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宽孔全多孔混合模式辛基/吡啶键合硅胶材料,具有 pH 依赖性表面电荷反转,用于蛋白质的高性能疏水电荷诱导色谱。

Wide-pore fully porous mixed-mode octyl/pyridyl-bonded silica material with pH-dependent surface charge reversal for high-performance hydrophobic charge-induction chromatography of proteins.

机构信息

Institute of Pharmaceutical Sciences, Pharmaceutical (Bio-)Analysis, University of Tübingen, Auf der Morgenstelle 8, Tübingen 72076, Germany.

Institute of Organic Chemistry, University of Tübingen, Auf der Morgenstelle 18, Tübingen 72076, Germany.

出版信息

J Chromatogr A. 2024 Nov 22;1737:465429. doi: 10.1016/j.chroma.2024.465429. Epub 2024 Oct 9.

DOI:10.1016/j.chroma.2024.465429
PMID:39426258
Abstract

In an attempt to overcome silanophilic interactions like observed on popular reversed-phase butyl‑bonded silica stationary phases in protein HPLC, a mixed-mode stationary phase based on wide pore silica (3 µm, 300 Å) was prepared by co-immobilization of octyl and 2-pyridylethyl ligands. The surface modification was performed by a new approach using synthesized functional silatranes of the above ligands and prewetted silica. It allowed to generate a dense polymeric siloxane layer on the silica surface. Butyl-bonded silica and octyl/3-aminopropyl-bonded mixed-mode silica phases were prepared for comparison. The modified silicas were subsequently characterized by elemental analysis regarding ligand densities, by solid-state Si and C cross polarization/magic angle spinning nuclear magnetic resonance spectroscopy for confirming the surface-bonded structure, and by pH-dependent ζ-potential measurements via electrophoretic light scattering providing net surface charge information at distinct pH values. While the classical butyl‑bonded stationary phase revealed negative ζ-potential over the entire pH range investigated (pH 3.5-9.5) due to residual silanols and the mixed-mode octyl/3-aminopropyl-bonded silica positive ζ-potential over the entire pH range, pH-dependent charge reversal was observed at approximately pH 5.5 for the octyl/pyridyl-bonded stationary phase. Then, a test set of proteins differing in hydrophobicities and isoelectric points was employed to evaluate the retention characteristics of all three synthesized stationary phases over the pH range of 3 to 7.5 by acetonitrile-gradient elution reversed-phase HPLC. Under acidic conditions (pH 3) the mixed-mode phases octyl/pyridyl-silica and octyl/aminopropyl-silica showed reduced retention and improved peak shapes due to repulsive interactions preventing silanophilic interactions, while protein separations by their hydrophobicities were achieved (repulsive charge-assisted protein RPLC). Finally, the prepared novel mixed-mode octyl/pyridyl-bonded stationary phase was evaluated in hydrophobic charge induction chromatography mode for protein separation of the same test set. Instead of an organic modifier gradient, elution was enforced by a pH gradient from almost neutral to acidic pH at constant organic modifier content of 10 %. This chromatographic mode showed orthogonal retention characteristics and reversed elution order compared to above organic gradient RP-HPLC. In addition, significantly less organic solvent was used under these conditions, classifying it as a green protein LC technology.

摘要

为了克服在蛋白质 HPLC 中常用的反相丁基键合硅胶固定相上观察到的硅烷亲合相互作用,通过共固定化辛基和 2-吡啶乙基配体,制备了一种基于大孔硅胶(3 µm,300 Å)的混合模式固定相。表面修饰是通过使用上述配体的合成功能硅烷三醇和预湿硅胶的新方法进行的。它允许在硅胶表面上生成致密的聚合物硅氧烷层。还制备了丁基键合硅胶和辛基/3-氨丙基键合混合模式硅胶相进行比较。通过元素分析、固态 Si 和 C 交叉极化/魔角旋转核磁共振光谱对修饰后的硅胶进行了配体密度的表征,通过电泳光散射进行 pH 依赖性 ζ-电势测量,提供了在不同 pH 值下的净表面电荷信息。虽然经典的丁基键合固定相由于残留的硅醇而在整个研究的 pH 范围内(pH 3.5-9.5)呈现负 ζ-电势,而混合模式的辛基/3-氨丙基键合硅胶在整个 pH 范围内呈现正 ζ-电势,但在 pH 约 5.5 时观察到辛基/吡啶基键合固定相的 pH 依赖性电荷反转。然后,使用一组疏水性和等电点不同的蛋白质来评估所有三种合成固定相在 pH 3 到 7.5 范围内的保留特性,通过乙腈梯度洗脱反相 HPLC。在酸性条件下(pH 3),由于排斥相互作用阻止了硅烷亲合相互作用,混合模式相辛基/吡啶硅胶和辛基/氨基丙基硅胶显示出降低的保留和改善的峰形,而通过疏水性实现了蛋白质分离(排斥电荷辅助蛋白质 RPLC)。最后,在疏水性电荷感应色谱模式下评估了制备的新型混合模式辛基/吡啶键合固定相用于相同测试集的蛋白质分离。与有机改性剂梯度洗脱不同,通过在恒定有机改性剂含量为 10%的情况下从近中性到酸性 pH 的 pH 梯度强制洗脱。与上述有机梯度 RP-HPLC 相比,这种色谱模式显示出正交保留特性和相反的洗脱顺序。此外,在这些条件下使用的有机溶剂显著减少,将其归类为绿色蛋白质 LC 技术。

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