Levi-Schaffer F, Austen K F, Caulfield J P, Hein A, Bloes W F, Stevens R L
J Immunol. 1985 Nov;135(5):3454-62.
Rat serosal heparin-containing mast cells (HP-MC) were maintained in vitro for as long as 30 days when co-cultured with mouse skin-derived 3T3 fibroblasts. In contrast, when the mast cells were cultured alone, on fibronectin-, gelatin-, or dermal-collagen-coated dishes, on acid and heat-killed fibroblasts in the presence or absence of 24 hr fibroblast-conditioned medium, or on a monolayer of mouse serosal macrophages, they failed to adhere to the dishes, released significant amounts of their histamine and lactate dehydrogenase, and stained with trypan blue, indicating a loss of viability. The rat serosal HP-MC cultured with the 3T3 fibroblasts became so adherent to the fibroblasts that the two cell types could be separated from one another only by trypsinization. The cultured HP-MC stained with both alcian blue and safranin and continued to synthesize proteoglycan at a rate comparable to that of freshly isolated cells. The 35S-labeled proteoglycan synthesized by these cultured cells, like that produced by freshly isolated rat serosal HP-MC, was a 750,000 to 1,000,000 m.w. proteoglycan containing only heparin glycosaminoglycans of 50,000 to 100,000 m.w. When HP-MC were cultured for 1 wk with the fibroblasts and were then incubated for 5 min with a 1/20 dilution of rabbit anti-rat IgE, they generated and released an average of 22 +/- 10 ng (mean +/- SD, n = 5) of prostaglandin D2 per 10(6) cells and exocytosed a higher net percentage of their total histamine content (44 +/- 11% [mean +/- SD, n = 8]) than did cells just isolated from the animal (6 +/- 4% [mean +/- SD, n = 4]). As assessed by electron microscopy, many of the cultured HP-MC resembled freshly isolated cells except that some secretory granules had fused with one another in some cells. Morphologically, after activation the cultured HP-MC underwent compound exocytosis like freshly isolated cells. These results demonstrate that the in vivo differentiated rat HP-MC maintain their histology, morphology, immunologic responsiveness, histamine content, and ability to synthesize heparin proteoglycan when co-cultured with living fibroblasts.
当与小鼠皮肤来源的3T3成纤维细胞共培养时,大鼠浆膜含肝素肥大细胞(HP - MC)可在体外维持长达30天。相比之下,当肥大细胞单独培养时,无论是在纤连蛋白、明胶或真皮胶原蛋白包被的培养皿上,还是在有或没有24小时成纤维细胞条件培养基的情况下与经酸处理和热灭活的成纤维细胞共培养,又或是在小鼠浆膜巨噬细胞单层上培养,它们都无法黏附在培养皿上,会释放大量组胺和乳酸脱氢酶,并用台盼蓝染色,表明细胞活力丧失。与3T3成纤维细胞共培养的大鼠浆膜HP - MC与成纤维细胞紧密黏附,以至于只有通过胰蛋白酶消化才能将这两种细胞类型分离。培养的HP - MC用阿尔辛蓝和番红染色,并继续以与新鲜分离细胞相当的速率合成蛋白聚糖。这些培养细胞合成的35S标记蛋白聚糖,与新鲜分离的大鼠浆膜HP - MC产生的蛋白聚糖一样,是一种分子量为750,000至1,000,000的蛋白聚糖,仅含有分子量为50,000至100,000的肝素糖胺聚糖。当HP - MC与成纤维细胞共培养1周,然后用兔抗大鼠IgE的1/20稀释液孵育5分钟时,每10(6)个细胞平均产生并释放22±10 ng(平均值±标准差,n = 5)的前列腺素D2,并且其组胺总含量的胞吐净百分比(44±11% [平均值±标准差,n = 8])高于刚从动物体内分离的细胞(6±4% [平均值±标准差,n = 4])。通过电子显微镜评估,许多培养的HP - MC与新鲜分离的细胞相似,只是在一些细胞中一些分泌颗粒相互融合。在形态上,激活后培养的HP - MC像新鲜分离的细胞一样经历复合胞吐作用。这些结果表明,体内分化的大鼠HP - MC与活的成纤维细胞共培养时,其组织学、形态学、免疫反应性、组胺含量以及合成肝素蛋白聚糖的能力得以维持。
