Molecular mechanisms of viral and host cell substrate recognition by hepatitis C virus NS3/4A protease
| dc.contributor.author | Romano, Keith P. | |
| dc.contributor.author | Laine, Jennifer M. | |
| dc.contributor.author | Deveau, Laura M. | |
| dc.contributor.author | Cao, Hong | |
| dc.contributor.author | Massi, Francesca | |
| dc.contributor.author | Schiffer, Celia A. | |
| dc.date | 2022-08-11T08:08:00.000 | |
| dc.date.accessioned | 2022-08-23T15:38:45Z | |
| dc.date.available | 2022-08-23T15:38:45Z | |
| dc.date.issued | 2011-07-22 | |
| dc.date.submitted | 2011-11-22 | |
| dc.identifier.citation | J Virol. 2011 Jul;85(13):6106-16. Epub 2011 Apr 20. <a href="http://dx.doi.org/10.1128/JVI.00377-11">Link to article on publisher's site</a> | |
| dc.identifier.issn | 0022-538X (Linking) | |
| dc.identifier.doi | 10.1128/JVI.00377-11 | |
| dc.identifier.pmid | 21507982 | |
| dc.identifier.uri | http://hdl.handle.net/20.500.14038/26004 | |
| dc.description.abstract | Hepatitis C NS3/4A protease is a prime therapeutic target that is responsible for cleaving the viral polyprotein at junctions 3-4A, 4A4B, 4B5A, and 5A5B and two host cell adaptor proteins of the innate immune response, TRIF and MAVS. In this study, NS3/4A crystal structures of both host cell cleavage sites were determined and compared to the crystal structures of viral substrates. Two distinct protease conformations were observed and correlated with substrate specificity: (i) 3-4A, 4A4B, 5A5B, and MAVS, which are processed more efficiently by the protease, form extensive electrostatic networks when in complex with the protease, and (ii) TRIF and 4B5A, which contain polyproline motifs in their full-length sequences, do not form electrostatic networks in their crystal complexes. These findings provide mechanistic insights into NS3/4A substrate recognition, which may assist in a more rational approach to inhibitor design in the face of the rapid acquisition of resistance. | |
| dc.language.iso | en_US | |
| dc.relation | <a href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=pubmed&cmd=Retrieve&list_uids=21507982&dopt=Abstract">Link to Article in PubMed</a> | |
| dc.relation.url | http://dx.doi.org/10.1128/JVI.00377-11 | |
| dc.subject | Adaptor Proteins, Signal Transducing | |
| dc.subject | Carrier Proteins | |
| dc.subject | Catalytic Domain | |
| dc.subject | Crystallization | |
| dc.subject | Humans | |
| dc.subject | Magnetic Resonance Spectroscopy | |
| dc.subject | Membrane Proteins | |
| dc.subject | Models, Molecular | |
| dc.subject | Polyproteins | |
| dc.subject | Protein Conformation | |
| dc.subject | Static Electricity | |
| dc.subject | Substrate Specificity | |
| dc.subject | Viral Nonstructural Proteins | |
| dc.subject | Biochemistry, Biophysics, and Structural Biology | |
| dc.subject | Microbiology | |
| dc.title | Molecular mechanisms of viral and host cell substrate recognition by hepatitis C virus NS3/4A protease | |
| dc.type | Journal Article | |
| dc.source.journaltitle | Journal of virology | |
| dc.source.volume | 85 | |
| dc.source.issue | 13 | |
| dc.identifier.legacycoverpage | https://escholarship.umassmed.edu/bmp_pp/134 | |
| dc.identifier.contextkey | 2367984 | |
| html.description.abstract | <p>Hepatitis C NS3/4A protease is a prime therapeutic target that is responsible for cleaving the viral polyprotein at junctions 3-4A, 4A4B, 4B5A, and 5A5B and two host cell adaptor proteins of the innate immune response, TRIF and MAVS. In this study, NS3/4A crystal structures of both host cell cleavage sites were determined and compared to the crystal structures of viral substrates. Two distinct protease conformations were observed and correlated with substrate specificity: (i) 3-4A, 4A4B, 5A5B, and MAVS, which are processed more efficiently by the protease, form extensive electrostatic networks when in complex with the protease, and (ii) TRIF and 4B5A, which contain polyproline motifs in their full-length sequences, do not form electrostatic networks in their crystal complexes. These findings provide mechanistic insights into NS3/4A substrate recognition, which may assist in a more rational approach to inhibitor design in the face of the rapid acquisition of resistance.</p> | |
| dc.identifier.submissionpath | bmp_pp/134 | |
| dc.contributor.department | Department of Biochemistry and Molecular Pharmacology | |
| dc.source.pages | 6106-16 |
This item appears in the following Collection(s)
Related items
Showing items related by title, author, creator and subject.
-
Dynamic Regulation at the Neuronal Plasma Membrane: Novel Endocytic Mechanisms Control Anesthetic-Activated Potassium Channels and Amphetamine-Sensitive Dopamine Transporters: A DissertationEndocytic trafficking dynamically regulates neuronal plasma membrane protein presentation and activity, and plays a central role in excitability and plasticity. Over the course of my dissertation research I investigated endocytic mechanisms regulating two neuronal membrane proteins: the anesthetic-activated potassium leak channel, KCNK3, as well as the psychostimulant-sensitive dopamine transporter (DAT). My results indicate that KCNK3 internalizes in response to Protein Kinase C (PKC) activation, using a novel pathway that requires the phosphoserine binding protein, 14-3-3β, and demonstrates for the first time regulated KCNK3 channel trafficking in neurons. Additionally, PKC-mediated KCNK3 trafficking requires a non-canonical endocytic motif, which is shared exclusively between KCNK3 and sodium-dependent neurotransmitter transporters, such as DAT. DAT trafficking studies in intact ex vivo adult striatal slices indicate that DAT endocytic trafficking has both dynamin-dependent and –independent components. Moreover, DAT segregates into two populations at the neuronal plasma membrane: trafficking-competent and -incompetent. Taken together, these results demonstrate that novel, non-classical endocytic mechanisms dynamically control the plasma membrane presentation of these two important neuronal proteins.
-
Selective interaction of JNK protein kinase isoforms with transcription factorsThe JNK protein kinase is a member of the MAP kinase group that is activated in response to dual phosphorylation on threonine and tyrosine. Ten JNK isoforms were identified in human brain by molecular cloning. These protein kinases correspond to alternatively spliced isoforms derived from the JNK1, JNK2 and JNK3 genes. The protein kinase activity of these JNK isoforms was measured using the transcription factors ATF2, Elk-1 and members of the Jun family as substrates. Treatment of cells with interleukin-1 (IL-1) caused activation of the JNK isoforms. This activation was blocked by expression of the MAP kinase phosphatase MKP-1. Comparison of the binding activity of the JNK isoforms demonstrated that the JNK proteins differ in their interaction with ATF2, Elk-1 and Jun transcription factors. Individual members of the JNK group may therefore selectively target specific transcription factors in vivo.
-
Role of the Raf/mitogen-activated protein kinase pathway in p21ras desensitizationDesensitization of p21(ras) after stimulation of cells by growth factors and phorbol 12-myristate 13-acetate (PMA) correlates with hyperphosphorylation of the guanine nucleotide exchange factor Son-of-sevenless (Sos) and its dissociation from the adaptor protein Grb2 (Cherniack, A., Klarlund, J. K., Conway, B. R., and Czech, M. P. (1995) J. Biol. Chem. 270, 1485-1488). To test the role of the Raf/mitogen-activated protein (MAP) kinase pathway, we utilized cells expressing a chimera composed of the catalytic domain of p74Raf-1 and the hormone binding domain of the estradiol receptor (DeltaRaf-1:ER). Estradiol markedly stimulated DeltaRaf-1:ER and the downstream MEK and MAP kinases in these cells as well as Sos phosphorylation. However, the dissociation of Grb2 from Sos observed in response to PMA was not apparent upon DeltaRaf-1:ER activation. Furthermore, stimulation of DeltaRaf-1:ER did not impair GTP loading of p21(ras) in response to platelet-derived growth factor or epidermal growth factor. We conclude that activation of the Raf/MAP kinase pathway alone in these cells is insufficient to cause disassembly of Sos from Grb2 or to interrupt the ability of Sos to catalyze activation of p21(ras).
