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用于结合富含精氨酸蛋白质的亲和膜吸附剂。

Affinity membrane adsorbers for binding arginine-rich proteins.

作者信息

Chenette Heather C S, Welsh James M, Husson Scott M

机构信息

Department of Chemical and Biomolecular Engineering and Center for Advanced Engineering Fibers and Films, Clemson University, Clemson, SC 29634, USA.

出版信息

Sep Sci Technol. 2017;52(2):276-286. doi: 10.1080/01496395.2016.1206934. Epub 2016 Aug 17.

DOI:10.1080/01496395.2016.1206934
PMID:37830059
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC10569433/
Abstract

Delivering protein chemotherapeutics into cancer cells is a challenge. Fusing the protein to an arginine-rich cell-penetrating peptide offers a possible solution. The goal of this work was to develop an affinity membrane for purification of Arg-rich fusion proteins via capture chromatography. Membranes were prepared by grafting polymers bearing diethyl-4-aminobenzyl phosphonate (D4ABP) ligands from macroporous membrane supports. Incorporation of D4ABP was studied by infrared spectroscopy and energy dispersive spectroscopy. Protein binding capacities of 3 mg lysozyme/mL were measured. While further studies are required to evaluate binding kinetics and Arg-selectivity, achieving higher protein binding capacity is needed before investment in such studies.

摘要

将蛋白质类化疗药物递送至癌细胞是一项挑战。将蛋白质与富含精氨酸的细胞穿透肽融合提供了一种可能的解决方案。这项工作的目标是开发一种亲和膜,用于通过捕获色谱法纯化富含精氨酸的融合蛋白。通过将带有二乙基-4-氨基苄基膦酸酯(D4ABP)配体的聚合物接枝到大孔膜载体上来制备膜。通过红外光谱和能量色散光谱研究了D4ABP的掺入情况。测得蛋白质结合容量为3 mg溶菌酶/ mL。虽然需要进一步研究来评估结合动力学和精氨酸选择性,但在进行此类研究之前,需要实现更高的蛋白质结合容量。

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