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两种CD23单克隆抗体的特性鉴定,其反应性与该分化簇内的其他抗体不同。

Characterization of two CD23 monoclonal antibodies with reactivity distinct from other antibodies within this cluster of differentiation.

作者信息

Goff L K, Armitage R J, Beverley P C

机构信息

Imperial Cancer Research Fund, Human Tumour Immunology Group, London, U.K.

出版信息

Immunology. 1988 Oct;65(2):213-20.

PMID:2461344
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1384916/
Abstract

We have produced two CD23 monoclonal antibodies (mAb), LA1 and LA2, which differ significantly in their patterns of reactivity compared to other mAb within this cluster. Unlike other CD23 mAb, LA1 and LA2 show virtually no reactivity with freshly isolated tonsil B lymphocytes or mantle zone lymphocytes in tissue section. That LA1 and LA2 are CD23 mAb is confirmed by their precipitation of a 45,000 MW surface protein from B cells and strong reactivity with a CD23 transfectant. Cross-blocking studies with four well-characterized CD23 mAb show that LA1 and LA2 recognize the same, distinct epitope of the CD23 molecule. However, similar to other CD23 mAb, expression of LA1 and LA2 increases after activation. Following removal of cells staining with the well-characterized CD23 mAb MHM6, using a highly efficient magnetic bead technique, LA1 and LA2, but not other CD23 mAb, react with a subpopulation of the remaining cells when activated with interleukin-4 (IL-4) or phorbol ester. Soluble LA1 and MHM6 both provide a co-stimulatory signal for phorbol ester-induced B-cell proliferation. This response is increased if these mAb are used to cross-link the CD23 molecule. Interestingly, despite the fact that LA2 and LA1 cross-block, LA2 has no effect on functional responses in its soluble form but can elicit a comparable increase in proliferation when cross-linked. Results presented here suggest that the novel CD23 mAb, LA1 and LA2, recognize a distinct form of the CD23 molecule, expressed only on activation. These mAb define a subpopulation of activated B cells which do not stain with other CD23 mAb.

摘要

我们制备了两种CD23单克隆抗体(mAb),LA1和LA2,与该簇内的其他单克隆抗体相比,它们的反应模式有显著差异。与其他CD23单克隆抗体不同,LA1和LA2对新鲜分离的扁桃体B淋巴细胞或组织切片中的套区淋巴细胞几乎没有反应性。LA1和LA2是CD23单克隆抗体这一点通过它们从B细胞中沉淀出45,000 MW的表面蛋白以及与CD23转染体的强反应性得到证实。用四种特征明确的CD23单克隆抗体进行的交叉阻断研究表明,LA1和LA2识别CD23分子相同的、独特的表位。然而,与其他CD23单克隆抗体类似,LA1和LA2的表达在激活后增加。在用特征明确的CD23单克隆抗体MHM6染色的细胞被去除后,使用高效磁珠技术,当用白细胞介素-4(IL-4)或佛波酯激活时,LA1和LA2而非其他CD23单克隆抗体与剩余细胞的一个亚群发生反应。可溶性LA1和MHM6都为佛波酯诱导的B细胞增殖提供共刺激信号。如果使用这些单克隆抗体交联CD23分子,这种反应会增强。有趣的是,尽管LA2和LA1能交叉阻断,但LA2的可溶性形式对功能反应没有影响,但交联时能引发类似的增殖增加。此处呈现的结果表明,新型CD23单克隆抗体LA1和LA2识别一种仅在激活时表达的CD23分子的独特形式。这些单克隆抗体定义了一个不被其他CD23单克隆抗体染色的活化B细胞亚群。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2a6e/1384916/2ef0809d1beb/immunology00150-0054-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2a6e/1384916/9544aa4b4f0a/immunology00150-0053-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2a6e/1384916/2ef0809d1beb/immunology00150-0054-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2a6e/1384916/9544aa4b4f0a/immunology00150-0053-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2a6e/1384916/2ef0809d1beb/immunology00150-0054-a.jpg

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本文引用的文献

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Biosynthesis of HLA-A and HLA-B antigens in vivo.体内HLA - A和HLA - B抗原的生物合成。
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The low-affinity receptor for IgE (CD23) on B lymphocytes is spatially associated with HLA-DR antigens.B淋巴细胞上的IgE低亲和力受体(CD23)在空间上与HLA-DR抗原相关联。
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Coordinated action of IgE and a B-cell-stimulatory factor on the CD23 receptor molecule up-regulates B-lymphocyte growth.IgE与一种B细胞刺激因子对CD23受体分子的协同作用上调B淋巴细胞生长。
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Human recombinant interleukin 4 induces Fc epsilon receptors (CD23) on normal human B lymphocytes.人重组白细胞介素4可诱导正常人B淋巴细胞上的Fcε受体(CD23)。
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Molecular structure of human lymphocyte receptor for immunoglobulin E.人免疫球蛋白E淋巴细胞受体的分子结构
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Triggering of B lymphocytes through CD23: epitope mapping and studies using antibody derivatives indicate an allosteric mechanism of signalling.通过CD23触发B淋巴细胞:表位作图及使用抗体衍生物的研究表明一种变构信号传导机制。
Immunology. 1987 Apr;60(4):517-21.
10
Ligation of the CD23,p45 (BLAST-2,EBVCS) antigen triggers the cell-cycle progression of activated B lymphocytes.CD23、p45(BLAST-2、EBVCS)抗原的结扎触发活化B淋巴细胞的细胞周期进程。
Eur J Immunol. 1986 Sep;16(9):1075-80. doi: 10.1002/eji.1830160908.