cytometry (Protocol 1).

Determine the EC50 value for the binding of the murine BBK2 antibody to the CD137-expressing Jurkat cells (Protocol 1).

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