Specific covalent inhibition of MALT1 paracaspase suppresses B cell lymphoma growth
Lorena Fontán, … , Nathanael S. Gray, Ari Melnick
Lorena Fontán, … , Nathanael S. Gray, Ari Melnick
Published July 19, 2018
Citation Information: J Clin Invest. 2018;128(10):4397-4412. https://doi.org/10.1172/JCI99436.
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Research Article Oncology Therapeutics

Specific covalent inhibition of MALT1 paracaspase suppresses B cell lymphoma growth

Abstract

The paracaspase MALT1 plays an essential role in activated B cell–like diffuse large B cell lymphoma (ABC DLBCL) downstream of B cell and TLR pathway genes mutated in these tumors. Although MALT1 is considered a compelling therapeutic target, the development of tractable and specific MALT1 protease inhibitors has thus far been elusive. Here, we developed a target engagement assay that provides a quantitative readout for specific MALT1-inhibitory effects in living cells. This enabled a structure-guided medicinal chemistry effort culminating in the discovery of pharmacologically tractable, irreversible substrate-mimetic compounds that bind the MALT1 active site. We confirmed that MALT1 targeting with compound 3 is effective at suppressing ABC DLBCL cells in vitro and in vivo. We show that a reduction in serum IL-10 levels exquisitely correlates with the drug pharmacokinetics and degree of MALT1 inhibition in vitro and in vivo and could constitute a useful pharmacodynamic biomarker to evaluate these compounds in clinical trials. Compound 3 revealed insights into the biology of MALT1 in ABC DLBCL, such as the role of MALT1 in driving JAK/STAT signaling and suppressing the type I IFN response and MHC class II expression, suggesting that MALT1 inhibition could prime lymphomas for immune recognition by cytotoxic immune cells.

Authors

Lorena Fontán, Qi Qiao, John M. Hatcher, Gabriella Casalena, Ilkay Us, Matt Teater, Matt Durant, Guangyan Du, Min Xia, Natalia Bilchuk, Spandan Chennamadhavuni, Giuseppe Palladino, Giorgio Inghirami, Ulrike Philippar, Hao Wu, David A. Scott, Nathanael S. Gray, Ari Melnick

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Figure 8

Compound 3 suppresses the growth of DLBCL PDXs ex vivo.

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Compound 3 suppresses the growth of DLBCL PDXs ex vivo. (A) Western blot...
(A) Western blots for MALT1 targets Roquin, CYLD, and uncleaved BCL10 in PDX specimens were used to establish the MALT1 activation state in each specimen. (B) Cell counts relative to vehicle-treated cells for the indicated DLBCL PDX specimens ex vivo. Four different concentrations of compound 3 were assayed. Data represent the mean ± SD of 1 representative experiment. Each experiment was performed at least twice with similar results. (C) CFSE dilution assay results for 2 different concentrations of compound 3 in the indicated PDX specimens. (D) CFSE MFI FC relative to the mean of the vehicle-treated cells. (E) hIL-10 levels in the supernatant of PDX ex vivo culture. Data represent the mean ± SEM of 1 representative experiment performed in quadruplicate. **P ≤ 0.01, ***P < 0.001, and ****P < 0.0001, by ANOVA with Dunnett’s multiple comparisons adjustment (B and D) and unpaired, 2-tailed Student’s t test (E).