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通过柱后络合滴定的高效液相色谱法对二磷酸肌醇磷酸酯进行合成及非放射性微量分析。

Synthesis and nonradioactive micro-analysis of diphosphoinositol phosphates by HPLC with postcolumn complexometry.

作者信息

Lin Hongying, Lindner Karsten, Mayr Georg W

机构信息

Institut für Biochemie und Molekularbiologie I: Zelluläre Signaltransduktion, Universitätsklinikum Hamburg-Eppendorf, Hamburg, Germany.

出版信息

Methods Mol Biol. 2010;645:103-22. doi: 10.1007/978-1-60327-175-2_7.

Abstract

A nonradioactive high-performance anion-exchange chromatographic method based on MDD-HPLC (Mayr Biochem. J. 254:585-591, 1988) was developed for the separation of inositol hexakisphosphate (InsP(6), phytic acid) and most isomers of pyrophosphorylated inositol phosphates, such as diphosphoinositol pentakisphosphate (PPInsP(5) or InsP(7)) and bis-diphosphoinositol tetrakisphosphate (bisPPInsP(4) or InsP(8)). With an acidic elution, the anion-exchange separation led to the resolution of four separable PPInsP(5) isomers (including pairs of enantiomers) into three peaks and of nine separable bisPPInsP(4) isomers into nine peaks. The whole separation procedure was completed within 20-36 min after optimization. Reference standards of all bisPPInsP(4) isomers were generated by a nonenzymatic shotgun synthesis from InsP(6). Hereby, the phosphorylation was brought about nonenzymatically when concentrated InsP(6) bound to the solid surface of anion-exchange beads was incubated with creatine phosphate under optimal pH conditions. From the mixture of pyrophosphorylated InsP(6) derivatives containing all theoretically possible isomers of PPInsP(5), bisPPInsP(4), and also some isomers of trisPPInsP(3), isomers were separated by anion-exchange chromatography and fractions served as reference standards of bisPPInsP(4) isomers for further investigation. Their isomeric nature could be partly assigned by comparison with position specifically synthesized or NMR-characterized purified protozoan reference compounds and partly by limited hydrolysis to PPInsP(5) isomers. By applying this nonradioactive analysis technique to cellular studies, the isomeric nature of the major bisPPInsP(4) in mammalian cells could be identified without the need to obtain sufficient material for NMR analysis.

摘要

基于MDD-HPLC(迈尔生物化学杂志,第254卷,第585 - 591页,1988年)开发了一种非放射性高效阴离子交换色谱法,用于分离肌醇六磷酸(InsP(6),植酸)和焦磷酸化肌醇磷酸的大多数异构体,如二磷酸肌醇五磷酸(PPInsP(5)或InsP(7))和双二磷酸肌醇四磷酸(双PPInsP(4)或InsP(8))。通过酸性洗脱,阴离子交换分离将四种可分离的PPInsP(5)异构体(包括对映体对)分离为三个峰,将九种可分离的双PPInsP(4)异构体分离为九个峰。优化后,整个分离过程在20 - 36分钟内完成。所有双PPInsP(4)异构体的参考标准品通过从InsP(6)进行非酶随机合成产生。在此过程中,当结合到阴离子交换珠固体表面的浓缩InsP(6)在最佳pH条件下与磷酸肌酸孵育时,非酶促实现磷酸化。从含有PPInsP(5)、双PPInsP(4)所有理论上可能的异构体以及一些三磷酸肌醇三磷酸(trisPPInsP(3))异构体的焦磷酸化InsP(6)衍生物混合物中,通过阴离子交换色谱法分离异构体,各馏分用作双PPInsP(4)异构体的参考标准品以供进一步研究。通过与位置特异性合成或经NMR表征的纯化原生动物参考化合物比较,以及部分通过有限水解为PPInsP(5)异构体,可部分确定它们的异构体性质。通过将这种非放射性分析技术应用于细胞研究,无需获得足够用于NMR分析的材料即可鉴定哺乳动物细胞中主要双PPInsP(4)的异构体性质。

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