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质粒大小对苯甲膜吸附剂纯化模型质粒 DNA 疫苗的影响。

Impact of plasmid size on the purification of model plasmid DNA vaccines by phenyl membrane adsorbers.

机构信息

IBB - Institute for Biotechnology and Bioengineering, Centre for Biological and Chemical Engineering, Instituto Superior Técnico, Lisboa, Portugal; DBE - Department of Bioengineering, Instituto Superior Técnico, Av. Rovisco Pais 1, 1049-001 Lisboa, Portugal.

出版信息

J Chromatogr A. 2013 Nov 8;1315:145-51. doi: 10.1016/j.chroma.2013.09.076. Epub 2013 Sep 27.

DOI:10.1016/j.chroma.2013.09.076
PMID:24103809
Abstract

Plasmid DNA (pDNA) offers a versatile platform for the development of new pharmaceuticals. This versatility also adds in variability among plasmid products most of the times sharing only the same basic molecular structure. Membrane chromatography experiments performed with a Sartorius(®) Phenyl 3 mL spiral cartridge and differently sized plasmids (3.70 kbp, 6.05 kbp and 10.4 kbp) show that the strength of interaction of pDNA isoforms with HIC membrane adsorbers depends on size. These differences in relative binding strength were explored using a stepwise elution strategy of decreasing buffer conductivities in order to increase the purity of supercoiled (SC) pDNA isoforms. The open circular (OC) isoforms of all plasmids eluted earlier at a similar conductivity of 190 mS/cm, independently of the hydrodynamic diameter (Dh). A drop in conductivity of 16.0 mS/cm, 23 mS/cm and 19 mS/cm had to be imposed to elute the supercoiled (SC) counterparts of the 3.70 kbp, 6.05 kbp and 10.4 kbp, respectively. This corresponds to relative binding strengths of the SC over OC isoforms of 1.09, 1.14 and 1.11. Unlike the OC isoforms, the behavior of SC isoforms was dependent of the Dh. The purified and pooled plasmid fractions were assayed and demonstrated high degree of purity, compliant with regulatory agencies criteria: over 99% RNA removal, endotoxin levels below 0.001 EU/μg pDNA and undetectable protein content by BCA assay.

摘要

质粒 DNA(pDNA)为新药物的开发提供了一个多功能平台。这种多功能性也增加了质粒产品的可变性,大多数情况下,它们仅共享相同的基本分子结构。使用 Sartorius(®)Phenyl 3 mL 螺旋柱和不同大小的质粒(3.70 kbp、6.05 kbp 和 10.4 kbp)进行的膜色谱实验表明,pDNA 同种型与 HIC 膜吸附剂的相互作用强度取决于大小。使用逐步降低缓冲液电导率的洗脱策略来增加超螺旋(SC)pDNA 同种型的纯度,探索了这些相对结合强度的差异。所有质粒的开环(OC)同种型在相似的电导率 190 mS/cm 处较早洗脱,与流体动力学直径(Dh)无关。必须将电导率降低 16.0 mS/cm、23 mS/cm 和 19 mS/cm,才能分别洗脱 3.70 kbp、6.05 kbp 和 10.4 kbp 的超螺旋(SC)对应物。这对应于 SC 对 OC 同种型的相对结合强度为 1.09、1.14 和 1.11。与 OC 同种型不同,SC 同种型的行为取决于 Dh。对纯化和汇集的质粒级分进行了检测,结果表明其具有高纯度,符合监管机构的标准:超过 99%的 RNA 去除、内毒素水平低于 0.001 EU/μg pDNA 和通过 BCA 测定法检测不到的蛋白质含量。

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