Your search keyword '"Blake Wood"' showing total 10 results

1. Virulence assessment of Australian Pyrenophora tritici‐repentis isolates

Author

Nikki Schultz, Kalai A. Marathamuthu, Caroline S. Moffat, Kefei Chen, Blake Wood, Manisha Shankar, and Pao Theen See

Subjects

Genetics, Pyrenophora, Virulence, Plant Science, Horticulture, Biology, biology.organism_classification, Agronomy and Crop Science

Published

2021

2. Antibody Specificities Associated with Neutralization Breadth in Plasma from Human Immunodeficiency Virus Type 1 Subtype C-Infected Blood Donors

Author

John R. Mascola, Natasha Taylor, George M. Shaw, Blake Wood, Elin S. Gray, Allan C. deCamp, Diane Wycuff, Adrian Puren, David C. Montefiori, Georgia D. Tomaras, Lynn Morris, James M. Binley, Penny L. Moore, Peter B. Gilbert, Constantinos Kurt Wibmer, and Barton F. Haynes

Subjects

Immunology, Blood Donors, Cross Reactions, HIV Antibodies, Microbiology, Virus, Epitope, Neutralization, Antibody Specificity, Neutralization Tests, Virology, Humans, chemistry.chemical_classification, biology, Antibody titer, biology.organism_classification, Molecular biology, Epitope mapping, chemistry, Antibodies, Anticardiolipin, Insect Science, Lentivirus, HIV-1, biology.protein, Pathogenesis and Immunity, Antibody, Glycoprotein, Epitope Mapping

Abstract

Defining the specificities of the anti-human immunodeficiency virus type 1 (HIV-1) envelope antibodies able to mediate broad heterologous neutralization will assist in identifying targets for an HIV-1 vaccine. We screened 70 plasmas from chronically HIV-1-infected individuals for neutralization breadth. Of these, 16 (23%) were found to neutralize 80% or more of the viruses tested. Anti-CD4 binding site (CD4bs) antibodies were found in almost all plasmas independent of their neutralization breadth, but they mainly mediated neutralization of the laboratory strain HxB2 with little effect on the primary virus, Du151. Adsorption with Du151 monomeric gp120 reduced neutralizing activity to some extent in most plasma samples when tested against the matched virus, although these antibodies did not always confer cross-neutralization. For one plasma, this activity was mapped to a site overlapping the CD4-induced (CD4i) epitope and CD4bs. Anti-membrane-proximal external region (MPER) ( r = 0.69; P < 0.001) and anti-CD4i ( r = 0.49; P < 0.001) antibody titers were found to be correlated with the neutralization breadth. These anti-MPER antibodies were not 4E10- or 2F5-like but spanned the 4E10 epitope. Furthermore, we found that anti-cardiolipin antibodies were correlated with the neutralization breadth ( r = 0.67; P < 0.001) and anti-MPER antibodies ( r = 0.6; P < 0.001). Our study suggests that more than one epitope on the envelope glycoprotein is involved in the cross-reactive neutralization elicited during natural HIV-1 infection, many of which are yet to be determined, and that polyreactive antibodies are possibly involved in this phenomenon.

Published

2009

3. Factors Associated with the Development of Cross-Reactive Neutralizing Antibodies during Human Immunodeficiency Virus Type 1 Infection

Author

D. Noah Sather, Xuesong Yu, Leonidas Stamatatos, Jakob Armann, Steve Self, Lance K. Ching, Angeliki Mavrantoni, George Sellhorn, Zachary Caldwell, Spyros A. Kalams, and Blake Wood

Subjects

Male, Author's Correction, Immunology, Human immunodeficiency virus (HIV), HIV Infections, Cross immunity, Cross Reactions, HIV Antibodies, medicine.disease_cause, Gp41, Microbiology, Epitope, Epitopes, Neutralization Tests, Virology, medicine, Humans, Avidity, HIV vaccine, Neutralizing antibody, biology, env Gene Products, Human Immunodeficiency Virus, virus diseases, Epitope mapping, Insect Science, HIV-1, biology.protein, Pathogenesis and Immunity, Female, Antibody, Epitope Mapping

Abstract

The characterization of the cross-reactive, or heterologous, neutralizing antibody responses developed during human immunodeficiency virus type 1 (HIV-1) infection and the identification of factors associated with their generation are relevant to the development of an HIV vaccine. We report that in healthy HIV-positive, antiretroviral-naïve subjects, the breadth of plasma heterologous neutralizing antibody responses correlates with the time since infection, plasma viremia levels, and the binding avidity of anti-Env antibodies. Anti-CD4-binding site antibodies are responsible for the exceptionally broad cross-neutralizing antibody responses recorded only in rare plasma samples. However, in most cases examined, antibodies to the variable regions and to the CD4-binding site of Env modestly contributed in defining the overall breadth of these responses. Plasmas with broad cross-neutralizing antibody responses were identified that targeted the gp120 subunit, but their precise epitopes mapped outside the variable regions and the CD4-binding site. Finally, although several plasmas were identified with cross-neutralizing antibody responses that were not directed against gp120, only one plasma with a moderate breadth of heterologous neutralizing antibody responses contained cross-reactive neutralizing antibodies against the 4E10 epitope, which is within the gp41 transmembrane subunit. Overall, our study indicates that more than one pathway leads to the development of broad cross-reactive neutralizing antibodies during HIV infection and that the virus continuously escapes their action.

Published

2009

4. Profiling the Specificity of Neutralizing Antibodies in a Large Panel of Plasmas from Patients Chronically Infected with Human Immunodeficiency Virus Type 1 Subtypes B and C

Author

John R. Mascola, James E. Robinson, Lynn Morris, Cory Nathe, Elizabeth A. Lybarger, Diane Wycuff, Douglas D. Richman, Emma T. Crooks, Frederic Bibollet-Ruche, James M. Binley, Blake Wood, Linda Harris, Elin S. Gray, David C. Montefiori, Natalie Hawkins, George M. Shaw, Julie M. Decker, Georgia D. Tomaras, Katie L. Davis, and Michael S. Seaman

Subjects

Receptors, CCR5, Guinea Pigs, Immunology, Enzyme-Linked Immunosorbent Assay, HIV Antibodies, HIV Envelope Protein gp120, Gp41, Microbiology, Virus, Epitope, Neutralization, Immunoglobulin G, Antibody Specificity, Neutralization Tests, Virology, Animals, Humans, Primary isolate, Neutralizing antibody, Acquired Immunodeficiency Syndrome, biology, env Gene Products, Human Immunodeficiency Virus, Molecular biology, HIV Envelope Protein gp41, Peptide Fragments, Immunoglobulin A, Insect Science, CD4 Antigens, Chronic Disease, HIV-1, biology.protein, Pathogenesis and Immunity, Electrophoresis, Polyacrylamide Gel, Antibody

Abstract

Identifying the viral epitopes targeted by broad neutralizing antibodies (NAbs) that sometimes develop in human immunodeficiency virus type 1 (HIV-1)-infected subjects should assist in the design of vaccines to elicit similar responses. Here, we investigated the activities of a panel of 24 broadly neutralizing plasmas from subtype B- and C-infected donors using a series of complementary mapping methods, focusing mostly on JR-FL as a prototype subtype B primary isolate. Adsorption with gp120 immobilized on beads revealed that an often large but variable fraction of plasma neutralization was directed to gp120 and that in some cases, neutralization was largely mediated by CD4 binding site (CD4bs) Abs. The results of a native polyacrylamide gel electrophoresis assay using JR-FL trimers further suggested that half of the subtype B and a smaller fraction of subtype C plasmas contained a significant proportion of NAbs directed to the CD4bs. Anti-gp41 neutralizing activity was detected in several plasmas of both subtypes, but in all but one case, constituted only a minor fraction of the overall neutralization activity. Assessment of the activities of the subtype B plasmas against chimeric HIV-2 viruses bearing various fragments of the membrane proximal external region (MPER) of HIV-1 gp41 revealed mixed patterns, implying that MPER neutralization was not dominated by any single specificity akin to known MPER-specific monoclonal Abs. V3 and 2G12-like NAbs appeared to make little or no contribution to JR-FL neutralization titers. Overall, we observed significant titers of anti-CD4bs NAbs in several plasmas, but approximately two-thirds of the neutralizing activity remained undefined, suggesting the existence of NAbs with specificities unlike any characterized to date.

Published

2008

5. Development and implementation of an international proficiency testing program for a neutralizing antibody assay for HIV-1 in TZM-bl cells

Author

Peter B. Gilbert, Ronald Brown, Kelli Greene, Maggie Wang, Yunda Huang, Xuesong Yu, Daniel A. Ozaki, Christopher A. Todd, Gary Li, Hongmei Gao, Blake Wood, M. Patricia D'Souza, Marcella Sarzotti-Kelsoe, and David C. Montefiori

Subjects

Quality Control, medicine.medical_specialty, Laboratory Proficiency Testing, Standardization, Immunology, Human immunodeficiency virus (HIV), HIV Infections, HIV Antibodies, medicine.disease_cause, Article, Neutralization Tests, Cell Line, Tumor, Proficiency testing, Immunology and Allergy, Medicine, Humans, Medical physics, Neutralizing antibody, Reference standards, Luciferase reporter gene, AIDS Vaccines, biology, Extramural, business.industry, Reference Standards, Virology, Antibodies, Neutralizing, biology.protein, HIV-1, business

Abstract

Recent advances in assay technology have led to major improvements in how HIV-1 neutralizing antibodies are measured. A luciferase reporter gene assay performed in TZM-bl (JC53bl-13) cells has been optimized and validated. Because this assay has been adopted by multiple laboratories worldwide, an external proficiency testing program was developed to ensure data equivalency across laboratories performing this neutralizing antibody assay for HIV/AIDS vaccine clinical trials. The program was optimized by conducting three independent rounds of testing, with an increased level of stringency from the first to third round. Results from the participating domestic and international laboratories improved each round as factors that contributed to inter-assay variability were identified and minimized. Key contributors to increased agreement were experience among laboratories and standardization of reagents. A statistical qualification rule was developed using a simulation procedure based on the three optimization rounds of testing, where a laboratory qualifies if at least 25 of the 30 ID50 values lie within the acceptance ranges. This ensures no more than a 20% risk that a participating laboratory fails to qualify when it should, as defined by the simulation procedure. Five experienced reference laboratories were identified and tested a series of standardized reagents to derive the acceptance ranges for pass–fail criteria. This Standardized Proficiency Testing Program is the first available for the evaluation and documentation of assay equivalency for laboratories performing HIV-1 neutralizing antibody assays and may provide guidance for the development of future proficiency testing programs for other assay platforms.

Published

2011

6. Tiered Categorization of a Diverse Panel of HIV-1 Env Pseudoviruses for Assessment of Neutralizing Antibodies ▿

Author

Francine E. McCutchan, Peter B. Gilbert, Blake Wood, John R. Mascola, Natalie Hawkins, Michael S. Seaman, Colleen Devoy, Holly Janes, Alan Lapedes, Tanmoy Bhattacharya, Linda Harris, Ayush Giri, Bette T. Korber, Victoria R. Polonis, David C. Montefiori, Lauren E. Grandpre, Steve Self, Rory Coffey, and Marcus Daniels

Subjects

biology, Immunology, Human immunodeficiency virus (HIV), Gene Products, env, HIV Infections, biology.organism_classification, medicine.disease_cause, Microbiology, Virology, Antibodies, Neutralizing, Virus, Neutralization, Cell Line, Insect Science, Lentivirus, Vaccines and Antiviral Agents, biology.protein, medicine, HIV-1, Humans, Antibody, Clade, Neutralizing antibody

Abstract

The restricted neutralization breadth of vaccine-elicited antibodies is a major limitation of current human immunodeficiency virus-1 (HIV-1) candidate vaccines. In order to permit the efficient identification of vaccines with enhanced capacity for eliciting cross-reactive neutralizing antibodies (NAbs) and to assess the overall breadth and potency of vaccine-elicited NAb reactivity, we assembled a panel of 109 molecularly cloned HIV-1 Env pseudoviruses representing a broad range of genetic and geographic diversity. Viral isolates from all major circulating genetic subtypes were included, as were viruses derived shortly after transmission and during the early and chronic stages of infection. We assembled a panel of genetically diverse HIV-1-positive (HIV-1 + ) plasma pools to assess the neutralization sensitivities of the entire virus panel. When the viruses were rank ordered according to the average sensitivity to neutralization by the HIV-1 + plasmas, a continuum of average sensitivity was observed. Clustering analysis of the patterns of sensitivity defined four subgroups of viruses: those having very high (tier 1A), above-average (tier 1B), moderate (tier 2), or low (tier 3) sensitivity to antibody-mediated neutralization. We also investigated potential associations between characteristics of the viral isolates (clade, stage of infection, and source of virus) and sensitivity to NAb. In particular, higher levels of NAb activity were observed when the virus and plasma pool were matched in clade. These data provide the first systematic assessment of the overall neutralization sensitivities of a genetically and geographically diverse panel of circulating HIV-1 strains. These reference viruses can facilitate the systematic characterization of NAb responses elicited by candidate vaccine immunogens.

Published

2009

7. Anti-V3 Monoclonal Antibodies Display Broad Neutralizing Activities against Multiple HIV-1 Subtypes

Author

Terri Wrin, Susan Zolla-Pazner, Blake Wood, Xuesong Yu, Steve Self, Catarina E. Hioe, Constance Williams, Michael S. Seaman, and Miroslaw K. Gorny

Subjects

medicine.drug_class, lcsh:Medicine, HIV Infections, Cross Reactions, HIV Envelope Protein gp120, V3 loop, Biology, Antibodies, Viral, Monoclonal antibody, Virus, Neutralization, 03 medical and health sciences, Receptors, HIV, Immunology/Immunity to Infections, medicine, Humans, lcsh:Science, Neutralizing antibody, Virology/Vaccines, Conserved Sequence, 030304 developmental biology, chemistry.chemical_classification, 0303 health sciences, Multidisciplinary, 030306 microbiology, lcsh:R, Antibodies, Monoclonal, Infectious Diseases/HIV Infection and AIDS, Antibodies, Neutralizing, Virology, Peptide Fragments, 3. Good health, chemistry, Area Under Curve, Data Interpretation, Statistical, Immunology/Immune Response, Monoclonal, Immunology, HIV-1, biology.protein, lcsh:Q, Virology/Host Antiviral Responses, Antibody, Glycoprotein, Research Article

Abstract

Background: The V3 loop of the HIV-1 envelope (Env) glycoprotein gp120 was identified as the ‘‘principal neutralizing domain’’ of HIV-1, but has been considered too variable to serve as a neutralizing antibody (Ab) target. Structural and immunochemical data suggest, however, that V3 contains conserved elements which explain its role in binding to virus coreceptors despite its sequence variability. Despite this evidence of V3 conservation, the ability of anti-V3 Abs to neutralize a significant proportion of HIV-1 isolates from different subtypes (clades) has remained controversial. Methods: HIV-1 neutralization experiments were conducted in two independent laboratories to test human anti-V3 monoclonal Abs (mAbs) against pseudoviruses (psVs) expressing Envs of diverse HIV-1 subtypes from subjects with acute and chronic infections. Neutralization was defined by 50% inhibitory concentrations (IC50), and was statistically assessed based on the area under the neutralization titration curves (AUC). Results: Using AUC analyses, statistically significant neutralization was observed by $1 anti-V3 mAbs against 56/98 (57%) psVs expressing Envs of diverse subtypes, including subtypes A, AG, B, C and D. Even when the 10 Tier 1 psVs tested were excluded from the analysis, significant neutralization was detected by $1 anti-V3 mAbs against 46/88 (52%) psVs from diverse HIV-1 subtypes. Furthermore, 9/24 (37.5%) Tier 2 viruses from the clade B and C standard reference panels were neutralized by $1 anti-V3 mAbs. Each anti-V3 mAb tested was able to neutralize 28–42% of the psVs tested. By IC50 criteria, 40/98 (41%) psVs were neutralized by $1 anti-V3 mAbs. Conclusions: Using standard and new statistical methods of data analysis, 6/7 anti-V3 human mAbs displayed cross-clade neutralizing activity and revealed that a significant proportion of viruses can be neutralized by anti-V3 Abs. The new statistical method for analysis of neutralization data provides many advantages to previously used analyses.

Published

2010

8. P04-10. Neutralization of Tier 1 and Tier 2 pseudoviruses by human anti-V3 monoclonal antibodies

Author

Phillipe N. Nyambi, Alok Choudhary, Constance Williams, Timothy O'Neal, Kalpana Luthra, Seaman, Miroslaw K. Gorny, Blake Wood, and Susan Zolla-Pazner

Subjects

lcsh:Immunologic diseases. Allergy, biology, business.industry, medicine.drug_class, Bioinformatics, Monoclonal antibody, Virology, Neutralization, Tier 1 network, Infectious Diseases, Tier 2 network, Poster Presentation, biology.protein, Medicine, Antibody, lcsh:RC581-607, business

Published

2009

9. P15-04. Development and implementation of an international proficiency testing program for a neutralizing antibody assay for HIV-1 in TZM-bl cells

Author

Peter B. Gilbert, Christopher A. Todd, Xuesong Yu, Daniel A. Ozaki, Marcella Sarzotti-Kelsoe, M Wang, Blake Wood, Hongmei Gao, Kelli Greene, and David C. Montefiori

Subjects

lcsh:Immunologic diseases. Allergy, biology, business.industry, Human immunodeficiency virus (HIV), medicine.disease_cause, Virology, Infectious Diseases, Poster Presentation, biology.protein, Proficiency testing, Medicine, Antibody, Neutralizing antibody, business, lcsh:RC581-607

10. LabKey Server NAb: A tool for analyzing, visualizing and sharing results from neutralizing antibody assays

Author

Mark Igra, Sarah Ramsay, Elizabeth Nelson, Hongmei Gao, Josh Eckels, David C. Montefiori, Karl Lum, Kelli Greene, Blake Wood, Michael S. Seaman, and Britt Piehler

Subjects

lcsh:Immunologic diseases. Allergy, Computer science, Interface (computing), Statistics as Topic, Immunology, Human immunodeficiency virus (HIV), Information Storage and Retrieval, Bioinformatics, medicine.disease_cause, computer.software_genre, 03 medical and health sciences, 0302 clinical medicine, Software, Neutralization Tests, medicine, Animals, Humans, Macro, Neutralizing antibody, 030304 developmental biology, 0303 health sciences, biology, business.industry, Information Dissemination, High-Throughput Screening Assays, Identifier, Databases as Topic, 030220 oncology & carcinogenesis, Benchmark (computing), biology.protein, Operating system, business, lcsh:RC581-607, Serum dilution, computer

Abstract

Background Multiple types of assays allow sensitive detection of virus-specific neutralizing antibodies. For example, the extent of antibody neutralization of HIV-1, SIV and SHIV can be measured in the TZM-bl cell line through the degree of luciferase reporter gene expression after infection. In the past, neutralization curves and titers for this standard assay have been calculated using an Excel macro. Updating all instances of such a macro with new techniques can be unwieldy and introduce non-uniformity across multi-lab teams. Using Excel also poses challenges in centrally storing, sharing and associating raw data files and results. Results We present LabKey Server's NAb tool for organizing, analyzing and securely sharing data, files and results for neutralizing antibody (NAb) assays, including the luciferase-based TZM-bl NAb assay. The customizable tool supports high-throughput experiments and includes a graphical plate template designer, allowing researchers to quickly adapt calculations to new plate layouts. The tool calculates the percent neutralization for each serum dilution based on luminescence measurements, fits a range of neutralization curves to titration results and uses these curves to estimate the neutralizing antibody titers for benchmark dilutions. Results, curve visualizations and raw data files are stored in a database and shared through a secure, web-based interface. NAb results can be integrated with other data sources based on sample identifiers. It is simple to make results public after publication by updating folder security settings. Conclusions Standardized tools for analyzing, archiving and sharing assay results can improve the reproducibility, comparability and reliability of results obtained across many labs. LabKey Server and its NAb tool are freely available as open source software at http://www.labkey.com under the Apache 2.0 license. Many members of the HIV research community can also access the LabKey Server NAb tool without installing the software by using the Atlas Science Portal (https://atlas.scharp.org). Atlas is an installation of LabKey Server.