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纤连蛋白介导腹膜巨噬细胞对明胶包被乳胶颗粒的摄取。

Fibronectin-mediated uptake of gelatin-coated latex particles by peritoneal macrophages.

作者信息

Gudewicz P W, Molnar J, Lai M Z, Beezhold D W, Siefring G E, Credo R B, Lorand L

出版信息

J Cell Biol. 1980 Nov;87(2 Pt 1):427-33. doi: 10.1083/jcb.87.2.427.

Abstract

The present study demonstrates the ability of plasma fibronectin or cold-insoluble globulin (Clg) to promote the uptake of 125I-labeled, gelatin-coated latex beads (g-Ltx*) by monolayers of peritoneal macrophages (PM). The uptake of g-Ltx* by PM was enhanced by Clg in a concentration-dependent fashion and required the presence of heparin (10 U/ml) as an obligatory cofactor for maximal particle uptake. Treatment of PM monolayers with trypsin (1 mg/ml) for 15 min at 37 degrees C after particle uptake removed less than 15% of the radioactivity incorporated by the monolayers. However, a similar trypsin treatment of the monolayers before the addition of latex particles depressed Clg-dependent uptake by greater than 75%. Pretreatment of PM monolayers with inhibitors of glycolysis effectively reduced the Clg-dependent uptake of latex. Similarly, pretreatment of monolayers with either inhibitors of protein synthesis or agents that disrupt cytoskeletal elements also significantly depressed Clg-dependent particle uptake. Phagocytosis of g-Ltx* by PM in the presence of Clg and heparin was confirmed by electron microscopy. Finally, g-Ltx* could also be effectively opsonized with Clg at 37 degrees C before their addition to the monolayers. These studies suggest that the recognition of g-Ltx* in the presence of Clg required cell surface protein(s) and that subsequent phagocytosis of these particles by PM was energy dependent and required intact intracellular cytoskeleton elements. Thus, PM monolayers provide a suitable system for further studies on the function of Clg in the recognition and phagocytosis of gelatin-coated particles by phagocytic cells.

摘要

本研究证明了血浆纤连蛋白或冷不溶性球蛋白(Clg)能够促进腹膜巨噬细胞(PM)单层细胞对125I标记的、明胶包被的乳胶珠(g-Ltx*)的摄取。Clg以浓度依赖的方式增强了PM对g-Ltx的摄取,并且需要肝素(10 U/ml)作为最大颗粒摄取的必需辅助因子。在颗粒摄取后,于37℃用胰蛋白酶(1 mg/ml)处理PM单层细胞15分钟,去除的单层细胞摄取的放射性不到15%。然而,在添加乳胶颗粒之前,对单层细胞进行类似的胰蛋白酶处理可使Clg依赖的摄取降低超过75%。用糖酵解抑制剂预处理PM单层细胞可有效降低Clg依赖的乳胶摄取。同样,用蛋白质合成抑制剂或破坏细胞骨架成分的试剂预处理单层细胞也显著降低了Clg依赖的颗粒摄取。通过电子显微镜证实了在Clg和肝素存在下PM对g-Ltx的吞噬作用。最后,在将g-Ltx添加到单层细胞之前,也可在37℃用Clg有效地对其进行调理。这些研究表明,在Clg存在下对g-Ltx的识别需要细胞表面蛋白,并且随后PM对这些颗粒的吞噬作用是能量依赖的,并且需要完整的细胞内细胞骨架成分。因此,PM单层细胞为进一步研究Clg在吞噬细胞识别和吞噬明胶包被颗粒中的功能提供了一个合适的系统。

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