首页> 外文OA文献 >Fibroblasts that proliferate near denervated synaptic sites in skeletal muscle synthesize the adhesive molecules tenascin(J1), N-CAM, fibronectin, and a heparan sulfate proteoglycan
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Fibroblasts that proliferate near denervated synaptic sites in skeletal muscle synthesize the adhesive molecules tenascin(J1), N-CAM, fibronectin, and a heparan sulfate proteoglycan

机译:在骨骼肌中神经支配的突触位点附近增殖的成纤维细胞合成了黏附分子Tenascin(J1),N-CAM,纤连蛋白和硫酸乙酰肝素蛋白聚糖

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摘要

Four adhesive molecules, tenascin(J1), N-CAM, fibronectin, and a heparan sulfate proteoglycan, accumulate in interstitial spaces near synaptic sites after denervation of rat skeletal muscle (Sanes, J. R., M. Schachner, and J. Covault. 1986. J. Cell Biol. 102:420-431). We have now asked which cells synthesize these molecules, and how this synthesis is regulated. Electron microscopy revealed that mononucleated cells selectively accumulate in perisynaptic interstitial spaces beginning 2 d after denervation. These cells were identified as fibroblasts by ultrastructural and immunohistochemical criteria; [3H]thymidine autoradiography revealed that their accumulation results from local proliferation. Electron microscopic immunohistochemistry demonstrated that N-CAM is associated with the surface of the fibroblasts, while tenascin(J1) is associated with collagen fibers that abut fibroblasts. Using immunofluorescence and immunoprecipitation methods, we found that fibroblasts isolated from perisynaptic regions of denervated muscle synthesize N-CAM, tenascin(J1), fibronectin, and a heparan sulfate proteoglycan in vitro. Thus, fibroblasts that selectively proliferate in interstitial spaces near synaptic sites are likely to be the cellular source of the interstitial deposits of adhesive molecules in denervated muscle. To elucidate factors that might regulate the accumulation of these molecules in vivo, we analyzed the expression of tenascin(J1) and fibronectin by cultured fibroblasts. Fibroblasts from synapse-free regions of denervated muscle, as well as skin, lung, and 3T3 fibroblasts accumulate high levels of tenascin(J1) and fibronectin in culture, showing that perisynaptic fibroblasts are not unique in this regard. However, when they are first placed in culture, fibroblasts from denervated muscle bear more tenascin(J1) than fibroblasts from innervated muscle, indicating that expression of this molecule by fibroblasts is regulated by the muscle's state of innervation; this difference is no longer apparent after a few days in culture. In 3T3 cells, accumulation of tenascin(J1) is high in proliferating cultures, depressed in confluent cultures, and reactivated in cells stimulated to proliferate by replating at low density or by wounding a confluent monolayer. Thus, synthesis of tenascin(J1) is regulated in parallel with mitotic activity. In contrast, levels of fibronectin, which increase less dramatically after denervation in vivo, are similar in fibroblasts from innervated and denervated muscle and in proliferating and quiescent 3T3 cells.(ABSTRACT TRUNCATED AT 400 WORDS)
机译:大鼠骨骼肌失神经后,四个黏附分子Tenascin(J1),N-CAM,纤连蛋白和硫酸乙酰肝素蛋白聚糖积聚在突触部位附近的间隙中(Sanes,JR,M.Schachner和J.Covault.1986。 J.Cell Biol.102:420-431)。现在,我们询问了哪些细胞合成这些分子,以及如何调节这种合成。电子显微镜检查显示,去神经后2 d开始,单核细胞选择性地聚集在突触周间隙中。通过超微结构和免疫组织化学标准将这些细胞鉴定为成纤维细胞。 [3H]胸苷放射自显影显示其积累是局部增殖的结果。电子显微镜免疫组织化学表明,N-CAM与成纤维细胞表面有关,而腱生蛋白(J1)与邻接成纤维细胞的胶原纤维有关。使用免疫荧光和免疫沉淀方法,我们发现从神经支配的神经突触周围区域分离的成纤维细胞在体外合成了N-CAM,腱糖蛋白(J1),纤连蛋白和硫酸乙酰肝素蛋白聚糖。因此,在突触部位附近的间隙中选择性增殖的成纤维细胞很可能是失神经肌肉中粘附分子间隙沉积的细胞来源。为了阐明可能调节这些分子在体内积累的因素,我们分析了培养的成纤维细胞中腱生蛋白(J1)和纤连蛋白的表达。来自无神经支配的无突触区域的成纤维细胞以及皮肤,肺和3T3成纤维细胞在培养物中积累高水平的腱生蛋白(J1)和纤连蛋白,这表明突触周围成纤维细胞在这方面不是唯一的。然而,当它们首次被放置在培养物中时,来自神经支配的肌肉的成纤维细胞比来自神经支配的肌肉的成纤维细胞具有更多的腱生蛋白(J1),这表明由纤维母细胞表达的该分子受肌肉神经支配状态的调节。经过几天的培养,这种差异不再明显。在3T3细胞中,腱生蛋白(J1)在增殖培养物中的蓄积高,在融合培养物中抑制,并在低密度下铺板或融合的单层伤口刺激增殖的细胞中重新活化。因此,腱生蛋白(J1)的合成与有丝分裂活性并行调节。相比之下,体内神经支配后纤连蛋白的水平增加不那么剧烈,而神经支配和神经支配的肌肉中的成纤维细胞以及增殖和静止的3T3细胞中的纤连蛋白水平相似(摘要截短了400字)。

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