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Sulphation by cultured cells. Cysteine cysteinesulphinic acid and sulphite as sources for proteoglycan sulphate.

机译:培养细胞的硫化。半胱氨酸半胱氨酸磺酸和亚硫酸盐是蛋白多糖硫酸盐的来源。

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摘要

Bovine aortic smooth-muscle cells, bovine aortic endothelial cells, and IMR-90 human embryonic lung fibroblasts were tested to determine their ability to use cysteine or cysteine metabolites as a source of sulphate (SO4). Cells were incubated in SO4-depleted medium containing [3H]glucosamine plus 0.2 mM-cystine, 0.3 mM-cysteinesulphinic acid or 0.3 mM-sulphite (SO3). The [3H]chondroitin sulphate produced by the different cells was found to vary considerably in degree of sulphation under these conditions. One line of smooth-muscle cells utilized cysteine effectively as a SO4 source and thus produced chondroitin sulphate which was highly sulphated. IMR-90 fibroblasts produced partly sulphated chondroitin sulphate under these conditions, while another smooth-muscle cell line could not utilize cysteine, but could utilize cysteinesulphinic acid as a partial SO4 source. In contrast with the above cells, endothelial cells could not use cysteine or cysteinesulphinic acid as a source of SO4 and produced chondroitin with almost no SO4. All of the cells were able to utilize SO3. Incubation of the cells in the SO4-depleted medium containing [35S]cysteine confirmed that only the first line of smooth-muscle cells could convert significant amounts of [35S]cysteine to 35SO4. Furthermore, the addition of 0.4 mM inorganic SO4 did not inhibit the production of SO4 from cysteine by these cells.
机译:测试了牛主动脉平滑肌细胞,牛主动脉内皮细胞和IMR-90人胚肺成纤维细胞,以确定它们使用半胱氨酸或半胱氨酸代谢物作为硫酸盐(SO4)来源的能力。将细胞在含有[3H]葡糖胺加0.2 mM-胱氨酸,0.3 mM-半胱氨酸磺酸或0.3 mM-亚硫酸盐(SO3)的SO4耗尽培养基中孵育。发现在这些条件下,由不同细胞产生的[3H]软骨素硫酸盐的硫酸盐度变化很大。一条平滑肌细胞系有效地利用了半胱氨酸作为SO4来源,因此产生了高度硫酸化的软骨素硫酸盐。在这些条件下,IMR-90成纤维细胞产生部分硫酸化的硫酸软骨素,而另一条平滑肌细胞系不能利用半胱氨酸,但可以利用半胱氨酸作为部分SO4来源。与上述细胞相反,内皮细胞不能使用半胱氨酸或半胱氨酸磺酸作为SO 4的来源,而产生的软骨素几乎没有SO 4。所有的细胞都能够利用SO3。将细胞在含有[35S]半胱氨酸的SO4耗尽培养基中孵育,确认只有第一条平滑肌细胞才能将大量[35S]半胱氨酸转化为35SO4。此外,添加0.4 mM无机SO4不会抑制这些细胞从半胱氨酸生产SO4。

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