A sensitive method to quantitate gangliosides of the gangliotetraose series directly on chromatograms using peroxidase conjugated cholera toxin.

L D Cambron, K C Leskawa
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引用次数: 9

Abstract

A method is described whereby ganglioside GM1 can be quantitated directly on thin-layer chromatograms using cholera toxin subunit B conjugated to horseradish peroxidase and visualized with chloronaphthol. Overlay and color development were performed after separating gangliosides on nano-TLC plates, and fixing with polyisobutylmethacrylate. Absolute quantitation was realized using a Shimadzu CS-9000 integrating spectrodensitometer, scanning at 580 nm. A correlation coefficient of 0.98 was obtained in a linear range of detection from 10(-11) to 10(-16) moles. Statistical analysis revealed good reproducibility and over 99% of the added gangliosides remained with the chromatogram during all overlay and washing procedures. By comparison, standard chemical visualization by resorcinol-HCl was linear in the nanomole range with a detection limit of only 10(-10) moles. Since the carbohydrate portion of gangliosides immobilized in this manner is susceptible to the action of enzymes including neuraminidase, this technique can be applied to all structures of the gangliotetraose series.

用过氧化物酶结合霍乱毒素在色谱上直接定量神经节四糖系列神经节苷的灵敏方法。
本文描述了一种方法,利用霍乱毒素亚基B与辣根过氧化物酶偶联,并用氯萘酚可视化,可以直接在薄层色谱上定量神经节苷脂GM1。在纳米薄层色谱板上分离神经节苷脂,用聚异丁基甲基丙烯酸酯固定后进行复盖和显色。采用岛津CS-9000积分光谱密度计进行绝对定量,扫描波长580 nm。在10(-11)~ 10(-16)摩尔的线性检测范围内,相关系数为0.98。统计分析显示了良好的再现性,在所有覆盖和洗涤过程中,超过99%的添加神经节苷脂保留在色谱中。相比之下,间苯二酚-盐酸标准化学可视化在纳米摩尔范围内呈线性,检出限仅为10(-10)摩尔。由于以这种方式固定的神经节苷脂的碳水化合物部分易受包括神经氨酸酶在内的酶的作用,因此该技术可应用于神经节四糖系列的所有结构。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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