人单核吞噬细胞上β-葡聚糖受体的分离与鉴定
Isolation and characterization of beta-glucan receptors on human mononuclear phagocytes.
作者信息
Czop J K, Kay J
机构信息
Department of Medicine, Harvard Medical School, Boston, Massachusetts 02115.
出版信息
J Exp Med. 1991 Jun 1;173(6):1511-20. doi: 10.1084/jem.173.6.1511.
beta-glucan receptors, with ligand specificity for yeast and fungal carbohydrate polymers, have been studied as phagocytic receptors of human monocytes. To characterize their structure, binding studies were carried out with human U937 cells and a rabbit IgG anti-Id that recognizes epitopes on monocyte beta-glucan receptors. Unstimulated U937 cells specifically bound large amounts of the anti-Id, but almost none of the control anti-isotype. At saturation, the number of anti-Id molecules bound per U937 cell was 2.6 x 10(6) with an apparent Ka of 1.9 x 10(7) M-1. Immunoprecipitates from detergent lysates of surface-radioiodinated U937 cells contained only two membrane proteins with antigenic specificity for the anti-Id, one having a mol wt of 180 kD and the other 160 kD. Both proteins were disulfide-linked and presented, after reduction, as five polypeptides of 95, 88, 60, 27, and 20 kD. Detergent lysates of unlabeled U937 cells, purified by affinity chromatography on anti-Id-Sepharose, yielded the same two nonreduced proteins and five reduction products in slab gels stained with Coomassie blue. In Western blots probed with the anti-Id, the most immunoreactive nonreduced and reduced affinity-purified products were the 160 and 20 kD molecules, respectively. Immunoblots of two-dimensional gels showed the 180 and 160 kD proteins to express a common epitope through disulfide linkage to the 20 kD polypeptide. By immunoblot analysis, U937 cell glucan-binding proteins from detergent lysates contained two cell proteins antigenic for the anti-Id that were indistinguishable from affinity-purified molecules in size and subunit composition. Studies of affinity-purified proteins from detergent lysed human monocytes were characterized by immunoblot analysis and found to be identical to U937 cell beta-glucan receptors. They consisted of two disulfide-linked proteins, with mol wt of 180 and 160 kD, and had in common a 20 kD polypeptide with the anti-Id epitope.
β-葡聚糖受体对酵母和真菌碳水化合物聚合物具有配体特异性,已被作为人类单核细胞的吞噬受体进行研究。为了表征其结构,使用人U937细胞和识别单核细胞β-葡聚糖受体表位的兔IgG抗独特型抗体进行了结合研究。未刺激的U937细胞特异性结合大量的抗独特型抗体,但几乎不结合对照抗同种型抗体。在饱和状态下,每个U937细胞结合的抗独特型抗体分子数为2.6×10⁶,表观解离常数为1.9×10⁷M⁻¹。来自表面放射性碘化U937细胞去污剂裂解物的免疫沉淀物仅包含两种对抗独特型抗体具有抗原特异性的膜蛋白,一种分子量为180kD,另一种为160kD。两种蛋白通过二硫键连接,还原后呈现为95、88、60、27和20kD的五种多肽。未标记U937细胞的去污剂裂解物通过抗独特型抗体-琼脂糖亲和层析纯化,在考马斯亮蓝染色的平板凝胶中产生相同的两种非还原蛋白和五种还原产物。在用抗独特型抗体探测的Western印迹中,免疫反应性最强的非还原和还原亲和纯化产物分别是160kD和20kD分子。二维凝胶的免疫印迹显示180kD和160kD蛋白通过与20kD多肽的二硫键连接表达共同表位。通过免疫印迹分析,来自去污剂裂解物的U937细胞葡聚糖结合蛋白包含两种对抗独特型抗体具有抗原性的细胞蛋白,其大小和亚基组成与亲和纯化分子无法区分。对来自去污剂裂解的人类单核细胞的亲和纯化蛋白的研究通过免疫印迹分析进行表征,发现与U937细胞β-葡聚糖受体相同。它们由两种通过二硫键连接的蛋白组成,分子量分别为180kD和160kD,并共同具有带有抗独特型抗体表位的20kD多肽。
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