Hogg N, Ross G D, Jones D B, Slusarenko M, Walport M J, Lachmann P J
Eur J Immunol. 1984 Mar;14(3):236-43. doi: 10.1002/eji.1830140307.
A monoclonal antibody (E11) was produced by immunization of mice with intact human cells of monocyte lineage. Despite the finding that E11 did not inhibit rosettes with C3b-coated sheep erythrocytes (EC3b), several lines of evidence indicated that E11 was specific for complement receptor type one (CR1). All monocytes, neutrophils, lymphocytes and erythrocytes that reacted with E11 formed EC3b rosettes. The E11 antigen on these cells was shown to be a molecule of 222 +/- 10 kDa. Treatment of lymphocytes, monocytes, and neutrophils with E11 followed by fluorescein-coupled F(ab')2 anti-mouse-IgG at 37 degrees C in buffer lacking sodium azide, led to capping or apparent endocytosis of the E11 antigen and a diminution in CR1 activity of 88%, 59% and 25%, respectively. This same treatment had no detectable effect on monocyte or neutrophil CR3 activity (EC3bi rosettes). Furthermore, with E11-capped lymphocytes, the residual EC3b rosetting was capped directly over the E11-fluorescence cap, whereas EC3d,g rosetting (CR2 specific) was undiminished and distributed evenly around the circumference of cells containing E11-fluorescence caps. Finally, the binding of E11 to cells was inhibited by the prior treatment of these cells with a well characterized rabbit polyclonal anti-CR1. These data indicated that E11 was specific for a site in CR1 that was distal from the C3b-binding site, so that E11 was unable to block CR1 activity. E11 proved to be useful for identifying CR1 on various cells in tissue sections, and for quantitating CR1 on erythrocytes and neutrophils. Erythrocytes and neutrophils from normal individuals were found to bind an average of 610 and 4.6 X 10(4) 125I-labeled E11 molecules per cell. When E11 was visualized in tissues by immunoperoxidase staining, the cells that apparently contained the greatest amounts of CR1 were dendritic reticulum cells and kidney podocytes. The E11 reactive dentritic reticulum cells were characteristic of both follicular and diffuse follicular center cell tumors. Lymphocytes from patients with chronic lymphocytic leukemia (CLL) characteristically expressed little E11, confirming earlier studies that CLL cells lacked CR1 activity detected by EAC1-3b rosette formation. Because normal B cells have been shown to express CR1 at a very early stage of maturation, the absence of CR1 on CLL cells is discordant with the immature nature of CLL cells defined by immunoglobulin expression.
用完整的人单核细胞系细胞免疫小鼠,制备了一种单克隆抗体(E11)。尽管发现E11不抑制与C3b包被的绵羊红细胞(EC3b)形成的玫瑰花结,但多条证据表明E11对I型补体受体(CR1)具有特异性。所有与E11反应的单核细胞、中性粒细胞、淋巴细胞和红细胞均形成EC3b玫瑰花结。这些细胞上的E11抗原显示为一种分子量为222±10 kDa的分子。在缺乏叠氮化钠的缓冲液中,于37℃用E11处理淋巴细胞、单核细胞和中性粒细胞,随后用荧光素偶联的F(ab')2抗小鼠IgG处理,导致E11抗原出现帽化或明显的内吞作用,CR1活性分别降低88%、59%和25%。相同处理对单核细胞或中性粒细胞的CR3活性(EC3bi玫瑰花结)无明显影响。此外,对于E11帽化的淋巴细胞,剩余的EC3b玫瑰花结直接在E11荧光帽上方形成帽化,而EC3d,g玫瑰花结(CR2特异性)未减少,均匀分布在含有E11荧光帽的细胞周边。最后,用一种特征明确的兔多克隆抗CR1预先处理这些细胞,可抑制E11与细胞的结合。这些数据表明,E11对CR1中远离C3b结合位点的一个位点具有特异性,因此E11无法阻断CR1活性。事实证明,E11可用于鉴定组织切片中各种细胞上的CR1,以及定量红细胞和中性粒细胞上的CR1。发现正常个体的红细胞和中性粒细胞平均每个细胞分别结合610个和4.6×10⁴个¹²⁵I标记的E11分子。当通过免疫过氧化物酶染色在组织中观察E11时,明显含有最多CR1的细胞是树突状网状细胞和肾足细胞。E11反应性树突状网状细胞是滤泡性和弥漫性滤泡中心细胞肿瘤的特征。慢性淋巴细胞白血病(CLL)患者的淋巴细胞通常很少表达E11,这证实了早期研究中CLL细胞缺乏通过EAC1 - 3b玫瑰花结形成检测到的CR1活性。由于已证明正常B细胞在成熟的非常早期阶段就表达CR1,CLL细胞上CR1的缺失与通过免疫球蛋白表达定义的CLL细胞的未成熟性质不一致。
