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采用一步法制备的三维打印阴离子交换整体柱对蛋白质的捕获和分离。

Demonstration of protein capture and separation using three-dimensional printed anion exchange monoliths fabricated in one-step.

机构信息

School of Engineering, Institute for Bioengineering, University of Edinburgh, Edinburgh, UK.

School of Biological Sciences, SynthSys & Institute of Molecular Plant Sciences, University of Edinburgh, Edinburgh, UK.

出版信息

J Sep Sci. 2021 Mar;44(6):1078-1088. doi: 10.1002/jssc.202000722. Epub 2020 Oct 26.

Abstract

Three-dimensional printing applications in separation science are currently limited by the lack of materials compatible with chromatographic operations and three-dimensional printing technologies. In this work, we propose a new material for Digital Light Processing printing to fabricate functional ion exchange monoliths in a single step. Through copolymerization of the bifunctional monomer [2-(acryloyloxy)ethyl] trimethylammonium chloride, monolithic structures with quaternary amine ligands were fabricated. The novel formulation was optimized in terms of protein binding and recovery, microporous structure, and its swelling susceptibility by increasing its cross-link density and employing cyclohexanol and dodecanol as pore forming agents. In static conditions, the material demonstrated a maximum binding capacity of 104.2 ± 10.6 mg/mL for bovine serum albumin, in line with commercially available materials. Its anion exchange behavior was validated by separating bovine serum albumin and myoglobin on a monolithic bed with Schoen gyroid morphology. The same column geometry was tested for the purification of C-phycocyanin from clarified as well as cell-laden Arthrospira platensis feedstocks. This represents the first demonstration of one-step printed stationary phases to capture proteins directly from solid-laden feedstocks. We believe that the material presented here represents a significant improvement towards implementation of three-dimensional printed chromatography media in the field of separation science.

摘要

目前,三维打印在分离科学中的应用受到缺乏与色谱操作和三维打印技术兼容的材料的限制。在这项工作中,我们提出了一种新的用于数字光处理打印的材料,以一步法制造功能离子交换整体柱。通过双功能单体[2-(丙烯酰氧基)乙基]三甲基氯化铵的共聚,制备了带有季铵配体的整体结构。通过增加交联密度并使用环己醇和十二醇作为致孔剂,对新型配方进行了优化,以提高蛋白质结合和回收、微孔结构及其溶胀敏感性。在静态条件下,该材料对牛血清白蛋白的最大结合容量为 104.2±10.6mg/mL,与市售材料相当。通过在具有肖恩翼形体形态的整体床层上分离牛血清白蛋白和肌红蛋白,验证了其阴离子交换行为。相同的柱几何形状也用于从澄清和含细胞的节旋藻进料中纯化 C-藻蓝蛋白。这是首次证明一步打印固定相可直接从固载进料中捕获蛋白质。我们相信,这里提出的材料代表了在分离科学领域实施三维打印色谱介质的重大进展。

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