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通过硼酸盐吸附从含有质粒的裂解液中清除宿主细胞杂质。

Clearance of host cell impurities from plasmid-containing lysates by boronate adsorption.

机构信息

IBB - Institute for Biotechnology and Bioengineering, Centre for Biological and Chemical Engineering, Instituto Superior Técnico, 1049-001 Lisboa, Portugal.

出版信息

J Chromatogr A. 2010 Apr 9;1217(15):2262-6. doi: 10.1016/j.chroma.2010.02.015. Epub 2010 Feb 16.

DOI:10.1016/j.chroma.2010.02.015
PMID:20219199
Abstract

The ability of boronate adsorption to clear Escherichia coli impurities directly from plasmid-containing lysates (approximately pH 5.2) was evaluated. Results show that 3-aminophenyl boronate (PB) controlled pore glass (CPG) is able to adsorb not only those species that bear cis-diol groups (RNA, lipopolysaccharides-LPS), and are thus able to form covalent bonds with boronate, but also cis-diol-free proteins and genomic DNA (gDNA) fragments, while leaving most plasmid DNA in solution. Control runs performed with phenyl Sepharose and with PB-free CPG beads ruled out hydrophobic interactions with the phenyl ring and non-specific interactions with the glass matrix, respectively, as being responsible for RNA and gDNA adsorption. In batch mode, up to 97.6+/-3.1% of RNA, 94.6+/-0.8% of proteins and 96.7+/-11.7% of gDNA were cleared after 30 min, with a plasmid yield of 64%. In fixed-bed mode, most of the plasmid was recovered in the flowthrough (96.2+/-4.0%), even though the RNA (65.5+/-2.8%), protein (84.4+/-1.3%) and gDNA clearance (44.7+/-14.1%) were not as effective. In both cases, the LPS content was removed to a residual value of less than 0.005 EU/ml. The method is fast and straightforward, circumvents the need for pre-treatment of the feed and may contribute to shorten plasmid purification processes, as the treated streams can proceed directly to the final polishing steps.

摘要

硼酸盐吸附能力可直接从含有质粒的裂解液(约 pH5.2)中清除大肠杆菌杂质。结果表明,3-氨基苯硼酸(PB)控制孔玻璃(CPG)不仅能够吸附那些带有顺式二醇基团的物质(RNA、脂多糖-LPS),从而能够与硼酸盐形成共价键,还能够吸附无顺式二醇的蛋白质和基因组 DNA(gDNA)片段,而使大多数质粒 DNA 留在溶液中。用苯琼脂糖和无 PB 的 CPG 珠粒进行的对照实验分别排除了与苯环的疏水性相互作用和与玻璃基质的非特异性相互作用是导致 RNA 和 gDNA 吸附的原因。在批量模式下,经过 30 分钟,高达 97.6+/-3.1%的 RNA、94.6+/-0.8%的蛋白质和 96.7+/-11.7%的 gDNA 被清除,质粒产量为 64%。在固定床模式下,即使 RNA(65.5+/-2.8%)、蛋白质(84.4+/-1.3%)和 gDNA 清除率(44.7+/-14.1%)不是很高,大部分质粒仍在流穿液中回收(96.2+/-4.0%)。在这两种情况下,LPS 含量均降低到残留值小于 0.005 EU/ml。该方法快速简便,无需对进料进行预处理,可能有助于缩短质粒纯化过程,因为处理后的料流可直接进入最终的抛光步骤。

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