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1. The HIV-1 late domain-2 S40A polymorphism in antiretroviral (or ART)-exposed individuals influences protease inhibitor susceptibility

Author

Watanabe, Susan M, Simon, Viviana, Durham, Natasha D, Kemp, Brittney R, Machihara, Satoshi, Kemal, Kimdar Sherefa, Shi, Binshan, Foley, Brian, Li, Hongru, Chen, Benjamin K, Weiser, Barbara, Burger, Harold, Anastos, Kathryn, Chen, Chaoping, and Carter, Carol A

Subjects
Microbiology, Biological Sciences, Genetics, HIV/AIDS, Aetiology, 2.1 Biological and endogenous factors, Infection, Antiretroviral Therapy, Highly Active, Female, HEK293 Cells, HIV Infections, HIV Protease, HIV Protease Inhibitors, HIV-1, Humans, Mutation, Polymorphism, Genetic, Reproductive Tract Infections, Transcription Factors, Virus Release, Virus Replication, gag Gene Products, Human Immunodeficiency Virus, HIV Gag, HIV protease, Protease inhibitors, Late domain, Anti-retroviral drugs, ESCRT, Clinical Sciences, Virology
Abstract

BackgroundThe p6 region of the HIV-1 structural precursor polyprotein, Gag, contains two motifs, P7TAP11 and L35YPLXSL41, designated as late (L) domain-1 and -2, respectively. These motifs bind the ESCRT-I factor Tsg101 and the ESCRT adaptor Alix, respectively, and are critical for efficient budding of virus particles from the plasma membrane. L domain-2 is thought to be functionally redundant to PTAP. To identify possible other functions of L domain-2, we examined this motif in dominant viruses that emerged in a group of 14 women who had detectable levels of HIV-1 in both plasma and genital tract despite a history of current or previous antiretroviral therapy.ResultsRemarkably, variants possessing mutations or rare polymorphisms in the highly conserved L domain-2 were identified in seven of these women. A mutation in a conserved residue (S40A) that does not reduce Gag interaction with Alix and therefore did not reduce budding efficiency was further investigated. This mutation causes a simultaneous change in the Pol reading frame but exhibits little deficiency in Gag processing and virion maturation. Whether introduced into the HIV-1 NL4-3 strain genome or a model protease (PR) precursor, S40A reduced production of mature PR. This same mutation also led to high level detection of two extended forms of PR that were fairly stable compared to the WT in the presence of IDV at various concentrations; one of the extended forms was effective in trans processing even at micromolar IDV.ConclusionsOur results indicate that L domain-2, considered redundant in vitro, can undergo mutations in vivo that significantly alter PR function. These may contribute fitness benefits in both the absence and presence of PR inhibitor.

Published
2016

10. P2X1 Selective Antagonists Block HIV-1 Infection through Inhibition of Envelope Conformation-Dependent Fusion

Author

Soare, Alexandra Y., primary, Malik, Hagerah S., additional, Durham, Natasha D., additional, Freeman, Tracey L., additional, Alvarez, Raymond, additional, Patel, Foramben, additional, Satija, Namita, additional, Upadhyay, Chitra, additional, Hioe, Catarina E., additional, Chen, Benjamin K., additional, and Swartz, Talia H., additional

Published
2020
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13. Broadly neutralizing human antibodies against dengue virus identified by single B cell transcriptomics

Author

Durham, Natasha D, primary, Agrawal, Aditi, additional, Waltari, Eric, additional, Croote, Derek, additional, Zanini, Fabio, additional, Fouch, Mallorie, additional, Davidson, Edgar, additional, Smith, Olivia, additional, Carabajal, Esteban, additional, Pak, John E, additional, Doranz, Benjamin J, additional, Robinson, Makeda, additional, Sanz, Ana M, additional, Albornoz, Ludwig L, additional, Rosso, Fernando, additional, Einav, Shirit, additional, Quake, Stephen R, additional, McCutcheon, Krista M, additional, and Goo, Leslie, additional

Published
2019
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14. Author response: Broadly neutralizing human antibodies against dengue virus identified by single B cell transcriptomics

Author

Durham, Natasha D, primary, Agrawal, Aditi, additional, Waltari, Eric, additional, Croote, Derek, additional, Zanini, Fabio, additional, Fouch, Mallorie, additional, Davidson, Edgar, additional, Smith, Olivia, additional, Carabajal, Esteban, additional, Pak, John E, additional, Doranz, Benjamin J, additional, Robinson, Makeda, additional, Sanz, Ana M, additional, Albornoz, Ludwig L, additional, Rosso, Fernando, additional, Einav, Shirit, additional, Quake, Stephen R, additional, McCutcheon, Krista M, additional, and Goo, Leslie, additional

Published
2019
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15. Functional characterization and lineage analysis of broadly neutralizing human antibodies against dengue virus identified by single B cell transcriptomics

Author

Durham, Natasha D., primary, Agrawal, Aditi, additional, Waltari, Eric, additional, Croote, Derek, additional, Zanini, Fabio, additional, Davidson, Edgar, additional, Fouch, Mallorie, additional, Smith, Olivia, additional, Carabajal, Esteban, additional, Pak, John E., additional, Doranz, Benjamin J., additional, Robinson, Makeda, additional, Sanz, Ana M., additional, Albornoz, Ludwig L., additional, Rosso, Fernando, additional, Einav, Shirit, additional, Quake, Stephen R., additional, McCutcheon, Krista M., additional, and Goo, Leslie, additional

Published
2019
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16. P2X1 selective antagonists block HIV-1 infection through inhibition of envelope conformation-dependent fusion

Author

Soare, Alexandra Y., primary, Malik, Hagerah S., additional, Durham, Natasha D., additional, Freeman, Tracey L., additional, Alvarez, Raymond, additional, Patel, Foramben, additional, Satija, Namita, additional, Upadhyay, Chitra, additional, Hioe, Catarina E., additional, Chen, Benjamin K., additional, and Swartz, Talia H., additional

Published
2019
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18. P2X Antagonists Inhibit HIV-1 Productive Infection and Inflammatory Cytokines Interleukin-10 (IL-10) and IL-1β in a Human Tonsil Explant Model

Author

Soare, Alexandra Y., primary, Durham, Natasha D., additional, Gopal, Ramya, additional, Tweel, Benjamin, additional, Hoffman, Kevin W., additional, Brown, Julia A., additional, O’Brien, Megan, additional, Bhardwaj, Nina, additional, Lim, Jean K., additional, Chen, Benjamin K., additional, and Swartz, Talia H., additional

Published
2019
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20. Conformational changes in the Ebola virus membrane fusion machine induced by pH, Ca2+, and receptor binding.

Author

Das, Dibyendu Kumar, Bulow, Uriel, Diehl, William E., Durham, Natasha D., Senjobe, Fernando, Chandran, Kartik, Luban, Jeremy, and Munro, James B.

Subjects
MEMBRANE fusion, EBOLA virus, VIRAL envelope proteins, FLUORESCENCE resonance energy transfer, VIRAL envelopes
Abstract

The Ebola virus (EBOV) envelope glycoprotein (GP) is a membrane fusion machine required for virus entry into cells. Following endocytosis of EBOV, the GP1 domain is cleaved by cellular cathepsins in acidic endosomes, removing the glycan cap and exposing a binding site for the Niemann-Pick C1 (NPC1) receptor. NPC1 binding to cleaved GP1 is required for entry. How this interaction translates to GP2 domain-mediated fusion of viral and endosomal membranes is not known. Here, using a bulk fluorescence dequenching assay and single-molecule Förster resonance energy transfer (smFRET)-imaging, we found that acidic pH, Ca2+, and NPC1 binding synergistically induce conformational changes in GP2 and permit virus-liposome lipid mixing. Acidic pH and Ca2+ shifted the GP2 conformational equilibrium in favor of an intermediate state primed for NPC1 binding. Glycan cap cleavage on GP1 enabled GP2 to transition from a reversible intermediate to an irreversible conformation, suggestive of the postfusion 6-helix bundle; NPC1 binding further promoted transition to the irreversible conformation. Thus, the glycan cap of GP1 may allosterically protect against inactivation of EBOV by premature triggering of GP2. The Ebola virus envelope glycoprotein is a membrane fusion machine required for the virus to enter into host cells. This study presents direct observation of the conformational changes that the envelope glycoprotein undergoes during the membrane fusion process. [ABSTRACT FROM AUTHOR]

Published
2020
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21. P2X antagonists inhibit HIV-1 productive infection and inflammatory cytokines IL-10 and IL-1β in a human tonsil explant model

Author

Soare, Alexandra Y., primary, Durham, Natasha D., additional, Gopal, Ramya, additional, Tweel, Benjamin, additional, Hoffman, Kevin W., additional, Brown, Julia A., additional, O’Brien, Megan, additional, Bhardwaj, Nina, additional, Lim, Jean K., additional, Chen, Benjamin K., additional, and Swartz, Talia H., additional

Published
2018
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22. Single-molecule imaging reveals allosteric stimulation of SARS-CoV-2 spike receptor binding domain by host sialic acid.

Author

Díaz-Salinas, Marco A., Jain, Aastha, Durham, Natasha D., and Munro, James B.

Subjects
*SARS-CoV-2, *SIALIC acids, *FLUORESCENCE resonance energy transfer, *ANGIOTENSIN converting enzyme
Abstract

Conformational dynamics of the severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) spike glycoprotein (S) mediate exposure of the binding site for the cellular receptor, angiotensin-converting enzyme 2 (ACE2). The N-terminal domain (NTD) of S binds terminal sialic acid (SA) moieties on the cell surface, but the functional role of this interaction in virus entry is unknown. Here, we report that NTD-SA interaction enhances both S-mediated virus attachment and ACE2 binding. Through single-molecule Förster resonance energy transfer imaging of individual S trimers, we demonstrate that SA binding to the NTD allosterically shifts the S conformational equilibrium, favoring enhanced exposure of the ACE2-binding site. Antibodies that target the NTD block SA binding, which contributes to their mechanism of neutralization. These findings inform on mechanisms of S activation at the cell surface. [ABSTRACT FROM AUTHOR]

Published
2024
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23. Enhanced FCGR2A and FCGR3A signaling by HIV viremic controller IgG

Author

Alvarez, Raymond A., primary, Maestre, Ana M., additional, Law, Kenneth, additional, Durham, Natasha D., additional, Barria, Maria Ines, additional, Ishii-Watabe, Akiko, additional, Tada, Minoru, additional, Kapoor, Manav, additional, Hotta, Mathew T., additional, Rodriguez-Caprio, Gabriela, additional, Fierer, Daniel S., additional, Fernandez-Sesma, Ana, additional, Simon, Viviana, additional, and Chen, Benjamin K., additional

Published
2017
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28. The HIV-1 late domain-2 S40A polymorphism in antiretroviral (or ART)-exposed individuals influences protease inhibitor susceptibility.

Author

Watanabe, Susan M., Simon, Viviana, Durham, Natasha D., Kemp, Brittney R., Machihara, Satoshi, Kemal, Kimdar Sherefa, Shi, Binshan, Foley, Brian, Hongru Li, Chen, Benjamin K., Weiser, Barbara, Burger, Harold, Anastos, Kathryn, Chaoping Chen, and Carter, Carol A.

Subjects
HIV infection genetics, GENETICS of disease susceptibility, GENETIC polymorphisms, ANTIRETROVIRAL agents, PROTEASE inhibitors
Abstract

Background: The p6 region of the HIV-1 structural precursor polyprotein, Gag, contains two motifs, P7TAP11 and L35YPLXSL41, designated as late (L) domain-1 and -2, respectively. These motifs bind the ESCRT-I factor Tsg101 and the ESCRT adaptor Alix, respectively, and are critical for efficient budding of virus particles from the plasma membrane. L domain-2 is thought to be functionally redundant to PTAP. To identify possible other functions of L domain-2, we examined this motif in dominant viruses that emerged in a group of 14 women who had detectable levels of HIV-1 in both plasma and genital tract despite a history of current or previous antiretroviral therapy. Results: Remarkably, variants possessing mutations or rare polymorphisms in the highly conserved L domain-2 were identified in seven of these women. A mutation in a conserved residue (S40A) that does not reduce Gag interaction with Alix and therefore did not reduce budding efficiency was further investigated. This mutation causes a simultaneous change in the Pol reading frame but exhibits little deficiency in Gag processing and virion maturation. Whether introduced into the HIV-1 NL4-3 strain genome or a model protease (PR) precursor, S40A reduced production of mature PR. This same mutation also led to high level detection of two extended forms of PR that were fairly stable compared to the WT in the presence of IDV at various concentrations; one of the extended forms was effective in trans processing even at micromolar IDV. Conclusions: Our results indicate that L domain-2, considered redundant in vitro, can undergo mutations in vivo that significantly alter PR function. These may contribute fitness benefits in both the absence and presence of PR inhibitor. [ABSTRACT FROM AUTHOR]

Published
2016
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31. MOESM1 of The HIV-1 late domain-2 S40A polymorphism in antiretroviral (or ART)-exposed individuals influences protease inhibitor susceptibility

Author

Watanabe, Susan, Simon, Viviana, Durham, Natasha, Kemp, Brittney, Machihara, Satoshi, Kimdar Kemal, Binshan Shi, Foley, Brian, Hongru Li, Chen, Benjamin, Weiser, Barbara, Burger, Harold, Anastos, Kathryn, Chaoping Chen, and Carter, Carol

Subjects
3. Good health
Abstract

Additional file 1: Figure S1. Quantification of PR-V5 and p6*-PR-HA b produced by four different L-MBP fusion precursors (A-D). Signal value of each band (see Methods) was determined by the Image Studio software to represent band intensity. The solid lines denote p6*-PR-HAb detected in the cell lysates; the dashes line denote PR-V5 produced by trans processing.

32. MOESM1 of The HIV-1 late domain-2 S40A polymorphism in antiretroviral (or ART)-exposed individuals influences protease inhibitor susceptibility

Author

Watanabe, Susan, Simon, Viviana, Durham, Natasha, Kemp, Brittney, Machihara, Satoshi, Kimdar Kemal, Binshan Shi, Foley, Brian, Hongru Li, Chen, Benjamin, Weiser, Barbara, Burger, Harold, Anastos, Kathryn, Chaoping Chen, and Carter, Carol

Subjects
3. Good health
Abstract

Additional file 1: Figure S1. Quantification of PR-V5 and p6*-PR-HA b produced by four different L-MBP fusion precursors (A-D). Signal value of each band (see Methods) was determined by the Image Studio software to represent band intensity. The solid lines denote p6*-PR-HAb detected in the cell lysates; the dashes line denote PR-V5 produced by trans processing.

33. MOESM2 of The HIV-1 late domain-2 S40A polymorphism in antiretroviral (or ART)-exposed individuals influences protease inhibitor susceptibility

Author

Watanabe, Susan, Simon, Viviana, Durham, Natasha, Kemp, Brittney, Machihara, Satoshi, Kimdar Kemal, Binshan Shi, Foley, Brian, Hongru Li, Chen, Benjamin, Weiser, Barbara, Burger, Harold, Anastos, Kathryn, Chaoping Chen, and Carter, Carol

Subjects
3. Good health
Abstract

Additional file 2: Figure S2. The S40A and S40F mutants were placed into a fluorescent protein-expressing HIV (NLSF-GI construct) and examined by cell-free and cell-cell transmission using previously described assays [48]. S40A and S40F mutations were introduced into NLSF-GI constructs using restriction sites EcoR1 and Sph1 and previously described methodology. Cell-free virus particles were made in 293T cells transfected with WT NLSF-GI (includes NL4-3 env), Î env NLSF-GI, or the mutants. For cell-to-cell infection, 293Ts were used 24h after transfection as donors (removed using cell dissociation buffer). Donors were also diluted 1:1 or 1:3 with uninfected 293Ts to reduce input infection levels. Media was changed at 18h post infection (cell-free) or post co-culture with MT-4 cells (cell-cell) to media with 10uM AZT. The cells were fixed and examined by flow cytometry @ 40h. The average of triplicate samples was used to calculate values. The raw values were normalized to WT level for comparison. The cell-free infectivity of virus produced in 293T cells was severely reduced in the case of the S40F, but not the WT or the S40A mutant (panel A). In cell-to-cell infection with 293T as the producer cell, the same transmission efficiency exhibited by the S40A mutant in the cell-free assay was observed in the cell-to-cell assay (panel B). However the defective S40F infectivity apparent in the cell-free assay (panel A) was rescued by cell-to-cell transmission, reaching a level comparable to the WT (panel B). Overall, we can conclude that the infectivity defect of S40F can be rescued by cell-cell transmission.

34. Ebola Virus Glycoprotein Strongly Binds to Membranes in the Absence of Receptor Engagement.

Author

Vaknin A, Grossman A, Durham ND, Lupovitz I, Goren S, Golani G, Roichman Y, Munro JB, and Sorkin R

Subjects
Humans, Protein Binding, Virus Internalization, Niemann-Pick C1 Protein metabolism, Cell Membrane metabolism, Cell Membrane virology, Hemorrhagic Fever, Ebola virology, Hydrogen-Ion Concentration, Ebolavirus metabolism, Ebolavirus physiology, Ebolavirus genetics, Ebolavirus chemistry, Viral Envelope Proteins metabolism, Viral Envelope Proteins chemistry, Viral Envelope Proteins genetics
Abstract

Ebola virus (EBOV) is an enveloped virus that must fuse with the host cell membrane in order to release its genome and initiate infection. This process requires the action of the EBOV envelope glycoprotein (GP), encoded by the virus, which resides in the viral envelope and consists of a receptor binding subunit, GP1, and a membrane fusion subunit, GP2. Despite extensive research, a mechanistic understanding of the viral fusion process is incomplete. To investigate GP-membrane association, a key step in the fusion process, we used two approaches: high-throughput measurements of single-particle diffusion and single-molecule measurements with optical tweezers. Using these methods, we show that the presence of the endosomal Niemann-Pick C1 (NPC1) receptor is not required for primed GP-membrane binding. In addition, we demonstrate this binding is very strong, likely attributed to the interaction between the GP fusion loop and the membrane's hydrophobic core. Our results also align with previously reported findings, emphasizing the significance of acidic pH in the protein-membrane interaction. Beyond Ebola virus research, our approach provides a powerful toolkit for studying other protein-membrane interactions, opening new avenues for a better understanding of protein-mediated membrane fusion events.

Published
2024
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35. Regulation of Ebola GP conformation and membrane binding by the chemical environment of the late endosome.

Author

Jain A, Govindan R, Berkman A, Luban J, Durham ND, and Munro J

Abstract

Interaction between the Ebola virus envelope glycoprotein (GP) and the endosomal membrane is an essential step during virus entry into the cell. Acidic pH and Ca2+ have been implicated in mediating the GP-membrane interaction. However, the molecular mechanism by which these environmental factors regulate the conformational changes that enable engagement of GP with the target membrane is unknown. Here, we apply fluorescence correlation spectroscopy (FCS) and single-molecule Forster resonance energy transfer (smFRET) imaging to elucidate how the acidic pH, Ca2+ and anionic phospholipids in the late endosome promote GP-membrane interaction, thereby facilitating virus entry. We find that bis(monoacylglycero)phosphate (BMP), which is specific to the late endosome, is especially critical in determining the Ca2+-dependence of the GP-membrane interaction. Molecular dynamics (MD) simulations suggested residues in GP that sense pH and induce conformational changes that make the fusion loop available for insertion into the membrane. We similarly confirm residues in the fusion loop that mediate GPs interaction with Ca2+, which likely promotes local conformational changes in the fusion loop and mediates electrostatic interactions with the anionic phospholipids. Collectively, our results provide a mechanistic understanding of how the environment of the late endosome regulates the timing and efficiency of virus entry.

Published
2023
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36. P2X Antagonists Inhibit HIV-1 Productive Infection and Inflammatory Cytokines Interleukin-10 (IL-10) and IL-1β in a Human Tonsil Explant Model.

Author

Soare AY, Durham ND, Gopal R, Tweel B, Hoffman KW, Brown JA, O'Brien M, Bhardwaj N, Lim JK, Chen BK, and Swartz TH

Subjects
Benzenesulfonates pharmacology, Down-Regulation, Gene Expression Regulation, HIV Infections drug therapy, HIV-1 drug effects, HIV-1 immunology, Humans, Models, Biological, Palatine Tonsil drug effects, Palatine Tonsil immunology, Palatine Tonsil virology, Pyridines pharmacology, Tetrazoles pharmacology, Tissue Culture Techniques, Virulence drug effects, Zidovudine pharmacology, HIV Infections immunology, HIV-1 pathogenicity, Interleukin-10 metabolism, Interleukin-1beta metabolism, Palatine Tonsil cytology, Purinergic P2X Receptor Antagonists pharmacology
Abstract

HIV-1 causes a persistent infection of the immune system that is associated with chronic comorbidities. The mechanisms that underlie this inflammation are poorly understood. Emerging literature has implicated proinflammatory purinergic receptors and downstream signaling mediators in HIV-1 infection. This study probed whether inhibitors of purinergic receptors would reduce HIV-1 infection and HIV-1-stimulated inflammation. An ex vivo human tonsil histoculture infection model was developed to support HIV-1 productive infection and stimulated the inflammatory cytokine interleukin-1 beta (IL-1β) and the immunosuppressive cytokine interleukin-10 (IL-10). This study tests whether inhibitors of purinergic receptors would reduce HIV-1 infection and HIV-1-stimulated inflammation. The purinergic P2X1 receptor antagonist NF449, the purinergic P2X7 receptor antagonist A438079, and azidothymidine (AZT) were tested in HIV-1-infected human tonsil explants to compare levels of inhibition of HIV-1 infection and HIV-stimulated inflammatory cytokine production. All drugs limited HIV-1 productive infection, but P2X-selective antagonists (NF449 and A438079) significantly lowered HIV-stimulated IL-10 and IL-1β. We further observed that P2X1- and P2X7-selective antagonists can act differentially as inhibitors of both HIV-1 infection and HIV-1-stimulated inflammation. Our findings highlight the differential effects of HIV-1 on inflammation in peripheral blood compared to those in lymphoid tissue. For the first time, we demonstrate that P2X-selective antagonists act differentially as inhibitors of both HIV-1 infection and HIV-1-stimulated inflammation. Drugs that block these pathways can have independent inhibitory activities against HIV-1 infection and HIV-induced inflammation. IMPORTANCE Patients who are chronically infected with HIV-1 experience sequelae related to chronic inflammation. The mechanisms of this inflammation have not been elucidated. Here, we describe a class of drugs that target the P2X proinflammatory signaling receptors in a human tonsil explant model. This model highlights differences in HIV-1 stimulation of lymphoid tissue inflammation and peripheral blood. These drugs serve to block both HIV-1 infection and production of IL-10 and IL-1β in lymphoid tissue, suggesting a novel approach to HIV-1 therapeutics in which both HIV-1 replication and inflammatory signaling are simultaneously targeted., (Copyright © 2018 American Society for Microbiology.)

Published
2018
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37. Measuring T Cell-to-T Cell HIV-1 Transfer, Viral Fusion, and Infection Using Flow Cytometry.

Author

Durham ND and Chen BK

Subjects
Animals, Cell Communication, Cell Culture Techniques methods, HIV Infections virology, Humans, Jurkat Cells, Membrane Fusion, T-Lymphocytes cytology, Flow Cytometry methods, HIV Infections pathology, HIV-1 physiology, T-Lymphocytes pathology, T-Lymphocytes virology, Virus Internalization
Abstract

Direct T cell-to-T cell HIV-1 infection is a distinct mode of HIV-1 infection that requires physical contact between an HIV-1-infected "donor" cell and an uninfected, CD4-expressing "target" cell. In vitro studies indicate that HIV-1 cell-to-cell infection is much more efficient than infection by cell-free viral particles; however, the exact mechanisms of the enhanced efficiency of this infection pathway are still unclear. Several assays have been developed to study the mechanism of direct cell-to-cell HIV-1 transmission and to assess sensitivity to neutralizing antibodies and pharmacologic inhibitors. These assays are based on the coculture of donor and target cells. Here, we describe methods that utilize flow cytometry, which can discriminate donor and target cells and can assess different stages of entry and infection following cell-to-cell contact. HIV Gag-iGFP, a clone that makes fluorescent virus particles, can be used to measure cell-to-cell transfer of virus particles. HIV NL-GI, a clone that expresses GFP as an early gene, facilitates the measure of productive infection after cell-to-cell contact. Lastly, a variation of the β-lactamase (BlaM)-Vpr fusion assay can be used to measure the viral membrane fusion process after coculture of donor and target cells in a manner that is independent of cell-cell fusion. These assays can be performed in the presence of neutralizing antibodies/inhibitors to determine the 50 % inhibitory concentration (IC50) required to block infection specifically in the target cells.

Published
2016
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