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一种用于质粒 DNA 色谱纯化的多模态组氨酸配体。

A multimodal histamine ligand for chromatographic purification of plasmid DNA.

机构信息

BIA Separations d.o.o., Mirce 21, SI-5270 Ajdovščina, Slovenia.

出版信息

J Chromatogr A. 2013 Mar 15;1281:87-93. doi: 10.1016/j.chroma.2013.01.058. Epub 2013 Jan 23.

DOI:10.1016/j.chroma.2013.01.058
PMID:23398998
Abstract

To exploit different chromatographic modes for efficient plasmid DNA (pDNA) purification a novel monolithic chromatographic support bearing multimodal histamine (HISA) groups was developed and characterized. Electrostatic charge of HISA groups depends on the pH of the mobile phase, being neutral above pH 7 and becoming positively charged below. As a consequence, HISA groups exhibit predominantly ion-exchange character at low pH values, which decreases with titration of the HISA groups resulting in increased hydrophobicity. This feature enabled separation of supercoiled (sc) pDNA from other plasmid isoforms (and other process related impurities) by adjusting salt or pH gradient. The dynamic binding capacity (DBC) for a 5.1kbp large plasmid at pH 5 was 4.0 mg/ml under low salt binding conditions, remaining relatively high (3.0 mg/ml) even in the presence of 1.0 M NaCl due to the multimodal nature of HISA ligand. Only slightly lower DBC (2.7 mg/ml) was determined under preferentially hydrophobic conditions in 3.0 M (NH(4))(2)SO(4), pH 7.4. Open circular and sc pDNA isoforms were baseline separated in descending (NH(4))(2)SO(4) gradient. Furthermore, an efficient plasmid DNA separation was possible both on analytical as well as on preparative scale by applying the descending pH gradient at a constant concentration (above 3.0 M) of (NH(4))(2)SO(4).

摘要

为了利用不同的色谱模式来高效地纯化质粒 DNA(pDNA),我们开发并表征了一种新型的整体式色谱支撑物,其表面带有多模态组氨酸(HISA)基团。HISA 基团的静电荷取决于流动相的 pH 值,在 pH 值高于 7 时呈中性,低于 7 时带正电荷。因此,HISA 基团在低 pH 值下主要表现出离子交换特性,随着 HISA 基团的滴定,这种特性会降低,从而增加疏水性。这种特性使得可以通过调节盐度或 pH 梯度来分离超螺旋(sc)pDNA 与其他质粒异构体(和其他相关的工艺杂质)。在低盐结合条件下,pH 值为 5 时,对于 5.1kbp 大小的质粒,动态结合容量(DBC)为 4.0mg/ml,即使在存在 1.0 M NaCl 的情况下,由于 HISA 配体的多模态性质,DBC 仍相对较高(3.0mg/ml)。在 3.0 M(NH 4)2SO 4、pH 值为 7.4 的情况下,在优先疏水性条件下,DBC 略低(2.7mg/ml)。开环和 sc pDNA 异构体在(NH 4)2SO 4 下降梯度中基线分离。此外,通过在恒定浓度(高于 3.0 M)的(NH 4)2SO 4 下应用下降 pH 梯度,可以在分析和制备规模上有效地分离质粒 DNA。

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