Your search keyword '"Nunberg JH"' showing total 73 results

1. Adaptation to persistent growth in the H9 cell line renders a primary isolate of human immunodeficiency virus type 1 sensitive to neutralization by vaccine sera

Author

Joann Vennari, H Schuitemaker, T P Loh, T Wrin, Nunberg Jh, and Other departments

Subjects

viruses, Immunology, Guinea Pigs, Molecular Sequence Data, Biology, V3 loop, HIV Envelope Protein gp120, Antibodies, Viral, Virus Replication, Microbiology, Virus, Neutralization, Cell Line, Neutralization Tests, Virology, Animals, Humans, Amino Acid Sequence, Primary isolate, Tropism, Cytopathic effect, DNA Primers, AIDS Vaccines, Base Sequence, Viral culture, Antibodies, Monoclonal, Immunoglobulins, Intravenous, Adaptation, Physiological, Viral replication, Insect Science, HIV-1, Research Article

Abstract

Seven diverse primary isolates of human immunodeficiency virus type 1 (HIV-1) were examined and found to be refractory to neutralization by antisera to recombinant gp120 (rgp120) protein from HIV-1 MN. This stands in marked contrast to the sensitivity exhibited by certain laboratory-adapted viruses. To understand the difference between primary and laboratory-adapted viruses, we adapted the primary virus ACH 168.10 to growth in the FDA/H9 cell line. ACH 168.10 was chosen because the V3 region of gp120 closely matches that of MN. After 4 weeks, infection became evident. The virus (168A) replicated in FDA/H9 cells with extensive cytopathic effect but was unchanged in sensitivity to antibody-mediated neutralization. Thus, growth in cell lines is not sufficient to render primary virus sensitive to neutralization. The 168A virus was, however, partially sensitive to CD4 immunoadhesin (CD4-Ig). Adaptation was continued to produce a persistently infected FDA/H9 culture that displayed minimal cytopathic effect. The virus (168C) was now sensitive to neutralization by MN rgp120 vaccine sera and by MN-specific monoclonal antibodies and showed increased sensitivity to HIVIG and CD4-Ig. 168C encoded three amino acid changes in gp120, including one within the V3 loop (I-166-->R, I-282-->N, G-318-->R). MN-specific monoclonal antibodies bound equally to the surface of cells infected with either neutralization-resistant or -sensitive virus. The coincidence of changes in neutralization sensitivity with changes in cell tropism and cytopathic effect suggests a common underlying mechanism(s) acting through the whole of the envelope protein complex.

Published

1995

2. HIV-1MN recombinant gp120 vaccine serum, which fails to neutralize primary isolates of HIV-1, does not antagonize neutralization by antibodies from infected individuals

Author

Nunberg Jh and Wrin T

Subjects

Immunology, Human immunodeficiency virus (HIV), HIV Infections, HIV Antibodies, HIV Envelope Protein gp120, medicine.disease_cause, Neutralization, law.invention, law, Neutralization Tests, medicine, Immunology and Allergy, Humans, AIDS Vaccines, Acquired Immunodeficiency Syndrome, Vaccines, Synthetic, Primary (chemistry), biology, business.industry, Virology, Infectious Diseases, Recombinant DNA, biology.protein, HIV-1, Antibody, business

Published

1994

3. Restoration of virulence in the attenuated Candid#1 vaccine virus requires reversion at both positions 168 and 427 in the envelope glycoprotein GPC.

Author

Nunberg JH, Westover JB, York J, Jung KH, Bailey KW, Boardman KM, Li M, Furnell RS, Wasson SR, Murray JS, Kaundal R, Thomas AJ, and Gowen BB

Subjects

Animals, Guinea Pigs, Humans, Mice, Glycoproteins genetics, South American People, Vaccines, Attenuated genetics, Virulence, Hemorrhagic Fever, American prevention & control, Junin virus physiology, Viral Vaccines genetics

Abstract

Live-attenuated virus vaccines provide long-lived protection against viral disease but carry inherent risks of residual pathogenicity and genetic reversion. The live-attenuated Candid#1 vaccine was developed to protect Argentines against lethal infection by the Argentine hemorrhagic fever arenavirus, Junín virus. Despite its safety and efficacy in Phase III clinical study, the vaccine is not licensed in the US, in part due to concerns regarding the genetic stability of attenuation. Previous studies had identified a single F427I mutation in the transmembrane domain of the Candid#1 envelope glycoprotein GPC as the key determinant of attenuation, as well as the propensity of this mutation to revert upon passage in cell culture and neonatal mice. To ascertain the consequences of this reversion event, we introduced the I427F mutation into recombinant Candid#1 (I427F rCan) and investigated the effects in two validated small-animal models: in mice expressing the essential virus receptor (human transferrin receptor 1; huTfR1) and in the conventional guinea pig model. We report that I427F rCan displays only modest virulence in huTfR1 mice and appears attenuated in guinea pigs. Reversion at another attenuating locus in Candid#1 GPC (T168A) was also examined, and a similar pattern was observed. By contrast, virus bearing both revertant mutations (A168T+I427F rCan) approached the lethal virulence of the pathogenic Romero strain in huTfR1 mice. Virulence was less extreme in guinea pigs. Our findings suggest that genetic stabilization at both positions is required to minimize the likelihood of reversion to virulence in a second-generation Candid#1 vaccine.IMPORTANCELive-attenuated virus vaccines, such as measles/mumps/rubella and oral poliovirus, provide robust protection against disease but carry with them the risk of genetic reversion to the virulent form. Here, we analyze the genetics of reversion in the live-attenuated Candid#1 vaccine that is used to protect against Argentine hemorrhagic fever, an often-lethal disease caused by the Junín arenavirus. In two validated small-animal models, we find that restoration of virulence in recombinant Candid#1 viruses requires back-mutation at two positions specific to the Candid#1 envelope glycoprotein GPC, at positions 168 and 427. Viruses bearing only a single change showed only modest virulence. We discuss strategies to genetically harden Candid#1 GPC against these two reversion events in order to develop a safer second-generation Candid#1 vaccine virus., Competing Interests: The authors declare no conflict of interest.

Published

2024

4. Fusogenic structural changes in arenavirus glycoproteins are associated with viroporin activity.

Author

Zhang Y, York J, Brindley MA, Nunberg JH, and Melikyan GB

Subjects

Viroporin Proteins metabolism, Glycoproteins metabolism, Viral Envelope Proteins metabolism, Lassa virus, Virus Internalization, Arenavirus genetics

Abstract

Many enveloped viruses enter host cells by fusing with acidic endosomes. The fusion activity of multiple viral envelope glycoproteins does not generally affect viral membrane permeability. However, fusion induced by the Lassa virus (LASV) glycoprotein complex (GPc) is always preceded by an increase in viral membrane permeability and the ensuing acidification of the virion interior. Here, systematic investigation of this LASV fusion phenotype using single pseudovirus tracking in live cells reveals that the change in membrane barrier function is associated with the fusogenic conformational reorganization of GPc. We show that a small-molecule fusion inhibitor or mutations that impair viral fusion by interfering with GPc refolding into the post-fusion structure prevent the increase in membrane permeability. We find that the increase in virion membrane permeability occurs early during endosomal maturation and is facilitated by virus-cell contact. This increase is observed using diverse arenavirus glycoproteins, whether presented on lentivirus-based pseudoviruses or arenavirus-like particles, and in multiple different cell types. Collectively, these results suggest that conformational changes in GPc triggered by low pH and cell factor binding are responsible for virion membrane permeabilization and acidification of the virion core prior to fusion. We propose that this viroporin-like activity may augment viral fusion and/or post-fusion steps of infection, including ribonucleoprotein release into the cytoplasm., Competing Interests: The authors have declared that no competing interests exist., (Copyright: © 2023 Zhang et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.)

Published

2023

5. Second-Generation Live-Attenuated Candid#1 Vaccine Virus Resists Reversion and Protects against Lethal Junín Virus Infection in Guinea Pigs.

Author

Gowen BB, Hickerson BT, York J, Westover JB, Sefing EJ, Bailey KW, Wandersee L, and Nunberg JH

Subjects

Animals, Antibodies, Viral biosynthesis, Antibodies, Viral immunology, Chlorocebus aethiops, Guinea Pigs, Hemorrhagic Fever, American immunology, Immunogenicity, Vaccine, Junin virus genetics, Junin virus pathogenicity, Male, Vaccines, Attenuated genetics, Vaccines, Attenuated immunology, Vaccines, Synthetic genetics, Vaccines, Synthetic immunology, Vero Cells, Viral Vaccines genetics, Virulence, Hemorrhagic Fever, American prevention & control, Junin virus immunology, Viral Vaccines immunology

Abstract

Live-attenuated virus vaccines are highly effective in preventing viral disease but carry intrinsic risks of residual virulence and reversion to pathogenicity. The classically derived Candid#1 virus protects seasonal field workers in Argentina against zoonotic infection by Junín virus (JUNV) but is not approved in the United States, in part due to the potential for reversion at the attenuating locus, a phenylalanine-to-isoleucine substitution at position 427 in the GP2 subunit of the GPC envelope glycoprotein. Previously, we demonstrated facile reversion of recombinant Candid#1 (rCan) in cell culture and identified an epistatic interaction between the attenuating I427 and a secondary K33S mutation in the stable signal peptide (SSP) subunit of GPC that imposes an evolutionary barrier to reversion. The magnitude of this genetic barrier is manifest in our repeated failures to rescue the hypothetical revertant virus. In this study, we show that K33S rCan is safe and attenuated in guinea pigs and capable of eliciting potent virus-neutralizing antibodies. Immunized animals are fully protected against lethal challenge with virulent JUNV. In addition, we employed a more permissive model of infection in neonatal mice to investigate genetic reversion. RNA sequence analysis of the recovered virus identified revertant viruses in pups inoculated with the parental rCan virus and none in mice receiving K33S rCan ( P  < 0.0001). Taken together, our findings support the further development of K33S rCan as a safe second-generation JUNV vaccine. IMPORTANCE Our most successful vaccines comprise weakened strains of virus that initiate a limited and benign infection in immunized persons. The live-attenuated Candid#1 strain of Junín virus (JUNV) was developed to protect field workers in Argentina from rodent-borne hemorrhagic fever but is not licensed in the United States, in part due to the likelihood of genetic reversion to virulence. A single-amino-acid change in the GPC envelope glycoprotein of the virus is responsible for attenuation, and a single nucleotide change may regenerate the pathogenic virus. Here, we take advantage of a unique genetic interaction between GPC subunits to design a mutant Candid#1 virus that establishes an evolutionary barrier to reversion. The mutant virus (K33S rCan) is fully attenuated and protects immunized guinea pigs against lethal JUNV infection. We find no instances of reversion in mice inoculated with K33S rCan. This work supports the further development of K33S rCan as a second-generation JUNV vaccine.

Published

2021

6. SAR studies of 4-acyl-1,6-dialkylpiperazin-2-one arenavirus cell entry inhibitors.

Author

Plewe MB, Whitby LR, Naik S, Brown ER, Sokolova NV, Gantla VR, York J, Nunberg JH, Zhang L, Kalveram B, Freiberg AN, Boger DL, Henkel G, and McCormack K

Subjects

Antiviral Agents chemical synthesis, Antiviral Agents chemistry, Arenavirus metabolism, Dose-Response Relationship, Drug, Microbial Sensitivity Tests, Molecular Structure, Piperazines chemical synthesis, Piperazines chemistry, Structure-Activity Relationship, Viral Envelope Proteins metabolism, Antiviral Agents pharmacology, Arenavirus drug effects, Piperazines pharmacology, Viral Envelope Proteins antagonists & inhibitors

Abstract

Old World (Africa) and New World (South America) arenaviruses are associated with human hemorrhagic fevers. Efforts to develop small molecule therapeutics have yielded several chemical series including the 4-acyl-1,6-dialkylpiperazin-2-ones. Herein, we describe an extensive exploration of this chemotype. In initial Phase I studies, R 1 and R 4 scanning libraries were assayed to identify potent substituents against Old World (Lassa) virus. In subsequent Phase II studies, R 6 substituents and iterative R 1 , R 4 and R 6 substituent combinations were evaluated to obtain compounds with improved Lassa and New World (Machupo, Junin, and Tacaribe) arenavirus inhibitory activity, in vitro human liver microsome metabolic stability and aqueous solubility., (Copyright © 2019 Elsevier Ltd. All rights reserved.)

Published

2019

7. A Cell-Cell Fusion Assay to Assess Arenavirus Envelope Glycoprotein Membrane-Fusion Activity.

Author

York J and Nunberg JH

Subjects

Animals, Chlorocebus aethiops, Hydrogen-Ion Concentration, Membrane Fusion physiology, Vero Cells, Viral Envelope Proteins metabolism, beta-Galactosidase metabolism, Arenavirus metabolism, Biological Assay methods, Endosomes metabolism, Glycoproteins metabolism

Abstract

For many viruses that enter their target cells through pH-dependent fusion of the viral and endosomal membranes, cell-cell fusion assays can provide an experimental platform for investigating the structure-function relationships that promote envelope glycoprotein membrane-fusion activity. Typically, these assays employ effector cells expressing the recombinant envelope glycoprotein on the cell surface and target cells engineered to quantitatively report fusion with the effector cell. In the protocol described here, Vero cells are transfected with a plasmid encoding the arenavirus envelope glycoprotein complex GPC and infected with the vTF7-3 vaccinia virus expressing the bacteriophage T7 RNA polymerase. These effector cells are mixed with target cells infected with the vCB21R-lacZ vaccinia virus encoding a β-galactosidase reporter under the control of the T7 promoter. Cell-cell fusion is induced upon exposure to low-pH medium (pH 5.0), and the resultant expression of the β-galactosidase reporter is quantitated using a chemiluminescent substrate. We have utilized this robust microplate cell-cell fusion assay extensively to study arenavirus entry and its inhibition by small-molecule fusion inhibitors.

Published

2018

8. Epistastic Interactions within the Junín Virus Envelope Glycoprotein Complex Provide an Evolutionary Barrier to Reversion in the Live-Attenuated Candid#1 Vaccine.

Author

York J and Nunberg JH

Subjects

Animals, Chlorocebus aethiops, Evolution, Molecular, Genotype, Hemorrhagic Fever, American prevention & control, Humans, Junin virus metabolism, Junin virus pathogenicity, Membrane Fusion, Mutation, Vaccines, Attenuated genetics, Vero Cells, Virulence, Virus Internalization, Epistasis, Genetic, Glycoproteins genetics, Junin virus genetics, Junin virus immunology, Viral Envelope Proteins genetics, Viral Vaccines genetics

Abstract

The Candid#1 strain of Junín virus was developed using a conventional attenuation strategy of serial passage in nonhost animals and cultured cells. The live-attenuated Candid#1 vaccine is used in Argentina to protect at-risk individuals against Argentine hemorrhagic fever, but it has not been licensed in the United States. Recent studies have revealed that Candid#1 attenuation is entirely dependent on a phenylalanine-to-isoleucine substitution at position 427 in the fusion subunit (GP2) of the viral envelope glycoprotein complex (GPC), thereby raising concerns regarding the potential for reversion to virulence. In this study, we report the identification and characterization of an intragenic epistatic interaction between the attenuating F427I mutation in GP2 and a lysine-to-serine mutation at position 33 in the stable signal peptide (SSP) subunit of GPC, and we demonstrate the utility of this interaction in creating an evolutionary barrier against reversion to the pathogenic genotype. In the presence of the wild-type F427 residue, the K33S mutation abrogates the ability of ectopically expressed GPC to mediate membrane fusion at endosomal pH. This defect is rescued by the attenuating F427I mutation. We show that the recombinant Candid#1 (rCan) virus bearing K33S GPC is viable and retains its attenuated genotype under cell culture conditions that readily select for reversion in the parental rCan virus. If back-mutation to F427 offers an accessible pathway to increase fitness in rCan, reversion in K33S-GPC rCan is likely to be lethal. The epistatic interaction between K33S and F427I thus may minimize the likelihood of reversion and enhance safety in a second-generation Candid#1 vaccine. IMPORTANCE The live-attenuated Candid#1 vaccine strain of Junín virus is used to protect against Argentine hemorrhagic fever. Recent findings that a single missense mutation in the viral envelope glycoprotein complex (GPC) is responsible for attenuation raise the prospect of facile reversion to pathogenicity. Here, we characterize a genetic interaction between GPC subunits that evolutionarily forces retention of the attenuating mutation. By incorporating this secondary mutation into Candid#1 GPC, we hope to minimize the likelihood of reversion and enhance safety in a second-generation Candid#1 vaccine. A similar approach may guide the design of live-attenuated vaccines against Lassa and other arenaviral hemorrhagic fevers., (Copyright © 2017 American Society for Microbiology.)

Published

2017

9. Convergent immunological solutions to Argentine hemorrhagic fever virus neutralization.

Author

Zeltina A, Krumm SA, Sahin M, Struwe WB, Harlos K, Nunberg JH, Crispin M, Pinschewer DD, Doores KJ, and Bowden TA

Subjects

Antibodies, Monoclonal immunology, Antibodies, Viral immunology, Binding Sites, Crystallography, X-Ray, Enzyme-Linked Immunosorbent Assay, Epitopes chemistry, Glycoproteins chemistry, HEK293 Cells, Humans, Immune System, Junin virus, Protein Binding, Recombinant Proteins immunology, Viral Envelope Proteins chemistry, Antibodies, Neutralizing immunology, Hemorrhagic Fever, American immunology, Neutralization Tests

Abstract

Transmission of hemorrhagic fever New World arenaviruses from their rodent reservoirs to human populations poses substantial public health and economic dangers. These zoonotic events are enabled by the specific interaction between the New World arenaviral attachment glycoprotein, GP1, and cell surface human transferrin receptor (hTfR1). Here, we present the structural basis for how a mouse-derived neutralizing antibody (nAb), OD01, disrupts this interaction by targeting the receptor-binding surface of the GP1 glycoprotein from Junín virus (JUNV), a hemorrhagic fever arenavirus endemic in central Argentina. Comparison of our structure with that of a previously reported nAb complex (JUNV GP1-GD01) reveals largely overlapping epitopes but highly distinct antibody-binding modes. Despite differences in GP1 recognition, we find that both antibodies present a key tyrosine residue, albeit on different chains, that inserts into a central pocket on JUNV GP1 and effectively mimics the contacts made by the host TfR1. These data provide a molecular-level description of how antibodies derived from different germline origins arrive at equivalent immunological solutions to virus neutralization., Competing Interests: The authors declare no conflict of interest.

Published

2017

10. Myristoylation of the Arenavirus Envelope Glycoprotein Stable Signal Peptide Is Critical for Membrane Fusion but Dispensable for Virion Morphogenesis.

Author

York J and Nunberg JH

Subjects

Amino Acid Substitution, Animals, Chlorocebus aethiops, Glycoproteins genetics, Glycoproteins metabolism, Junin virus genetics, Membrane Glycoproteins genetics, Mutant Proteins genetics, Mutant Proteins metabolism, Reverse Genetics, Sequence Deletion, Vero Cells, Viral Envelope Proteins genetics, Virion metabolism, Junin virus physiology, Membrane Glycoproteins metabolism, Myristic Acid metabolism, Protein Processing, Post-Translational, Protein Sorting Signals, Viral Envelope Proteins metabolism, Virus Assembly, Virus Internalization

Abstract

Unlabelled: Arenaviruses are responsible for severe and often fatal hemorrhagic disease. In the absence of effective antiviral therapies and vaccines, these viruses pose serious threats to public health and biodefense. Arenaviruses enter the host cell by fusion of the viral and endosomal membranes, a process mediated by the virus envelope glycoprotein GPC. Unlike other class I viral fusion proteins, GPC retains its stable signal peptide (SSP) as an essential third subunit in the mature complex. SSP spans the membrane twice and is myristoylated at its cytoplasmic N terminus. Mutations that abolish SSP myristoylation have been shown to reduce pH-induced cell-cell fusion activity of ectopically expressed GPC to ∼20% of wild-type levels. In order to examine the role of SSP myristoylation in the context of the intact virus, we used reverse genetics to generate Junín viruses (Candid #1 isolate) in which the critical glycine-2 residue in SSP was either replaced by alanine (G2A) or deleted (ΔG2). These mutant viruses produced smaller foci of infection in Vero cells and showed an ∼5-fold reduction in specific infectivity, commensurate with the defect in cell-cell fusion. However, virus assembly and GPC incorporation into budded virions were unaffected. Our findings suggest that the myristate moiety is cryptically disposed in the prefusion GPC complex and may function late in the fusion process to promote merging of the viral and cellular membranes., Importance: Hemorrhagic fever arenaviruses pose significant threats to public health and biodefense. Arenavirus entry into the host cell is promoted by the virus envelope glycoprotein GPC. Unlike other viral envelope glycoproteins, GPC contains a myristoylated stable signal peptide (SSP) as an essential third subunit. Myristoylation has been shown to be important for the membrane fusion activity of recombinantly expressed GPC. Here, we use reverse genetics to study the role of SSP myristoylation in the context of the intact virion. We find that nonmyristoylated GPC mutants of the Candid #1 strain of Junín virus display a commensurate deficiency in their infectivity, albeit without additional defects in virion assembly and budding. These results suggest that SSP myristoylation may function late in the fusion process to facilitate merging of the viral and cellular membranes. Antiviral agents that target this novel aspect of GPC membrane fusion may be useful in the treatment of arenavirus hemorrhagic fevers., (Copyright © 2016, American Society for Microbiology. All Rights Reserved.)

Published

2016

11. Small-Molecule Fusion Inhibitors Bind the pH-Sensing Stable Signal Peptide-GP2 Subunit Interface of the Lassa Virus Envelope Glycoprotein.

Author

Shankar S, Whitby LR, Casquilho-Gray HE, York J, Boger DL, and Nunberg JH

Subjects

Animals, Chlorocebus aethiops, Humans, Hydrogen-Ion Concentration, Lassa virus, Protein Subunits, Vero Cells, Viral Envelope Proteins chemistry, Antiviral Agents pharmacology, Membrane Fusion drug effects, Protein Sorting Signals, Small Molecule Libraries pharmacology, Viral Envelope Proteins metabolism, Virus Internalization drug effects

Abstract

Unlabelled: Arenavirus species are responsible for severe life-threatening hemorrhagic fevers in western Africa and South America. Without effective antiviral therapies or vaccines, these viruses pose serious public health and biodefense concerns. Chemically distinct small-molecule inhibitors of arenavirus entry have recently been identified and shown to act on the arenavirus envelope glycoprotein (GPC) to prevent membrane fusion. In the tripartite GPC complex, pH-dependent membrane fusion is triggered through a poorly understood interaction between the stable signal peptide (SSP) and the transmembrane fusion subunit GP2, and our genetic studies have suggested that these small-molecule inhibitors act at this interface to antagonize fusion activation. Here, we have designed and synthesized photoaffinity derivatives of the 4-acyl-1,6-dialkylpiperazin-2-one class of fusion inhibitors and demonstrate specific labeling of both the SSP and GP2 subunits in a native-like Lassa virus (LASV) GPC trimer expressed in insect cells. Photoaddition is competed by the parental inhibitor and other chemically distinct compounds active against LASV, but not those specific to New World arenaviruses. These studies provide direct physical evidence that these inhibitors bind at the SSP-GP2 interface. We also find that GPC containing the uncleaved GP1-GP2 precursor is not susceptible to photo-cross-linking, suggesting that proteolytic maturation is accompanied by conformational changes at this site. Detailed mapping of residues modified by the photoaffinity adducts may provide insight to guide the further development of these promising lead compounds as potential therapeutic agents to treat Lassa hemorrhagic fever., Importance: Hemorrhagic fever arenaviruses cause lethal infections in humans and, in the absence of licensed vaccines or specific antiviral therapies, are recognized to pose significant threats to public health and biodefense. Lead small-molecule inhibitors that target the arenavirus envelope glycoprotein (GPC) have recently been identified and shown to block GPC-mediated fusion of the viral and cellular endosomal membranes, thereby preventing virus entry into the host cell. Genetic studies suggest that these inhibitors act through a unique pH-sensing intersubunit interface in GPC, but atomic-level structural information is unavailable. In this report, we utilize novel photoreactive fusion inhibitors and photoaffinity labeling to obtain direct physical evidence for inhibitor binding at this critical interface in Lassa virus GPC. Future identification of modified residues at the inhibitor-binding site will help elucidate the molecular basis for fusion activation and its inhibition and guide the development of effective therapies to treat arenaviral hemorrhagic fevers., (Copyright © 2016, American Society for Microbiology. All Rights Reserved.)

Published

2016

12. Arenavirus infection induces discrete cytosolic structures for RNA replication.

Author

Baird NL, York J, and Nunberg JH

Subjects

Animals, Arenaviruses, New World pathogenicity, Cell Membrane virology, Centrifugation, Density Gradient, Chlorocebus aethiops, Cytosol ultrastructure, Junin virus pathogenicity, Nucleoproteins, Phosphatidylinositol Phosphates analysis, RNA, Viral genetics, Transcription, Genetic, Vero Cells, Arenaviridae Infections virology, Arenaviruses, New World physiology, Cytosol virology, Junin virus physiology, RNA, Viral biosynthesis, Virus Replication

Abstract

Arenaviruses are responsible for acute hemorrhagic fevers with high mortality and pose significant threats to public health and biodefense. These enveloped negative-sense RNA viruses replicate in the cell cytoplasm and express four proteins. To better understand how these proteins insinuate themselves into cellular processes to orchestrate productive viral replication, we have identified and characterized novel cytosolic structures involved in arenavirus replication and transcription. In cells infected with the nonpathogenic Tacaribe virus or the attenuated Candid#1 strain of Junín virus, we find that newly synthesized viral RNAs localize to cytosolic puncta containing the nucleoprotein (N) of the virus. Density gradient centrifugation studies reveal that these replication-transcription complexes (RTCs) are associated with cellular membranes and contain full-length genomic- and antigenomic-sense RNAs. Viral mRNAs segregate at a higher buoyant density and are likewise scant in immunopurified RTCs, consistent with their translation on bulk cellular ribosomes. In addition, confocal microscopy analysis reveals that RTCs contain the lipid phosphatidylinositol-4-phosphate and proteins involved in cellular mRNA metabolism, including the large and small ribosomal subunit proteins L10a and S6, the stress granule protein G3BP1, and a subset of translation initiation factors. Elucidating the structure and function of RTCs will enhance our understanding of virus-cell interactions that promote arenavirus replication and mitigate against host cell immunity. This knowledge may lead to novel intervention strategies to limit viral virulence and pathogenesis.

Published

2012

13. Dissection of the role of the stable signal peptide of the arenavirus envelope glycoprotein in membrane fusion.

Author

Messina EL, York J, and Nunberg JH

Subjects

Amino Acid Sequence, Animals, Arenavirus genetics, Chlorocebus aethiops, Glycoproteins genetics, Models, Molecular, Molecular Sequence Data, Vero Cells, Viral Envelope Proteins genetics, Arenavirus physiology, Glycoproteins metabolism, Protein Sorting Signals, Viral Envelope Proteins metabolism, Virus Internalization

Abstract

The arenavirus envelope glycoprotein (GPC) retains a stable signal peptide (SSP) as an essential subunit in the mature complex. The 58-amino-acid residue SSP comprises two membrane-spanning hydrophobic regions separated by a short ectodomain loop that interacts with the G2 fusion subunit to promote pH-dependent membrane fusion. Small-molecule compounds that target this unique SSP-G2 interaction prevent arenavirus entry and infection. The interaction between SSP and G2 is sensitive to the phylogenetic distance between New World (Junín) and Old World (Lassa) arenaviruses. For example, heterotypic GPC complexes are unable to support virion entry. In this report, we demonstrate that the hybrid GPC complexes are properly assembled, proteolytically cleaved, and transported to the cell surface but are specifically defective in their membrane fusion activity. Chimeric SSP constructs reveal that this incompatibility is localized to the first transmembrane segment of SSP (TM1). Genetic changes in TM1 also affect sensitivity to small-molecule fusion inhibitors, generating resistance in some cases and inhibitor dependence in others. Our studies suggest that interactions of SSP TM1 with the transmembrane domain of G2 may be important for GPC-mediated membrane fusion and its inhibition.

Published

2012

14. The curious case of arenavirus entry, and its inhibition.

Author

Nunberg JH and York J

Subjects

Amino Acid Sequence, Animals, Antigens, CD physiology, Antiviral Agents pharmacology, Arenaviridae classification, Arenaviridae Infections virology, Conserved Sequence, Disease Reservoirs, Endosomes virology, Forecasting, Humans, Membrane Fusion drug effects, Membrane Glycoproteins chemistry, Membrane Glycoproteins physiology, Models, Molecular, Molecular Sequence Data, Phylogeny, Protein Conformation, Protein Sorting Signals physiology, Receptors, Transferrin physiology, Receptors, Virus physiology, Rodentia virology, Sequence Alignment, Sequence Homology, Amino Acid, Viral Envelope Proteins chemistry, Viral Envelope Proteins physiology, Arenaviridae physiology, Virus Internalization drug effects

Abstract

Arenaviruses comprise a diverse family of enveloped negative-strand RNA viruses that are endemic to specific rodent hosts worldwide. Several arenaviruses cause severe hemorrhagic fevers in humans, including Junín and Machupo viruses in South America and Lassa fever virus in western Africa. Arenavirus entry into the host cell is mediated by the envelope glycoprotein complex, GPC. The virion is endocytosed on binding to a cell-surface receptor, and membrane fusion is initiated in response to physiological acidification of the endosome. As with other class I virus fusion proteins, GPC-mediated membrane fusion is promoted through a regulated sequence of conformational changes leading to formation of the classical postfusion trimer-of-hairpins structure. GPC is, however, unique among the class I fusion proteins in that the mature complex retains a stable signal peptide (SSP) as a third subunit, in addition to the canonical receptor-binding and fusion proteins. We will review the curious properties of the tripartite GPC complex and describe evidence that SSP interacts with the fusion subunit to modulate pH-induced activation of membrane fusion. This unusual solution to maintaining the metastable prefusion state of GPC on the virion and activating the class I fusion cascade at acidic pH provides novel targets for antiviral intervention.

Published

2012

15. Biochemical reconstitution of hemorrhagic-fever arenavirus envelope glycoprotein-mediated membrane fusion.

Author

Thomas CJ, Shankar S, Casquilho-Gray HE, York J, Sprang SR, and Nunberg JH

Subjects

Animals, Antibodies, Neutralizing immunology, Chlorocebus aethiops, Furin metabolism, Humans, Hydrogen-Ion Concentration, Lipids chemistry, Mutant Proteins metabolism, Neutralization Tests, Protein Conformation, Proteolipids metabolism, Proteolysis, Recombinant Proteins metabolism, Surface Plasmon Resonance, Vero Cells, Virus Shedding, Glycoproteins metabolism, Junin virus metabolism, Membrane Fusion, Viral Envelope Proteins metabolism

Abstract

The membrane-anchored proteins of enveloped viruses form labile spikes on the virion surface, primed to undergo large-scale conformational changes culminating in virus-cell membrane fusion and viral entry. The prefusion form of these envelope glycoproteins thus represents an important molecular target for antiviral intervention. A critical roadblock to this endeavor has been our inability to produce the prefusion envelope glycoprotein trimer for biochemical and structural analysis. Through our studies of the GPC envelope glycoprotein of the hemorrhagic fever arenaviruses, we have shown that GPC is unique among class I viral fusion proteins in that the mature complex retains a stable signal peptide (SSP) in addition to the conventional receptor-binding and transmembrane fusion subunits. In this report we show that the recombinant GPC precursor can be produced as a discrete native-like trimer and that its proteolytic cleavage generates the mature glycoprotein. Proteoliposomes containing the cleaved GPC mediate pH-dependent membrane fusion, a characteristic feature of arenavirus entry. This reaction is inhibited by arenavirus-specific monoclonal antibodies and small-molecule fusion inhibitors. The in vitro reconstitution of GPC-mediated membrane-fusion activity offers unprecedented opportunities for biochemical and structural studies of arenavirus entry and its inhibition. To our knowledge, this report is the first to demonstrate functional reconstitution of membrane fusion by a viral envelope glycoprotein.

Published

2012

16. A specific interaction of small molecule entry inhibitors with the envelope glycoprotein complex of the Junín hemorrhagic fever arenavirus.

Author

Thomas CJ, Casquilho-Gray HE, York J, DeCamp DL, Dai D, Petrilli EB, Boger DL, Slayden RA, Amberg SM, Sprang SR, and Nunberg JH

Subjects

Animals, Antigens, CD genetics, Antiviral Agents chemistry, Arenaviridae Infections genetics, Arenaviridae Infections metabolism, Chlorocebus aethiops, Humans, Junin virus genetics, Receptors, Transferrin genetics, Vero Cells, Viral Envelope Proteins genetics, Virus Internalization drug effects, Antigens, CD metabolism, Antiviral Agents pharmacology, Arenaviridae Infections drug therapy, Junin virus metabolism, Receptors, Transferrin metabolism, Viral Envelope Proteins antagonists & inhibitors, Viral Envelope Proteins metabolism

Abstract

Arenaviruses are responsible for acute hemorrhagic fevers worldwide and are recognized to pose significant threats to public health and biodefense. Small molecule compounds have recently been discovered that inhibit arenavirus entry and protect against lethal infection in animal models. These chemically distinct inhibitors act on the tripartite envelope glycoprotein (GPC) through its unusual stable signal peptide subunit to stabilize the complex against pH-induced activation of membrane fusion in the endosome. Here, we report the production and characterization of the intact transmembrane GPC complex of Junín arenavirus and its interaction with these inhibitors. The solubilized GPC is antigenically indistinguishable from the native protein and forms a homogeneous trimer in solution. When reconstituted into a lipid bilayer, the purified complex interacts specifically with its cell-surface receptor transferrin receptor-1. We show that small molecule entry inhibitors specific to New World or Old World arenaviruses bind to the membrane-associated GPC complex in accordance with their respective species selectivities and with dissociation constants comparable with concentrations that inhibit GPC-mediated membrane fusion. Furthermore, competitive binding studies reveal that these chemically distinct inhibitors share a common binding pocket on GPC. In conjunction with previous genetic studies, these findings identify the pH-sensing interface of GPC as a highly vulnerable target for antiviral intervention. This work expands our mechanistic understanding of arenavirus entry and provides a foundation to guide the development of small molecule compounds for the treatment of arenavirus hemorrhagic fevers.

Published

2011

17. T-705 (favipiravir) inhibition of arenavirus replication in cell culture.

Author

Mendenhall M, Russell A, Juelich T, Messina EL, Smee DF, Freiberg AN, Holbrook MR, Furuta Y, de la Torre JC, Nunberg JH, and Gowen BB

Subjects

Animals, Arenaviruses, New World physiology, Cell Line, Chlorocebus aethiops, Humans, Junin virus drug effects, Junin virus physiology, Lymphocytic choriomeningitis virus drug effects, Lymphocytic choriomeningitis virus physiology, Microbial Sensitivity Tests methods, Ribavirin pharmacology, Vero Cells, Amides pharmacology, Antiviral Agents pharmacology, Arenaviruses, New World drug effects, Pyrazines pharmacology, Virus Replication drug effects

Abstract

A number of New World arenaviruses (Junín [JUNV], Machupo [MACV], and Guanarito [GTOV] viruses) can cause human disease ranging from mild febrile illness to a severe and often fatal hemorrhagic fever syndrome. These highly pathogenic viruses and the Old World Lassa fever virus pose a significant threat to public health and national security. The only licensed antiviral agent with activity against these viruses, ribavirin, has had mixed success in treating severe arenaviral disease and is associated with significant toxicities. A novel pyrazine derivative currently in clinical trials for the treatment of influenza virus infections, T-705 (favipiravir), has demonstrated broad-spectrum activity against a number of RNA viruses, including arenaviruses. T-705 has also been shown to be effective against Pichinde arenavirus infection in a hamster model. Here, we demonstrate the robust antiviral activity of T-705 against authentic highly pathogenic arenaviruses in cell culture. We show that T-705 disrupts an early or intermediate stage in viral replication, distinct from absorption or release, and that its antiviral activity in cell culture is reversed by the addition of purine bases and nucleosides, but not with pyrimidines. Specific inhibition of viral replication/transcription by T-705 was demonstrated using a lymphocytic choriomeningitis arenavirus replicon system. Our findings indicate that T-705 acts to inhibit arenavirus replication/transcription and may directly target the viral RNA-dependent RNA polymerase.

Published

2011

18. Structure of a zinc-binding domain in the Junin virus envelope glycoprotein.

Author

Briknarová K, Thomas CJ, York J, and Nunberg JH

Subjects

Amino Acid Sequence, Conserved Sequence, Hydrogen-Ion Concentration, Junin virus metabolism, Membrane Glycoproteins genetics, Membrane Glycoproteins metabolism, Molecular Sequence Data, Nuclear Magnetic Resonance, Biomolecular, Protein Binding, Protein Interaction Domains and Motifs physiology, Protein Sorting Signals physiology, Protein Structure, Tertiary, Viral Envelope Proteins genetics, Viral Envelope Proteins metabolism, Zinc metabolism, Zinc Fingers physiology, Junin virus chemistry, Membrane Glycoproteins chemistry, Viral Envelope Proteins chemistry, Virus Internalization, Zinc chemistry

Abstract

Arenaviruses cause acute hemorrhagic fevers with high mortality. Entry of the virus into the host cell is mediated by the viral envelope glycoprotein, GPC. In contrast to other class I viral envelope glycoproteins, the mature GPC complex contains a cleaved stable signal peptide (SSP) in addition to the canonical receptor-binding (G1) and transmembrane fusion (G2) subunits. SSP is critical for intracellular transport of the GPC complex to the cell surface and for its membrane-fusion activity. Previous studies have suggested that SSP is retained in GPC through interaction with a zinc-binding domain (ZBD) in the cytoplasmic tail of G2. Here we used NMR spectroscopy to determine the structure of Junín virus (JUNV) ZBD (G2 residues 445-485) and investigate its interaction with a conserved Cys residue (Cys-57) in SSP. We show that JUNV ZBD displays a novel fold containing two zinc ions. One zinc ion is coordinated by His-447, His-449, Cys-455, and His-485. The second zinc ion is coordinated by His-459, Cys-467, and Cys-469 and readily accepts Cys-57 from SSP as the fourth ligand. Our studies describe the structural basis for retention of the unique SSP subunit and suggest a mechanism whereby SSP is positioned in the GPC complex to modulate pH-dependent membrane fusion.

Published

2011

19. An antibody directed against the fusion peptide of Junin virus envelope glycoprotein GPC inhibits pH-induced membrane fusion.

Author

York J, Berry JD, Ströher U, Li Q, Feldmann H, Lu M, Trahey M, and Nunberg JH

Subjects

Amino Acid Sequence, Animals, Arenaviridae Infections immunology, Arenaviridae Infections virology, Chlorocebus aethiops, Glycoproteins chemistry, Glycoproteins genetics, Hydrogen-Ion Concentration, Junin virus chemistry, Junin virus drug effects, Junin virus genetics, Molecular Sequence Data, Sequence Alignment, Vero Cells, Viral Fusion Proteins chemistry, Viral Fusion Proteins genetics, Antibodies pharmacology, Glycoproteins immunology, Junin virus physiology, Membrane Fusion drug effects, Viral Fusion Proteins immunology

Abstract

The arenavirus envelope glycoprotein (GPC) initiates infection in the host cell through pH-induced fusion of the viral and endosomal membranes. As in other class I viral fusion proteins, this process proceeds through a structural reorganization in GPC in which the ectodomain of the transmembrane fusion subunit (G2) engages the host cell membrane and subsequently refolds to form a highly stable six-helix bundle structure that brings the two membranes into apposition for fusion. Here, we describe a G2-directed monoclonal antibody, F100G5, that prevents membrane fusion by binding to an intermediate form of the protein on the fusion pathway. Inhibition of syncytium formation requires that F100G5 be present concomitant with exposure of GPC to acidic pH. We show that F100G5 recognizes neither the six-helix bundle nor the larger trimer-of-hairpins structure in the postfusion form of G2. Rather, Western blot analysis using recombinant proteins and a panel of alanine-scanning GPC mutants revealed that F100G5 binding is dependent on an invariant lysine residue (K283) near the N terminus of G2, in the so-called fusion peptide that inserts into the host cell membrane during the fusion process. The F100G5 epitope is located in the internal segment of the bipartite GPC fusion peptide, which also contains four conserved cysteine residues, raising the possibility that this fusion peptide may be highly structured. Collectively, our studies indicate that F100G5 identifies an on-path intermediate form of GPC. Binding to the transiently exposed fusion peptide may interfere with G2 insertion into the host cell membrane. Strategies to effectively target fusion peptide function in the endosome may lead to novel classes of antiviral agents.

Published

2010

20. Assembly of arenavirus envelope glycoprotein GPC in detergent-soluble membrane microdomains.

Author

Agnihothram SS, Dancho B, Grant KW, Grimes ML, Lyles DS, and Nunberg JH

Subjects

Animals, Cell Membrane virology, Chlorocebus aethiops, Immunohistochemistry, Membrane Microdomains chemistry, Microscopy, Confocal methods, Microscopy, Electron methods, Myristic Acid metabolism, Octoxynol pharmacology, Protein Structure, Tertiary, Vero Cells, Viral Envelope Proteins chemistry, Arenavirus metabolism, Cell Membrane metabolism, Detergents pharmacology, Glycoproteins chemistry

Abstract

The family Arenaviridae includes a number of highly pathogenic viruses that are responsible for acute hemorrhagic fevers in humans. Genetic diversity among arenavirus species in their respective rodent hosts supports the continued emergence of new pathogens. In the absence of available vaccines or therapeutic agents, the hemorrhagic fever arenaviruses remain a serious public health and biodefense concern. Arenaviruses are enveloped virions that assemble and bud from the plasma membrane. In this study, we have characterized the microdomain organization of the virus envelope glycoprotein (GPC) on the cell surface by using immunogold electron microscopy. We find that Junín virus (JUNV) GPC clusters into discrete microdomains of 120 to 160 nm in diameter and that this property of GPC is independent of its myristoylation and of coexpression with the virus matrix protein Z. In cells infected with the Candid#1 strain of JUNV, and in purified Candid#1 virions, these GPC microdomains are soluble in cold Triton X-100 detergent and are thus distinct from conventional lipid rafts, which are utilized by numerous other viruses for assembly. Virion morphogenesis ultimately requires colocalization of viral components, yet our dual-label immunogold staining studies failed to reveal a spatial association of Z with GPC microdomains. This observation may reflect either rapid Z-dependent budding of virus-like particles upon coassociation or a requirement for additional viral components in the assembly process. Together, these results provide new insight into the molecular basis for arenavirus morphogenesis.

Published

2009

21. Intersubunit interactions modulate pH-induced activation of membrane fusion by the Junin virus envelope glycoprotein GPC.

Author

York J and Nunberg JH

Subjects

Amino Acid Sequence, Animals, Chlorocebus aethiops, Glycoproteins chemistry, Glycoproteins genetics, Hydrogen-Ion Concentration, Junin virus genetics, Molecular Sequence Data, Mutation genetics, Peptides genetics, Peptides metabolism, Protein Subunits chemistry, Protein Subunits genetics, Protein Subunits metabolism, Sequence Alignment, Vero Cells, Viral Envelope Proteins chemistry, Viral Envelope Proteins genetics, Glycoproteins metabolism, Junin virus metabolism, Membrane Fusion, Viral Envelope Proteins metabolism, Virus Internalization

Abstract

The mature arenavirus envelope glycoprotein GPC is a tripartite complex comprising a stable signal peptide (SSP) in addition to the receptor-binding (G1) and transmembrane fusion (G2) subunits. We have shown previously that SSP is a key element in GPC-mediated membrane fusion, and that GPC sensitivity to acidic pH is modulated in part through the lysine residue at position 33 in the ectodomain loop of SSP (J. York and J. H. Nunberg, J. Virol. 80:7775-7780, 2006). A glutamine substitution at this position stabilizes the native GPC complex and thereby prevents the induction of pH-dependent membrane fusion. In efforts to identify the intersubunit interactions of K33, we performed alanine-scanning mutagenesis at charged residues in the membrane-proximal ectodomain of G2 and determined the ability of these mutations to rescue the fusion deficiency in K33Q GPC. Four second-site mutations that specifically complement K33Q were identified (D400A, E410A, R414A, and K417A). Moreover, complementation was also observed at three hydrophobic positions in the membrane-spanning domain of G2 (F427, W428, and F438). Interestingly, all of the complementing mutations restored wild-type pH sensitivity to the K33Q mutant, while none themselves affected the pH of membrane fusion. Our studies demonstrate a specific interaction between SSP and G2 that is involved in priming the native GPC complex for pH-induced membrane fusion. Importantly, this pH-dependent interaction has been shown to be vulnerable to small-molecule compounds that stabilize the native complex and prevent the activation of membrane fusion. A detailed mechanistic understanding of the control of GPC-mediated membrane fusion will be important in guiding the development of effective therapeutics against arenaviral hemorrhagic fever.

Published

2009

22. pH-induced activation of arenavirus membrane fusion is antagonized by small-molecule inhibitors.

Author

York J, Dai D, Amberg SM, and Nunberg JH

Subjects

Amino Acid Sequence, Amino Acid Substitution genetics, Antiviral Agents pharmacology, Drug Resistance, Viral, Hydrogen-Ion Concentration, Models, Biological, Models, Molecular, Molecular Sequence Data, Protein Binding, Sequence Alignment, Urea pharmacology, Arenavirus drug effects, Arenavirus physiology, Membrane Fusion drug effects, Membrane Fusion physiology, Sulfonamides pharmacology, Urea analogs & derivatives, Viral Envelope Proteins metabolism, Virus Internalization drug effects

Abstract

The arenavirus envelope glycoprotein (GPC) mediates viral entry through pH-induced membrane fusion in the endosome. This crucial process in the viral life cycle can be specifically inhibited in the New World arenaviruses by the small-molecule compound ST-294. Here, we show that ST-294 interferes with GPC-mediated membrane fusion by targeting the interaction of the G2 fusion subunit with the stable signal peptide (SSP). We demonstrate that amino acid substitutions at lysine-33 of the Junín virus SSP confer resistance to ST-294 and engender de novo sensitivity to ST-161, a chemically distinct inhibitor of the Old World Lassa fever virus. These compounds, as well as a broadly active inhibitor, ST-193, likely share a molecular target at the SSP-G2 interface. We also show that both ST-294 and ST-193 inhibit pH-induced dissociation of the G1 receptor-binding subunit from GPC, a process concomitant with fusion activation. Interestingly, the inhibitory activity of these molecules can in some cases be overcome by further lowering the pH used for activation. Our results suggest that these small molecules act to stabilize the prefusion GPC complex against acidic pH. The pH-sensitive interaction between SSP and G2 in GPC represents a robust molecular target for the development of antiviral compounds for the treatment of arenavirus hemorrhagic fevers.

Published

2008

23. Unique small molecule entry inhibitors of hemorrhagic fever arenaviruses.

Author

Lee AM, Rojek JM, Spiropoulou CF, Gundersen AT, Jin W, Shaginian A, York J, Nunberg JH, Boger DL, Oldstone MB, and Kunz S

Subjects

Animals, Antiviral Agents therapeutic use, Chlorocebus aethiops, Drug Evaluation, Preclinical, HeLa Cells, Humans, Vero Cells, Virion metabolism, Antiviral Agents chemistry, Antiviral Agents pharmacology, Arenaviridae Infections drug therapy, Arenavirus, Communicable Diseases, Emerging drug therapy, Hemorrhagic Fevers, Viral drug therapy, Viral Fusion Proteins antagonists & inhibitors

Abstract

Viral hemorrhagic fevers caused by the arenaviruses Lassa virus in Africa and Machupo, Guanarito, Junin, and Sabia virus in South America are among the most devastating emerging human diseases with fatality rates of 15-35% and a limited antiviral therapeutic repertoire available. Here we used high throughput screening of synthetic combinatorial small molecule libraries to identify inhibitors of arenavirus infection using pseudotyped virion particles bearing the glycoproteins (GPs) of highly pathogenic arenaviruses. Our screening efforts resulted in the discovery of a series of novel small molecule inhibitors of viral entry that are highly active against both Old World and New World hemorrhagic arenaviruses. We observed potent inhibition of infection of human and primate cells with live hemorrhagic arenaviruses (IC(50)=500-800 nm). Investigations of the mechanism of action revealed that the candidate compounds efficiently block pH-dependent fusion by the arenavirus GPs (IC(50) of 200-350 nm). Although our lead compounds were potent against phylogenetically distant arenaviruses, they did not show activity against other enveloped viruses with class I viral fusion proteins, indicating specificity for arenavirus GP-mediated membrane fusion.

Published

2008

24. A novel zinc-binding domain is essential for formation of the functional Junín virus envelope glycoprotein complex.

Author

York J and Nunberg JH

Subjects

Amino Acid Motifs, Amino Acid Sequence, Animals, Chlorocebus aethiops, Glycoproteins chemistry, Glycoproteins genetics, Hydrogen-Ion Concentration, Junin virus chemistry, Junin virus genetics, Membrane Fusion, Molecular Sequence Data, Protein Sorting Signals, Vero Cells, Viral Envelope Proteins chemistry, Viral Envelope Proteins genetics, Viral Fusion Proteins chemistry, Viral Fusion Proteins genetics, Zinc Fingers genetics, Glycoproteins metabolism, Junin virus metabolism, Viral Envelope Proteins metabolism, Viral Fusion Proteins metabolism, Zinc metabolism

Abstract

The envelope glycoprotein of the Junín arenavirus (GP-C) mediates entry into target cells through a pH-dependent membrane fusion mechanism. Unlike other class I viral fusion proteins, the mature GP-C complex retains a cleaved, 58-amino-acid signal peptide (SSP) as an essential subunit, required both for trafficking of GP-C to the cell surface and for the activation of membrane fusion. SSP has been shown to associate noncovalently in GP-C via the cytoplasmic domain (CTD) of the transmembrane fusion subunit G2. In this report we investigate the molecular basis for this intersubunit interaction. We identify an invariant series of six cysteine and histidine residues in the CTD of G2 that is essential for incorporation of SSP in the GP-C complex. Moreover, we show that a CTD peptide fragment containing His-447, His-449, and Cys-455 specifically binds Zn(2+) at subnanomolar concentrations. Together, these results suggest a zinc finger-like domain structure in the CTD of G2. We propose that the remaining residues in the series (His-459, Cys-467, and Cys-469) form an intersubunit zinc-binding center that incorporates Cys-57 of SSP. This unusual motif may act to retain SSP in the GP-C complex and position the ectodomain loop of SSP for its role in modulating membrane fusion activity. The unique tripartite organization of GP-C could provide novel molecular targets for therapeutic intervention in arenaviral disease.

Published

2007

25. Bitopic membrane topology of the stable signal peptide in the tripartite Junín virus GP-C envelope glycoprotein complex.

Author

Agnihothram SS, York J, Trahey M, and Nunberg JH

Subjects

Amino Acid Sequence, Cell Fusion, Detergents pharmacology, Digitonin pharmacology, Hydrophobic and Hydrophilic Interactions, Junin virus physiology, Microscopy, Confocal, Models, Molecular, Molecular Sequence Data, Viral Envelope Proteins metabolism, Virus Assembly physiology, Cell Membrane chemistry, Cell Membrane virology, Cytoplasm chemistry, Junin virus chemistry, Protein Sorting Signals, Viral Envelope Proteins chemistry

Abstract

The stable signal peptide (SSP) of the GP-C envelope glycoprotein of the Junín arenavirus plays a critical role in trafficking of the GP-C complex to the cell surface and in its membrane fusion activity. SSP therefore may function on both sides of the lipid membrane. In this study, we have investigated the membrane topology of SSP by confocal microscopy of cells treated with the detergent digitonin to selectively permeabilize the plasma membrane. By using an affinity tag to mark the termini of SSP in the properly assembled GP-C complex, we find that both the N and C termini reside in the cytosol. Thus, SSP adopts a bitopic topology in which the C terminus is translocated from the lumen of the endoplasmic reticulum to the cytoplasm. This model is supported by (i) the presence of two conserved hydrophobic regions in SSP (hphi1 and hphi2) and (ii) our previous demonstration that lysine-33 in the ectodomain loop is essential for pH-dependent membrane fusion. Moreover, we demonstrate that the introduction of a charged side chain or single amino acid deletion in the membrane-spanning hphi2 region significantly diminishes SSP association in the GP-C complex and abolishes membrane fusion activity. Taken together, our results suggest that bitopic membrane insertion of SSP is centrally important in the assembly and function of the tripartite GP-C complex.

Published

2007

26. Transferrin receptor 1 is a cellular receptor for New World haemorrhagic fever arenaviruses.

Author

Radoshitzky SR, Abraham J, Spiropoulou CF, Kuhn JH, Nguyen D, Li W, Nagel J, Schmidt PJ, Nunberg JH, Andrews NC, Farzan M, and Choe H

Subjects

Antibodies immunology, Antibodies pharmacology, Antigens, CD genetics, Antigens, CD immunology, Arenaviruses, New World drug effects, Arenaviruses, New World physiology, Culture Media chemistry, Glycoproteins metabolism, Humans, Iron analysis, Iron pharmacology, Receptors, Transferrin antagonists & inhibitors, Receptors, Transferrin genetics, Receptors, Transferrin immunology, Viral Envelope Proteins metabolism, Virus Replication drug effects, Antigens, CD metabolism, Arenaviruses, New World metabolism, Receptors, Transferrin metabolism, Receptors, Virus metabolism

Abstract

At least five arenaviruses cause viral haemorrhagic fevers in humans. Lassa virus, an Old World arenavirus, uses the cellular receptor alpha-dystroglycan to infect cells. Machupo, Guanarito, Junin and Sabia viruses are New World haemorrhagic fever viruses that do not use alpha-dystroglycan. Here we show a specific, high-affinity association between transferrin receptor 1 (TfR1) and the entry glycoprotein (GP) of Machupo virus. Expression of human TfR1, but not human transferrin receptor 2, in hamster cell lines markedly enhanced the infection of viruses pseudotyped with the GP of Machupo, Guanarito and Junin viruses, but not with those of Lassa or lymphocytic choriomeningitis viruses. An anti-TfR1 antibody efficiently inhibited the replication of Machupo, Guanarito, Junin and Sabia viruses, but not that of Lassa virus. Iron depletion of culture medium enhanced, and iron supplementation decreased, the efficiency of infection by Junin and Machupo but not Lassa pseudoviruses. These data indicate that TfR1 is a cellular receptor for New World haemorrhagic fever arenaviruses.

Published

2007

27. Distinct requirements for signal peptidase processing and function in the stable signal peptide subunit of the Junín virus envelope glycoprotein.

Author

York J and Nunberg JH

Subjects

Amino Acid Sequence, Animals, Biological Transport, Chlorocebus aethiops, Junin virus genetics, Membrane Fusion, Molecular Sequence Data, Mutagenesis, Site-Directed, Protein Precursors chemistry, Protein Precursors immunology, Protein Precursors metabolism, Protein Sorting Signals genetics, Vero Cells, Viral Envelope Proteins chemistry, Viral Envelope Proteins genetics, Junin virus physiology, Membrane Proteins metabolism, Protein Sorting Signals physiology, Serine Endopeptidases metabolism, Viral Envelope Proteins metabolism

Abstract

The arenavirus envelope glycoprotein (GP-C) retains a cleaved and stable signal peptide (SSP) as an essential subunit of the mature complex. This 58-amino-acid residue peptide serves as a signal sequence and is additionally required to enable transit of the assembled GP-C complex to the Golgi, and for pH-dependent membrane fusion activity. We have investigated the C-terminal region of the Junín virus SSP to study the role of the cellular signal peptidase (SPase) in generating SSP. Site-directed mutagenesis at the cleavage site (positions -1 and -3) reveals a pattern of side-chain preferences consistent with those of SPase. Although position -2 is degenerate for SPase cleavage, this residue in the arenavirus SSP is invariably a cysteine. In the Junín virus, this cysteine is not involved in disulfide bonding. We show that replacement with alanine or serine is tolerated for SPase cleavage but prevents the mutant SSP from associating with GP-C and enabling transport to the cell surface. Conversely, an arginine mutation at position -1 that prevents SPase cleavage is fully compatible with GP-C-mediated membrane fusion activity when the mutant SSP is provided in trans. These results point to distinct roles of SSP sequences in SPase cleavage and GP-C biogenesis. Further studies of the unique structural organization of the GP-C complex will be important in identifying novel opportunities for antiviral intervention against arenaviral hemorrhagic disease.

Published

2007

28. Oligomerization of hepatitis C virus core protein is crucial for interaction with the cytoplasmic domain of E1 envelope protein.

Author

Nakai K, Okamoto T, Kimura-Someya T, Ishii K, Lim CK, Tani H, Matsuo E, Abe T, Mori Y, Suzuki T, Miyamura T, Nunberg JH, Moriishi K, and Matsuura Y

Subjects

Amino Acid Sequence, Glycosylation, Hepacivirus genetics, Immunoprecipitation, Molecular Sequence Data, Protein Binding, Protein Conformation, Protein Interaction Mapping, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Sequence Deletion, Two-Hybrid System Techniques, Viral Core Proteins chemistry, Viral Core Proteins genetics, Viral Envelope Proteins chemistry, Viral Envelope Proteins genetics, Hepacivirus physiology, Viral Core Proteins metabolism, Viral Envelope Proteins metabolism

Abstract

Hepatitis C virus (HCV) contains two membrane-associated envelope glycoproteins, E1 and E2, which assemble as a heterodimer in the endoplasmic reticulum (ER). In this study, predictive algorithms and genetic analyses of deletion mutants and glycosylation site variants of the E1 glycoprotein were used to suggest that the glycoprotein can adopt two topologies in the ER membrane: the conventional type I membrane topology and a polytopic topology in which the protein spans the ER membrane twice with an intervening cytoplasmic loop (amino acid residues 288 to 360). We also demonstrate that the E1 glycoprotein is able to associate with the HCV core protein, but only upon oligomerization of the core protein in the presence of tRNA to form capsid-like structures. Yeast two-hybrid and immunoprecipitation analyses reveal that oligomerization of the core protein is promoted by amino acid residues 72 to 91 in the core. Furthermore, the association between the E1 glycoprotein and the assembled core can be recapitulated using a fusion protein containing the putative cytoplasmic loop of the E1 glycoprotein. This fusion protein is also able to compete with the intact E1 glycoprotein for binding to the core. Mutagenesis of the cytoplasmic loop of E1 was used to define a region of four amino acids (residues 312 to 315) that is important for interaction with the assembled HCV core. Taken together, our studies suggest that interaction between the self-oligomerized HCV core and the E1 glycoprotein is mediated through the cytoplasmic loop present in a polytopic form of the E1 glycoprotein.

Published

2006

29. Role of the stable signal peptide of Junín arenavirus envelope glycoprotein in pH-dependent membrane fusion.

Author

York J and Nunberg JH

Subjects

Amino Acid Sequence, Amino Acid Substitution, Animals, Cell Fusion, Chlorocebus aethiops, Glycoproteins genetics, Hydrogen-Ion Concentration, Junin virus genetics, Lysine genetics, Lysine metabolism, Molecular Sequence Data, Protein Precursors chemistry, Protein Precursors metabolism, Protein Processing, Post-Translational, Sequence Homology, Amino Acid, Vero Cells, Viral Envelope Proteins genetics, Glycoproteins metabolism, Junin virus metabolism, Membrane Fusion, Protein Sorting Signals physiology, Viral Envelope Proteins metabolism

Abstract

The envelope glycoprotein of the arenaviruses (GP-C) is unusual in that the mature complex retains the cleaved, 58-amino-acid signal peptide. Association of this stable signal peptide (SSP) has been shown to be essential for intracellular trafficking and proteolytic maturation of the GP-C complex. We identify here a specific and previously unrecognized role of SSP in pH-dependent membrane fusion. Amino acid substitutions that alter the positive charge at lysine K33 in SSP affect the ability of GP-C to mediate cell-cell fusion and the threshold pH at which membrane fusion is triggered. Based on the presumed location of K33 at or near the luminal domain of SSP, we postulate that SSP interacts with the membrane-proximal or transmembrane regions of the G2 fusion protein. This unique organization of the GP-C complex may suggest novel strategies for intervention in arenavirus infection.

Published

2006

30. Furin cleavage of the SARS coronavirus spike glycoprotein enhances cell-cell fusion but does not affect virion entry.

Author

Follis KE, York J, and Nunberg JH

Subjects

Amino Acid Sequence, Animals, COS Cells, Cell Fusion, Chlorocebus aethiops, Membrane Glycoproteins chemistry, Membrane Glycoproteins genetics, Molecular Sequence Data, Spike Glycoprotein, Coronavirus, Viral Envelope Proteins chemistry, Viral Envelope Proteins genetics, Virion genetics, Virion physiology, Furin metabolism, Membrane Glycoproteins physiology, Severe acute respiratory syndrome-related coronavirus physiology, Viral Envelope Proteins physiology

Abstract

The fusogenic potential of Class I viral envelope glycoproteins is activated by proteloytic cleavage of the precursor glycoprotein to generate the mature receptor-binding and transmembrane fusion subunits. Although the coronavirus (CoV) S glycoproteins share membership in this class of envelope glycoproteins, cleavage to generate the respective S1 and S2 subunits appears absent in a subset of CoV species, including that responsible for the severe acute respiratory syndrome (SARS). To determine whether proteolytic cleavage of the S glycoprotein might be important for the newly emerged SARS-CoV, we introduced a furin recognition site at single basic residues within the putative S1-S2 junctional region. We show that furin cleavage at the modified R667 position generates discrete S1 and S2 subunits and potentiates membrane fusion activity. This effect on the cell-cell fusion activity by the S glycoprotein is not, however, reflected in the infectivity of pseudotyped lentiviruses bearing the cleaved glycoprotein. The lack of effect of furin cleavage on virion infectivity mirrors that observed in the normally cleaved S glycoprotein of the murine coronavirus and highlights an additional level of complexity in coronavirus entry.

Published

2006

31. Role of the stable signal peptide and cytoplasmic domain of G2 in regulating intracellular transport of the Junín virus envelope glycoprotein complex.

Author

Agnihothram SS, York J, and Nunberg JH

Subjects

Animals, Biological Transport, Chlorocebus aethiops, Glycoproteins genetics, Protein Structure, Tertiary, Vero Cells, Viral Fusion Proteins chemistry, Viral Fusion Proteins metabolism, Glycoproteins metabolism, Junin virus chemistry, Protein Sorting Signals physiology, Viral Envelope Proteins metabolism

Abstract

Enveloped viruses utilize the membranous compartments of the host cell for the assembly and budding of new virion particles. In this report, we have investigated the biogenesis and trafficking of the envelope glycoprotein (GP-C) of the Junín arenavirus. The mature GP-C complex is unusual in that it retains a stable signal peptide (SSP) as an essential component in association with the typical receptor-binding (G1) and transmembrane fusion (G2) subunits. We demonstrate that, in the absence of SSP, the G1-G2 precursor is restricted to the endoplasmic reticulum (ER). This constraint is relieved by coexpression of SSP in trans, allowing transit of the assembled GP-C complex through the Golgi and to the cell surface, the site of arenavirus budding. Transport of a chimeric CD4 glycoprotein bearing the transmembrane and cytoplasmic domains of G2 is similarly regulated by SSP association. Truncations to the cytoplasmic domain of G2 abrogate SSP association yet now permit transport of the G1-G2 precursor to the cell surface. Thus, the cytoplasmic domain of G2 is an important determinant for both ER localization and its control through SSP binding. Alanine mutations to either of two dibasic amino acid motifs in the G2 cytoplasmic domain can also mobilize the G1-G2 precursor for transit through the Golgi. Taken together, our results suggest that SSP binding masks endogenous ER localization signals in the cytoplasmic domain of G2 to ensure that only the fully assembled, tripartite GP-C complex is transported for virion assembly. This quality control process points to an important role of SSP in the structure and function of the arenavirus envelope glycoprotein.

Published

2006

32. Genetic analysis of heptad-repeat regions in the G2 fusion subunit of the Junín arenavirus envelope glycoprotein.

Author

York J, Agnihothram SS, Romanowski V, and Nunberg JH

Subjects

Amino Acid Sequence, Animals, Chlorocebus aethiops, Humans, Hydrogen-Ion Concentration, Junin virus pathogenicity, Junin virus physiology, Membrane Fusion, Models, Molecular, Molecular Sequence Data, Mutagenesis, Insertional, Protein Structure, Tertiary, Protein Subunits, Recombinant Proteins chemistry, Recombinant Proteins genetics, Sequence Homology, Amino Acid, Vero Cells, Viral Envelope Proteins chemistry, Viral Fusion Proteins chemistry, Junin virus genetics, Viral Envelope Proteins genetics, Viral Fusion Proteins genetics

Abstract

The G2 fusion subunit of the Junín virus envelope glycoprotein GP-C contains two hydrophobic heptad-repeat regions that are postulated to form a six-helix bundle structure required for the membrane fusion activity of Class I viral fusion proteins. We have investigated the role of these heptad-repeat regions and, specifically, the importance of the putative interhelical a and d position sidechains by using alanine-scanning mutagenesis. All the mutant glycoproteins were expressed and transported to the cell surface. Proteolytic maturation at the subtilisin kexin isozyme-1/site-1-protease (SKI-1/S1P) cleavage site was observed in all but two of the mutants. Among the adequately cleaved mutant glycoproteins, four positions in the N-terminal region (I333, L336, L347 and L350) and two positions in the C-terminal region (R392 and W395) were shown to be important determinants of cell-cell fusion. Taken together, our results indicate that alpha-helical coiled-coil structures are likely critical in promoting arenavirus membrane fusion. These findings support the inclusion of the arenavirus GP-C among the Class I viral fusion proteins and suggest pharmacologic and immunologic strategies for targeting arenavirus infection and hemorrhagic fever.

Published

2005

33. Serine-scanning mutagenesis studies of the C-terminal heptad repeats in the SARS coronavirus S glycoprotein highlight the important role of the short helical region.

Author

Follis KE, York J, and Nunberg JH

Subjects

Amino Acid Sequence, Animals, COS Cells, Chlorocebus aethiops, Membrane Fusion genetics, Membrane Fusion physiology, Membrane Glycoproteins physiology, Models, Molecular, Molecular Sequence Data, Mutagenesis, Protein Structure, Secondary, Recombinant Proteins chemistry, Recombinant Proteins genetics, Repetitive Sequences, Amino Acid, Severe acute respiratory syndrome-related coronavirus pathogenicity, Spike Glycoprotein, Coronavirus, Transfection, Viral Envelope Proteins physiology, Membrane Glycoproteins chemistry, Membrane Glycoproteins genetics, Severe acute respiratory syndrome-related coronavirus genetics, Severe acute respiratory syndrome-related coronavirus physiology, Viral Envelope Proteins chemistry, Viral Envelope Proteins genetics

Abstract

The fusion subunit of the SARS-CoV S glycoprotein contains two regions of hydrophobic heptad-repeat amino acid sequences that have been shown in biophysical studies to form a six-helix bundle structure typical of the fusion-active core found in Class I viral fusion proteins. Here, we have applied serine-scanning mutagenesis to the C-terminal-most heptad-repeat region in the SARS-CoV S glycoprotein to investigate the functional role of this region in membrane fusion. We show that hydrophobic sidechains at a and d positions only within the short helical segment of the C-terminal heptad-repeat region (I1161, I1165, L1168, A1172, and L1175) are critical for cell-cell fusion. Serine mutations at outlying heptad-repeat residues that form an extended chain in the core structure (V1158, L1179, and L1182) do not affect fusogenicity. Our study provides genetic evidence for the important role of alpha-helical packing in promoting S glycoprotein-mediated membrane fusion.

Published

2005

34. The signal peptide of the Junín arenavirus envelope glycoprotein is myristoylated and forms an essential subunit of the mature G1-G2 complex.

Author

York J, Romanowski V, Lu M, and Nunberg JH

Subjects

Amino Acid Sequence, Amino Acid Substitution, Animals, CD4 Antigens genetics, CD4 Antigens metabolism, Cell Fusion, Chlorocebus aethiops, Conserved Sequence, Glycoproteins metabolism, Hydrogen-Ion Concentration, Membrane Fusion, Molecular Sequence Data, Protein Precursors chemistry, Protein Precursors metabolism, Protein Processing, Post-Translational, Sequence Homology, Amino Acid, Vero Cells, Viral Envelope Proteins metabolism, Viral Fusion Proteins chemistry, Viral Fusion Proteins metabolism, Glycoproteins chemistry, Junin virus chemistry, Protein Sorting Signals physiology, Protein Subunits metabolism, Viral Envelope Proteins chemistry

Abstract

Arenaviruses comprise a diverse family of rodent-borne viruses that are responsible for recurring and emerging outbreaks of viral hemorrhagic fevers worldwide. The Junín virus, a member of the New World arenaviruses, is endemic to the pampas grasslands of Argentina and is the etiologic agent of Argentine hemorrhagic fever. In this study, we have analyzed the assembly and function of the Junín virus envelope glycoproteins. The mature envelope glycoprotein complex is proteolytically processed from the GP-C precursor polypeptide and consists of three noncovalently associated subunits, G1, G2, and a stable 58-amino-acid signal peptide. This tripartite organization is found both on virions of the attenuated Candid 1 strain and in cells expressing the pathogenic MC2 strain GP-C gene. Replacement of the Junín virus GP-C signal peptide with that of human CD4 has little effect on glycoprotein assembly while abolishing the ability of the G1-G2 complex to mediate pH-dependent cell-cell fusion. In addition, we demonstrate that the Junín virus GP-C signal peptide subunit is myristoylated at its N-terminal glycine. Alanine substitution for the modified glycine residue in the GP-C signal peptide does not affect formation of the tripartite envelope glycoprotein complex but markedly reduces its membrane fusion activity. In contrast to the classical view that signal peptides act primarily in targeting nascent polypeptides to the endoplasmic reticulum, we suggest that the signal peptide of the arenavirus GP-C may serve additional functions in envelope glycoprotein structure and trafficking.

Published

2004

35. Evidence for a polytopic form of the E1 envelope glycoprotein of Hepatitis C virus.

Author

Migliaccio CT, Follis KE, Matsuura Y, and Nunberg JH

Subjects

Amino Acid Sequence, Animals, Antibodies, Monoclonal immunology, Antibodies, Monoclonal metabolism, Antigens, Viral chemistry, Antigens, Viral genetics, Antigens, Viral immunology, Antigens, Viral metabolism, Dimerization, Epitopes immunology, Hepatitis C Antibodies immunology, Hepatitis C Antibodies metabolism, Humans, Mice, Molecular Sequence Data, Protein Conformation, Protein Folding, Protein Processing, Post-Translational, Protein Structure, Tertiary, Protein Transport, Proteolipids immunology, Proteolipids metabolism, Viral Envelope Proteins genetics, Viral Envelope Proteins immunology, Hepacivirus physiology, Viral Envelope Proteins chemistry, Viral Envelope Proteins metabolism

Abstract

The polyprotein precursor of the Hepatitis C virus (HCV) contains multiple membrane-spanning domains that define the membrane topology and subsequent maturation of the viral structural proteins. In order to examine the biogenesis of the E1-E2 heterodimeric complex, we inserted an affinity tag (S-peptide) at specific locations within the envelope glycoproteins. In particular, and based on the prediction that the E1 glycoprotein may be able to assume a polytopic topology containing two membrane-spanning domains, we inserted the affinity tag within a putative cytoplasmic loop of the E1 glycoprotein. The HCV structural polyprotein containing this tag (at amino acids 295/296) was highly expressed and able to form a properly processed and noncovalently associated E1-E2 complex. This complex was bound by murine and conformation-dependent human monoclonal antibodies (MAbs) comparably to the native untagged complex. In addition, MAb recognition was retained upon reconstituting the tagged E1-E2 complex in lipid membrane as topologically constrained proteoliposomes. Our findings are consistent with the model of a topologically flexible E1 glycoprotein that is able to adopt a polytopic form. This form of the E1-E2 complex may be important in the HCV life cycle and in pathogenesis.

Published

2004

36. Role of hydrophobic residues in the central ectodomain of gp41 in maintaining the association between human immunodeficiency virus type 1 envelope glycoprotein subunits gp120 and gp41.

Author

York J and Nunberg JH

Subjects

Amino Acid Sequence, Animals, COS Cells, Chlorocebus aethiops, Giant Cells, HIV Envelope Protein gp120 genetics, HIV Envelope Protein gp41 genetics, Humans, Membrane Fusion, Mutagenesis, Site-Directed, Mutation, Protein Conformation, HIV Envelope Protein gp120 metabolism, HIV Envelope Protein gp41 chemistry, HIV Envelope Protein gp41 metabolism, HIV-1 pathogenicity, Hydrophobic and Hydrophilic Interactions

Abstract

The interaction between the gp120 and gp41 subunits of the human immunodeficiency virus envelope glycoprotein serves to stabilize the virion form of the complex and to transmit receptor-induced conformational changes in gp120 to trigger the membrane fusion activity of gp41. In this study, we used site-directed mutagenesis to identify amino acid residues in the central ectodomain of gp41 that contribute to the stability of the gp120-gp41 association. We identified alanine mutations at six positions, including four tryptophan residues, which result in mutant envelope glycoprotein complexes that fail to retain gp120 on the cell surface. These envelope glycoproteins readily shed their gp120 and are unable to mediate cell-cell fusion. These findings suggest an important role for the conserved bulky hydrophobic residues in stabilizing the gp120-gp41 complex.

Published

2004

37. Genetic evidence that interhelical packing interactions in the gp41 core are critical for transition of the human immunodeficiency virus type 1 envelope glycoprotein to the fusion-active state.

Author

Follis KE, Larson SJ, Lu M, and Nunberg JH

Subjects

Amino Acid Sequence, Antibodies, Monoclonal immunology, HIV Envelope Protein gp120 genetics, HIV Envelope Protein gp41 genetics, HIV Envelope Protein gp41 immunology, HIV-1 pathogenicity, Humans, Molecular Sequence Data, Protein Conformation, HIV Envelope Protein gp120 metabolism, HIV Envelope Protein gp41 chemistry, HIV Envelope Protein gp41 metabolism, HIV-1 metabolism, Membrane Fusion, Mutation

Abstract

The envelope glycoprotein complex (gp120-gp41) of human immunodeficiency virus type 1 (HIV-1) promotes the fusion of viral and cellular membranes through formation of the fusion-active six-helix bundle in the gp41 ectodomain. This gp41 core structure consists of three C-terminal helices packed in an antiparallel manner into hydrophobic grooves on the surface of the N-terminal trimeric coiled coil. Alanine mutations that destabilize the N- and C-terminal interhelical packing interactions also reduce viral infectivity. Here we show that viruses bearing these mutations exhibit a marked potentiation of inhibition by peptides that make up the gp41 core. By contrast, these viruses are unchanged in their sensitivities to soluble CD4, the CXCR4 coreceptor ligand SDF-1alpha, and human anti-HIV immunoglobulin, reagents that impact the initial, receptor-induced conformational changes in the envelope glycoprotein. Our results support the notion that these alanine mutations specifically affect the conformational transition to the fusion-active gp41 structure. The mutations also increase viral sensitivity to the gp41-directed monoclonal antibody 2F5, suggesting that this broadly neutralizing antibody may also interfere with this transition. The conformational activation of the HIV-1 envelope glycoprotein likely represents a viable target for vaccine and antiviral drug development.

Published

2002

38. Interhelical interactions in the gp41 core: implications for activation of HIV-1 membrane fusion.

Author

Wang S, York J, Shu W, Stoller MO, Nunberg JH, and Lu M

Subjects

Alanine genetics, Amino Acid Sequence, Animals, COS Cells, Cell Line, Transformed, Coculture Techniques, Crystallography, X-Ray, Gene Products, env biosynthesis, Gene Products, env genetics, Gene Products, env physiology, Glycoproteins biosynthesis, Glycoproteins genetics, Glycoproteins physiology, HIV Envelope Protein gp41 chemistry, HIV Envelope Protein gp41 genetics, HIV Envelope Protein gp41 physiology, HIV-1 genetics, Humans, Isoleucine genetics, Membrane Fusion genetics, Molecular Sequence Data, Mutagenesis, Site-Directed, Peptide Fragments chemistry, Peptide Fragments genetics, Peptide Fragments metabolism, Peptide Fragments physiology, Protein Structure, Secondary genetics, Protein Structure, Tertiary genetics, Virus Activation genetics, HIV Envelope Protein gp41 metabolism, HIV-1 physiology, Membrane Fusion physiology, Virus Activation physiology

Abstract

The human immunodeficiency virus type 1 (HIV-1) envelope glycoprotein complex (gp120-gp41) promotes viral entry by mediating the fusion of viral and cellular membranes. Formation of a stable trimer-of-hairpins structure in the gp41 ectodomain brings the two membranes into proximity, leading to membrane fusion. The core of this hairpin structure is a six-helix bundle in which three carboxyl-terminal outer helices pack against an inner trimeric coiled coil. Here we investigate the role of these conserved interhelical interactions on the structure and function of both the envelope glycoprotein and the gp41 core. We have replaced each of the eight amino acids at the buried face of the carboxyl-terminal helix with a representative amino acid, alanine. Structural and physicochemical characterization of the alanine mutants shows that hydrophobic interactions are a dominant factor in the stabilization of the six-helix bundle. Alanine substitutions at the Trp628, Trp631, Ile635, and Ile642 residues also affected envelope processing and/or gp120-gp41 association and abrogated the ability of the envelope glycoprotein to mediate cell-cell fusion. These results suggest that the amino-terminal region of the gp41 outer-layer alpha-helix plays a key role in the sequence of events associated with HIV-1 entry and have implications for the development of antibodies and small-molecule inhibitors of this conserved element.

Published

2002

39. Retraction.

Author

Nunberg JH

Published

2002

40. Structural and functional analysis of interhelical interactions in the human immunodeficiency virus type 1 gp41 envelope glycoprotein by alanine-scanning mutagenesis.

Author

Lu M, Stoller MO, Wang S, Liu J, Fagan MB, and Nunberg JH

Subjects

Alanine, Amino Acid Sequence, Animals, COS Cells, Cell Fusion, Crystallization, HIV Envelope Protein gp41 physiology, Molecular Sequence Data, Mutagenesis, Protein Conformation, HIV Envelope Protein gp41 chemistry, HIV-1 chemistry

Abstract

Membrane fusion by human immunodeficiency virus type 1 (HIV-1) is promoted by the refolding of the viral envelope glycoprotein into a fusion-active conformation. The structure of the gp41 ectodomain core in its fusion-active state is a trimer of hairpins in which three antiparallel carboxyl-terminal helices pack into hydrophobic grooves on the surface of an amino-terminal trimeric coiled coil. In an effort to identify amino acid residues in these grooves that are critical for gp41 activation, we have used alanine-scanning mutagenesis to investigate the importance of individual side chains in determining the biophysical properties of the gp41 core and the membrane fusion activity of the gp120-gp41 complex. Alanine substitutions at Leu-556, Leu-565, Val-570, Gly-572, and Arg-579 positions severely impaired membrane fusion activity in envelope glycoproteins that were for the most part normally expressed. Whereas alanine mutations at Leu-565 and Val-570 destabilized the trimer-of-hairpins structure, mutations at Gly-572 and Arg-579 led to the formation of a stable gp41 core. Our results suggest that the Leu-565 and Val-570 residues are important determinants of conserved packing interactions between the amino- and carboxyl-terminal helices of gp41. We propose that the high degree of sequence conservation at Gly-572 and Arg-579 may result from selective pressures imposed by prefusogenic conformations of the HIV-1 envelope glycoprotein. Further analysis of the gp41 activation process may elucidate targets for antiviral intervention.

Published

2001

41. Structural and functional analysis of the HIV gp41 core containing an Ile573 to Thr substitution: implications for membrane fusion.

Author

Liu J, Shu W, Fagan MB, Nunberg JH, and Lu M

Subjects

Amino Acid Sequence, Cell Line, Conserved Sequence, Crystallography, X-Ray, HIV Envelope Protein gp41 physiology, HIV-1 pathogenicity, Humans, Molecular Sequence Data, Protein Conformation, Protein Structure, Secondary genetics, Protein Structure, Tertiary genetics, Repetitive Sequences, Amino Acid, Structure-Activity Relationship, Transfection, Tumor Cells, Cultured, Virion genetics, Virion pathogenicity, Virulence, Amino Acid Substitution genetics, HIV Envelope Protein gp41 chemistry, HIV Envelope Protein gp41 genetics, HIV-1 genetics, Isoleucine genetics, Membrane Fusion genetics, Threonine genetics

Abstract

The envelope glycoprotein of HIV-1 consists of the surface subunit gp120 and the transmembrane subunit gp41. Binding of gp120 to target cell receptors induces a conformational change in gp41, which then mediates the fusion of viral and cellular membranes. A buried isoleucine (Ile573) in a central trimeric coiled coil within the fusion-active gp41 ectodomain core is thought to favor this conformational activation. The role of Ile573 in determining the structure and function of the gp120-gp41 complex was investigated by mutating this residue to threonine, a nonconservative substitution in HIV-1 that occurs naturally in SIV. While the introduction of Thr573 markedly destabilized the gp41 core, the three-dimensional structure of the mutant trimer of hairpins was very similar to that of the wild-type molecule. A new hydrogen-bonding interaction between the buried Thr573 and Thr569 residues appears to allow formation of the trimer-of-hairpins structure at physiological temperature. The mutant envelope glycoprotein expressed in 293T cells and incorporated within pseudotyped virions displayed only a moderate reduction in syncytium-inducing capacity and virus infectivity, respectively. Our results demonstrate that the proper folding of the gp41 core underlies the membrane fusion properties of the gp120-gp41 complex. An understanding of the gp41 activation process may suggest novel strategies for vaccine and antiviral drug development.

Published

2001

42. Antibody binding and neutralization of primary and T-cell line-adapted isolates of human immunodeficiency virus type 1.

Author

York J, Follis KE, Trahey M, Nyambi PN, Zolla-Pazner S, and Nunberg JH

Subjects

Antibody Affinity, Cell Line, Flow Cytometry, Gene Products, env immunology, HIV Infections immunology, HIV-1 metabolism, HIV-1 pathogenicity, Humans, Neutralization Tests, T-Lymphocytes virology, Transfection, Virion immunology, Virion pathogenicity, Antibodies, Monoclonal immunology, HIV Antibodies immunology, HIV Infections virology, HIV-1 immunology

Abstract

The relative resistance of human immunodeficiency virus type 1 (HIV-1) primary isolates (PIs) to neutralization by a wide range of antibodies remains a theoretical and practical barrier to the development of an effective HIV vaccine. One model to account for the differential neutralization sensitivity between Pls and laboratory (or T-cell line-adapted [TCLA]) strains of HIV suggests that the envelope protein (Env) complex is made more accessible to antibody binding as a consequence of adaptation to growth in established cell lines. Here, we revisit this question using genetically related PI and TCLA viruses and molecularly cloned env genes. By using complementary techniques of flow cytometry and virion binding assays, we show that monoclonal antibodies targeting the V3 loop, CD4-binding site, CD4-induced determinant of gp120, or the ectodomain of gp41 bind equally well to PI and TCLA Env complexes, despite large differences in neutralization outcome. The data suggest that the differential neutralization sensitivity of PI and TCLA viruses may derive not from differences in the initial antibody binding event but rather from differences in the subsequent functioning of the PI and TCLA Envs during virus entry. An understanding of these as yet undefined differences may enhance our ability to generate broadly neutralizing HIV vaccine immunogens.

Published

2001

43. Turning a corner on HIV neutralization?

Author

Nunberg JH, Follis KE, Trahey M, and LaCasse RA

Subjects

Animals, HIV Envelope Protein gp120 immunology, Humans, Neutralization Tests, Peptide Fragments immunology, AIDS Vaccines immunology, HIV immunology, HIV Infections prevention & control, Vaccines, Synthetic immunology

Abstract

HIV vaccine development has been hampered by the inability of conventional immunogens to elicit antibodies capable of neutralizing primary isolates of the virus. Recent studies using 'fusion-competent' immunogens that capture transitional intermediate structures of the functioning envelope protein suggest that this goal may now be achievable.

Published

2000

44. Fusion-competent vaccines: broad neutralization of primary isolates of HIV.

Author

LaCasse RA, Follis KE, Trahey M, Scarborough JD, Littman DR, and Nunberg JH

Subjects

Animals, CD4 Antigens metabolism, Cell Fusion, Coculture Techniques, Epitopes immunology, Gene Products, env chemistry, Gene Products, env metabolism, Giant Cells, HIV Antibodies biosynthesis, HIV Antigens chemistry, HIV Envelope Protein gp120 chemistry, HIV Envelope Protein gp120 immunology, HIV Envelope Protein gp120 metabolism, HIV Envelope Protein gp41 chemistry, HIV Envelope Protein gp41 immunology, HIV Envelope Protein gp41 metabolism, HIV Infections virology, HIV-1 isolation & purification, HIV-1 physiology, Humans, Mice, Mice, Transgenic, Neutralization Tests, Protein Conformation, Receptors, CCR5 metabolism, Tumor Cells, Cultured, AIDS Vaccines immunology, Gene Products, env immunology, HIV Antibodies immunology, HIV Antigens immunology, HIV-1 immunology

Abstract

Current recombinant human immunodeficiency virus (HIV) gp120 protein vaccine candidates are unable to elicit antibodies capable of neutralizing infectivity of primary isolates from patients. Here, "fusion-competent" HIV vaccine immunogens were generated that capture the transient envelope-CD4-coreceptor structures that arise during HIV binding and fusion. In a transgenic mouse immunization model, these formaldehyde-fixed whole-cell vaccines elicited antibodies capable of neutralizing infectivity of 23 of 24 primary HIV isolates from diverse geographic locations and genetic clades A to E. Development of these fusion-dependent immunogens may lead to a broadly effective HIV vaccine.

Published

1999

45. Continued utilization of CCR5 coreceptor by a newly derived T-cell line-adapted isolate of human immunodeficiency virus type 1.

Author

Follis KE, Trahey M, LaCasse RA, and Nunberg JH

Subjects

Adaptation, Biological, Base Sequence, DNA, Viral, HIV Envelope Protein gp120 genetics, HIV-1 genetics, HIV-1 immunology, Humans, Molecular Sequence Data, Neutralization Tests, Sequence Analysis, DNA, Tumor Cells, Cultured, HIV-1 metabolism, Receptors, CCR5 metabolism, T-Lymphocytes virology

Abstract

The differential use of CC chemokine receptor 5 (CCR5) and CXC chemokine receptor 4 (CXCR4) may be intimately involved in the transmission and progression of human immunodeficiency virus infection. Changes in coreceptor utilization have also been noted upon adaptation of primary isolates (PI) to growth in established T-cell lines. All of the T-cell line-adapted (TCLA) viruses studied to date utilize CXCR4 but not CCR5. This observation had been suggested as an explanation for the sensitivity of TCLA, but not PI, viruses to neutralization by recombinant gp120 antisera and V3-directed monoclonal antibodies, but recent studies have shown coreceptor utilization to be independent of neutralization sensitivity. Here we describe a newly isolated TCLA virus that is sensitive to neutralization but continues to utilize both CXCR4 and CCR5 for infection. This finding further divorces coreceptor specificity from neutralization sensitivity and from certain changes in cell tropism. That the TCLA virus can continue to utilize CCR5 despite the changes that occur upon adaptation and in the apparent absence of CCR5 expression in the FDA/H9 T-cell line suggests that the interaction between envelope protein and coreceptor may be mediated by multiple weak interactions along a diffuse surface.

Published

1998

46. Coreceptor utilization by human immunodeficiency virus type 1 is not a primary determinant of neutralization sensitivity.

Author

LaCasse RA, Follis KE, Moudgil T, Trahey M, Binley JM, Planelles V, Zolla-Pazner S, and Nunberg JH

Subjects

Animals, Base Sequence, COS Cells, Cell Line, Cloning, Molecular, DNA, Viral, Genes, env, HIV Antibodies immunology, HIV-1 genetics, HIV-1 isolation & purification, Humans, Molecular Sequence Data, Neutralization Tests, Antibodies, Monoclonal immunology, HIV Antigens immunology, HIV Envelope Protein gp120 immunology, HIV-1 immunology, HIV-1 metabolism, Peptide Fragments immunology, Receptors, CCR5 metabolism, Receptors, CXCR4 metabolism

Abstract

We have examined the relationship between coreceptor utilization and sensitivity to neutralization in a primary isolate of human immunodeficiency virus type 1 and its T-cell line-adapted (TCLA) derivative. We determined that adaptation of the primary-isolate (PI) virus 168P results in the loss of the unique capacity of PI viruses to utilize the CCR5 coreceptor and in the acquisition by the TCLA 168C virus of sensitivity to neutralization by V3-directed monoclonal antibodies (MAbs). In experiments wherein infection by 168P is directed via either the CCR5 or the CXCR4 pathway, we demonstrate that the virus, as well as pseudotyped virions bearing a molecularly cloned 168P envelope protein, remains refractory to neutralization by MAbs 257-D, 268-D, and 50.1 regardless of the coreceptor utilized. This study suggests that coreceptor utilization is not a primary determinant of differential neutralization sensitivity in PI and TCLA viruses.

Published

1998

47. Synthetic peptides from P. falciparum sexual stage 25-kDa protein induce antibodies that react with the native protein: the role of IL-2 and conformational structure on immunogenicity of Pfs25.

Author

Quakyi IA, Miller LH, Good MF, Ahlers JD, Isaacs SN, Nunberg JH, Houghten RA, Keister DB, Coligan JE, and Moss B

Subjects

Amino Acid Sequence, Animals, Antibodies, Monoclonal, Epitopes chemistry, Epitopes immunology, Female, Humans, Immunization, Male, Mice, Mice, Inbred A, Mice, Inbred BALB C, Molecular Sequence Data, Peptide Fragments chemistry, Plasmodium falciparum chemistry, Protein Conformation, Recombinant Proteins pharmacology, Antibodies, Protozoan immunology, Interleukin-2 pharmacology, Peptide Fragments immunology, Plasmodium falciparum immunology, Protozoan Proteins chemistry, Protozoan Proteins immunology

Abstract

To identify B-cell epitopes of the Plasmodium falciparum 25-kDa ookinete protein, Pfs25, 41 overlapping synthetic peptides spanning the entire length of the protein were used individually to immunize CAF1 (F1 hybrid of BALB/c female and A/J male) mice. Antipeptide sera were tested for reactivity to live intact zygote/early ookinete (post-fertilization stage) by immunofluorescence, and by Western blot analysis under nonreducing and reducing conditions, immunoprecipitation of 35S-cysteine-labeled antigen, and ELISA using a vaccinia recombinant Pfs25 antigen. Fourteen B-cell epitopes were identified. These peptides were immunogenic only when administered with high-dose recombinant interleukin-2. Antibodies to 11 peptides recognized only the native conformational structure, one peptide induced antibodies that recognized both reduced and native protein, and two other peptides, after primary immunization, made antibodies to denatured Pfs25, but after boosting the antibodies reacted to both denatured and native Pfs25. Anti-sera to peptides in the first (peptide 7) and fourth (peptide 34) epidermal growth factor-like domains of Pfs25 reacted most strongly with zygotes/ookinetes by immunofluorescence assay. The antibodies elicited by immunization with peptide 34 suppressed infectivity of the parasite to mosquitoes. We further observed that the secondary structure of Pfs25 may be important for immunogenicity because monoclonal antibodies (MAbs) 1C7 and 1D2, both transmission-blocking MAbs, protected enzyme cleavage sites in Pfs25 from proteolysis, suggesting that discontinuous segments of Pfs25 may come together to form immunogenic epitopic sites. Thus, definition of B- and T-cell epitopes may be required to construct a Pfs25 vaccine for optimum immunogenicity.

Published

1995

48. Adaptation to persistent growth in the H9 cell line renders a primary isolate of human immunodeficiency virus type 1 sensitive to neutralization by vaccine sera.

Author

Wrin T, Loh TP, Vennari JC, Schuitemaker H, and Nunberg JH

Subjects

AIDS Vaccines immunology, Amino Acid Sequence, Animals, Antibodies, Monoclonal immunology, Base Sequence, Cell Line, DNA Primers, Guinea Pigs, HIV Envelope Protein gp120 immunology, Humans, Immunoglobulins, Intravenous immunology, Molecular Sequence Data, Virus Replication, Adaptation, Physiological, Antibodies, Viral immunology, HIV-1 immunology, HIV-1 physiology, Neutralization Tests

Abstract

Seven diverse primary isolates of human immunodeficiency virus type 1 (HIV-1) were examined and found to be refractory to neutralization by antisera to recombinant gp120 (rgp120) protein from HIV-1 MN. This stands in marked contrast to the sensitivity exhibited by certain laboratory-adapted viruses. To understand the difference between primary and laboratory-adapted viruses, we adapted the primary virus ACH 168.10 to growth in the FDA/H9 cell line. ACH 168.10 was chosen because the V3 region of gp120 closely matches that of MN. After 4 weeks, infection became evident. The virus (168A) replicated in FDA/H9 cells with extensive cytopathic effect but was unchanged in sensitivity to antibody-mediated neutralization. Thus, growth in cell lines is not sufficient to render primary virus sensitive to neutralization. The 168A virus was, however, partially sensitive to CD4 immunoadhesin (CD4-Ig). Adaptation was continued to produce a persistently infected FDA/H9 culture that displayed minimal cytopathic effect. The virus (168C) was now sensitive to neutralization by MN rgp120 vaccine sera and by MN-specific monoclonal antibodies and showed increased sensitivity to HIVIG and CD4-Ig. 168C encoded three amino acid changes in gp120, including one within the V3 loop (I-166-->R, I-282-->N, G-318-->R). MN-specific monoclonal antibodies bound equally to the surface of cells infected with either neutralization-resistant or -sensitive virus. The coincidence of changes in neutralization sensitivity with changes in cell tropism and cytopathic effect suggests a common underlying mechanism(s) acting through the whole of the envelope protein complex.

Published

1995

49. HIV-1MN recombinant gp120 vaccine serum, which fails to neutralize primary isolates of HIV-1, does not antagonize neutralization by antibodies from infected individuals.

Author

Wrin T and Nunberg JH

Subjects

Acquired Immunodeficiency Syndrome blood, HIV Antibodies blood, HIV Infections blood, HIV-1 isolation & purification, Humans, Neutralization Tests, AIDS Vaccines immunology, Acquired Immunodeficiency Syndrome immunology, HIV Antibodies immunology, HIV Envelope Protein gp120 immunology, HIV Infections immunology, HIV-1 immunology, Vaccines, Synthetic immunology

Published

1994

50. Development of a single-shot subunit vaccine for HIV-1.

Author

Cleland JL, Powell MF, Lim A, Barrón L, Berman PW, Eastman DJ, Nunberg JH, Wrin T, and Vennari JC

Subjects

AIDS Vaccines administration & dosage, Adjuvants, Immunologic administration & dosage, Alum Compounds administration & dosage, Animals, Delayed-Action Preparations, Guinea Pigs, HIV Antibodies biosynthesis, HIV Envelope Protein gp120 administration & dosage, HIV Envelope Protein gp120 immunology, HIV Envelope Protein gp120 isolation & purification, Humans, Microspheres, Neutralization Tests, Peptide Fragments immunology, Polylactic Acid-Polyglycolic Acid Copolymer, Polymers administration & dosage, Saponins administration & dosage, Vaccines, Synthetic administration & dosage, Vaccines, Synthetic isolation & purification, AIDS Vaccines isolation & purification, HIV-1 immunology, Lactic Acid, Polyglycolic Acid

Abstract

The successful development of an AIDS vaccine will require formulations that not only invoke the desired immunological response, but also are stable and easy to administer. A single shot MN rgp120 vaccine formulation comprised of MN rgp120 encapsulated in poly (lactic-coglycolic) acid (PLGA) microspheres was developed to provide an in vivo autoboost of antigen. These formulations were designed to yield an in vivo autoboost at 1, 2, 3 or 4-6 months. In addition, PLGA microspheres containing the adjuvant, QS21, were also prepared to provide an in vivo autoboost concomitant with antigen. In guinea pigs, these formulations yielded higher anti-MN rgp120 and anti-V3 loop antibody titers than alum formulations that were administered at higher antigen doses. Different doses of encapsulated MN rgp120 provided a clear and well-defined dose response curve for both anti-MN rgp120 and anti-V3 loop antibody titers. When soluble QS21 was mixed with the encapsulated MN rgp120, the antibody titers were increased by a factor of 5 over the titers with encapsulated MN rgp120 alone. An additional fivefold increase in antibody titers was observed for guinea pigs immunized with encapsulated MN rgp120 and QS21 on the same microspheres. These results suggest that the adjuvant properties of QS21 can be increased by microencapsulation in PLGA. Furthermore, antibodies induced by these preparations neutralized the MN strain of HIV-1. The neutralization titers for sera from animals immunized with MN rgp120-PLGA and soluble QS21 were greater than the titers obtained from guinea pigs that were treated with MN rgp120 and soluble QS21 at the same dose. Overall, these studies validate the in vivo autoboost concept, reveal a method for improving the adjuvant properties of QS21, and indicate the potential of future single shot vaccine formulations.

Published

1994