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2
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Effect of bivalent interaction upon apparent antibody affinity: experimental confirmation of theory using fluorescence photobleaching and implications for antibody binding assays.二价相互作用对表观抗体亲和力的影响:利用荧光光漂白对理论的实验验证及对抗体结合测定的意义
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Preparation of iodine-131 labelled human growth hormone of high specific activity.高比活度碘-131标记人生长激素的制备
Nature. 1962 May 5;194:495-6. doi: 10.1038/194495a0.
2
THE REACTION WITH RED CELLS OF 7S RABBIT ANTIBODY, ITS SUB-UNITS AND THEIR RECOMBINANTS.7S兔抗体及其亚基和重组体与红细胞的反应
Immunology. 1965 Apr;8(4):420-31.
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HLA-A2 as a target for cell-mediated lympholysis: evidence from immunoselected HLA-A2 negative mutant cell lines.HLA - A2作为细胞介导的淋巴细胞溶解的靶点:来自免疫选择的HLA - A2阴性突变细胞系的证据。
Hum Immunol. 1980 Jul;1(1):77-86. doi: 10.1016/0198-8859(80)90011-7.
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A beginner's guide to major histocompatibility complex function.
Nature. 1982 Jun 24;297(5868):628. doi: 10.1038/297628a0.
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The kinetics of antibody binding to membrane antigens in solution and at the cell surface.抗体与溶液中和细胞表面膜抗原结合的动力学。
Biochem J. 1980 Apr 1;187(1):1-20. doi: 10.1042/bj1870001.
6
Gamma ray-induced loss of expression of HLA and glyoxalase I alleles in lymphoblastoid cells.γ射线诱导淋巴母细胞中HLA和乙二醛酶I等位基因表达缺失。
Proc Natl Acad Sci U S A. 1980 Jul;77(7):4251-5. doi: 10.1073/pnas.77.7.4251.
7
Cell surface properties of HLA antigens on Epstein-Barr virus-transformed cell lines.爱泼斯坦-巴尔病毒转化细胞系上HLA抗原的细胞表面特性
Proc Natl Acad Sci U S A. 1982 Jan;79(2):608-12. doi: 10.1073/pnas.79.2.608.
8
Quantitative analysis of cell surface HLA structures by means of monoclonal antibodies.利用单克隆抗体对细胞表面HLA结构进行定量分析。
Hum Immunol. 1980 Oct;1(3):233-43. doi: 10.1016/0198-8859(80)90018-x.
9
The antigenic structure of HLA-A2: an analysis with competitive binding assays and monoclonal antibodies.HLA - A2的抗原结构:竞争性结合试验和单克隆抗体分析
J Immunol. 1983 Aug;131(2):856-63.
10
Enhancement of monoclonal antibodies against HLA-A2 is due to antibody bivalency.抗HLA - A2单克隆抗体的增强作用归因于抗体的二价性。
J Biol Chem. 1983 Feb 10;258(3):1580-6.

单克隆抗体与细胞表面分子的结合。针对人类移植抗原HLA - A2的两个同种异体抗原决定簇的免疫球蛋白G定量分析。

The binding of monoclonal antibodies to cell-surface molecules. A quantitative analysis with immunoglobulin G against two alloantigenic determinants of the human transplantation antigen HLA-A2.

作者信息

Ways J P, Parham P

出版信息

Biochem J. 1983 Nov 15;216(2):423-32. doi: 10.1042/bj2160423.

DOI:10.1042/bj2160423
PMID:6197968
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1152520/
Abstract

Monoclonal IgG1 (immunoglobulin G1) PA2.1 and MA2.1 antibodies recognize polymorphic sites of the human transplantation antigen HLA-A2. They are distinguishable because MA2.1 binds HLA-A2 and HLA-B17, whereas PA2.1 binds HLA-A2 and HLA-A28. The affinities of PA2.1-Fab for HLA-A2, three HLA-A2 variants and HLA-A28 are similar and relatively low (1.9 X 10(7) M-1). The affinities of MA2.1-Fab for HLA-A2, three HLA-A2 variants and HLA-B17 are similar and high (1.2 X 10(9) M-1). The difference in affinity is due to the rates of dissociation, which give half-times of dissociation of 290 min for MA2.1-Fab and 4 min for PA2.1-Fab. For both Fab, equilibrium measurements and kinetic determinations gave consistent estimates for affinity. When PA2.1-F(ab)2 or IgG is incubated with cells it reaches equilibrium within 3 h, with most molecules bound bivalently to the cell. Under similar conditions, MA2.1-F(ab)2 does not reach equilibrium and a significant proportion of molecules bound with one and two sites are found. For the lower-affinity antibody (PA2.1), estimates of the binding constants for one- and two-site interactions could be made. By simple Scatchard analysis the avidity of F(ab)2 or IgG is 1.3 X 10(9) M-1, giving an enhancement factor of 68 between bivalent and univalent binding. This is a measure of the equilibrium constant for the interchange between bivalent and univalent binding. Analysis of the results with more realistic models indicates that the actual value is larger (10(3)-10(4) M-1) than 68 M-1. The avidities of F(ab)2 and IgG for HLA-A2 are identical, showing the Fc does not interfere with bivalent binding to cells.

摘要

单克隆IgG1(免疫球蛋白G1)PA2.1和MA2.1抗体识别人类移植抗原HLA - A2的多态性位点。它们是可区分的,因为MA2.1结合HLA - A2和HLA - B17,而PA2.1结合HLA - A2和HLA - A28。PA2.1 - Fab对HLA - A2、三种HLA - A2变体和HLA - A28的亲和力相似且相对较低(1.9×10⁷ M⁻¹)。MA2.1 - Fab对HLA - A2、三种HLA - A2变体和HLA - B17的亲和力相似且较高(1.2×10⁹ M⁻¹)。亲和力的差异归因于解离速率,MA2.1 - Fab的解离半衰期为290分钟,PA2.1 - Fab的解离半衰期为4分钟。对于这两种Fab,平衡测量和动力学测定给出了一致的亲和力估计值。当PA2.1 - F(ab)₂或IgG与细胞一起孵育时,它在3小时内达到平衡,大多数分子以二价形式结合到细胞上。在类似条件下,MA2.1 - F(ab)₂未达到平衡,并且发现有相当比例的分子以一个和两个位点结合。对于低亲和力抗体(PA2.1),可以对一位点和二位点相互作用的结合常数进行估计。通过简单的Scatchard分析,F(ab)₂或IgG的亲和力为1.3×10⁹ M⁻¹,二价结合与单价结合之间的增强因子为68。这是二价结合与单价结合之间互换的平衡常数的一种度量。用更实际的模型分析结果表明,实际值比68 M⁻¹更大(10³ - 10⁴ M⁻¹)。F(ab)₂和IgG对HLA - A2的亲和力相同,表明Fc不干扰与细胞的二价结合。