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采用双电解洗脱液产生法对溶菌多糖单加氧酶产生的氧化的纤维寡糖进行色谱分析。

Chromatographic analysis of oxidized cello-oligomers generated by lytic polysaccharide monooxygenases using dual electrolytic eluent generation.

机构信息

Norwegian University of Life Sciences (NMBU), Faculty of Chemistry, Biotechnology, and Food Science, P.O. Box 5003, Ås N-1432, Norway.

Norwegian University of Life Sciences (NMBU), Faculty of Chemistry, Biotechnology, and Food Science, P.O. Box 5003, Ås N-1432, Norway.

出版信息

J Chromatogr A. 2022 Jan 11;1662:462691. doi: 10.1016/j.chroma.2021.462691. Epub 2021 Nov 19.

Abstract

Research on oligosaccharides, including the complicated product mixtures generated by lytic polysaccharide monooxygenases (LPMOs), is growing at a rapid pace. LPMOs are gaining major interest, and the ability to efficiently and accurately separate and quantify their native and oxidized products chromatographically is essential in furthering our understanding of these oxidative enzymes. Here we present a novel set of methods based on dual electrolytic eluent generation, where the conventional sodium acetate/sodium hydroxide (NaOAc/NaOH) eluents in high-performance anion-exchange chromatography (HPAEC) are replaced by electrolytically-generated potassium methane sulfonate/potassium hydroxide (KMSA/KOH). The new methods separate all compounds of interest within 24-45 min and with high sensitivity; limits of detection and quantification were in the range of 0.0001-0.0032 mM and 0.0002-0.0096 mM, respectively. In addition, an average of 3.5 times improvement in analytical CV was obtained. This chromatographic platform overcomes drawbacks associated with manual preparation of eluents and offers simplified operation and rapid method optimization, with increased precision for less abundant LPMO-derived products.

摘要

寡糖的研究,包括溶菌多糖单加氧酶(LPMOs)产生的复杂产物混合物,正在迅速发展。LPMOs 引起了人们的极大兴趣,能够高效、准确地通过色谱法分离和定量其天然和氧化产物对于进一步了解这些氧化酶至关重要。在这里,我们提出了一套基于双电解洗脱液生成的新方法,其中取代了高效阴离子交换色谱(HPAEC)中传统的乙酸钠/氢氧化钠(NaOAc/NaOH)洗脱液,采用电解生成的甲烷磺酸钾/氢氧化钾(KMSA/KOH)。新方法在 24-45 分钟内分离出所有感兴趣的化合物,具有较高的灵敏度;检测限和定量限分别在 0.0001-0.0032 mM 和 0.0002-0.0096 mM 范围内。此外,分析 CV 的平均改善了 3.5 倍。这种色谱平台克服了手动制备洗脱液的缺点,提供了简化的操作和快速的方法优化,对于较少丰度的 LPMO 衍生产物具有更高的精度。

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