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鉴定出一种自发脱落的含有C3d结合位点的二型B细胞补体受体(CR2)片段。

Identification of a spontaneously shed fragment of B cell complement receptor type two (CR2) containing the C3d-binding site.

作者信息

Myones B L, Ross G D

出版信息

Complement. 1987;4(2):87-98. doi: 10.1159/000463012.

DOI:10.1159/000463012
PMID:3497773
Abstract

CR2 is a 140-kilodalton glycoprotein expressed on B lymphocytes which binds to both C3d and Epstein-Barr virus (EBV). The present study identified a 72-kilodalton C3d-binding protein (gp72) in the spent culture media of Raji B lymphoblastoid cells as a spontaneously shed fragment of the 140-kilodalton CR2 molecule. Both polyclonal and monoclonal antibodies (AB) were used in several assay systems to detect antigenic determinants shared between the gp72 fragment and CR2. Rabbit antibodies to either intact CR2 or gp72 blocked C3d receptor activity, and this inhibitory activity was removed by absorption of anti-CR2 with purified gp72.OKB7, a monoclonal anti-CR2 AB that blocks both C3d and EBV binding to CR2, reacted specifically with both CR2 and gp72, whereas both anti-B2 and HB-5 monoclonal anti-CR2 AB, that block neither of these receptor sites, were unreactive with gp72. The data suggested that the gp72 fragment was not present as such in intact cells, but rather was a product of cells generated by proteolysis of CR2. Thus, intrinsically labeled gp72 was isolated from Raji cell media by affinity chromatography on OKB7-Sepharose, but only intact CR2 was isolated from the Raji cell fraction solubilized in the presence of protease inhibitors. Several lines of evidence suggested that gp72 was not a second type of C3d receptor that was distinct from CR2. First, Raji cells expressed nearly identical amounts of OKB7 and HB-5 epitopes when analyzed by flow cytometry or radioimmune assay, excluding the possibility that B cells expressed OKB7 antigens in both CR2 and a distinct HB-5-negative C3d receptor. Second, all Raji cell surface C3d receptor activity was associated with HB-5-reactive CR2 molecules. We conclude that gp72 represents a spontaneously shed proteolytic fragment of CR2 that contains the C3d-binding site and the closely associated OKB7 epitope.

摘要

CR2是一种在B淋巴细胞上表达的140千道尔顿糖蛋白,它能与C3d和爱泼斯坦-巴尔病毒(EBV)结合。本研究在Raji B淋巴母细胞的用过的培养基中鉴定出一种72千道尔顿的C3d结合蛋白(gp72),它是140千道尔顿CR2分子的自发脱落片段。在多个检测系统中使用多克隆抗体和单克隆抗体(AB)来检测gp72片段和CR2之间共有的抗原决定簇。针对完整CR2或gp72的兔抗体可阻断C3d受体活性,并且这种抑制活性可通过用纯化的gp72吸收抗CR2而消除。OKB7是一种单克隆抗CR2抗体,可阻断C3d和EBV与CR2的结合,它能与CR2和gp72特异性反应,而既不阻断这些受体位点的抗B2和HB-5单克隆抗CR2抗体与gp72无反应。数据表明,gp72片段在完整细胞中并非以这种形式存在,而是CR2蛋白水解产生的细胞产物。因此,通过在OKB7-琼脂糖上进行亲和层析从Raji细胞培养基中分离出内在标记的gp72,但在存在蛋白酶抑制剂的情况下溶解的Raji细胞组分中仅分离出完整的CR2。几条证据表明,gp72不是一种与CR2不同的第二种C3d受体。首先,通过流式细胞术或放射免疫分析时,Raji细胞表达的OKB7和HB-5表位数量几乎相同,排除了B细胞在CR2和一种独特的HB-5阴性C3d受体中都表达OKB7抗原的可能性。其次,所有Raji细胞表面C3d受体活性都与HB-5反应性CR2分子相关。我们得出结论,gp72代表CR2的一种自发脱落的蛋白水解片段,它包含C3d结合位点和紧密相关的OKB7表位。

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