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Dive into the research topics where Bryan C. Tieman is active.

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Featured researches published by Bryan C. Tieman.


Clinical and Vaccine Immunology | 2010

Generation and Characterization of Chimeric Antibodies against NS3, NS4, NS5, and Core Antigens of Hepatitis C Virus

Bailin Tu; Robert N. Ziemann; Bryan C. Tieman; David J. Hawksworth; Joan D. Tyner; James W. Scheffel; Mary S. Pinkus; Susan E. Brophy; Jeffrey M. Werneke; Robin A. Gutierrez; Michael White

ABSTRACT Mouse-human chimeric antibodies (cAbs) against hepatitis C virus (HCV) core, NS3 (nonstructural), NS4, and NS5 antigens were developed as quality control (QC) reagents to replace the use of human sera/plasma for Abbott HCV immunoassays. The cAb retains the mouse monoclonal antibody (MAb) specificity and affinity but still reacts in the existing HCV assay format, which measures human anti-HCV immunoglobulin. Mouse heavy-chain (VH) and light-chain (VL) variable regions of anti-HCV core, NS3, NS4, and NS5 antigens were PCR amplified from hybridoma lines and then cloned with human IgG1 heavy-chain (CH) and light-chain (CL) constant regions, respectively. A single mammalian expression plasmid containing both heavy-chain and light-chain immunoglobulin genes was constructed and transfected into dihydrofolate reductase (DHFR)-deficient Chinese hamster ovary (CHO) cells. The transfected CHO cells were selected using hypoxanthine- and thymidine-free medium and screened by an enzyme immunoassay (EIA). The clone secreting the highest level of antibody was isolated from the CHO transfectants and further subcloned. Each cAb-expressing CHO cell line was weaned into serum-free medium, and the cAb was purified by protein A affinity chromatography. The levels of cAb production for the various CHO cell lines varied from 10 to 20 mg/liter. Purified anti-HCV cAbs were tested with Abbott HCV immunoassays and showed reactivity. Moreover, yeast surface display combined with alanine-scanning mutagenesis was used to map the epitope at the individual amino acid level. Our results suggest that these HCV cAbs are ideal controls, calibrators, and/or QC reagents for HCV assay standardization.


Hybridoma | 2012

Generation of Human Neutrophil Gelatinase-Associated Lipocalin Monoclonal Antibodies for Use in ARCHITECT® Assay

David J. Hawksworth; Bailin Tu; Bryan C. Tieman; Susan E. Brophy; Joan D. Tyner; A. Scott Muerhoff; Robert N. Ziemann

Development of a robust immunoassay requires the selection of monoclonal antibodies with desired properties. These properties generally include kinetics parameters such as on-rate and off-rate (i.e., binding affinity), and, often times, the ability to form a sandwich with the analyte of interest. We sought to obtain antibodies suitable for development of an immunoassay capable of detecting human neutrophil gelatinase-associated lipocalin (NGAL), a glycosylated lipocalin of 25 kDa expressed in kidney tubules in response to injury that has been shown to be a urinary biomarker capable of diagnosing acute kidney injury. We immunized CAF1/J and RBF/DnJ mouse strains with recombinant NGAL, and a robust immune response, as measured by serum antibody titer, was observed among all CAF1/J mice. Antibodies secreted from mouse B cell-myeloma hybridomas were screened by enzyme immunoassay (EIA) and by surface plasmon resonance using a method we termed hybrid supernatant kinetic screening. Approximately 300 hybrid clones were evaluated by this technique to identify antibodies with the kinetic binding parameters meeting criteria required for further assay development (i.e., rapid association and slow dissociation). This data, along with epitope grouping, cell growth, cell viability, and antibody secretion, were used to identify antibodies for testing in the ARCHITECT assay.


Archive | 2008

IMMUNOASSAYS AND KITS FOR THE DETECTION OF NGAL

Larry G. Birkenmeyer; Suresh M. Desai; Frank C. Grenier; David J. Hawksworth; Edward T. Olejniczak; Qiaoqiao Ruan; Robert W. Siegel; Sergey Y. Tetin; Bryan C. Tieman; Bailin Tu; Joan D. Tyner; Ryan F. Workman; Robert N. Ziemann; Lowell J. Tyner


Archive | 2008

ANTIBODIES THAT BIND TO MAMMALIAN NGAL AND USES THEREOF

Larry G. Birkenmeyer; Suresh M. Desai; David J. Hawksworth; Edward T. Olejniczak; Qiaoqiao Ruan; Robert W. Siegel; Sergey Y. Tetin; Bryan C. Tieman; Bailin Tu; Joan D. Tyner; Robert N. Ziemann


Archive | 2006

Human ring specific bnp antibodies

Jessie W. Shih; Joan D. Tyner; Matthew S. Matias; Mary S. Pinkus; Susan E. Brophy; David J. Dagfal; David J. Hawksworth; Bryan C. Tieman


Archive | 2009

SOLUBLE FMS-LIKE TYROSINE KINASE-1 (sFLT-1) ANTIBODY AND RELATED COMPOSITION, KIT, METHODS OF USING, AND MATERIALS AND METHOD FOR MAKING

Susan E. Brophy; Saul A. Datwyler; David J. Hawksworth; Don C. Laird; Sharmila Manoj; Dominick Pucci; Bryan C. Tieman; Joan D. Tyner; Zhiguang Yu


Archive | 2008

Anti-t. cruzi antibodies and methods of use

Susan E. Brophy; David J. Hawksworth; Dinesh O. Shah; Robert W. Siegel; Bryan C. Tieman; Bailin Tu; Joan D. Tyner; Robert N. Ziemann


Archive | 2013

HCV core lipid binding domain monoclonal antibodies

Robert N. Ziemann; April Ahlberg; David J. Hawksworth; Bryan C. Tieman; A. Scott Muerhoff; Christopher Marohnic; Kathy Otis


Archive | 2014

Anti-gp73 monoclonal antibodies and methods of obtaining the same

Bailin Tu; Robert N. Ziemann; Bryan C. Tieman; Philip M. Hemken; Carol S. Ramsay; Carolyn J. Strobel; David J. Hawksworth; Larry G. Birkenmeyer; Cheng Zhao; Susan E. Brophy; Barry L. Dowell; Anthony S. Muerhoff


Archive | 2016

Detection methods employing hcv core lipid and dna binding domain monoclonal antibodies

Robert N. Ziemann; April Ahlberg; David J. Hawksworth; Bryan C. Tieman; A. Scott Muerhoff; Christopher Marohnic; Kathy Otis; Andrea D. Branch; Francis J. Eng

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David J. Hawksworth

Icahn School of Medicine at Mount Sinai

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Robert N. Ziemann

Icahn School of Medicine at Mount Sinai

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Larry G. Birkenmeyer

National Institutes of Health

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A. Scott Muerhoff

Icahn School of Medicine at Mount Sinai

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April Ahlberg

Icahn School of Medicine at Mount Sinai

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