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石墨化碳柱上糖肽和寡糖的高效液相色谱法

High-performance liquid chromatography of glycopeptides and oligosaccharides on graphitized carbon columns.

作者信息

Fan J Q, Kondo A, Kato I, Lee Y C

机构信息

Department of Biology, Johns Hopkins University, Baltimore, Maryland 21218.

出版信息

Anal Biochem. 1994 Jun;219(2):224-9. doi: 10.1006/abio.1994.1261.

Abstract

High-performance liquid chromatography of carbohydrate materials on graphitized carbon columns (GCC) has some advantages over other types of chromatography. Oligosaccharides and glycopeptides with few amino acids are barely retained on reversed-phase columns even under high salt or low pH conditions, but can be retained effectively on a graphitized carbon column. Moreover, elution of GCC requires concentrations of organic solvents lower than that required for normal-phase columns. The usefulness of graphitized carbon columns is exemplified by the following results: (i) Man9GlcNAc2 with only Asn or Asn-Phe (derived from soybean agglutinin) was not retained by a C18 reversed-phase column, but could be separated on a GCC with a gradient of 10-45% CH3CN in 30 min. (ii) Ribonuclease B glycopeptides obtained by Pronase digestion could be separated on GCC with a gradient of 10-30% CH3CN, but they were not retained on a C18 reversed-phase column even with water as eluent. (iii) Oligosaccharides released from ribonuclease B by endo-beta-N-acetylglucosaminidase were separated from each other and peptides on GCC with a linear gradient of 10 mM NH4OH to 10 mM NH4OH-12.5% CH3CN in 50 min at 70 degrees C. Silica-based columns do not allow such an alkaline eluent. (iv) Chito-oligosaccharides (DP 1-9) are well separated within 40 min on GCC with a gradient (10 mM NH4OH-10 mM NH4OH with 25% CH3CN) at 50 degrees C. Chito-oligosaccharides could not be separated by high-performance anion exchange columns such as Carbopac PA-1.

摘要

在石墨化碳柱(GCC)上对碳水化合物材料进行高效液相色谱分析比其他类型的色谱分析具有一些优势。即使在高盐或低pH条件下,含少量氨基酸的寡糖和糖肽在反相柱上几乎不保留,但在石墨化碳柱上能有效保留。此外,GCC洗脱所需的有机溶剂浓度低于正相柱所需的浓度。石墨化碳柱的实用性通过以下结果得以体现:(i)仅含天冬酰胺或天冬酰胺 - 苯丙氨酸(源自大豆凝集素)的Man9GlcNAc2不被C18反相柱保留,但可在GCC上于30分钟内用10 - 45% CH3CN梯度分离。(ii)经链霉蛋白酶消化得到的核糖核酸酶B糖肽可在GCC上用10 - 30% CH3CN梯度分离,但即使以水作为洗脱剂,它们也不被C18反相柱保留。(iii)通过内切β - N - 乙酰氨基葡萄糖苷酶从核糖核酸酶B释放的寡糖在GCC上彼此分离,并与肽分离,在70℃下于50分钟内用10 mM NH4OH至10 mM NH4OH - 12.5% CH3CN的线性梯度。基于硅胶的柱不允许使用这种碱性洗脱剂。(iv)壳寡糖(聚合度1 - 9)在50℃下于40分钟内在GCC上用梯度(10 mM NH4OH - 含25% CH3CN的10 mM NH4OH)良好分离。壳寡糖不能通过诸如Carbopac PA - 1的高效阴离子交换柱分离。

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