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通过新型冷冻凝胶化方法将纳米刺整合到疏水性冷冻凝胶的结构中:质粒 DNA 纯化的替代吸附剂。

Nanospines incorporation into the structure of the hydrophobic cryogels via novel cryogelation method: an alternative sorbent for plasmid DNA purification.

机构信息

Hacettepe University, Department of Chemistry, 06381, Beytepe, Ankara, Turkey.

出版信息

Colloids Surf B Biointerfaces. 2013 Feb 1;102:243-50. doi: 10.1016/j.colsurfb.2012.08.020. Epub 2012 Aug 28.

DOI:10.1016/j.colsurfb.2012.08.020
PMID:23006565
Abstract

In this study, it was aimed to prepare hydrophobic cryogels for plasmid DNA (pDNA) purification from Escherichia coli lysate. The hydrophobicity was achieved by incorporating a hydrophobic ligand, N-methacryloyl-(L)-phenylalanine (MAPA), into the cryogel backbone. In addition to the conventional cryogelation process, freeze-drying step was included to create nanospines. Three different cryogels {poly(2-hydoxyethyl methacrylate-N-methacryloyl-L-phenylalanine)-freeze dried, [P(HEMA-MAPA)-FD]; poly(2-hydoxyethyl methacrylate-N-methacryloyl-L-phenylalanine, [P(HEMA-MAPA)] and poly(2-hydoxyethyl methacrylate)-freeze dried, [P(HEMA)-FD]} were prepared, characterized, and used for DNA (salmon sperm DNA) adsorption studies from aqueous solution. The specific surface areas of cryogels were determined to be 21.4 m(2)/g for P(HEMA)-FD, 17.65 m(2)/g for P(HEMA-MAPA) and 36.0 m(2)/g for P(HEMA-MAPA)-FD. The parameters affecting adsorption such as temperature, initial DNA concentration, salt type and concentration were examined in continuous mode. The maximum adsorption capacities were observed as 45.31 mg DNA/g, 27.08 mg DNA/g and 1.81 mg DNA/g for P(HEMA-MAPA)-FD, P(HEMA-MAPA) and P(HEMA)-FD, respectively. Desorption process was performed using acetate buffer (pH 5.50) without salt. First, pDNA was isolated from E. coli lysate and the purity of pDNA was then determined by agarose gel electrophoresis. Finally, the chromatographic performance of P(HEMA-MAPA)-FD cryogel for pDNA purification was tested in FPLC. The resolution (R(s)) was 2.84, and the specific selectivity for pDNA was 237.5-folds greater than all impurities.

摘要

本研究旨在制备疏水性水凝胶以从大肠杆菌裂解物中纯化质粒 DNA(pDNA)。通过将疏水性配体 N-丙烯酰基-L-苯丙氨酸(MAPA)掺入水凝胶骨架中来实现疏水性。除了常规的水凝胶化过程外,还包括了冷冻干燥步骤以创建纳米刺。制备了三种不同的水凝胶:聚(2-羟乙基甲基丙烯酸酯-N-丙烯酰基-L-苯丙氨酸)-冷冻干燥,[P(HEMA-MAPA)-FD];聚(2-羟乙基甲基丙烯酸酯-N-丙烯酰基-L-苯丙氨酸),[P(HEMA-MAPA)]和聚(2-羟乙基甲基丙烯酸酯)-冷冻干燥,[P(HEMA)-FD],并对其进行了表征,并用于从水溶液中吸附 DNA(鲑鱼精子 DNA)的研究。水凝胶的比表面积分别为 P(HEMA)-FD 为 21.4 m²/g,P(HEMA-MAPA)为 17.65 m²/g,P(HEMA-MAPA)-FD 为 36.0 m²/g。以连续模式研究了影响吸附的参数,如温度、初始 DNA 浓度、盐的类型和浓度。对于 P(HEMA-MAPA)-FD、P(HEMA-MAPA)和 P(HEMA)-FD,最大吸附容量分别为 45.31、27.08 和 1.81 mg DNA/g。使用无盐的乙酸缓冲液(pH 5.50)进行解吸过程。首先从大肠杆菌裂解物中分离 pDNA,然后通过琼脂糖凝胶电泳确定 pDNA 的纯度。最后,在 FPLC 中测试了 P(HEMA-MAPA)-FD 水凝胶对 pDNA 纯化的色谱性能。分辨率(R(s))为 2.84,pDNA 的特定选择性比所有杂质高 237.5 倍。

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