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人单核细胞体外分化过程中糖胺聚糖生物合成的变化

Changes in glycosaminoglycan biosynthesis during differentiation in vitro of human monocytes.

作者信息

Kolset S O, Kjellén L, Seljelid R, Lindahl U

出版信息

Biochem J. 1983 Mar 15;210(3):661-7. doi: 10.1042/bj2100661.

Abstract

Monocytes isolated from human blood were maintained in vitro on plastic culture dishes. After 3-4 days, adherent cells displayed morphological changes previously attributed to differentiation of the cells into histiocytes. 35S-labelled glycosaminoglycans were isolated after incubation of the cells with inorganic [35S]sulphate. Polysaccharide recovered from the culture medium after labelling from day 0 to day 2 or from day 5 to day 7 in vitro was approximately 90% galactosaminoglycan (resistant to deamination by HNO2), irrespective of labelling period. Whereas day-0-2 material was extensively degraded to disaccharide on incubation with the bacterial eliminase chondroitinase AC, a significant portion, about 30%, of the day-5-7 material resisted degradation under the same conditions. The resistant portion was readily depolymerized by treatment with chondroitinase ABC and may be dermatan sulphate. Paper electrophoresis and paper chromatography of the disaccharides obtained by eliminase digestion identified the day-0-2 labelled galactosaminoglycan as chondroitin 4-sulphate. In contrast, the corresponding day-5-7 material yielded approximately 20% disulphated disaccharide, both on digestion with chondroitinase AC and on subsequent enzymic degradation of the chondroitinase AC-resistant fraction. Further treatment of the disulphated disaccharide with chondro-4-sulphatase and chondro-6-sulphatase indicated that both sulphate groups were located on the N-acetylgalactosamine residue. In accordance with these findings, the day-5-7 polysaccharide showed a higher negative charge density than the day-0-2 material on ion-exchange chromatography. It is concluded that the novel properties acquired by the monocyte during prolonged culturing on plastic include the ability to synthesize glycosaminoglycan(s) containing 4,6-disulphated N-acetylgalactosamine units.

摘要

从人血液中分离出的单核细胞在塑料培养皿中进行体外培养。3 - 4天后,贴壁细胞呈现出先前归因于细胞分化为组织细胞的形态变化。在用无机[35S]硫酸盐孵育细胞后,分离出35S标记的糖胺聚糖。无论标记期如何,在体外从第0天到第2天或从第5天到第7天标记后从培养基中回收的多糖约90%是半乳糖胺聚糖(对HNO2脱氨有抗性)。与细菌消除酶软骨素酶AC孵育时,第0 - 2天的物质被广泛降解为二糖,而在相同条件下,第5 - 7天的物质有相当一部分(约30%)抵抗降解。通过用软骨素酶ABC处理,抗性部分很容易解聚,可能是硫酸皮肤素。对消除酶消化得到的二糖进行纸电泳和纸色谱分析,确定第0 - 2天标记的半乳糖胺聚糖为硫酸软骨素4 - 硫酸酯。相比之下,相应的第5 - 7天的物质在用软骨素酶AC消化以及随后对软骨素酶AC抗性部分进行酶促降解时,均产生约20%的二硫酸化二糖。用软骨素4 - 硫酸酯酶和软骨素6 - 硫酸酯酶对二硫酸化二糖进行进一步处理表明,两个硫酸基团都位于N - 乙酰半乳糖胺残基上。根据这些发现,在塑料上长时间培养期间单核细胞获得的新特性包括合成含有4,6 - 二硫酸化N - 乙酰半乳糖胺单元的糖胺聚糖的能力。

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