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与吞噬溶酶体胞质表面相关的细胞内抗原。

Intracellular antigens associated with the cytoplasmic surface of phagolysosomes.

作者信息

Vaux D J, Gordon S

出版信息

J Cell Sci. 1985 Aug;77:109-27. doi: 10.1242/jcs.77.1.109.

Abstract

Monoclonal antibodies were prepared to study the cytoplasmic face of latex phagolysosomes isolated from thioglycollate-elicited mouse peritoneal macrophages. Phagolysosomes obtained by sucrose flotation contained latent beta-glucuronidase activity and tightly associated cellular proteins and glycoproteins. Fluorescence-activated cell sorter analysis, scanning and transmission electron microscopy showed that the particle preparation contained greater than 98% monomers and dimers, invested with a smooth layer of membrane and minimally contaminated with cytoplasmic adhesions. Sera for immunized rats bound preferentially to isolated phagolysosomes rather than intact cells and monoclonal antibodies PL-1 and PL-4 were isolated on this basis. Indirect fluorescent, radio- and peroxidase immunobinding assays with intact and methanol-permeabilized cells confirmed that antigens PL-1 and PL-4 were exclusively intracellular and that well-washed phagolysosomes bound both antibodies. These antigens were found in a variety of cells from several species and in macrophages not fed latex. Although the PL-1 antigen could not be immunoprecipitated, intracellular staining was characteristic of intermediate filament distribution, that is, it was in the form of a fine intersecting network, which collapsed, reversibly, in a rim round the nucleus upon treatment with colcemid. The staining pattern was undetectable in cells 1 h after adherence to a substratum, but gradually appeared after 6-12 h. The PL-4 antibody has been shown elsewhere to define a Ca2+-binding protein of approximately 20 000 molecular weight, which is phosphorylated during phagocytosis. This antibody stained stress fibres and revealed a widespread punctate distribution of antigen within cells at all stages after adhesion. The nature of the association between these intracellular antigens and phagolysosomes and their possible role in phagocytosis are not known.

摘要

制备单克隆抗体以研究从巯基乙酸盐诱导的小鼠腹腔巨噬细胞中分离出的乳胶吞噬溶酶体的胞质面。通过蔗糖浮选获得的吞噬溶酶体含有潜在的β-葡萄糖醛酸酶活性以及紧密结合的细胞蛋白和糖蛋白。荧光激活细胞分选分析、扫描和透射电子显微镜显示,颗粒制剂包含大于98%的单体和二聚体,外包一层光滑的膜,且极少被胞质粘连物污染。免疫大鼠的血清优先与分离出的吞噬溶酶体结合,而非完整细胞,并在此基础上分离出单克隆抗体PL-1和PL-4。对完整细胞和甲醇通透处理的细胞进行间接荧光、放射和过氧化物酶免疫结合试验,证实抗原PL-1和PL-4仅存在于细胞内,且充分洗涤后的吞噬溶酶体与两种抗体均结合。这些抗原存在于多个物种的多种细胞以及未摄取乳胶的巨噬细胞中。尽管PL-1抗原无法被免疫沉淀,但其细胞内染色具有中间丝分布的特征,即呈精细的交叉网络形式,在用秋水仙酰胺处理后,围绕细胞核的边缘会可逆性塌陷。在细胞贴壁于基质1小时后,这种染色模式无法检测到,但在6 - 12小时后逐渐出现。PL-4抗体在其他地方已被证明可识别一种分子量约为20000的钙结合蛋白,该蛋白在吞噬过程中会被磷酸化。这种抗体可使应力纤维染色,并显示出在细胞粘附后所有阶段抗原在细胞内广泛的点状分布。这些细胞内抗原与吞噬溶酶体之间的关联性质及其在吞噬作用中的可能作用尚不清楚。

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