Kumarasuriyar Arjuna, Dombrowski Christian, Rider David A, Nurcombe Victor, Cool Simon M
Institute of Molecular and Cell Biology, Singapore, Singapore.
J Mol Histol. 2007 Oct;38(5):435-47. doi: 10.1007/s10735-007-9136-z. Epub 2007 Sep 21.
Several methods to alter cell surface glycosaminoglycan (GAG) expression have previously been described, including treatments with chlorate to reduce the addition of charged sulfate groups, xyloside compounds to displace GAGs from their core proteins, and GAG lyases, such as heparinase and chondroitinase, to release GAG fragments from the cell layer. While these methods are useful in identifying cellular mechanisms which are dependent on GAGs, they must be stringently validated to assess results in the appropriate context. To determine the most useful technique for the evaluation of GAG function in osteogenesis, MG-63 osteosarcoma cells were systematically treated with these agents and evaluated for changes in cell surface GAGs using a TAT-EGFP fusion protein. TAT, a protein transduction domain from the HIV-1 virus, requires cell surface GAGs to traverse cell membranes. The EGFP component provides a method to assess protein entry into cells in both qualitative and quantitative tests. Here, TAT-EGFP transduction analysis confirmed radiochemical and physiological data that chlorate effectively disrupts GAG expression. TAT-EGFP entry into cells was also inhibited by the exogenous application of commercial heparin and GAGs extracted from MG-63 cells as well as by the pre-treatment of cells with chondroitinase ABC. However, neither heparinase III treatment nor the addition of exogenous chondroitin-6-sulfate affected TAT-EGFP entry into cells. In addition, xyloside-beta-D-naphthol and xyloside-beta-D-cis/trans-decahydro-2-naphthol treatment could not induce significant phenotypic change in these cells, and the unaffected TAT-EGFP transduction confirmed that this was due to an inability to efficiently prime GAG synthesis. The use of TAT-EGFP is thus a useful technique to specifically evaluate cell surface GAG expression in a simple, quantifiable manner, and avoids the complications involved with conventional radiochemical assays or analytical chromatography.
先前已经描述了几种改变细胞表面糖胺聚糖(GAG)表达的方法,包括用氯酸盐处理以减少带电荷硫酸基团的添加、用木糖苷化合物从其核心蛋白上置换GAG,以及用GAG裂解酶,如肝素酶和软骨素酶,从细胞层释放GAG片段。虽然这些方法在识别依赖于GAG的细胞机制方面很有用,但必须进行严格验证以在适当的背景下评估结果。为了确定评估GAG在骨生成中功能的最有用技术,用这些试剂对MG-63骨肉瘤细胞进行系统处理,并使用TAT-EGFP融合蛋白评估细胞表面GAG的变化。TAT是来自HIV-1病毒的蛋白质转导结构域,需要细胞表面GAG才能穿过细胞膜。EGFP成分提供了一种在定性和定量测试中评估蛋白质进入细胞的方法。在这里,TAT-EGFP转导分析证实了放射化学和生理学数据,即氯酸盐有效地破坏了GAG表达。商业肝素和从MG-63细胞中提取的GAG的外源应用以及用软骨素酶ABC对细胞进行预处理也抑制了TAT-EGFP进入细胞。然而,肝素酶III处理和外源添加硫酸软骨素-6-硫酸盐均未影响TAT-EGFP进入细胞。此外,β-D-萘酚木糖苷和β-D-顺式/反式十氢-2-萘酚木糖苷处理不能在这些细胞中诱导明显的表型变化,未受影响的TAT-EGFP转导证实这是由于无法有效启动GAG合成。因此,使用TAT-EGFP是一种以简单、可量化的方式特异性评估细胞表面GAG表达的有用技术,并且避免了传统放射化学分析或分析色谱法所涉及的复杂性。
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