| Literature DB >> 24726805 |
L Nathan Tumey1, Diane H Boschelli2, Niala Bhagirath2, Jaechul Shim2, Elizabeth A Murphy3, Deborah Goodwin3, Eric M Bennett4, Mengmeng Wang5, Lih-Ling Lin3, Barry Press2, Marina Shen3, Richard K Frisbie2, Paul Morgan3, Shashi Mohan3, Julia Shin3, Vikram R Rao3.
Abstract
IRAK4 is responsible for initiating signaling from Toll-like receptors (TLRs) and members of the IL-1/18 receptor family. Kinase-inactive knock-ins and targeted deletions of IRAK4 in mice cause reductions in TLR induced pro-inflammatory cytokines and these mice are resistant to various models of arthritis. Herein we report the identification and optimization of a series of potent IRAK4 inhibitors. Representative examples from this series showed excellent selectivity over a panel of kinases, including the kinases known to play a role in TLR-mediated signaling. The compounds exhibited low nM potency in LPS- and R848-induced cytokine assays indicating that they are blocking the TLR signaling pathway. A key compound (26) from this series was profiled in more detail and found to have an excellent pharmaceutical profile as measured by predictive assays such as microsomal stability, TPSA, solubility, and clogP. However, this compound was found to afford poor exposure in mouse upon IP or IV administration. We found that removal of the ionizable solubilizing group (32) led to increased exposure, presumably due to increased permeability. Compounds 26 and 32, when dosed to plasma levels corresponding to ex vivo whole blood potency, were shown to inhibit LPS-induced TNFα in an in vivo murine model. To our knowledge, this is the first published in vivo demonstration that inhibition of the IRAK4 pathway by a small molecule can recapitulate the phenotype of IRAK4 knockout mice.Entities:
Keywords: IRAK4; Indoloquinoline; Inflammation; Kinase inhibitor; TLR signaling
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Year: 2014 PMID: 24726805 DOI: 10.1016/j.bmcl.2014.03.056
Source DB: PubMed Journal: Bioorg Med Chem Lett ISSN: 0960-894X Impact factor: 2.823