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蛋白聚糖合成抑制对培养的大鼠雪旺细胞分化的影响。

Effects of inhibition of proteoglycan synthesis on the differentiation of cultured rat Schwann cells.

作者信息

Carey D J, Rafferty C M, Todd M S

出版信息

J Cell Biol. 1987 Aug;105(2):1013-21. doi: 10.1083/jcb.105.2.1013.

Abstract

Schwann cells synthesize two heparan sulfate proteoglycans, one that is a component of the Schwann cell basement membrane and a smaller one that is an integral component of the Schwann cell plasma membrane. To determine the functions of these molecules, Schwann cell-nerve cell cultures were grown in medium containing a specific inhibitor of proteoglycan biosynthesis, 4-methylumbelliferyl-beta-D-xyloside. Treatment with 1 mM beta-D-xyloside caused a 90% reduction in the accumulation of 35SO4-labeled proteoglycans in the cell layer of the cultures. Gel filtration analysis revealed that both the basement membrane and plasma membrane proteoglycans were affected. Inhibition of proteoglycan biosynthesis was accompanied by an inhibition of laminin deposition into extracellular matrix as determined by immunostaining of cultures and by immunoblotting of cell-associated proteins. This occurred even though there was no decrease in the amount of laminin detected in the medium of beta-D-xyloside-treated cultures. Deposition of collagen type IV was similarly affected. In addition, there was no myelin produced in beta-D-xyloside treated cultures. However, when beta-xyloside-treated cultures were supplied with exogenous basement membrane, Schwann cells produced numerous myelin segments. These results indicate that Schwann cell proteoglycans play an essential role in basement membrane assembly, and that the integral plasma membrane proteoglycan is not required for the basement membrane to exert its effects on Schwann cell differentiation.

摘要

施万细胞合成两种硫酸乙酰肝素蛋白聚糖,一种是施万细胞基底膜的组成成分,另一种较小的是施万细胞质膜的固有成分。为了确定这些分子的功能,将施万细胞 - 神经细胞培养物在含有蛋白聚糖生物合成特异性抑制剂4 - 甲基伞形酮基 - β - D - 木糖苷的培养基中培养。用1 mM β - D - 木糖苷处理导致培养物细胞层中35SO4标记的蛋白聚糖积累减少90%。凝胶过滤分析表明基底膜和质膜蛋白聚糖均受到影响。通过培养物的免疫染色和细胞相关蛋白的免疫印迹测定,蛋白聚糖生物合成的抑制伴随着层粘连蛋白沉积到细胞外基质中的抑制。即使在β - D - 木糖苷处理的培养物的培养基中检测到的层粘连蛋白量没有减少,这种情况仍会发生。IV型胶原的沉积也受到类似影响。此外,在β - D - 木糖苷处理的培养物中没有产生髓磷脂。然而,当向β - 木糖苷处理的培养物提供外源性基底膜时,施万细胞产生了大量髓鞘节段。这些结果表明施万细胞蛋白聚糖在基底膜组装中起重要作用,并且基底膜对施万细胞分化发挥作用并不需要固有质膜蛋白聚糖。

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