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Sequential two-step chromatographic purification of infectious poliovirus using ceramic fluoroapatite and ceramic hydroxyapatite columns

机译:陶瓷氟磷灰石和陶瓷羟基磷灰石柱对脊灰病毒的连续两步色谱纯化

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摘要

Infectious virus purification techniques are important for vaccine development and gene therapy applications. However, the standardized one-step purification technique using ceramic hydroxyapatite (CHAp) has proven unsuitable for poliovirus. Therefore, we designed a sequential two-step chromatographic technique for purification of the infectious Sabin type 2 vaccine strain of poliovirus from the cell culture supernatant. In the first step, we removed protein contaminants from the Sabin type 2 virus fraction by pH gradient elution on a ceramic fluoroapatite column. In the second step, we removed double-stranded DNA derived from host cells by diluting the virus fraction, directly loading it on a CHAp column, and purifying it using a phosphate gradient with 1 M sodium chloride. This process achieved removal rates of more than 99.95% and 99.99% for proteins and double-stranded DNA, respectively, and was highly reproducible and scalable. Furthermore, it is likely that it will be applicable to other virus species.
机译:传染性病毒纯化技术对于疫苗开发和基因治疗应用很重要。但是,已证明使用陶瓷羟基磷灰石(CHAp)的标准化一步纯化技术不适用于脊髓灰质炎病毒。因此,我们设计了一种连续的两步色谱技术,用于从细胞培养上清液中纯化脊髓灰质炎病毒的传染性Sabin 2型疫苗株。第一步,我们通过在陶瓷氟磷灰石柱上进行pH梯度洗脱,从Sabin 2型病毒级分中去除了蛋白质污染物。在第二步中,我们通过稀释病毒部分,直接将其上样到CHAp柱上,并使用1 M氯化钠的磷酸盐梯度纯化来去除源自宿主细胞的双链DNA。此过程对蛋白质和双链DNA的去除率分别超过99.95%和99.99%,并且具有很高的重现性和可扩展性。此外,它可能将适用于其他病毒种类。

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