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巨噬细胞外膜蛋白的鉴定及其在细胞黏附中的可能作用。

Identification of macrophage external membrane proteins and their possible role in cell adhesion.

作者信息

Pearlstein E, Dienstman S R, Defendi V

出版信息

J Cell Biol. 1978 Oct;79(1):263-7. doi: 10.1083/jcb.79.1.263.

Abstract

Starch-activated mouse peritoneal macrophages (STpMAC) plated on plastic demonstrate the adhesive properties typical for activated pMAC: attaching as round cells and, within 15 min, spreading out with marginal membrane ruffles. These attached STpMAC were labeled by lactoperoxidase-catalysed 125I surface iodination, sodium dodecyl-sulfate-lysed, and the lysates electrophoresed on polyacrylamide gels which were examined by autoradiography. The STpMAC morphological phenotype correlates with the labeling of a particular protein (195,000, estimated mol wt). Normal pMAC (NpMAC), from unstimulated mice, do not spread and do not display the 195,000 band. Both pMAC band patterns, including the 195,000 band, are relatively resistant to trypsin digestion, as is pMAC adhesion itself trypsin-resistant. Neither class of pMAC exhibits fibronectin (Cell Adhesion Factor, LETS protein) which is a component in the adhesive matrix of cells forming trypsin-sensitive monolayers. When pMAC are tested against antifibronectin antibody, these cells do not give immunofluorescent staining. In summary, two functions in pMAC adhesion, enzyme resistance and the ability to spread, appear related to molecular properties distinctive for pMAC surface protein.

摘要

接种在塑料培养皿上的淀粉激活的小鼠腹腔巨噬细胞(STpMAC)表现出激活的腹腔巨噬细胞(pMAC)典型的黏附特性:以圆形细胞形式附着,并在15分钟内展开,边缘有膜皱褶。这些附着的STpMAC通过乳过氧化物酶催化的125I表面碘化进行标记,经十二烷基硫酸钠裂解,裂解物在聚丙烯酰胺凝胶上进行电泳,然后通过放射自显影进行检测。STpMAC的形态表型与一种特定蛋白质(估计分子量为195,000)的标记相关。来自未受刺激小鼠的正常pMAC(NpMAC)不会展开,也不会显示出195,000的条带。两种pMAC的条带模式,包括195,000的条带,对胰蛋白酶消化相对具有抗性,就像pMAC的黏附本身对胰蛋白酶具有抗性一样。这两类pMAC均未表现出纤连蛋白(细胞黏附因子,LETS蛋白),而纤连蛋白是形成对胰蛋白酶敏感单层的细胞黏附基质的一个成分。当用抗纤连蛋白抗体检测pMAC时,这些细胞不会产生免疫荧光染色。总之,pMAC黏附中的两种功能,即酶抗性和展开能力,似乎与pMAC表面蛋白独特的分子特性有关。

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Fibronectin is produced by human macrophages.纤连蛋白由人类巨噬细胞产生。
J Exp Med. 1980 Mar 1;151(3):602-13. doi: 10.1084/jem.151.3.602.

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