Communication between the active sites and dimer interface of a herpesvirus protease revealed by a transition-state inhibitor

Marnett, Alan B.; Nomura, Anson M.; Shimba, Nobuhisa; Montellano, Paul R. Ortiz de; Craik, Charles S.

doi:10.1073/pnas.0401613101

Cited by 43 publications

(69 citation statements)

References 40 publications

(43 reference statements)

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“…Samples incorporating isotopically labeled Ala, Cys, His, Pro, or Arg were recombinantly expressed in E. coli strain BL21(DE3) in M9 media supplemented with all amino acids, nucleosides, and vitamins (35) 13 C, and 15 N. Protease concentrations were determined using a calculated 280 ) 0.931 mg/mL for wild-type and M197D proteins, 280 ) 1.000 mg/mL for ∆, and 280 ) 0.957 mg/mL for inhibited wild-type protease covalently modified with the inhibitor acetyl-Pro-Val-TyrtBug-Gln-AlaP-(OPh) 2 after hydrolysis of the two phenoxy moieties. The inhibitor was synthesized both with and without a biotin moiety on the amino terminus as previously described (33).…”

Section: Methodsmentioning

confidence: 99%

“…The Tyr-Val-tBug-Ala-ACC substrate was synthesized and purified as described (36), and substrate turnover was monitored for 1 h with an excitation wavelength of 380 nm and an emission wavelength of 460 nm. Protease samples were diluted into assay buffer and allowed to equilibrate for at least 1 h. The concentration of dimeric protease was calculated using the previously determined dissociation constant of 1.8 µM and the total concentration of protease using the equation previously derived (33).…”

Section: Methodsmentioning

confidence: 99%

“…Use of the inhibitor, which stabilizes the dimeric conformation of KSHV Pr (33), has allowed the direct comparison of the R-helical content between the monomeric and dimeric conformations of a herpesvirus protease, revealing a loss of 31% R-helicity upon dissociation.…”

Section: Quantification Of Structural Differences Between the Monomermentioning

confidence: 99%

“…A direct comparison between the monomer and dimer has been conducted through the use of an M197D mutation, which yields inactive monomers, and a hexapeptide diphenyl phosphonate covalent inhibitor, which stabilizes the protease dimer (33). Comparison of multiple engineered mutations in the KSHV Pr interfacial helix, adjacent to the active site and in the active site, which result in obligate monomers, has shown that loss of dimerization and activity is not linked to any specific point mutant, such as M197D (18; data not shown).…”

Section: Quantification Of Structural Differences Between the Monomermentioning

confidence: 99%

“…Herpesvirus proteases require dimerization for activity (17,18,(27)(28)(29)(30)(31) with binding affinities in the low micromolar to high nanomolar range; however, the dimeric X-ray structures all show the presence of intact active sites in each monomer, which are separate from the dimer interface. Early studies led to the hypothesis that a conformational change connects the active site and dimer interface, linking enzymatic activity to the protein oligomeric state (18,19,21,25,26,32,33). Recently, NMR spectroscopy and engineering of a redox switch, which allowed protease activity to be controlled by the addition of small molecule effectors (34), revealed that dissociation of herpesvirus dimers leads to unfolding of the two carboxyl-terminal R-helices.…”

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One Functional Switch Mediates Reversible and Irreversible Inactivation of a Herpesvirus Protease

et al. 2006

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Distinct mechanisms have evolved to regulate the function of proteolytic enzymes. Viral proteases in particular have developed novel regulatory mechanisms, presumably due to their comparatively rapid life cycles and responses to constant evolutionary pressure. Herpesviruses are a family of human pathogens that require a viral protease with a concentration-dependent zymogen activation involving folding of two R-helices and activation of the catalytic machinery, which results in formation of infectious virions. Kaposi's sarcoma-associated herpesvirus protease (KSHV Pr) is unique among the herpesvirus proteases in possessing an autolysis site in the dimer interface, which removes the carboxyl-terminal 27 amino acids comprising an R-helix adjacent to the active site. Truncation results in the irreversible loss of dimerization and concomitant inactivation. We characterized the conformational and functional differences between the active dimer, inactive monomer, and inactive truncated protease to determine the different protease regulatory mechanisms that control the KSHV lytic cycle. Circular dichroism revealed a loss of 31% R-helicity upon dimer dissociation. Comparison of the full-length and truncated monomers by NMR showed differences in 21% of the protein structure, mainly located adjacent to the dimer interface, with little perturbation of the overall protein upon truncation. Fluorescence polarization and active site labeling, with a transition state mimetic, characterized the functional effects of these conformational changes. Substrate turnover is abolished in both the full-length and truncated monomers; however, substrate binding remained intact. Disruption of the helix 6 interaction with the active site oxyanion loop is therefore used in two independent regulatory mechanisms of proteolytic activity.The nine known human herpesviruses (HHVs) 1 are responsible for diseases ranging from herpes labialis, caused by Herpes simplex virus-1, to Kaposi's sarcoma (KS), caused by Kaposi's sarcoma-associated herpesvirus (KSHV, HHV8) (1-3). These nine HHVs are grouped into three families, based on phenotypic and genomic similarities. Although the R-, the -, and the γ-herpesviruses (including KSHV) vary in tissue distribution and disease states, all herpesviruses possess homologous structural and enzymatic proteins involved in their lytic cycles. Among these proteins are the protease (Pr) and assembly protein (AP), which are necessary for infectious virion formation (4-8). Pr is expressed as a Pr/AP fusion (9-13), AP binds the major capsid protein, and the complex translocates to the nucleus where the immature capsid is assembled around the AP scaffold (14). Pr cleaves the Pr/AP fusion at the release site (R-site) and the maturation site (M-site) (10,11,13,15,16), allowing DNA packaging, formation of the infectious virion, and completion of the lytic cycle. Additional internal cleavage sites have been identified in multiple herpesvirus proteases; however, KSHV Pr is unique in that autolysis at the D-site (dimer d...

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Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Quantification Of Structural Differences Between the Monomermentioning

confidence: 99%

Section: Quantification Of Structural Differences Between the Monomermentioning

confidence: 99%

mentioning

confidence: 99%

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One Functional Switch Mediates Reversible and Irreversible Inactivation of a Herpesvirus Protease

et al. 2006

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Discovery and Evaluation of New Activity‐Based Probes for Serine Hydrolases

et al. 2019

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Serine hydrolases play crucial biological roles and are important therapeutic targets in many clinical applications. Activity‐based protein profiling of serine hydrolases by using fluorophosphonate probes, pioneered by Cravatt and co‐workers, has been a powerful tool for interrogating serine hydrolases in various biological systems. Herein, we present new phenyl phosphonate probes with an azide handle for click chemistry that offer remarkable improvements over the classical fluorophosphonate serine hydrolase activity‐based probes including ease of preparation, excellent cell permeability, and distinct reactivity profiles, as controlled by the phenolate leaving group. Thus, these new activity‐based serine hydrolase probes are valuable tools to further interrogate this important class of enzymes.

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Enantioselective Merger of Aminocatalysis with π‐Lewis Acid Metal Catalysis: Asymmetric Preparation of Carbo‐ and Heterocycles

et al. 2013

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The metallo‐organocatalyzed enantioselective synthesis of various five‐membered carbo‐ and heterocyclic structures through the merger of aminocatalysis with the catalytic indium(III) or copper(I) activation of α‐disubstituted formyl alkynes is described. The use of indium trichloride associated with the (R)‐1,1′‐bis‐(2‐naphthylamine) ligand led to encouraging results with up to 85:15 enantiomeric ratio. After a careful examination of several other strategies, the best synergic catalytic system, which combines a chiral copper(I) complex with cyclohexylamine, afforded the enantioselective preparations of cyclopentane, indane, and pyrrolidine scaffolds with moderate to excellent control of the all‐carbon quaternary stereogenic centers created through such cyclization processes.

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Communication between the active sites and dimer interface of a herpesvirus protease revealed by a transition-state inhibitor

Cited by 43 publications

References 40 publications

One Functional Switch Mediates Reversible and Irreversible Inactivation of a Herpesvirus Protease

One Functional Switch Mediates Reversible and Irreversible Inactivation of a Herpesvirus Protease

Discovery and Evaluation of New Activity‐Based Probes for Serine Hydrolases

Enantioselective Merger of Aminocatalysis with π‐Lewis Acid Metal Catalysis: Asymmetric Preparation of Carbo‐ and Heterocycles

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