Chen A, Gaddipati S, Hong Y, Volkman D J, Peerschke E I, Ghebrehiwet B
Department of Medicine, State University of New York, Stony Brook 11794.
J Immunol. 1994 Aug 15;153(4):1430-40.
Although the receptor that binds to the collagen-like domain of human C1q (C1qR) is expressed on a wide variety of cell types, the presence or absence of this receptor on human T lymphocytes has been debatable. The current studies were undertaken to re-examine whether human T cells possess specific binding sites for C1q by using a combination of techniques, including radioligand binding studies, flow cytometric analysis, and epifluorescence imaging techniques. Radioligand binding studies indicate that both peripheral T cells and the cultured T cell line, MOLT4, bind 125I-labeled C1q in a specific and apparently saturable manner, reaching equilibrium within 30 min at 37 degrees C under conditions of subphysiologic (90 mM NaCl) ionic strength. Western blot analysis with anti-C1qR of membrane proteins derived from Raji and MOLT4 cells showed an apparent single band of approximately 60 kDa under nonreducing conditions. Furthermore, when peripheral blood T cells were stimulated with 12,-o-tetradecanoyl phorbol-13-ester acetate for 5 days at 37 degrees C and assessed by FACS for their ability to bind anti-C1qR, the mitogen-induced cells were found to bind 40 to 50% more than their unstimulated counterparts. In addition, both CD4+ and CD8+ T cells were found to bind anti-C1qR. When the cells were mitogen induced with either 12,-o-tetradecanoyl phorbol-13-ester acetate, Con A, or PWM for 48 h in the presence or absence of 50 micrograms/ml C1q then pulsed with 1 microCi [3H]thymidine for 16 h at 37 degrees C, proliferation was significantly inhibited (40 to 80%, n = 7) as assessed by reduced [3H]thymidine incorporation. Taken together, the data suggest that: 1) Human T cells express C1qR in which immunoblots reveal a 60-kDa single chain protein. 2) C1qR expression is up-regulated by mitogens that induce T cell proliferation. 3) The primary ligand, C1q, induces an antiproliferative signal, which suggests that the C1qR plays a role in T cell activation and proliferation. In addition, the data contribute to the characterization of C1qRs on cells in peripheral blood and indicate that all cells, with the exception of erythrocytes, bear functional C1q receptors.
尽管与人C1q胶原样结构域结合的受体(C1qR)在多种细胞类型上均有表达,但人T淋巴细胞上该受体的有无一直存在争议。目前的研究旨在通过结合放射性配体结合研究、流式细胞术分析和落射荧光成像技术等多种技术,重新检验人T细胞是否具有C1q的特异性结合位点。放射性配体结合研究表明,外周血T细胞和培养的T细胞系MOLT4均以特异性且明显可饱和的方式结合125I标记的C1q,在37℃、亚生理离子强度(90 mM NaCl)条件下30分钟内达到平衡。用抗C1qR对源自Raji和MOLT4细胞的膜蛋白进行蛋白质印迹分析,在非还原条件下显示出一条约60 kDa的明显单带。此外,当外周血T细胞在37℃用12 - O - 十四烷酰佛波醇 - 13 - 乙酸酯刺激5天,并通过流式细胞术评估其结合抗C1qR的能力时,发现有丝分裂原诱导的细胞比未刺激的细胞结合能力高40%至50%。另外,发现CD4 +和CD8 + T细胞均能结合抗C1qR。当细胞在有或无50微克/毫升C1q存在的情况下,用12 - O - 十四烷酰佛波醇 - 13 - 乙酸酯、刀豆蛋白A或美洲商陆丝裂原进行有丝分裂原诱导48小时,然后在37℃用1微居里[3H]胸苷脉冲标记16小时,通过[3H]胸苷掺入量减少评估,增殖受到显著抑制(40%至80%,n = 7)。综上所述,数据表明:1)人T细胞表达C1qR,免疫印迹显示为一种60 kDa的单链蛋白。2)C1qR的表达受诱导T细胞增殖的有丝分裂原上调。3)主要配体C1q诱导抗增殖信号,这表明C1qR在T细胞活化和增殖中起作用。此外,这些数据有助于对外周血细胞上的C1qR进行表征,并表明除红细胞外,所有细胞均带有功能性C1q受体。
