首页   按字顺浏览 期刊浏览 卷期浏览 Preferential Antibody Recognition of Structurally Distinct HIV‐1 gp120 Molecules
Preferential Antibody Recognition of Structurally Distinct HIV‐1 gp120 Molecules

 

作者: T. VanCott,   F. Bethke,   V. Kalyanaraman,   D. Burke,   R. Redfield,   D. Birx,  

 

期刊: Journal of Acquired Immune Deficiency Syndromes  (OVID Available online 1994)
卷期: Volume 7, issue 11  

页码: 1103-1115

 

ISSN:0894-9255

 

年代: 1994

 

出版商: OVID

 

关键词: Human immunodeficiency virus;gp120 envelope;AIDS vaccines;Bio-specific interaction analysis;Biosensors

 

数据来源: OVID

 

摘要:

We have developed an assay, using a biosensor matrix and surface plasmon resonance, that rapidly and reproducibly measures antibody reactivity to human immunodeficiency virus type 1 (HIV-1) gp120 in various structural conformations. In particular, antibodies displaying preferential reactivity to a CD4-binding competent (“native,” rgp120) or CD4-binding incompetent (“reduced,” rcmgp120) monomeric gp120 molecule were distinguished. This technique has advantages over conventional enzyme-linked immunosorbent assay (ELISA) methodology in which it is difficult to control the concentration of protein adsorbed to the ELISA wells and a significant disruption of protein structure occurs on adsorption. A population of gp120 molecules that lacked CD4 receptor binding capacity and bound antibodies specific for reduced gp120 was found in several native gp120 preparations. The relative amount of this CD4-binding incompetent population varied among the various preparations studied. This presence of CD4-binding incompetent molecules within various native recombinant gp120 preparations may have implications for HIV-1 envelope vaccine development. By measuring antibody-binding ratios, several monoclonal antibodies were identified, which, although elicited by immunization with various native gp120 preparations, bound specifically to reduced gp120. The ability to screen antibody specificity against HIV-1 envelope proteins with different conformations will assist in determining the quality of antibodies induced by various HIV-1 envelope vaccine candidates.

 

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