Kinetic Characterization and Molecular Docking of a Novel, Potent, and Selective Slow-Binding Inhibitor of Human Cathepsin L

Shah, Parag P.; Myers, Michael C.; Beavers, Mary Pat; Purvis, Jeremy E.; Jing, Huiyan; Grieser, Heather; Sharlow, Elizabeth R.; Napper, Andrew D.; Huryn, Donna M.; Cooperman, Barry S.; Smith, Amos B.; Diamond, Scott L.

doi:10.1124/mol.108.046219

Cited by 42 publications

(45 citation statements)

References 23 publications

(18 reference statements)

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“…A cellular cytotoxicity assay was conducted with human aortic endothelial cells (HAEC) and human hepatocellular liver carcinoma cells (HepG2) as previously described (27) to measure viability after 24 h of incubation.…”

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confidence: 99%

Discovery of Potent Small-Molecule Inhibitors of Multidrug-Resistant Plasmodium falciparum Using a Novel Miniaturized High-Throughput Luciferase-Based Assay

Lucumi¹,

Darling²,

et al. 2010

Antimicrob Agents Chemother

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Malaria is a global health problem that causes significant mortality and morbidity, with more than 1 million deaths per year caused by Plasmodium falciparum. Most antimalarial drugs face decreased efficacy due to the emergence of resistant parasites, which necessitates the discovery of new drugs. To identify new antimalarials, we developed an automated 384-well plate screening assay using P. falciparum parasites that stably express cytoplasmic firefly luciferase. After initial optimization, we tested two different types of compound libraries: known bioactive collections (Library of Pharmacologically Active Compounds [LOPAC] and the library from the National Institute of Neurological Disorders and Stroke [NINDS]) and a library of uncharacterized compounds (ChemBridge). A total of 12,320 compounds were screened at 5.5 M. Selecting only compounds that reduced parasite growth by 85% resulted in 33 hits from the combined bioactive collection and 130 hits from the ChemBridge library. Fifteen novel drug-like compounds from the bioactive collection were found to be active against P. falciparum. Twelve new chemical scaffolds were found from the ChemBridge hits, the most potent of which was a series based on the 1,4-naphthoquinone scaffold, which is structurally similar to the FDA-approved antimalarial atovaquone. However, in contrast to atovaquone, which acts to inhibit the bc 1 complex and block the electron transport chain in parasite mitochondria, we have determined that our new 1,4-napthoquinones act in a novel, non-bc 1 -dependent mechanism and remain potent against atovaquone-and chloroquine-resistant parasites. Ultimately, this study may provide new probes to understand the molecular details of the malaria life cycle and to identify new antimalarials.

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confidence: 99%

Discovery of Potent Small-Molecule Inhibitors of Multidrug-Resistant Plasmodium falciparum Using a Novel Miniaturized High-Throughput Luciferase-Based Assay

Lucumi¹,

Darling²,

et al. 2010

Antimicrob Agents Chemother

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“…15,24 Compound 1 demonstrated selectivity towards cathepsin L versus other cysteine proteases, including cathepsins V, S, B, and K, with the greatest selectivity index observed for cathepsin K (150). 23 The details of a structure activity relationship study for cathepsin L inhibition in the carbazate series are being published separately 25 , but reveal that removal of the NHBoc group causes a dramatic loss of cathepsin L inhibitory activity. This single synthetic change to the carbazate scaffold of 1 removes both the potential for hydrogen bonding with Asp 148 and the hydrophobic contact of the tert-butoxy group in the S3 subsite, resulting in a 400-fold reduction in cathepsin L inhibition.…”

Section: Resultsmentioning

confidence: 99%

“…Most notably, the rate of inhibitor dissociation (k off ) from cathepsin L was extremely slow, leading to a K i = k off / k on = 0.890 nM. 23 Alternative reaction schemes for steady-state and irreversible inhibitor binding were also tested, but did not fit the data as well as the 5-parameter model. Taken together, the results from the docking and kinetic analyses suggest a covalent but slowly reversible mechanism of inhibition that is aided by strong non-covalent interactions.…”

Section: Resultsmentioning

confidence: 99%

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Molecular Docking of Cathepsin L Inhibitors in the Binding Site of Papain

Beavers¹,

Myers²,

Shah³

et al. 2010

J. Chem. Inf. Model.

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The papain/CLIK-148 coordinate system was employed as a model to study the interactions of a non-peptide thiocarbazate inhibitor of cathepsin L (1). This small molecule inhibitor, a thiol ester containing a diacyl hydrazine functionality and one stereogenic center, was most active as the Senantiomer, with an IC 50 of 56 nM; the R-enantiomer (2) displayed only weak activity (33 μM). Correspondingly, molecular docking studies with Extra Precision Glide revealed a correlation between score and biological activity for the two thiocarbazate enantiomers when a structural water was preserved. The molecular interactions between 1 and papain were very similar to the interactions observed for CLIK-148 (3a and 3b) with papain, especially with regard to the hydrogen bonding and lipophilic interactions of the ligands with conserved residues in the catalytic binding site. Subsequent docking of virtual compounds in the binding site led to the identification of a more potent inhibitor (5), with an IC 50 of 7.0 nM. These docking studies revealed that favorable energy scores and correspondingly favorable biological activities could be realized when the virtual compound design included occupation of the S2, S3 and S1′ subsites by hydrophobic and aromatic functionalities of the ligand, and at least three hydrogen bonding contacts between the ligand and the conserved binding site residues of the protein.

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“…Second, docking studies of 15a (R 1 =H, R 2 = o -ethylphenyl) placed the C2 carbonyl in close proximity to the active site cysteine xxxix. The kinetic characterization of 15a revealed a slowly reversible inhibition xl. Additional studies provided further insight into the mode of action of these inhibitors.…”

Section: Characterization Of Thiocarbazate’s Inhibitionmentioning

confidence: 97%

The Identification, Characterization and Optimization of Small Molecule Probes of Cysteine Proteases: Experiences of the Penn Center for Molecular Discovery with Cathepsin B and Cathepsin L

Huryn

Smith²

2009

CTMC

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During the pilot phase of the NIH Molecular Library Screening Network, the Penn Center for Molecular Discovery focused on a series of projects aimed at high throughput screening and the development of probes of a variety of protease targets. This review provides our medicinal chemistry experience with two such targets -cathepsin B and cathepsin L. We describe our approach for hit validation, characterization and triage that led to a critical understanding of the nature of hits from the cathepsin B project. In addition, we detail our experience at hit identification and optimization that led to the development of a novel thiocarbazate probe of cathepsin L.

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Kinetic Characterization and Molecular Docking of a Novel, Potent, and Selective Slow-Binding Inhibitor of Human Cathepsin L

Cited by 42 publications

References 23 publications

Discovery of Potent Small-Molecule Inhibitors of Multidrug-Resistant Plasmodium falciparum Using a Novel Miniaturized High-Throughput Luciferase-Based Assay

Discovery of Potent Small-Molecule Inhibitors of Multidrug-Resistant Plasmodium falciparum Using a Novel Miniaturized High-Throughput Luciferase-Based Assay

Molecular Docking of Cathepsin L Inhibitors in the Binding Site of Papain

The Identification, Characterization and Optimization of Small Molecule Probes of Cysteine Proteases: Experiences of the Penn Center for Molecular Discovery with Cathepsin B and Cathepsin L

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