Your search keyword '"Doms RW"' showing total 252 results

1. 2G12/PGT-binding yeast glycoprotein Gp38 elicits mannose-specific HIV-1 Env cross-reactive antibodies

Author

Zhang H, Fu H, Liu B, Luallen RJ, Doms RW, Smith DF, and Geng Y

Subjects

Immunologic diseases. Allergy, RC581-607

Published

2012

2. Viral entry denied.

Author

Doms RW

Published

2004

3. Differential escape patterns within the dominant HLA-B*57:03-restricted HIV Gag epitope reflect distinct clade-specific functional constraints

Author

Richard Haubrich, S. Branch, P. R. Harrigan, Anne Edwards, Simon Mallal, Emily Adland, Eric Hunter, Zabrina L. Brumme, Pjr Goulder, Philippa C Matthews, Jonathan M. Carlson, JP Jooste, T. Strong, John Frater, Beatriz Mothe, Christian Brander, Steven G. Deeks, Henrik N. Kløverpris, Fabian Chen, Rebecca Payne, C Landis, Mina John, Bruce D. Walker, Lynn Riddell, Catherine K. Koofhethile, Julia G. Prado, Roger L. Shapiro, Thumbi Ndung'u, Ellen M. Leitman, and Doms, RW

Subjects

Male, Cytotoxic, T-Lymphocytes, HIV Infections, Medical and Health Sciences, gag Gene Products, Human Immunodeficiency Virus, Epitope, Cohort Studies, Epitopes, 2.2 Factors relating to the physical environment, 2.1 Biological and endogenous factors, Aetiology, Biological Sciences, Middle Aged, HLA-B, Infectious Diseases, HIV/AIDS, Female, Infection, Viral load, Human Immunodeficiency Virus, Adult, Genotype, Immunology, Mutation, Missense, Human leukocyte antigen, Biology, Microbiology, Virus, Immune system, Genetic, Clinical Research, Virology, Genetics, Humans, Selection, Genetic, Selection, gag Gene Products, Immune Evasion, Agricultural and Veterinary Sciences, Chronic infection, CTL, Good Health and Well Being, HLA-B Antigens, Insect Science, Mutation, Pathogenesis and Immunity, Immunization, Missense, T-Lymphocytes, Cytotoxic

Abstract

HLA-B*57:01 and HLA-B*57:03, the most prevalent HLA-B*57 subtypes in Caucasian and African populations, respectively, are the HLA alleles most protective against HIV disease progression. Understanding the mechanisms underlying this immune control is of critical importance, yet they remain unclear. Unexplained differences are observed in the impact of the dominant cytotoxic T lymphocyte (CTL) response restricted by HLA-B*57:01 and HLA-B*57:03 in chronic infection on the Gag epitope KAFSPEVIPMF (KF11; Gag 162 to 172). We previously showed that the HLA-B*57:03-KF11 response is associated with a >1-log-lower viral setpoint in C clade virus infection and that this response selects escape mutants within the epitope. We first examined the relationship of KF11 responses in B clade virus-infected subjects with HLA-B*57:01 to immune control and observed that a detectable KF11 response was associated with a >1-log-higher viral load ( P = 0.02). No evidence of HLA-B*57:01-KF11-associated selection pressure was identified in previous comprehensive analyses of >1,800 B clade virus-infected subjects. We then studied a B clade virus-infected cohort in Barbados, where HLA-B*57:03 is highly prevalent. In contrast to findings for B clade virus-infected subjects expressing HLA-B*57:01, we observed strong selection pressure driven by the HLA-B*57:03-KF11 response for the escape mutation S173T. This mutation reduces recognition of virus-infected cells by HLA-B*57:03-KF11 CTLs and is associated with a >1-log increase in viral load in HLA-B*57:03-positive subjects ( P = 0.009). We demonstrate functional constraints imposed by HIV clade relating to the residue at Gag 173 that explain the differential clade-specific escape patterns in HLA-B*57:03 subjects. Further studies are needed to evaluate the role of the KF11 response in HLA-B*57:01-associated HIV disease protection. IMPORTANCE HLA-B*57 is the HLA class I molecule that affords the greatest protection against disease progression in HIV infection. Understanding the key mechanism(s) underlying immunosuppression of HIV is of importance in guiding therapeutic and vaccine-related approaches to improve the levels of HIV control occurring in nature. Numerous mechanisms have been proposed to explain the HLA associations with differential HIV disease outcome, but no consensus exists. These studies focus on two subtypes of HLA-B*57 prevalent in Caucasian and African populations, HLA-B*57:01 and HLA-B*57:03, respectively. These alleles appear equally protective against HIV disease progression. The CTL epitopes presented are in many cases identical, and the dominant response in chronic infection in each case is to the Gag epitope KF11. However, there the similarity ends. This study sought to better understand the reasons for these differences and what they teach us about which immune responses contribute to immune control of HIV infection.

Published

2016

4. Timing of galectin-1 exposure differentially modulates Nipah virus entry and syncytium formation in endothelial cells

Author

Alexander N. Freiberg, Tatyana Yun, Hector C. Aguilar, Benhur Lee, Thomas A. Bowden, Omai B. Garner, Arnold Park, Linda G. Baum, Olivier Pernet, and Doms, RW

Subjects

Galectin 1, Cells, viruses, Immunology, Biology, Medical and Health Sciences, Microbiology, Giant Cells, Virus, Vaccine Related, Viral life cycle, Biodefense, Virology, otorhinolaryngologic diseases, 2.2 Factors relating to the physical environment, 2.1 Biological and endogenous factors, Humans, Antibody-dependent enhancement, Aetiology, Cells, Cultured, Galectin, Syncytium, Cultured, Innate immune system, Agricultural and Veterinary Sciences, Prevention, Nipah Virus, Endothelial Cells, Biological Sciences, Virus Internalization, Cell biology, Virus-Cell Interactions, Endothelial stem cell, Infectious Diseases, Emerging Infectious Diseases, Good Health and Well Being, Insect Science, Galectin-1, Host-Pathogen Interactions, Infection

Abstract

Author(s): Garner, Omai B; Yun, Tatyana; Pernet, Olivier; Aguilar, Hector C; Park, Arnold; Bowden, Thomas A; Freiberg, Alexander N; Lee, Benhur; Baum, Linda G | Abstract: UnlabelledNipah virus (NiV) is a deadly emerging enveloped paramyxovirus that primarily targets human endothelial cells. Endothelial cells express the innate immune effector galectin-1 that we have previously shown can bind to specific N-glycans on the NiV envelope fusion glycoprotein (F). NiV-F mediates fusion of infected endothelial cells into syncytia, resulting in endothelial disruption and hemorrhage. Galectin-1 is an endogenous carbohydrate-binding protein that binds to specific glycans on NiV-F to reduce endothelial cell fusion, an effect that may reduce pathophysiologic sequelae of NiV infection. However, galectins play multiple roles in regulating host-pathogen interactions; for example, galectins can promote attachment of HIV to T cells and macrophages and attachment of HSV-1 to keratinocytes but can also inhibit influenza entry into airway epithelial cells. Using live Nipah virus, in the present study, we demonstrate that galectin-1 can enhance NiV attachment to and infection of primary human endothelial cells by bridging glycans on the viral envelope to host cell glycoproteins. In order to exhibit an enhancing effect, galectin-1 must be present during the initial phase of virus attachment; in contrast, addition of galectin-1 postinfection results in reduced production of progeny virus and syncytium formation. Thus, galectin-1 can have dual and opposing effects on NiV infection of human endothelial cells. While various roles for galectin family members in microbial-host interactions have been described, we report opposing effects of the same galectin family member on a specific virus, with the timing of exposure during the viral life cycle determining the outcome.ImportanceNipah virus is an emerging pathogen that targets endothelial cells lining blood vessels; the high mortality rate (up to 70%) in Nipah virus infections results from destruction of these cells and resulting catastrophic hemorrhage. Host factors that promote or prevent Nipah virus infection are not well understood. Endogenous human lectins, such as galectin-1, can function as pattern recognition receptors to reduce infection and initiate immune responses; however, lectins can also be exploited by microbes to enhance infection of host cells. We found that galectin-1, which is made by inflamed endothelial cells, can both promote Nipah virus infection of endothelial cells by "bridging" the virus to the cell, as well as reduce production of progeny virus and reduce endothelial cell fusion and damage, depending on timing of galectin-1 exposure. This is the first report of spatiotemporal opposing effects of a host lectin for a virus in one type of host cell.

Published

2016

5. Ineffectual Targeting of HIV-1 Nef by Cytotoxic T Lymphocytes in Acute Infection Results in No Functional Impairment or Viremia Reduction

Author

Martha J. Lewis, Thomas Vollbrecht, Otto O. Yang, Hwee L. Ng, Patricia Frohnen, Justin De La Cruz, Eric S. Daar, and Doms, RW

Subjects

Adoptive cell transfer, Cytotoxic, T-Lymphocytes, viruses, Immunology, Viremia, HIV Infections, Immunodominance, nef Gene Products, Biology, Major histocompatibility complex, Medical and Health Sciences, Microbiology, Vaccine Related, Clinical Research, Virology, medicine, Cytotoxic T cell, Humans, nef Gene Products, Human Immunodeficiency Virus, Agricultural and Veterinary Sciences, virus diseases, Biological Sciences, medicine.disease, Chronic infection, CTL, Infectious Diseases, Good Health and Well Being, Insect Science, biology.protein, HIV-1, HIV/AIDS, Pathogenesis and Immunity, Immunization, Infection, Human Immunodeficiency Virus, CD8, Biotechnology, T-Lymphocytes, Cytotoxic

Abstract

The human immunodeficiency virus type 1 (HIV-1) accessory protein Nef is heavily targeted by CD8 + T lymphocytes (CTLs) during acute infection and therefore is included in many candidate vaccines. We investigated whether CTL targeting of Nef during acute infection contributes to immune control by disrupting the function of Nef. The sequence and function of Nef in parallel with CTL responses were assessed longitudinally from peak viremia until the viremia set point in a cohort of six subjects with acute infection. All but one individual had a single founder strain. Nef-specific CTL responses were detected in all subjects and declined in magnitude over time. These responses were associated with mutations, but none of the mutations were detected in important functional motifs. Nef-mediated downregulation of CD4 and major histocompatibility complex (MHC) class I molecules was better preserved in acute infection than in chronic infection. Finally, Nef-specific CTL responses were not associated with a reduction in viremia from its acute-phase peak. Our results indicate that CTLs targeting Nef epitopes outside critical functional domains have little effect on the pathogenic functions of Nef, rendering these responses ineffective in acute infection. IMPORTANCE These data indicate that using the whole Nef protein as a vaccine immunogen likely allows immunodominance that leads to targeting of CTL responses that are rapidly escaped with little effect on Nef-mediated pathogenic functions. Pursuing vaccination approaches that can more precisely direct responses to vulnerable areas would maximize efficacy. Until vaccine-induced targeting can be optimized, other approaches, such as the use of Nef function inhibitors or the pursuit of immunotherapies such as T cell receptor gene therapy or adoptive transfer, may be more likely to result in successful control of viremia.

Published

2014

6. Comparative Evaluation of Choose Your Own Adventure and Traditional Linear Case Formats in Radiology Small Group Teaching.

Author

Thomas SP, Fathy R, Aepli S, Clancy CB, Lipschik GY, Simpson SA, Katz SI, Doms RW, and Nachiappan AC

Subjects

Humans, Learning, Radiography, Surveys and Questionnaires, Teaching, Radiology education, Students, Medical

Abstract

Rationale and Objectives: We aim to compare Choose Your Own Adventure (CYOA) presentation format with linear case format as educational methods for teaching a radiology small group session to medical students., Materials and Methods: A radiology small group session was held for preclinical second-year medical students in the pulmonary course, whereby eight classrooms of students and eight radiology facilitators were each randomized to do either the linear case format or the nonlinear CYOA presentation format. All students in attendance were administered a survey at the end of the session, which assessed students' perceptions using five-point Likert-type questions. The survey also contained a four-question knowledge quiz on chest radiology. The facilitators were administered a qualitative survey as well. Between-group analyses were performed using Student's t-test., Results: Of the 144 students who attended the small group sessions, 143 students completed the survey (99.3%). The CYOA format group reported significantly greater engagement in the cases (4.5 ± 0.7 vs. 3.8 ± 0.7, p < 0.001), satisfaction with the format (4.6 ± 0.6 vs. 3.7 ± 0.9, p < 0.001), and enhancement of clinical decision making skills (4.5 ± 0.6 vs. 3.5 ± 0.9, p < 0.001). The linear format group reported a greater role for the facilitator to add value (4.6 ± 0.5 vs. 4.3 ± 1.1, p = 0.033). There was no significant difference between groups in performance on the knowledge quiz., Conclusion: Medical students reported higher satisfaction, engagement, and enhanced clinical decision making skills with the CYOA presentation method compared to linear case format for radiology small group learning., (Copyright © 2021 The Association of University Radiologists. Published by Elsevier Inc. All rights reserved.)

Published

2022

7. What Came First-the Virus or the Egg?

Author

Doms RW

Subjects

Dengue, Humans, Zika Virus, Zika Virus Infection, Germ Cells metabolism, Membrane Proteins metabolism

Abstract

Three recent studies find that the single-pass transmembrane protein HAP2 mediates gamete fusion and is remarkably similar to class II fusion proteins found in viruses such as dengue and Zika., (Copyright © 2017 Elsevier Inc. All rights reserved.)

Published

2017

8. Platelet Factor 4 Inhibits and Enhances HIV-1 Infection in a Concentration-Dependent Manner by Modulating Viral Attachment.

Author

Parker ZF, Rux AH, Riblett AM, Lee FH, Rauova L, Cines DB, Poncz M, Sachais BS, and Doms RW

Subjects

Humans, Protein Binding, HIV-1 physiology, Host-Pathogen Interactions, Platelet Factor 4 metabolism, Virus Attachment, env Gene Products, Human Immunodeficiency Virus metabolism

Abstract

Platelet factor 4 (PF4) has been recently shown to inhibit infection by a broad range of human immunodeficiency virus type 1 (HIV-1) isolates in vitro. We found that the inhibitory effects of PF4 are limited to a defined concentration range where PF4 exists largely in a monomeric state. Under these conditions, PF4 bound the HIV-1 envelope protein and inhibited HIV-1 attachment to the cell surface. However, as concentrations increased to the point where PF4 exists largely in tetrameric or higher-order forms, viral infection in vitro was enhanced. Enhancement could be inhibited by mutations in PF4 that shift the oligomeric equilibrium toward the monomeric state, or by using soluble glycosaminoglycans (GAGs) to which tetrameric PF4 avidly binds. We conclude that at physiologically relevant concentrations, oligomeric PF4 enhances infection by HIV-1 by interacting with the viral envelope protein as well as cell surface GAGs, enhancing virus attachment to the cell surface. This effect was not specific to HIV-1, as enhancement was seen with some but not all other viruses tested. The biphasic effects of PF4 on HIV-1 infection suggest that native PF4 will not be a useful antiviral agent and that PF4 could contribute to the hematologic abnormalities commonly seen in HIV-infected individuals by enhancing virus infection in the bone marrow.

Published

2016

9. Envelope residue 375 substitutions in simian-human immunodeficiency viruses enhance CD4 binding and replication in rhesus macaques.

Author

Li H, Wang S, Kong R, Ding W, Lee FH, Parker Z, Kim E, Learn GH, Hahn P, Policicchio B, Brocca-Cofano E, Deleage C, Hao X, Chuang GY, Gorman J, Gardner M, Lewis MG, Hatziioannou T, Santra S, Apetrei C, Pandrea I, Alam SM, Liao HX, Shen X, Tomaras GD, Farzan M, Chertova E, Keele BF, Estes JD, Lifson JD, Doms RW, Montefiori DC, Haynes BF, Sodroski JG, Kwong PD, Hahn BH, and Shaw GM

Subjects

Amino Acid Substitution, Animals, Humans, Macaca mulatta, CD4 Antigens metabolism, HIV Infections genetics, HIV Infections metabolism, HIV-1 physiology, Mutation, Missense, Simian Acquired Immunodeficiency Syndrome genetics, Simian Acquired Immunodeficiency Syndrome metabolism, Simian Immunodeficiency Virus physiology, Virus Replication genetics, env Gene Products, Human Immunodeficiency Virus genetics, env Gene Products, Human Immunodeficiency Virus metabolism

Abstract

Most simian-human immunodeficiency viruses (SHIVs) bearing envelope (Env) glycoproteins from primary HIV-1 strains fail to infect rhesus macaques (RMs). We hypothesized that inefficient Env binding to rhesus CD4 (rhCD4) limits virus entry and replication and could be enhanced by substituting naturally occurring simian immunodeficiency virus Env residues at position 375, which resides at a critical location in the CD4-binding pocket and is under strong positive evolutionary pressure across the broad spectrum of primate lentiviruses. SHIVs containing primary or transmitted/founder HIV-1 subtype A, B, C, or D Envs with genotypic variants at residue 375 were constructed and analyzed in vitro and in vivo. Bulky hydrophobic or basic amino acids substituted for serine-375 enhanced Env affinity for rhCD4, virus entry into cells bearing rhCD4, and virus replication in primary rhCD4 T cells without appreciably affecting antigenicity or antibody-mediated neutralization sensitivity. Twenty-four RMs inoculated with subtype A, B, C, or D SHIVs all became productively infected with different Env375 variants-S, M, Y, H, W, or F-that were differentially selected in different Env backbones. Notably, SHIVs replicated persistently at titers comparable to HIV-1 in humans and elicited autologous neutralizing antibody responses typical of HIV-1. Seven animals succumbed to AIDS. These findings identify Env-rhCD4 binding as a critical determinant for productive SHIV infection in RMs and validate a novel and generalizable strategy for constructing SHIVs with Env glycoproteins of interest, including those that in humans elicit broadly neutralizing antibodies or bind particular Ig germ-line B-cell receptors.

Published

2016

10. Making Bunyaviruses Talk: Interrogation Tactics to Identify Host Factors Required for Infection.

Author

Riblett AM and Doms RW

Subjects

Genetic Testing methods, High-Throughput Screening Assays, Humans, Bunyaviridae Infections immunology, Bunyaviridae Infections pathology, Host-Pathogen Interactions, Orthobunyavirus pathogenicity

Abstract

The identification of host cellular genes that act as either proviral or antiviral factors has been aided by the development of an increasingly large number of high-throughput screening approaches. Here, we review recent advances in which these new technologies have been used to interrogate host genes for the ability to impact bunyavirus infection, both in terms of technical advances as well as a summary of biological insights gained from these studies.

Published

2016

11. A Haploid Genetic Screen Identifies Heparan Sulfate Proteoglycans Supporting Rift Valley Fever Virus Infection.

Author

Riblett AM, Blomen VA, Jae LT, Altamura LA, Doms RW, Brummelkamp TR, and Wojcechowskyj JA

Subjects

Cell Line, Genetic Testing, Heparan Sulfate Proteoglycans genetics, Humans, Mutagenesis, Heparan Sulfate Proteoglycans metabolism, Rift Valley fever virus physiology, Virus Attachment

Abstract

Unlabelled: Rift Valley fever virus (RVFV) causes recurrent insect-borne epizootics throughout the African continent, and infection of humans can lead to a lethal hemorrhagic fever syndrome. Deep mutagenesis of haploid human cells was used to identify host factors required for RVFV infection. This screen identified a suite of enzymes involved in glycosaminoglycan (GAG) biogenesis and transport, including several components of the cis-oligomeric Golgi (COG) complex, one of the central components of Golgi complex trafficking. In addition, disruption of PTAR1 led to RVFV resistance as well as reduced heparan sulfate surface levels, consistent with recent observations that PTAR1-deficient cells exhibit altered Golgi complex morphology and glycosylation defects. A variety of biochemical and genetic approaches were utilized to show that both pathogenic and attenuated RVFV strains require GAGs for efficient infection on some, but not all, cell types, with the block to infection being at the level of virion attachment. Examination of other members of the Bunyaviridae family for GAG-dependent infection suggested that the interaction with GAGs is not universal among bunyaviruses, indicating that these viruses, as well as RVFV on certain cell types, employ additional unidentified virion attachment factors and/or receptors., Importance: Rift Valley fever virus (RVFV) is an emerging pathogen that can cause severe disease in humans and animals. Epizootics among livestock populations lead to high mortality rates and can be economically devastating. Human epidemics of Rift Valley fever, often initiated by contact with infected animals, are characterized by a febrile disease that sometimes leads to encephalitis or hemorrhagic fever. The global burden of the pathogen is increasing because it has recently disseminated beyond Africa, which is of particular concern because the virus can be transmitted by widely distributed mosquito species. There are no FDA-licensed vaccines or antiviral agents with activity against RVFV, and details of its life cycle and interaction with host cells are not well characterized. We used the power of genetic screening in human cells and found that RVFV utilizes glycosaminoglycans to attach to host cells. This furthers our understanding of the virus and informs the development of antiviral therapeutics., (Copyright © 2016, American Society for Microbiology. All Rights Reserved.)

Published

2015

12. Antibodies elicited by yeast glycoproteins recognize HIV-1 virions and potently neutralize virions with high mannose N-glycans.

Author

Zhang H, Fu H, Luallen RJ, Liu B, Lee FH, Doms RW, and Geng Y

Subjects

Animals, Humans, Neutralization Tests, Rabbits, Antibodies, Fungal immunology, Antibodies, Heterophile immunology, Antibodies, Neutralizing immunology, HIV-1 immunology, Polysaccharides immunology, Saccharomyces cerevisiae immunology

Abstract

The glycan shield on the human immunodeficiency virus 1 (HIV-1) envelope (Env) glycoprotein has drawn attention as a target for HIV-1 vaccine design given that an increasing number of potent and broadly neutralizing antibodies (bNAbs) recognize epitopes entirely or partially comprised of high mannose type N-linked glycans. In an attempt to generate immunogens that target the glycan shield of HIV-1, we previously engineered a triple mutant (TM) strain of Saccharomyces cerevisiae that results in exclusive presentation of high mannose type N-glycans, and identified five TM yeast glycoproteins that support strong binding of 2G12, a bNAb that targets a cluster of high mannose glycans on the gp120 subunit of Env. Here, we further analyzed the antigenicity and immunogenicity of these proteins in inducing anti-HIV responses. Our study demonstrated that the 2G12-reactive TM yeast glycoproteins efficiently bound to recently identified bNAbs including PGT125-130 and PGT135 that recognize high mannose glycan-dependent epitopes. Immunization of rabbits with a single TM yeast glycoprotein (Gp38 or Pst1), when conjugated to a promiscuous T-cell epitope peptide and coadministered with a Toll-like receptor 2 agonist, induced glycan-specific HIV-1 Env cross-reactive antibodies. The immune sera bound to both synthetic mannose oligosaccharides and gp120 proteins from a broad range of HIV-1 strains. The purified antibodies recognized and captured virions that contain both complex- and high mannose-type of N-glycans, and potently neutralized virions from different HIV-1 clades but only when the virions were enforced to retain high mannose N-glycans. This study provides insights into the elicitation of anti-carbohydrate, HIV-1 Env-cross reactive antibodies with a heterologous glycoprotein and may have applications in the design and administration of immunogens that target the viral glycan shield for development of an effective HIV-1 vaccine., (Copyright © 2015 Elsevier Ltd. All rights reserved.)

Published

2015

13. The major cellular sterol regulatory pathway is required for Andes virus infection.

Author

Petersen J, Drake MJ, Bruce EA, Riblett AM, Didigu CA, Wilen CB, Malani N, Male F, Lee FH, Bushman FD, Cherry S, Doms RW, Bates P, and Briley K Jr

Subjects

Cell Line, Flow Cytometry, Humans, Microscopy, Confocal, Mutagenesis, Site-Directed, Polymerase Chain Reaction, Signal Transduction physiology, Sterols metabolism, Transduction, Genetic, Virus Replication physiology, Cholesterol metabolism, Orthohantavirus pathogenicity, Hantavirus Infections metabolism, Host-Parasite Interactions physiology, Virus Internalization

Abstract

The Bunyaviridae comprise a large family of RNA viruses with worldwide distribution and includes the pathogenic New World hantavirus, Andes virus (ANDV). Host factors needed for hantavirus entry remain largely enigmatic and therapeutics are unavailable. To identify cellular requirements for ANDV infection, we performed two parallel genetic screens. Analysis of a large library of insertionally mutagenized human haploid cells and a siRNA genomic screen converged on components (SREBP-2, SCAP, S1P and S2P) of the sterol regulatory pathway as critically important for infection by ANDV. The significance of this pathway was confirmed using functionally deficient cells, TALEN-mediated gene disruption, RNA interference and pharmacologic inhibition. Disruption of sterol regulatory complex function impaired ANDV internalization without affecting virus binding. Pharmacologic manipulation of cholesterol levels demonstrated that ANDV entry is sensitive to changes in cellular cholesterol and raises the possibility that clinically approved regulators of sterol synthesis may prove useful for combating ANDV infection.

Published

2014

14. Simultaneous zinc-finger nuclease editing of the HIV coreceptors ccr5 and cxcr4 protects CD4+ T cells from HIV-1 infection.

Author

Didigu CA, Wilen CB, Wang J, Duong J, Secreto AJ, Danet-Desnoyers GA, Riley JL, Gregory PD, June CH, Holmes MC, and Doms RW

Subjects

Animals, CD4-Positive T-Lymphocytes cytology, Cell Proliferation, Female, HEK293 Cells, HIV Infections prevention & control, HIV Infections therapy, HIV-1, Humans, Male, Mice, Receptors, Chemokine metabolism, CD4-Positive T-Lymphocytes virology, Endodeoxyribonucleases metabolism, HIV Infections immunology, Receptors, CCR5 genetics, Receptors, CXCR4 genetics, Zinc Fingers

Abstract

HIV-1 entry into CD4(+) T cells requires binding of the virus to CD4 followed by engagement of either the C-C chemokine receptor 5 (CCR5) or C-X-C chemokine receptor 4 (CXCR4) coreceptor. Pharmacologic blockade or genetic inactivation of either coreceptor protects cells from infection by viruses that exclusively use the targeted coreceptor. We have used zinc-finger nucleases to drive the simultaneous genetic modification of both ccr5 and cxcr4 in primary human CD4(+) T cells. These gene-modified cells proliferated normally and were resistant to both CCR5- and CXCR4-using HIV-1 in vitro. When introduced into a humanized mouse model of HIV-1 infection, these coreceptor negative cells engraft and traffic normally, and are protected from infection with CCR5- and CXCR4-using HIV-1 strains. These data suggest that simultaneous disruption of the HIV coreceptors may provide a useful approach for the long-term, drug-free treatment of established HIV-1 infections.

Published

2014

15. Quantitative phosphoproteomics reveals extensive cellular reprogramming during HIV-1 entry.

Author

Wojcechowskyj JA, Didigu CA, Lee JY, Parrish NF, Sinha R, Hahn BH, Bushman FD, Jensen ST, Seeholzer SH, and Doms RW

Subjects

Cells, Cultured, Gene Expression Regulation, Humans, Proteomics methods, RNA Splicing, Virus Release, Virus Replication, CD4-Positive T-Lymphocytes virology, HIV-1 physiology, Host-Pathogen Interactions, Phosphoproteins analysis, Proteome analysis, Virus Internalization

Abstract

Receptor engagement by HIV-1 during host cell entry activates signaling pathways that can reprogram the cell for optimal viral replication. To obtain a global view of the signaling events induced during HIV-1 entry, we conducted a quantitative phosphoproteomics screen of primary human CD4(+) T cells after infection with an HIV-1 strain that engages the receptors CD4 and CXCR4. We quantified 1,757 phosphorylation sites with high stringency. The abundance of 239 phosphorylation sites from 175 genes, including several proteins in pathways known to be impacted by HIV-receptor binding, changed significantly within a minute after HIV-1 exposure. Several previously uncharacterized HIV-1 host factors were also identified and confirmed through RNAi depletion studies. Surprisingly, five serine/arginine-rich (SR) proteins involved in messenger RNA splicing, including the splicing factor SRm300 (SRRM2), were differentially phosophorylated. Mechanistic studies with SRRM2 suggest that HIV-1 modulates host cell alternative splicing machinery during entry in order to facilitate virus replication and release., (Copyright © 2013 Elsevier Inc. All rights reserved.)

Published

2013

16. Phenotypic properties of transmitted founder HIV-1.

Author

Parrish NF, Gao F, Li H, Giorgi EE, Barbian HJ, Parrish EH, Zajic L, Iyer SS, Decker JM, Kumar A, Hora B, Berg A, Cai F, Hopper J, Denny TN, Ding H, Ochsenbauer C, Kappes JC, Galimidi RP, West AP Jr, Bjorkman PJ, Wilen CB, Doms RW, O'Brien M, Bhardwaj N, Borrow P, Haynes BF, Muldoon M, Theiler JP, Korber B, Shaw GM, and Hahn BH

Subjects

Base Sequence, CD4-Positive T-Lymphocytes immunology, Cloning, Molecular, Enzyme-Linked Immunosorbent Assay, HIV Infections immunology, HIV Infections transmission, HIV-1 immunology, Humans, Linear Models, Molecular Sequence Data, Sequence Analysis, DNA, Dendritic Cells immunology, HIV-1 genetics, Phenotype, Viral Envelope Proteins metabolism, Virion pathogenicity

Abstract

Defining the virus-host interactions responsible for HIV-1 transmission, including the phenotypic requirements of viruses capable of establishing de novo infections, could be important for AIDS vaccine development. Previous analyses have failed to identify phenotypic properties other than chemokine receptor 5 (CCR5) and CD4+ T-cell tropism that are preferentially associated with viral transmission. However, most of these studies were limited to examining envelope (Env) function in the context of pseudoviruses. Here, we generated infectious molecular clones of transmitted founder (TF; n = 27) and chronic control (CC; n = 14) viruses of subtypes B (n = 18) and C (n = 23) and compared their phenotypic properties in assays specifically designed to probe the earliest stages of HIV-1 infection. We found that TF virions were 1.7-fold more infectious (P = 0.049) and contained 1.9-fold more Env per particle (P = 0.048) compared with CC viruses. TF viruses were also captured by monocyte-derived dendritic cells 1.7-fold more efficiently (P = 0.035) and more readily transferred to CD4+ T cells (P = 0.025). In primary CD4+ T cells, TF and CC viruses replicated with comparable kinetics; however, when propagated in the presence of IFN-α, TF viruses replicated to higher titers than CC viruses. This difference was significant for subtype B (P = 0.000013) but not subtype C (P = 0.53) viruses, possibly reflecting demographic differences of the respective patient cohorts. Together, these data indicate that TF viruses are enriched for higher Env content, enhanced cell-free infectivity, improved dendritic cell interaction, and relative IFN-α resistance. These viral properties, which likely act in concert, should be considered in the development and testing of AIDS vaccines.

Published

2013

17. Transmitted/founder and chronic HIV-1 envelope proteins are distinguished by differential utilization of CCR5.

Author

Parker ZF, Iyer SS, Wilen CB, Parrish NF, Chikere KC, Lee FH, Didigu CA, Berro R, Klasse PJ, Lee B, Moore JP, Shaw GM, Hahn BH, and Doms RW

Subjects

CCR5 Receptor Antagonists, CD4-Positive T-Lymphocytes immunology, CD4-Positive T-Lymphocytes metabolism, CD4-Positive T-Lymphocytes virology, Cell Line, HEK293 Cells, HIV Infections immunology, HIV Infections metabolism, HIV Infections virology, Humans, Maraviroc, Virus Attachment, Virus Internalization, Cyclohexanes pharmacology, HIV-1 physiology, Receptors, CCR5 metabolism, Triazoles pharmacology, env Gene Products, Human Immunodeficiency Virus immunology, env Gene Products, Human Immunodeficiency Virus metabolism

Abstract

Infection by HIV-1 most often results from the successful transmission and propagation of a single virus variant, termed the transmitted/founder (T/F) virus. Here, we compared the attachment and entry properties of envelope (Env) glycoproteins from T/F and chronic control (CC) viruses. Using a panel of 40 T/F and 47 CC Envs, all derived by single genome amplification, we found that 52% of clade C and B CC Envs exhibited partial resistance to the CCR5 antagonist maraviroc (MVC) on cells expressing high levels of CCR5, while only 15% of T/F Envs exhibited this same property. Moreover, subtle differences in the magnitude with which MVC inhibited infection on cells expressing low levels of CCR5, including primary CD4(+) T cells, were highly predictive of MVC resistance when CCR5 expression levels were high. These results are consistent with previous observations showing a greater sensitivity of T/F Envs to MVC inhibition on cells expressing very high levels of CCR5 and indicate that CC Envs are often capable of recognizing MVC-bound CCR5, albeit inefficiently on cells expressing physiologic levels of CCR5. When CCR5 expression levels are high, this phenotype becomes readily detectable. The utilization of drug-bound CCR5 conformations by many CC Envs was seen with other CCR5 antagonists, with replication-competent viruses, and did not obviously correlate with other phenotypic traits. The striking ability of clade C and B CC Envs to use MVC-bound CCR5 relative to T/F Envs argues that the more promiscuous use of CCR5 by these Env proteins is selected against at the level of virus transmission and is selected for during chronic infection.

Published

2013

18. Kruppel-like factor 2 modulates CCR5 expression and susceptibility to HIV-1 infection.

Author

Richardson MW, Jadlowsky J, Didigu CA, Doms RW, and Riley JL

Subjects

CCR5 Receptor Antagonists, CD4-Positive T-Lymphocytes immunology, CD4-Positive T-Lymphocytes metabolism, CD4-Positive T-Lymphocytes virology, Cell Line, Transformed, Down-Regulation genetics, Down-Regulation immunology, Drug Delivery Systems methods, HIV Infections genetics, HIV Infections metabolism, Humans, Kruppel-Like Transcription Factors metabolism, Lymphocyte Activation genetics, Lymphocyte Activation immunology, Primary Cell Culture, Protein Binding genetics, Protein Binding immunology, RNA, Small Interfering pharmacology, Receptors, CCR5 genetics, Resting Phase, Cell Cycle genetics, Resting Phase, Cell Cycle immunology, Genetic Predisposition to Disease etiology, HIV Infections immunology, HIV-1 immunology, Kruppel-Like Transcription Factors physiology, Receptors, CCR5 biosynthesis

Abstract

CCR5, a cell surface molecule critical for the transmission and spread of HIV-1, is dynamically regulated during T cell activation and differentiation. The molecular mechanism linking T cell activation to modulation of CCR5 expression remains undefined. Kruppel-like factor 2 (KLF2) is a transcription factor that promotes quiescence, survival, and in part by modulating chemokine receptor levels, induces homing to secondary lymphoid organs. Given the relationship between T cell activation and chemokine receptor expression, we tested whether the abundance of KLF2 after T cell activation regulates CCR5 expression and, thus, susceptibility of a T cell to CCR5-dependent HIV-1 strains (R5). We observed a strong correlation between T cell activation, expression of KLF2 and CCR5, and susceptibility to infection. To directly measure how KLF2 affects CCR5 regulation, we introduced small interfering RNA targeting KLF2 expression and demonstrated that reduced KLF2 expression also resulted in less CCR5. Chromatin immunoprecipitation assays identified KLF2 bound to the CCR5 promoter in resting but not CD3/28 activated T cells, suggesting that KLF2 directly regulates CCR5 expression. Introduction of KLF2 under control of a heterologous promoter could restore CCR5 expression and R5 susceptibility to CD3/28 costimulated T cells and some transformed cell lines. Thus, KLF2 is a host factor that modulates CCR5 expression in CD4 T cells and influences susceptibility to R5 infection.

Published

2012

19. HIV: cell binding and entry.

Author

Wilen CB, Tilton JC, and Doms RW

Subjects

CD4 Antigens metabolism, CD4-Positive T-Lymphocytes immunology, CD4-Positive T-Lymphocytes virology, Cell Transformation, Viral physiology, HIV immunology, HIV Envelope Protein gp120 metabolism, Humans, Integrins metabolism, Protein Binding, Receptors, CCR4 metabolism, Receptors, CCR5 metabolism, Signal Transduction physiology, Virion metabolism, HIV pathogenicity, HIV Infections immunology, env Gene Products, Human Immunodeficiency Virus metabolism

Abstract

The first step of the human immunodeficiency virus (HIV) replication cycle-binding and entry into the host cell-plays a major role in determining viral tropism and the ability of HIV to degrade the human immune system. HIV uses a complex series of steps to deliver its genome into the host cell cytoplasm while simultaneously evading the host immune response. To infect cells, the HIV protein envelope (Env) binds to the primary cellular receptor CD4 and then to a cellular coreceptor. This sequential binding triggers fusion of the viral and host cell membranes, initiating infection. Revealing the mechanism of HIV entry has profound implications for viral tropism, transmission, pathogenesis, and therapeutic intervention. Here, we provide an overview into the mechanism of HIV entry, provide historical context to key discoveries, discuss recent advances, and speculate on future directions in the field.

Published

2012

20. Efficient production of Hantaan and Puumala pseudovirions for viral tropism and neutralization studies.

Author

Higa MM, Petersen J, Hooper J, and Doms RW

Subjects

Animals, Antibodies, Viral immunology, Cell Line, Hantaan virus genetics, Hantaan virus immunology, Hemorrhagic Fever with Renal Syndrome genetics, Hemorrhagic Fever with Renal Syndrome immunology, Humans, Mice, Neutralization Tests, Puumala virus genetics, Puumala virus immunology, Hantaan virus physiology, Hemorrhagic Fever with Renal Syndrome virology, Puumala virus physiology, Viral Tropism, Virus Cultivation methods

Abstract

Puumala (PUUV) and Hantaan (HTNV) viruses are hantaviruses within the family Bunyaviridae and associated with Hemorrhagic Fever with Renal Syndrome (HFRS) in humans. Little is known about how these viruses interact with host cells, though pathogenic hantaviruses interact with α(v)β(3) integrin. To study host cell interactions and rapidly test the ability of antibodies to prevent infection, we produced HTNV and PUUV pseudovirions on a vesicular stomatitis virus (VSV) core. Similar to replication-competent hantaviruses, infection was low-pH-dependent. Despite broad cell tropism, several human T cell lines were poorly permissive to hantavirus pseudovirions, compared to VSV, indicating a relative block to infection at the level of entry. Stable expression of α(v)β(3) integrin in SupT1 cells did not restore infectivity. Finally, the pseudovirion system provided a rapid, quantitative, and specific method to screen for neutralizing antibodies in immune sera., (Copyright © 2011. Published by Elsevier Inc.)

Published

2012

21. Novel approaches to inhibit HIV entry.

Author

Didigu CA and Doms RW

Subjects

Drug Therapy methods, Genetic Therapy methods, HIV Infections prevention & control, Humans, Immunotherapy methods, Models, Biological, HIV pathogenicity, HIV Infections therapy, HIV Infections virology, Virus Internalization

Abstract

Human Immunodeficiency Virus (HIV) entry into target cells is a multi-step process involving binding of the viral glycoprotein, Env, to its receptor CD4 and a coreceptor-either CCR5 or CXCR4. Understanding the means by which HIV enters cells has led to the identification of genetic polymorphisms, such as the 32 base-pair deletion in the ccr5 gene (ccr5∆32) that confers resistance to infection in homozygous individuals, and has also resulted in the development of entry inhibitors-small molecule antagonists that block infection at the entry step. The recent demonstration of long-term control of HIV infection in a leukemic patient following a hematopoietic stem cell transplant using cells from a ccr5∆32 homozygous donor highlights the important role of the HIV entry in maintaining an established infection and has led to a number of attempts to treat HIV infection by genetically modifying the ccr5 gene. In this review, we describe the HIV entry process and provide an overview of the different classes of approved HIV entry inhibitors while highlighting novel genetic strategies aimed at blocking HIV infection at the level of entry.

Published

2012

22. Transmitted/founder and chronic subtype C HIV-1 use CD4 and CCR5 receptors with equal efficiency and are not inhibited by blocking the integrin α4β7.

Author

Parrish NF, Wilen CB, Banks LB, Iyer SS, Pfaff JM, Salazar-Gonzalez JF, Salazar MG, Decker JM, Parrish EH, Berg A, Hopper J, Hora B, Kumar A, Mahlokozera T, Yuan S, Coleman C, Vermeulen M, Ding H, Ochsenbauer C, Tilton JC, Permar SR, Kappes JC, Betts MR, Busch MP, Gao F, Montefiori D, Haynes BF, Shaw GM, Hahn BH, and Doms RW

Subjects

Antibodies, Neutralizing immunology, Antibodies, Viral immunology, CD4-Positive T-Lymphocytes cytology, CD4-Positive T-Lymphocytes immunology, CD4-Positive T-Lymphocytes virology, Cells, Cultured, Cloning, Molecular, HIV Envelope Protein gp120 chemistry, HIV Envelope Protein gp120 immunology, HIV Envelope Protein gp120 metabolism, HIV Infections metabolism, HIV-1 immunology, HIV-1 metabolism, Host-Pathogen Interactions, Humans, Integrins immunology, Mucous Membrane virology, Neutralization Tests, Viral Tropism, Virus Internalization, Virus Replication, CD4 Antigens metabolism, HIV Infections transmission, HIV-1 pathogenicity, Integrins metabolism, Receptors, CCR5 metabolism

Abstract

Sexual transmission of human immunodeficiency virus type 1 (HIV-1) most often results from productive infection by a single transmitted/founder (T/F) virus, indicating a stringent mucosal bottleneck. Understanding the viral traits that overcome this bottleneck could have important implications for HIV-1 vaccine design and other prevention strategies. Most T/F viruses use CCR5 to infect target cells and some encode envelope glycoproteins (Envs) that contain fewer potential N-linked glycosylation sites and shorter V1/V2 variable loops than Envs from chronic viruses. Moreover, it has been reported that the gp120 subunits of certain transmitted Envs bind to the gut-homing integrin α4β7, possibly enhancing virus entry and cell-to-cell spread. Here we sought to determine whether subtype C T/F viruses, which are responsible for the majority of new HIV-1 infections worldwide, share biological properties that increase their transmission fitness, including preferential α4β7 engagement. Using single genome amplification, we generated panels of both T/F (n = 20) and chronic (n = 20) Env constructs as well as full-length T/F (n = 6) and chronic (n = 4) infectious molecular clones (IMCs). We found that T/F and chronic control Envs were indistinguishable in the efficiency with which they used CD4 and CCR5. Both groups of Envs also exhibited the same CD4+ T cell subset tropism and showed similar sensitivity to neutralization by CD4 binding site (CD4bs) antibodies. Finally, saturating concentrations of anti-α4β7 antibodies failed to inhibit infection and replication of T/F as well as chronic control viruses, although the growth of the tissue culture-adapted strain SF162 was modestly impaired. These results indicate that the population bottleneck associated with mucosal HIV-1 acquisition is not due to the selection of T/F viruses that use α4β7, CD4 or CCR5 more efficiently.

Published

2012

23. Molecular mechanisms of HIV entry.

Author

Wilen CB, Tilton JC, and Doms RW

Subjects

CD4 Antigens metabolism, HIV Infections virology, Humans, Models, Molecular, Protein Conformation, Receptors, CCR5 chemistry, Receptors, CCR5 metabolism, Receptors, CXCR4 chemistry, Receptors, CXCR4 metabolism, env Gene Products, Human Immunodeficiency Virus chemistry, env Gene Products, Human Immunodeficiency Virus genetics, env Gene Products, Human Immunodeficiency Virus metabolism, HIV metabolism, Virus Internalization

Abstract

Human immunodeficiency virus (HIV) entry is a complex and intricate process that facilitates delivery of the viral genome to the host cell. The only viral surface protein, Envelope (Env), is composed of a trimer of gp120 and gp41 heterodimers. It is essentially a fusion machine cloaked in a shroud of carbohydrate structures and variable loops of amino acids that enable it to evade the humoral immune response. For entry to occur gp120 sequentially engages the host protein CD4 and then one of two chemokine coreceptors, either CCR5 or CXCR4. CD4 binding facilitates exposure and formation of the coreceptor-binding site, and coreceptor binding then triggers the membrane fusion machinery in the gp41 subunit. Our understanding of HIV entry has led to the development of successful small molecule inhibitors for the clinical treatment of HIV infection as well as insights into viral tropism and pathogenesis.

Published

2012

24. Primary infection by a human immunodeficiency virus with atypical coreceptor tropism.

Author

Jiang C, Parrish NF, Wilen CB, Li H, Chen Y, Pavlicek JW, Berg A, Lu X, Song H, Tilton JC, Pfaff JM, Henning EA, Decker JM, Moody MA, Drinker MS, Schutte R, Freel S, Tomaras GD, Nedellec R, Mosier DE, Haynes BF, Shaw GM, Hahn BH, Doms RW, and Gao F

Subjects

Amino Acid Motifs, Amino Acid Substitution genetics, Apelin Receptors, CD4-Positive T-Lymphocytes virology, Cells, Cultured, Gene Expression, Humans, Macrophages virology, Receptors, Formyl Peptide genetics, Receptors, Formyl Peptide metabolism, Receptors, G-Protein-Coupled genetics, Receptors, G-Protein-Coupled metabolism, Receptors, Lipoxin genetics, Receptors, Lipoxin metabolism, Receptors, Peptide genetics, Receptors, Peptide metabolism, env Gene Products, Human Immunodeficiency Virus genetics, HIV-1 physiology, Receptors, HIV metabolism, Viral Tropism

Abstract

The great majority of human immunodeficiency virus type 1 (HIV-1) strains enter CD4+ target cells by interacting with one of two coreceptors, CCR5 or CXCR4. Here we describe a transmitted/founder (T/F) virus (ZP6248) that was profoundly impaired in its ability to utilize CCR5 and CXCR4 coreceptors on multiple CD4+ cell lines as well as primary human CD4+ T cells and macrophages in vitro yet replicated to very high titers (>80 million RNA copies/ml) in an acutely infected individual. Interestingly, the envelope (Env) glycoprotein of this clade B virus had a rare GPEK sequence in the crown of its third variable loop (V3) rather than the consensus GPGR sequence. Extensive sequencing of sequential plasma samples showed that the GPEK sequence was present in virtually all Envs, including those from the earliest time points after infection. The molecularly cloned (single) T/F virus was able to replicate, albeit poorly, in cells obtained from ccr5Δ32 homozygous donors. The ZP6248 T/F virus could also infect cell lines overexpressing the alternative coreceptors GPR15, APJ, and FPRL-1. A single mutation in the V3 crown sequence (GPEK->GPGK) of ZP6248 restored its infectivity in CCR5+ cells but reduced its ability to replicate in GPR15+ cells, indicating that the V3 crown motif played an important role in usage of this alternative coreceptor. These results suggest that the ZP6248 T/F virus established an acute in vivo infection by using coreceptor(s) other than CCR5 or CXCR4 or that the CCR5 coreceptor existed in an unusual conformation in this individual.

Published

2011

25. Phenotypic and immunologic comparison of clade B transmitted/founder and chronic HIV-1 envelope glycoproteins.

Author

Wilen CB, Parrish NF, Pfaff JM, Decker JM, Henning EA, Haim H, Petersen JE, Wojcechowskyj JA, Sodroski J, Haynes BF, Montefiori DC, Tilton JC, Shaw GM, Hahn BH, and Doms RW

Subjects

Antibodies, Neutralizing immunology, CD4-Positive T-Lymphocytes virology, Dendritic Cells virology, Female, HIV-1 isolation & purification, Humans, Male, Virus Internalization, HIV Antibodies immunology, HIV Infections virology, HIV-1 immunology, HIV-1 pathogenicity, Viral Tropism, env Gene Products, Human Immunodeficiency Virus immunology, env Gene Products, Human Immunodeficiency Virus metabolism

Abstract

Sexual transmission of human immunodeficiency virus type 1 (HIV-1) across mucosal barriers is responsible for the vast majority of new infections. This relatively inefficient process results in the transmission of a single transmitted/founder (T/F) virus, from a diverse viral swarm in the donor, in approximately 80% of cases. Here we compared the biological activities of 24 clade B T/F envelopes (Envs) with those from 17 chronic controls to determine whether the genetic bottleneck that occurs during transmission is linked to a particular Env phenotype. To maximize the likelihood of an intact mucosal barrier in the recipients and to enhance the sensitivity of detecting phenotypic differences, only T/F Envs from individuals infected with a single T/F variant were selected. Using pseudotyping to assess Env function in single-round infectivity assays, we compared coreceptor tropism, CCR5 utilization efficiencies, primary CD4(+) T cell subset tropism, dendritic cell trans-infections, fusion kinetics, and neutralization sensitivities. T/F and chronic Envs were phenotypically equivalent in most assays; however, T/F Envs were modestly more sensitive to CD4 binding site antibodies b12 and VRC01, as well as pooled human HIV Ig. This finding was independently validated with a panel of 14 additional chronic HIV-1 Env controls. Moreover, the enhanced neutralization sensitivity was associated with more efficient binding of b12 and VRC01 to T/F Env trimers. These data suggest that there are subtle but significant structural differences between T/F and chronic clade B Envs that may have implications for HIV-1 transmission and the design of effective vaccines.

Published

2011

26. Fusing HIV and chemokine receptors.

Author

Doms RW

Subjects

HIV Infections metabolism, HIV Infections virology, Humans, Protein Binding, Receptors, CCR5 metabolism, Receptors, CXCR4 metabolism, HIV metabolism, Membrane Fusion, Receptors, Chemokine metabolism

Published

2011

27. Engineering HIV-resistant human CD4+ T cells with CXCR4-specific zinc-finger nucleases.

Author

Wilen CB, Wang J, Tilton JC, Miller JC, Kim KA, Rebar EJ, Sherrill-Mix SA, Patro SC, Secreto AJ, Jordan AP, Lee G, Kahn J, Aye PP, Bunnell BA, Lackner AA, Hoxie JA, Danet-Desnoyers GA, Bushman FD, Riley JL, Gregory PD, June CH, Holmes MC, and Doms RW

Subjects

Animals, CD4-Positive T-Lymphocytes metabolism, CD4-Positive T-Lymphocytes transplantation, Cell Proliferation, Deoxyribonucleases biosynthesis, Deoxyribonucleases genetics, Disease Models, Animal, Genetic Engineering, HIV Infections genetics, HIV Infections metabolism, HIV Infections therapy, HIV-1 genetics, HIV-1 metabolism, Humans, Macaca mulatta, Mice, Receptors, CCR5 genetics, Receptors, CCR5 immunology, Receptors, CCR5 metabolism, Receptors, CXCR4 genetics, Receptors, CXCR4 metabolism, Transplantation, Autologous, Transplantation, Heterologous, Virus Internalization, CD4-Positive T-Lymphocytes immunology, Deoxyribonucleases immunology, HIV Infections immunology, HIV-1 immunology, Receptors, CXCR4 immunology

Abstract

HIV-1 entry requires the cell surface expression of CD4 and either the CCR5 or CXCR4 coreceptors on host cells. Individuals homozygous for the ccr5Δ32 polymorphism do not express CCR5 and are protected from infection by CCR5-tropic (R5) virus strains. As an approach to inactivating CCR5, we introduced CCR5-specific zinc-finger nucleases into human CD4+ T cells prior to adoptive transfer, but the need to protect cells from virus strains that use CXCR4 (X4) in place of or in addition to CCR5 (R5X4) remains. Here we describe engineering a pair of zinc finger nucleases that, when introduced into human T cells, efficiently disrupt cxcr4 by cleavage and error-prone non-homologous DNA end-joining. The resulting cells proliferated normally and were resistant to infection by X4-tropic HIV-1 strains. CXCR4 could also be inactivated in ccr5Δ32 CD4+ T cells, and we show that such cells were resistant to all strains of HIV-1 tested. Loss of CXCR4 also provided protection from X4 HIV-1 in a humanized mouse model, though this protection was lost over time due to the emergence of R5-tropic viral mutants. These data suggest that CXCR4-specific ZFNs may prove useful in establishing resistance to CXCR4-tropic HIV for autologous transplant in HIV-infected individuals.

Published

2011

28. Yeast-elicited cross-reactive antibodies to HIV Env glycans efficiently neutralize virions expressing exclusively high-mannose N-linked glycans.

Author

Agrawal-Gamse C, Luallen RJ, Liu B, Fu H, Lee FH, Geng Y, and Doms RW

Subjects

Animals, Antibodies, Monoclonal immunology, Antibodies, Monoclonal metabolism, Broadly Neutralizing Antibodies, Cross Reactions, Enzyme-Linked Immunosorbent Assay, Glycoproteins metabolism, HIV Antibodies metabolism, HIV Envelope Protein gp120 metabolism, Humans, Immunization, Mannose metabolism, Microarray Analysis, Neutralization Tests, Polysaccharides metabolism, Rabbits, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Virion metabolism, Antibodies, Neutralizing immunology, HIV Antibodies immunology, HIV Envelope Protein gp120 immunology, Polysaccharides immunology, Saccharomyces cerevisiae immunology, Virion immunology

Abstract

The HIV envelope (Env) protein uses a dense coat of glycans to mask conserved domains and evade host humoral immune responses. The broadly neutralizing antibody 2G12, which binds a specific cluster of high-mannose glycans on HIV Env, shows that the glycan shield can also serve as a target for neutralizing antibodies. We have described a triple mutant Saccharomyces cerevisiae strain that expresses high-mannose glycoproteins that bind to 2G12. When used to immunize rabbits, this yeast elicits antibodies that bind to gp120-associated glycans but fail to neutralize virus. Here we sought to determine the reason for these discordant results. Affinity purification of sera over columns conjugated with three 2G12-reactive yeast glycoproteins showed that these proteins could adsorb 80% of the antibodies that bind to gp120 glycans. Despite binding to monomeric gp120, these mannose-specific antibodies failed to bind cell surface-expressed trimeric Env. However, when Env was expressed in the presence of the mannosidase inhibitor kifunensine to force retention of high-mannose glycans at all sites, the purified antibodies gained the abilities to bind trimeric Env and to strongly and broadly neutralize viruses produced under these conditions. Combined, these data show that the triple mutant yeast strain elicits antibodies that bind to high-mannose glycans presented on the HIV envelope, but only when they are displayed in a manner not found on native Env trimers. This implies that the underlying structure of the protein scaffold used to present the high-mannose glycans may be critical to allow elicitation of antibodies that recognize trimeric Env and neutralize virus.

Published

2011

29. Quantitative phosphoproteomics of CXCL12 (SDF-1) signaling.

Author

Wojcechowskyj JA, Lee JY, Seeholzer SH, and Doms RW

Subjects

Amino Acid Sequence, Blotting, Western, Cell Line, GTP-Binding Proteins metabolism, Humans, Isotope Labeling, Molecular Sequence Data, Phosphopeptides chemistry, Phosphopeptides metabolism, Phosphoproteins chemistry, Proteome chemistry, Proteome metabolism, Reproducibility of Results, Chemokine CXCL12 pharmacology, Phosphoproteins metabolism, Proteomics methods, Signal Transduction drug effects

Abstract

CXCL12 (SDF-1) is a chemokine that binds to and signals through the seven transmembrane receptor CXCR4. The CXCL12/CXCR4 signaling axis has been implicated in both cancer metastases and human immunodeficiency virus type 1 (HIV-1) infection and a more complete understanding of CXCL12/CXCR4 signaling pathways may support efforts to develop therapeutics for these diseases. Mass spectrometry-based phosphoproteomics has emerged as an important tool in studying signaling networks in an unbiased fashion. We employed stable isotope labeling with amino acids in cell culture (SILAC) quantitative phosphoproteomics to examine the CXCL12/CXCR4 signaling axis in the human lymphoblastic CEM cell line. We quantified 4,074 unique SILAC pairs from 1,673 proteins and 89 phosphopeptides were deemed CXCL12-responsive in biological replicates. Several well established CXCL12-responsive phosphosites such as AKT (pS473) and ERK2 (pY204) were confirmed in our study. We also validated two novel CXCL12-responsive phosphosites, stathmin (pS16) and AKT1S1 (pT246) by Western blot. Pathway analysis and comparisons with other phosphoproteomic datasets revealed that genes from CXCL12-responsive phosphosites are enriched for cellular pathways such as T cell activation, epidermal growth factor and mammalian target of rapamycin (mTOR) signaling, pathways which have previously been linked to CXCL12/CXCR4 signaling. Several of the novel CXCL12-responsive phosphoproteins from our study have also been implicated with cellular migration and HIV-1 infection, thus providing an attractive list of potential targets for the development of cancer metastasis and HIV-1 therapeutics and for furthering our understanding of chemokine signaling regulation by reversible phosphorylation.

Published

2011

30. Rift valley fever virus infection of human cells and insect hosts is promoted by protein kinase C epsilon.

Author

Filone CM, Hanna SL, Caino MC, Bambina S, Doms RW, and Cherry S

Subjects

Acetophenones pharmacology, Animals, Benzophenanthridines pharmacology, Benzopyrans pharmacology, Cell Line, Chlorocebus aethiops, Diptera genetics, Diptera metabolism, Diptera virology, Drug Evaluation, Preclinical, Enzyme Inhibitors pharmacology, Fluorescent Antibody Technique, HEK293 Cells, Humans, Immunoblotting, Insecta cytology, Insecta metabolism, Protein Kinase C-epsilon antagonists & inhibitors, Protein Kinase C-epsilon genetics, RNA Interference, Rift Valley fever virus drug effects, Vero Cells, Insecta virology, Protein Kinase C-epsilon metabolism, Rift Valley fever virus physiology

Abstract

As an arthropod-borne human pathogen, Rift Valley fever virus (RVFV) cycles between an insect vector and mammalian hosts. Little is known about the cellular requirements for infection in either host. Here we developed a tissue culture model for RVFV infection of human and insect cells that is amenable to high-throughput screening. Using this approach we screened a library of 1280 small molecules with pharmacologically defined activities and identified 59 drugs that inhibited RVFV infection with 15 inhibiting RVFV replication in both human and insect cells. Amongst the 15 inhibitors that blocked infection in both hosts was a subset that inhibits protein kinase C. Further studies found that infection is dependent upon the novel protein kinase C isozyme epsilon (PKCε) in both human and insect cells as well as in adult flies. Altogether, these data show that inhibition of cellular factors required for early steps in the infection cycle including PKCε can block RVFV infection, and may represent a starting point for the development of anti-RVFV therapeutics.

Published

2010

31. A maraviroc-resistant HIV-1 with narrow cross-resistance to other CCR5 antagonists depends on both N-terminal and extracellular loop domains of drug-bound CCR5.

Author

Tilton JC, Wilen CB, Didigu CA, Sinha R, Harrison JE, Agrawal-Gamse C, Henning EA, Bushman FD, Martin JN, Deeks SG, and Doms RW

Subjects

Base Sequence, Binding Sites genetics, Cell Line, Cohort Studies, DNA Primers genetics, Drug Resistance, Viral genetics, HIV Envelope Protein gp120 genetics, HIV Infections genetics, HIV-1 genetics, Humans, In Vitro Techniques, Maraviroc, Models, Biological, Mutant Proteins antagonists & inhibitors, Mutant Proteins chemistry, Mutant Proteins genetics, Mutation, Peptide Fragments genetics, Protein Structure, Tertiary, Receptors, CCR5 chemistry, Receptors, CCR5 genetics, CCR5 Receptor Antagonists, Cyclohexanes pharmacology, HIV Fusion Inhibitors pharmacology, HIV Infections drug therapy, HIV Infections virology, HIV-1 drug effects, Triazoles pharmacology

Abstract

CCR5 antagonists inhibit HIV entry by binding to a coreceptor and inducing changes in the extracellular loops (ECLs) of CCR5. In this study, we analyzed viruses from 11 treatment-experienced patients who experienced virologic failure on treatment regimens containing the CCR5 antagonist maraviroc (MVC). Viruses from one patient developed high-level resistance to MVC during the course of treatment. Although resistance to one CCR5 antagonist is often associated with broad cross-resistance to other agents, these viruses remained sensitive to most other CCR5 antagonists, including vicriviroc and aplaviroc. MVC resistance was dependent upon mutations within the V3 loop of the viral envelope (Env) protein and was modulated by additional mutations in the V4 loop. Deep sequencing of pretreatment plasma viral RNA indicated that resistance appears to have occurred by evolution of drug-bound CCR5 use, despite the presence of viral sequences predictive of CXCR4 use. Envs obtained from this patient before and during MVC treatment were able to infect cells expressing very low CCR5 levels, indicating highly efficient use of a coreceptor. In contrast to previous reports in which CCR5 antagonist-resistant viruses interact predominantly with the N terminus of CCR5, these MVC-resistant Envs were also dependent upon the drug-modified ECLs of CCR5 for entry. Our results suggest a model of CCR5 cross-resistance whereby viruses that predominantly utilize the N terminus are broadly cross-resistant to multiple CCR5 antagonists, whereas viruses that require both the N terminus and antagonist-specific ECL changes demonstrate a narrow cross-resistance profile.

Published

2010

32. Immunology. Prime, boost, and broaden.

Author

Doms RW

Subjects

Animals, Antibodies, Neutralizing biosynthesis, Antibodies, Viral biosynthesis, Cross Reactions, Ferrets, Haplorhini, Hemagglutinin Glycoproteins, Influenza Virus genetics, Hemagglutinin Glycoproteins, Influenza Virus immunology, Humans, Immunization Schedule, Immunization, Secondary, Mice, Vaccines, DNA administration & dosage, Vaccines, DNA immunology, Vaccines, Inactivated administration & dosage, Vaccines, Inactivated immunology, Antibodies, Neutralizing immunology, Antibodies, Viral immunology, Cross Protection, Influenza A Virus, H1N1 Subtype immunology, Influenza A virus immunology, Influenza Vaccines administration & dosage, Influenza Vaccines immunology

Published

2010

33. HIV-1 resistance to CCR5 antagonists associated with highly efficient use of CCR5 and altered tropism on primary CD4+ T cells.

Author

Pfaff JM, Wilen CB, Harrison JE, Demarest JF, Lee B, Doms RW, and Tilton JC

Subjects

Benzoates pharmacology, CCR5 Receptor Antagonists, Diketopiperazines, HIV Envelope Protein gp120 genetics, HIV Envelope Protein gp41 genetics, HIV-1 physiology, Humans, Mutation, Missense, Piperazines pharmacology, Receptors, HIV antagonists & inhibitors, Spiro Compounds pharmacology, Virus Attachment, Anti-HIV Agents pharmacology, CD4-Positive T-Lymphocytes virology, Drug Resistance, Viral, HIV-1 drug effects, Receptors, CCR5 physiology, Receptors, HIV physiology, Viral Tropism

Abstract

We previously reported on a panel of HIV-1 clade B envelope (Env) proteins isolated from a patient treated with the CCR5 antagonist aplaviroc (APL) that were drug resistant. These Envs used the APL-bound conformation of CCR5, were cross resistant to other small-molecule CCR5 antagonists, and were isolated from the patient's pretreatment viral quasispecies as well as after therapy. We analyzed viral and host determinants of resistance and their effects on viral tropism on primary CD4(+) T cells. The V3 loop contained residues essential for viral resistance to APL, while additional mutations in gp120 and gp41 modulated the magnitude of drug resistance. However, these mutations were context dependent, being unable to confer resistance when introduced into a heterologous virus. The resistant virus displayed altered binding between gp120 and CCR5 such that the virus became critically dependent on the N' terminus of CCR5 in the presence of APL. In addition, the drug-resistant Envs studied here utilized CCR5 very efficiently: robust virus infection occurred even when very low levels of CCR5 were expressed. However, recognition of drug-bound CCR5 was less efficient, resulting in a tropism shift toward effector memory cells upon infection of primary CD4(+) T cells in the presence of APL, with relative sparing of the central memory CD4(+) T cell subset. If such a tropism shift proves to be a common feature of CCR5-antagonist-resistant viruses, then continued use of CCR5 antagonists even in the face of virologic failure could provide a relative degree of protection to the T(CM) subset of CD4(+) T cells and result in improved T cell homeostasis and immune function.

Published

2010

34. A Potent, Broad-Spectrum Antiviral Agent that Targets Viral Membranes.

Author

Wojcechowskyj JA and Doms RW

Abstract

Commentary on Wolf, M.C.; Freiberg, A.N.; Zhang, T.; Akyol-Ataman, Z.; Grock, A.; Hong, P.W.; Li, J.; Watson, N.F.; Fang, A.Q.; Aguilar, H.C.; et al. A broad-spectrum antiviral targeting entry of enveloped viruses. Proc. Natl. Acad. Sci. U. S. A.2010, 107, 3157-3162.

Published

2010

35. Antibodies against Manalpha1,2-Manalpha1,2-Man oligosaccharide structures recognize envelope glycoproteins from HIV-1 and SIV strains.

Author

Luallen RJ, Agrawal-Gamse C, Fu H, Smith DF, Doms RW, and Geng Y

Subjects

Animals, Gene Products, env chemistry, Gene Products, env metabolism, Glycoproteins chemistry, Glycoproteins immunology, Glycoproteins metabolism, HIV Envelope Protein gp120 chemistry, HIV-1 chemistry, HIV-1 classification, Mannans chemistry, Mutation, Oligosaccharides chemistry, Oligosaccharides metabolism, Rabbits, Simian Immunodeficiency Virus chemistry, Simian Immunodeficiency Virus classification, HIV Antibodies immunology, HIV Envelope Protein gp120 immunology, HIV-1 immunology, Mannans immunology, Oligosaccharides immunology, Simian Immunodeficiency Virus immunology

Abstract

Design of an envelope glycoprotein (Env)-based vaccine against human immunodeficiency virus type-1 (HIV-1) is complicated by the large number of N-linked glycans that coat the protein and serve as a barrier to antibody-mediated neutralization. Compared to normal mammalian glycoproteins, high-mannose-type glycans are disproportionately represented on the gp120 subunit of Env. These N-glycans serve as a target for a number of anti-HIV molecules that bind terminal alpha1,2-linked mannose residues, including lectins and the monoclonal antibody 2G12. We created a Saccharomyces cerevisiae glycosylation mutant, Deltamnn1Deltamnn4, to expose numerous terminal Manalpha1,2-Man residues on endogenous hypermannosylated glycoproteins in the yeast cell wall. Immunization of rabbits with whole cells from this mutant induced antibodies that bound to a broad range of Env proteins, including clade A, B, and C of HIV and simian immunodeficiency virus (SIV). The gp120 binding activity of these immune sera was due to mannose-specific immunoglobulin, as removal of high-mannose glycans and alpha1,2-linked mannoses from gp120 abrogated serum binding. Glycan array analysis with purified IgG demonstrated binding mainly to glycans with Manalpha1,2-Manalpha1,2-Man trisaccharides. Altogether, these data demonstrate the immunogenicity of exposed polyvalent Manalpha1,2-Manalpha1,2-Man structures on the yeast cell wall mannan and their ability to induce antibodies that bind to the HIV Env protein. The yeast strain and sera from this study will be useful tools for determining the type of mannose-specific response that is needed to develop neutralizing antibodies to the glycan shield of HIV.

Published

2010

36. Entry inhibitors in the treatment of HIV-1 infection.

Author

Tilton JC and Doms RW

Subjects

Cyclohexanes history, Cyclohexanes pharmacology, Cyclohexanes therapeutic use, Drug Resistance, Viral, Enfuvirtide, HIV Envelope Protein gp41 history, HIV Envelope Protein gp41 pharmacology, HIV Envelope Protein gp41 therapeutic use, HIV Fusion Inhibitors history, History, 20th Century, History, 21st Century, Humans, Maraviroc, Peptide Fragments history, Peptide Fragments pharmacology, Peptide Fragments therapeutic use, Triazoles history, Triazoles pharmacology, Triazoles therapeutic use, HIV Fusion Inhibitors pharmacology, HIV Fusion Inhibitors therapeutic use, HIV Infections drug therapy, HIV-1 drug effects

Abstract

Infection of target cells by HIV is a complex, multi-stage process involving attachment to host cells and CD4 binding, coreceptor binding, and membrane fusion. Drugs that block HIV entry are collectively known as entry inhibitors, but comprise a complex group of drugs with multiple mechanisms of action depending on the stage of the entry process at which they act. Two entry inhibitors, maraviroc and enfuvirtide, have been approved for the treatment of HIV-1 infection, and a number of agents are in development. This review covers the entry inhibitors and their use in the management of HIV-1 infection. This article forms part of a special issue of Antiviral Research marking the 25th anniversary of antiretroviral drug discovery and development, Vol 85, issue 1, 2010., (Copyright 2009 Elsevier B.V. All rights reserved.)

Published

2010

37. HIV type 1 from a patient with baseline resistance to CCR5 antagonists uses drug-bound receptor for entry.

Author

Tilton JC, Amrine-Madsen H, Miamidian JL, Kitrinos KM, Pfaff J, Demarest JF, Ray N, Jeffrey JL, Labranche CC, and Doms RW

Subjects

Benzoates therapeutic use, Cell Line, Cells, Cultured, Diketopiperazines, HIV Fusion Inhibitors therapeutic use, Humans, Microbial Sensitivity Tests, Mutation, Missense, Piperazines therapeutic use, Sequence Analysis, DNA, Spiro Compounds therapeutic use, env Gene Products, Human Immunodeficiency Virus genetics, Benzoates pharmacology, Drug Resistance, Viral, HIV Fusion Inhibitors pharmacology, HIV Infections virology, HIV-1 physiology, Piperazines pharmacology, Receptors, HIV antagonists & inhibitors, Spiro Compounds pharmacology, Virus Internalization

Abstract

CCR5 antagonists are a new class of antiretroviral drugs that block viral entry by disrupting interactions between the viral envelope (Env) glycoprotein and coreceptor. During the CCR100136 (EPIC) Phase IIb study of the CCR5 antagonist aplaviroc (APL) in treatment-naive individuals, a patient was identified who harbored virus strains that exhibited partial resistance to APL at the time of virologic failure. Retrospectively, it was found that APL resistance was present at baseline as well. To investigate the mechanism of APL resistance in this patient, we cloned HIV-1 env genes from plasma obtained at baseline and after virologic failure. Approximately 85% of cloned Envs were functional, and all exhibited partial resistance to APL. All Envs were R5-tropic, were partially resistant to other CCR5 antagonists including maraviroc on cells with high CCR5 expression, but remained sensitive to the fusion inhibitor enfuvirtide. Competition studies with natural CCR5 ligands revealed that the mechanism of drug resistance entailed the use of the drug-bound conformation of CCR5 by the Env proteins obtained from this individual. The degree of drug resistance varied between Env clones, and also varied depending on the cell line used or the donor from whom the primary T cells were obtained. Thus, both virus and host factors contribute to CCR5 antagonist resistance. This study shows that R5 HIV-1 strains resistant to CCR5 inhibitors can arise in patients, confirming a mechanism of resistance previously characterized in vitro. In addition, some patients can harbor CCR5 antagonist-resistant viruses prior to treatment, which may have implications for the clinical use of this new class of antiretrovirals.

Published

2010

38. Adaptive mutations in a human immunodeficiency virus type 1 envelope protein with a truncated V3 loop restore function by improving interactions with CD4.

Author

Agrawal-Gamse C, Lee FH, Haggarty B, Jordan AP, Yi Y, Lee B, Collman RG, Hoxie JA, Doms RW, and Laakso MM

Subjects

Adaptation, Biological genetics, Animals, Antibodies, Monoclonal immunology, CCR5 Receptor Antagonists, Cell Line, Cyclohexanes metabolism, HIV-1 chemistry, Humans, Maraviroc, Receptors, CCR5 genetics, Recombinant Proteins immunology, Triazoles metabolism, Anti-HIV Agents immunology, CD4 Antigens immunology, HIV Envelope Protein gp120 chemistry, HIV Envelope Protein gp120 genetics, HIV Envelope Protein gp120 metabolism, HIV-1 immunology, Mutation, Receptors, CCR5 immunology

Abstract

We previously reported that a human immunodeficiency virus type 1 (HIV-1) clade B envelope protein with a severely truncated V3 loop regained function after passage in tissue culture. The adapted virus, termed TA1, retained the V3 truncation, was exquisitely sensitive to neutralization by the CD4 binding site monoclonal antibody b12 and by HIV-positive human sera, used CCR5 to enter cells, and was completely resistant to small molecule CCR5 antagonists. To examine the mechanistic basis for these properties, we singly and in combination introduced each of the 5 mutations from the adapted clone TA1 into the unadapted envelope. We found that single amino acid changes in the C3 region, the V3 loop, and in the fusion peptide were responsible for imparting near-normal levels of envelope function to TA1. T342A, which resulted in the loss of a highly conserved glycosylation site in C3, played the primary role. The adaptive amino acid changes had no impact on CCR5 antagonist resistance but made virus more sensitive to neutralization by antibodies to the CD4 binding site, modestly enhanced affinity for CD4, and made TA1 more responsive to CD4 binding. Specifically, TA1 was triggered by soluble CD4 more readily than the parental Env and, unlike the parental Env, could mediate entry on cells that express low levels of CD4. In contrast, TA1 interacted with CCR5 less efficiently and was highly sensitive to antibodies that bind to the CCR5 N terminus and ECL2. Therefore, enhanced utilization of CD4 is one mechanism by which HIV-1 can overcome mutations in the V3 region that negatively affect CCR5 interactions.

Published

2009

39. Inefficient entry of vicriviroc-resistant HIV-1 via the inhibitor-CCR5 complex at low cell surface CCR5 densities.

Author

Pugach P, Ray N, Klasse PJ, Ketas TJ, Michael E, Doms RW, Lee B, and Moore JP

Subjects

Cell Line, Drug Resistance, Viral, Humans, Virus Attachment, Virus Internalization drug effects, CCR5 Receptor Antagonists, HIV Infections virology, HIV-1 drug effects, HIV-1 physiology, Piperazines pharmacology, Pyrimidines pharmacology, Receptors, CCR5 physiology

Abstract

HIV-1 variants resistant to small molecule CCR5 inhibitors such as vicriviroc (VVC) have modified Env complexes that can use both the inhibitor-bound and -free forms of the CCR5 co-receptor to enter target cells. However, entry via the inhibitor-CCR5 complex is inefficient in some, but not all, cell types, particularly cell lines engineered to express CCR5. We investigated the effect of increasing CCR5 expression, and hence the density of the inhibitor-CCR5 complex when a saturating inhibitor (VVC) concentration was present, by using 293-Affinofile cells, in which CCR5 expression is up-regulated by the transcriptional activator, ponasterone. When CCR5 expression was low, the resistant virus entered the target cells to a lesser extent when VVC was present than absent. However, at a higher CCR5 level, there was much less entry inhibition at a constant, saturating VVC concentration. We conclude that the relative decrease in entry of a VVC-resistant virus in some cell types results from its less efficient use of the VVC-CCR5 complex, and that increasing the CCR5 expression level can compensate for this inefficiency.

Published

2009

40. A yeast glycoprotein shows high-affinity binding to the broadly neutralizing human immunodeficiency virus antibody 2G12 and inhibits gp120 interactions with 2G12 and DC-SIGN.

Author

Luallen RJ, Fu H, Agrawal-Gamse C, Mboudjeka I, Huang W, Lee FH, Wang LX, Doms RW, and Geng Y

Subjects

Amino Acid Sequence, Antibodies, Monoclonal metabolism, Antigen Presentation, Broadly Neutralizing Antibodies, Cell Adhesion Molecules metabolism, Cross Reactions, Enzyme-Linked Immunosorbent Assay, Glycoproteins metabolism, HIV Antibodies metabolism, HIV Envelope Protein gp120 metabolism, HIV-1 immunology, HIV-1 metabolism, Humans, Lectins, C-Type metabolism, Molecular Sequence Data, Polysaccharides metabolism, Receptors, Cell Surface metabolism, Saccharomyces cerevisiae immunology, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins metabolism, Surface Plasmon Resonance, Antibodies, Monoclonal immunology, Cell Adhesion Molecules immunology, Glycoproteins immunology, HIV Antibodies immunology, HIV Envelope Protein gp120 immunology, Lectins, C-Type immunology, Receptors, Cell Surface immunology, Saccharomyces cerevisiae Proteins immunology

Abstract

The human immunodeficiency virus type 1 (HIV-1) envelope (Env) protein contains numerous N-linked carbohydrates that shield conserved peptide epitopes and promote trans infection by dendritic cells via binding to cell surface lectins. The potent and broadly neutralizing monoclonal antibody 2G12 binds a cluster of high-mannose-type oligosaccharides on the gp120 subunit of Env, revealing a conserved and highly exposed epitope on the glycan shield. To find an effective antigen for eliciting 2G12-like antibodies, we searched for endogenous yeast proteins that could bind to 2G12 in a panel of Saccharomyces cerevisiae glycosylation knockouts and discovered one protein that bound weakly in a Delta pmr1 strain deficient in hyperglycosylation. 2G12 binding to this protein, identified as Pst1, was enhanced by adding the Delta mnn1 deletion to the Delta pmr1 background, ensuring the exposure of terminal alpha1,2-linked mannose residues on the D1 and D3 arms of high-mannose glycans. However, optimum 2G12 antigenicity was found when Pst1, a heavily N-glycosylated protein, was expressed with homogenous Man(8)GlcNAc(2) structures in Delta och1 Delta mnn1 Delta mnn4 yeast. Surface plasmon resonance analysis of this form of Pst1 showed high affinity for 2G12, which translated into Pst1 efficiently inhibiting gp120 interactions with 2G12 and DC-SIGN and blocking 2G12-mediated neutralization of HIV-1 pseudoviruses. The high affinity of the yeast glycoprotein Pst1 for 2G12 highlights its potential as a novel antigen to induce 2G12-like antibodies.

Published

2009

41. Enhanced exposure of the CD4-binding site to neutralizing antibodies by structural design of a membrane-anchored human immunodeficiency virus type 1 gp120 domain.

Author

Wu L, Zhou T, Yang ZY, Svehla K, O'Dell S, Louder MK, Xu L, Mascola JR, Burton DR, Hoxie JA, Doms RW, Kwong PD, and Nabel GJ

Subjects

Amino Acid Sequence, CD4 Antigens immunology, Cell Line, Epitopes immunology, Epitopes metabolism, HIV Antibodies immunology, HIV Envelope Protein gp120 immunology, HIV-1 immunology, Humans, Immunoglobulin G immunology, Immunoglobulin G metabolism, Models, Molecular, Molecular Sequence Data, Neutralization Tests, Protein Binding, Protein Engineering, Protein Structure, Tertiary, Structure-Activity Relationship, Substrate Specificity, Binding Sites, Antibody, CD4 Antigens metabolism, HIV Antibodies metabolism, HIV Envelope Protein gp120 metabolism

Abstract

The broadly neutralizing antibody immunoglobulin G1 (IgG1) b12 binds to a conformationally conserved surface on the outer domain of the human immunodeficiency virus type 1 (HIV-1) gp120 envelope (Env) glycoprotein. To develop outer domain proteins (ODs) that could be recognized selectively by CD4-binding-site (CD4-BS) antibodies, membrane-anchored ODs were generated from an HIV-1 clade B virus, TA1 R3A, which was highly sensitive to neutralization by the IgG1 b12 antibody. A 231-residue fragment of gp120 (residues 252 to 482) linked to transmembrane regions from CD4 showed b12 binding comparable to that of the native Env spike as measured by flow cytometry. Truncation of the beta 20-beta 21 hairpin (residues 422 to 436 to Gly-Gly) improved overall protein expression. Replacement of the immunodominant central 20 amino acids of the V3 loop (residues 302 to 323) with a basic hexapeptide (NTRGRR) increased b12 reactivity further. Surface calculations indicated that the ratio of b12 epitope to exposed immunogenic surface in the optimized OD increased to over 30%. This OD variant [OD(GSL)(Deltabeta 20-21)(hCD4-TM)] was recognized by b12 and another CD4-BS-reactive antibody, b13, but not by eight other CD4-BS antibodies with limited neutralization potency. Furthermore, optimized membrane-anchored OD selectively absorbed neutralizing activity from complex antisera and b12. Structurally designed membrane-anchored ODs represent candidate immunogens to elicit or to allow the detection of broadly neutralizing antibodies to the conserved site of CD4 binding on HIV-1 gp120.

Published

2009

42. HR-2 mutations in human immunodeficiency virus type 1 gp41 restore fusion kinetics delayed by HR-1 mutations that cause clinical resistance to enfuvirtide.

Author

Ray N, Blackburn LA, and Doms RW

Subjects

Cell Line, Enfuvirtide, HIV Antibodies immunology, HIV Envelope Protein gp41 immunology, HIV-1 immunology, HIV-1 physiology, Humans, Models, Molecular, Neutralization Tests, Anti-HIV Agents pharmacology, Drug Resistance, Viral, HIV Envelope Protein gp41 genetics, HIV Envelope Protein gp41 pharmacology, HIV-1 drug effects, Peptide Fragments pharmacology, Suppression, Genetic, Virus Internalization

Abstract

Enfuvirtide (ENF) prevents the entry of human immunodeficiency virus type 1 (HIV-1) into cells by binding to the HR-1 region of the viral envelope (Env) protein gp41 subunit. Resistance to ENF arises via mutations in the drug binding site in HR-1. In addition, HR-2 mutations are commonly observed in ENF-resistant Env proteins, though their role remains unclear. We explored the mechanistic basis for clinical resistance to ENF and the role of HR-2 mutations. Using panels of ENF resistance-associated mutants for two patients, we found that mutations in HR-1 slowed the fusion kinetics and that mutations in HR-2 restored fusion rates. We assessed the differences in the rates of fusion of these mutants from a temperature-arrested state and observed similar trends, suggesting that the step of delay occurs after coreceptor engagement. Sensitivity to neutralizing antibodies was unchanged by the HR-1 and HR-2 mutants in each panel. Since this result was in contrast to those of a previous in vitro analysis where enhanced sensitivity to neutralization was demonstrated for heterologous Envs with ENF resistance-associated HR-1 changes, we examined the context dependence of HR-1 and HR-2 mutations by transferring the mutations seen in one patient into the Env context of another. These studies revealed that some, but not all, HR-1 mutations, when placed out of context (i.e., in a patient Env where they did not originally arise), enhance sensitivity to neutralizing antibodies. However, in most cases, HR-1 mutations in ENF-treated patients evolve in a manner that preserves pretreatment neutralization sensitivity so as to evade the pressures of the immune system.

Published

2009

43. Baseline resistance of primary human immunodeficiency virus type 1 strains to the CXCR4 inhibitor AMD3100.

Author

Harrison JE, Lynch JB, Sierra LJ, Blackburn LA, Ray N, Collman RG, and Doms RW

Subjects

Animals, Benzylamines, Cells, Cultured, Cyclams, Drug Resistance, Viral, HIV Envelope Protein gp120 chemistry, HIV Envelope Protein gp120 physiology, Quail, Receptors, CCR5 chemistry, Receptors, CXCR4 chemistry, HIV Fusion Inhibitors pharmacology, HIV-1 drug effects, Heterocyclic Compounds pharmacology, Receptors, CXCR4 antagonists & inhibitors

Abstract

We screened a panel of R5X4 and X4 human immunodeficiency virus type 1 (HIV-1) strains for their sensitivities to AMD3100, a small-molecule CXCR4 antagonist that blocks HIV-1 infection via this coreceptor. While no longer under clinical development, AMD3100 is a useful tool with which to probe interactions between the viral envelope (Env) protein and CXCR4 and to identify pathways by which HIV-1 may become resistant to this class of antiviral agents. While infection by most virus strains was completely blocked by AMD3100, we identified several R5X4 and X4 isolates that exhibited plateau effects: as the AMD3100 concentration was increased, virus infection and membrane fusion diminished to variable degrees. Once saturating concentrations of AMD3100 were achieved, further inhibition was not observed, indicating a noncompetitive mode of viral resistance to the drug. The magnitude of the plateau varied depending on the virus isolate, as well as the cell type used, with considerable variation observed when primary human T cells from different human donors were used. Structure-function studies indicated that the V1/V2 region of the R5X4 HIV-1 isolate DH12 was necessary for AMD3100 resistance and could confer this property on two heterologous Env proteins. We conclude that some R5X4 and X4 HIV-1 isolates can utilize the AMD3100-bound conformation of CXCR4, with the efficiency being influenced by both viral and host factors. Baseline resistance to this CXCR4 antagonist could influence the clinical use of such compounds.

Published

2008

44. An engineered Saccharomyces cerevisiae strain binds the broadly neutralizing human immunodeficiency virus type 1 antibody 2G12 and elicits mannose-specific gp120-binding antibodies.

Author

Luallen RJ, Lin J, Fu H, Cai KK, Agrawal C, Mboudjeka I, Lee FH, Montefiori D, Smith DF, Doms RW, and Geng Y

Subjects

Amino Acid Sequence, Antibodies, Monoclonal metabolism, Antibodies, Viral metabolism, Blotting, Western, Broadly Neutralizing Antibodies, Enzyme-Linked Immunosorbent Assay, Genetic Engineering methods, HIV Antibodies, Immune Sera immunology, Immunoprecipitation, Mannose metabolism, Microscopy, Fluorescence, Molecular Sequence Data, Saccharomyces cerevisiae virology, Antibodies, Monoclonal immunology, Antibodies, Viral immunology, HIV Envelope Protein gp120 immunology, HIV-1 immunology, Saccharomyces cerevisiae immunology

Abstract

The glycan shield of the human immunodeficiency virus type 1 (HIV-1) envelope (Env) protein serves as a barrier to antibody-mediated neutralization and plays a critical role in transmission and infection. One of the few broadly neutralizing HIV-1 antibodies, 2G12, binds to a carbohydrate epitope consisting of an array of high-mannose glycans exposed on the surface of the gp120 subunit of the Env protein. To produce proteins with exclusively high-mannose carbohydrates, we generated a mutant strain of Saccharomyces cerevisiae by deleting three genes in the N-glycosylation pathway, Och1, Mnn1, and Mnn4. Glycan profiling revealed that N-glycans produced by this mutant were almost exclusively Man(8)GlcNAc(2), and four endogenous glycoproteins that were efficiently recognized by the 2G12 antibody were identified. These yeast proteins, like HIV-1 gp120, contain a large number and high density of N-linked glycans, with glycosidase digestion abrogating 2G12 cross-reactivity. Immunization of rabbits with whole Delta och1 Delta mnn1 Delta mnn4 yeast cells produced sera that recognized a broad range of HIV-1 and simian immunodeficiency virus (SIV) Env glycoproteins, despite no HIV/SIV-related proteins being used in the immunization procedure. Analyses of one of these sera on a glycan array showed strong binding to glycans with terminal Man alpha1,2Man residues, and binding to gp120 was abrogated by glycosidase removal of high-mannose glycans and terminal Man alpha1,2Man residues, similar to 2G12. Since S. cerevisiae is genetically pliable and can be grown easily and inexpensively, it will be possible to produce new immunogens that recapitulate the 2G12 epitope and may make the glycan shield of HIV Env a practical target for vaccine development.

Published

2008

45. N-terminal substitutions in HIV-1 gp41 reduce the expression of non-trimeric envelope glycoproteins on the virus.

Author

Dey AK, David KB, Ray N, Ketas TJ, Klasse PJ, Doms RW, and Moore JP

Subjects

Cell Fusion, Cell Line, Dimerization, Gene Expression Regulation, Viral, HIV-1 genetics, HIV-1 metabolism, HIV-1 pathogenicity, HeLa Cells, Humans, Virion metabolism, Virion pathogenicity, Amino Acid Substitution, HIV Envelope Protein gp160 metabolism, HIV Envelope Protein gp41 genetics, env Gene Products, Human Immunodeficiency Virus metabolism

Abstract

The native, functional HIV-1 envelope glycoprotein (Env) complex is a trimer of two non-covalently associated subunits: the gp120 surface glycoprotein and the gp41 transmembrane glycoprotein. However, various non-functional forms of Env are present on virus particles and HIV-1-infected cells, some of which probably arise as the native complex decays. The aberrant forms include gp120-gp41 monomers and oligomers, as well as gp41 subunits from which gp120 has dissociated. The presence of non-functional Env creates binding sites for antibodies that do not recognize native Env complexes and that are, therefore, non-neutralizing. Non-native Env forms (monomers, dimers, tetramers and aggregates) can also arise when soluble gp140 proteins, lacking the cytoplasmic and transmembrane domains of gp41, are expressed for vaccine studies. We recently identified five amino acids in the gp41 N-terminal region (I535, Q543, S553, K567 and R588) that promote gp140 trimerization. We have now studied their influence on the function and antigenic properties of JR-FL Env expressed on the surfaces of pseudoviruses and Env-transfected cells. The 5 substitutions in gp41 reduce the expression of non-trimeric gp160s, without affecting trimer levels. Pseudovirions bearing the mutant Env are fully infectious with similar kinetics of Env-mediated fusion. Various non-neutralizing antibodies bind less strongly to the Env mutant, but neutralizing antibody binding is unaffected. Hence the gp41 substitutions do not adversely affect Env structure, supporting their use for making new Env-based vaccines. The mutant Env might also help in studies intended to correlate antibody binding to virus neutralization. Of note is that the 5 residues are much more frequent, individually or collectively, in viruses from subtypes other than B.

Published

2008

46. Focused dampening of antibody response to the immunodominant variable loops by engineered soluble gp140.

Author

Selvarajah S, Puffer BA, Lee FH, Zhu P, Li Y, Wyatt R, Roux KH, Doms RW, and Burton DR

Subjects

Animals, Blotting, Western, Cell Line, Enzyme-Linked Immunosorbent Assay, Glycosylation, HIV genetics, Humans, Microscopy, Electron, Transmission, Neutralization Tests, Rabbits, env Gene Products, Human Immunodeficiency Virus genetics, env Gene Products, Human Immunodeficiency Virus metabolism, env Gene Products, Human Immunodeficiency Virus ultrastructure, Epitopes, B-Lymphocyte immunology, HIV immunology, HIV Antibodies blood, HIV Infections immunology, env Gene Products, Human Immunodeficiency Virus immunology

Abstract

Immunization studies with modified gp120 monomers using a hyperglycosylation strategy, in which undesired epitopes are masked by the selective incorporation of N-linked glycans, were described in a previous paper (Selvarajah S, et al., J Virol 2000;79:12148-12163). In this report, we applied the hyperglycosylation strategy to soluble uncleaved gp140 trimers to improve the antigenic and immunogenic profile in the context of a trimeric conformation of the immunogen. The JR-FL gp140 gene was added upstream of a soluble trimerization domain of chicken cartilage matrix (CART) protein and expressed predominantly as a trimer and called gp140-CART wild-type. In the hyperglycosylated gp140-CART mCHO(V) mutant, four extra sugar attachment motifs on the variable loops helped mask epitope recognition by monoclonal antibodies specific to the variable loops. The gp140-CART mCHO(V) mutant and gp140-CART wild-type soluble trimer protein were used to immunize rabbits. The gp140-CART mCHO(V) immune sera had reduced antibody response to the variable loops compared to gp140-CART wild-type immune sera as shown by peptide reactivity, competition assays, and the reduced ability of sera to neutralize SF162 virus (a variable loop neutralization-sensitive virus). The antibody response to the CD4 binding site was retained in the gp140-CART mCHO(V) mutant immune sera similar to gp140-CART wild-type immune sera. The results demonstrate that the strategy of hyperglycosylation is clearly useful in the context of a compact form of Env immunogen such as the soluble gp140 trimer in dampening responses to variable loops while maintaining responses to an important epitope, the CD4 binding site. However, the results also show that in order to elicit broadly neutralizing antibodies that target conserved epitopes, the soluble gp140 trimer immunogen template will require further modifications.

Published

2008

47. Modulation of HIV and SIV neutralization sensitivity by DC-SIGN and mannose-binding lectin.

Author

Marzi A, Mitchell DA, Chaipan C, Fisch T, Doms RW, Carrington M, Desrosiers RC, and Pöhlmann S

Subjects

Animals, Cell Line, Glycosylation, HIV chemistry, HIV immunology, HIV metabolism, HIV Infections transmission, HIV Infections virology, Humans, Neutralization Tests, Polysaccharides metabolism, Simian Acquired Immunodeficiency Syndrome transmission, Simian Acquired Immunodeficiency Syndrome virology, Simian Immunodeficiency Virus chemistry, Simian Immunodeficiency Virus immunology, Simian Immunodeficiency Virus metabolism, Antibodies, Viral immunology, Cell Adhesion Molecules metabolism, HIV pathogenicity, HIV Antibodies immunology, Lectins, C-Type metabolism, Mannose-Binding Lectin metabolism, Receptors, Cell Surface metabolism, Simian Immunodeficiency Virus pathogenicity

Abstract

The C-type lectin DC-SIGN binds to oligosaccharides on the human and simian immunodeficiency virus (HIV, SIV) envelope glycoproteins and promotes infection of susceptible cells. Here, we show that DC-SIGN recognizes glycans involved in SIV sensitivity to neutralizing antibodies and that binding to DC-SIGN confers neutralization resistance to an otherwise sensitive SIV variant. Moreover, we provide evidence that mannose-binding lectin (MBL) can interfere with HIV-1 neutralization by the carbohydrate-specific antibody 2G12.

Published

2007

48. Replication-competent variants of human immunodeficiency virus type 2 lacking the V3 loop exhibit resistance to chemokine receptor antagonists.

Author

Lin G, Bertolotti-Ciarlet A, Haggarty B, Romano J, Nolan KM, Leslie GJ, Jordan AP, Huang CC, Kwong PD, Doms RW, and Hoxie JA

Subjects

Anti-HIV Agents pharmacology, Benzylamines, CCR5 Receptor Antagonists, CD4 Antigens genetics, CD4 Antigens metabolism, Cell Line, Cyclams, HIV Envelope Protein gp120 genetics, HIV Envelope Protein gp41 genetics, HIV Envelope Protein gp41 metabolism, HIV-1 genetics, HIV-2 genetics, Heterocyclic Compounds pharmacology, Humans, Oligopeptides pharmacology, Protein Structure, Secondary genetics, Receptors, CCR5 genetics, Receptors, CCR5 metabolism, Receptors, CXCR4 antagonists & inhibitors, Receptors, CXCR4 genetics, Receptors, CXCR4 metabolism, Sequence Deletion genetics, Drug Resistance, Viral drug effects, Drug Resistance, Viral genetics, HIV Envelope Protein gp120 metabolism, HIV-1 metabolism, HIV-2 metabolism, Virus Internalization drug effects, Virus Replication drug effects, Virus Replication genetics

Abstract

Entry of human immunodeficiency virus type 1 (HIV-1) and HIV-2 requires interactions between the envelope glycoprotein (Env) on the virus and CD4 and a chemokine receptor, either CCR5 or CXCR4, on the cell surface. The V3 loop of the HIV gp120 glycoprotein plays a critical role in this process, determining tropism for CCR5- or CXCR4-expressing cells, but details of how V3 interacts with these receptors have not been defined. Using an iterative process of deletion mutagenesis and in vitro adaptation of infectious viruses, variants of HIV-2 were derived that could replicate without V3, either with or without a deletion of the V1/V2 variable loops. The generation of these functional but markedly minimized Envs required adaptive changes on the gp120 core and gp41 transmembrane glycoprotein. V3-deleted Envs exhibited tropism for both CCR5- and CXCR4-expressing cells, suggesting that domains on the gp120 core were mediating interactions with determinants shared by both coreceptors. Remarkably, HIV-2 Envs with V3 deletions became resistant to small-molecule inhibitors of CCR5 and CXCR4, suggesting that these drugs inhibit wild-type viruses by disrupting a specific V3 interaction with the coreceptor. This study represents a proof of concept that HIV Envs lacking V3 alone or in combination with V1/V2 that retain functional domains required for viral entry can be derived. Such minimized Envs may be useful in understanding Env function, screening for new inhibitors of gp120 core interactions with chemokine receptors, and designing novel immunogens for vaccines.

Published

2007

49. V3 loop truncations in HIV-1 envelope impart resistance to coreceptor inhibitors and enhanced sensitivity to neutralizing antibodies.

Author

Laakso MM, Lee FH, Haggarty B, Agrawal C, Nolan KM, Biscone M, Romano J, Jordan AP, Leslie GJ, Meissner EG, Su L, Hoxie JA, and Doms RW

Subjects

Base Sequence, Cell Line, HIV Antibodies immunology, HIV Envelope Protein gp120 chemistry, HIV Envelope Protein gp120 genetics, HIV Fusion Inhibitors chemistry, HIV Fusion Inhibitors immunology, HIV-1 chemistry, HIV-1 genetics, Humans, Molecular Sequence Data, Neutralization Tests, Peptide Fragments chemistry, Peptide Fragments genetics, Receptors, CCR5 chemistry, Receptors, CCR5 genetics, Receptors, CCR5 immunology, Receptors, Chemokine chemistry, Receptors, Chemokine genetics, Receptors, HIV physiology, Virus Replication, HIV Envelope Protein gp120 immunology, HIV-1 immunology, Peptide Fragments immunology, Receptors, Chemokine immunology, Receptors, HIV antagonists & inhibitors

Abstract

The V1/V2 region and the V3 loop of the human immunodeficiency virus type I (HIV-1) envelope (Env) protein are targets for neutralizing antibodies and also play an important functional role, with the V3 loop largely determining whether a virus uses CCR5 (R5), CXCR4 (X4), or either coreceptor (R5X4) to infect cells. While the sequence of V3 is variable, its length is highly conserved. Structural studies indicate that V3 length may be important for interactions with the extracellular loops of the coreceptor. Consistent with this view, genetic truncation of the V3 loop is typically associated with loss of Env function. We removed approximately one-half of the V3 loop from three different HIV-1 strains, and found that only the Env protein from the R5X4 strain R3A retained some fusion activity. Loss of V1/V2 (DeltaV1/V2) was well tolerated by this virus. Passaging of virus with the truncated V3 loop resulted in the derivation of a virus strain that replicated with wild-type kinetics. This virus, termed TA1, retained the V3 loop truncation and acquired several adaptive changes in gp120 and gp41. TA1 could use CCR5 but not CXCR4 to infect cells, and was extremely sensitive to neutralization by HIV-1 positive human sera, and by antibodies to the CD4 binding site and to CD4-induced epitopes in the bridging sheet region of gp120. In addition, TA1 was completely resistant to CCR5 inhibitors, and was more dependent upon the N-terminal domain of CCR5, a region of the receptor that is thought to contact the bridging sheet of gp120 and the base of the V3 loop, and whose conformation may not be greatly affected by CCR5 inhibitors. These studies suggest that the V3 loop protects HIV from neutralization by antibodies prevalent in infected humans, that CCR5 inhibitors likely act by disrupting interactions between the V3 loop and the coreceptor, and that altered use of CCR5 by HIV-1 associated with increased sensitivity to changes in the N-terminal domain can be linked to high levels of resistance to these antiviral compounds.

Published

2007

50. Identification of a novel C-terminal cleavage of Crimean-Congo hemorrhagic fever virus PreGN that leads to generation of an NSM protein.

Author

Altamura LA, Bertolotti-Ciarlet A, Teigler J, Paragas J, Schmaljohn CS, and Doms RW

Subjects

Animals, Biological Transport, Chlorocebus aethiops, Cricetinae, Epitopes chemistry, Golgi Apparatus metabolism, HeLa Cells, Humans, Plasmids metabolism, Protein Conformation, Protein Structure, Tertiary, RNA, Viral chemistry, Vero Cells, Hemorrhagic Fever Virus, Crimean-Congo metabolism, Hemorrhagic Fever, Crimean virology

Abstract

The structural glycoproteins of Crimean-Congo hemorrhagic fever virus (CCHFV; genus Nairovirus, family Bunyaviridae) are derived through endoproteolytic cleavage of a 1,684-amino-acid M RNA segment-encoded polyprotein. This polyprotein is cotranslationally cleaved into the PreGN and PreGC precursors, which are then cleaved by SKI-1 and a SKI-1-like protease to generate the N termini of GN and GC, respectively. However, the resulting polypeptide defined by the N termini of GN and GC is predicted to be larger (58 kDa) than mature GN (37 kDa). By analogy to the topologically similar M segment-encoded polyproteins of viruses in the Orthobunyavirus genus, the C-terminal region of PreGN that contains four predicted transmembrane domains may also contain a nonstructural protein, NSM. To characterize potential PreGN C-terminal cleavage events, a panel of epitope-tagged PreGN truncation and internal deletion mutants was developed. These constructs allowed for the identification of a C-terminal endoproteolytic cleavage within, or very proximal to, the second predicted transmembrane domain following the GN ectodomain and the subsequent generation of a C-terminal fragment. Pulse-chase experiments showed that PreGN C-terminal cleavage occurred shortly after synthesis of the precursor and prior to generation of the GN glycoprotein. The resulting fragment trafficked to the Golgi compartment, the site of virus assembly. Development of an antiserum specific to the second cytoplasmic loop of PreGN allowed detection of cell-associated NSM proteins derived from transient expression of the complete CCHFV M segment and also in the context of virus infection.

Published

2007