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首页> 外文期刊>Journal of chromatography, B. Analytical technologies in the biomedical and life sciences >Purification of human papillomavirus-like particles expressed in silkworm using a Bombyx mori nucleopolyhedrovirus bacmid expression system
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Purification of human papillomavirus-like particles expressed in silkworm using a Bombyx mori nucleopolyhedrovirus bacmid expression system

机译:使用Bombyx Mori核多核细胞核表达系统纯化在家蚕中表达的人乳头瘤病毒样粒子

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摘要

A three-stage chromatography protocol for the purification of human papillomavirus-like particles (HPV-LPs) from the silkworm-based Bombyx mori nucleopolyhedrovirus bacmid expression system was developed. For host cell DNA separation, anion exchange chromatography was used after screening for a suitable stationary phase. Using the two separation principles of cation exchange chromatography and metal affinity of ceramic hydroxyapatite (CHT) as a second stage, the amount of baculovirus in the sample was reduced to less than the detection limit of qPCR. The CHT separation was optimized with respect to the elution buffer used; 150-600 mM sodium phosphate, pH 7.2, resulted in the highest recovery of HPV-LPs. Using heparin chromatography, it was possible to reduce the sample volume and to thus highly concentrate the target protein during the separation of contaminating proteins. During the second purification stage, over 99.3% of the DNA was removed, and no infectious baculoviruses remained. After concentration by heparin column chromatography, over 99.9% of the DNA and protein had been removed. The purity achieved by this method exceeds that obtained by DDDDK-tag-based affinity chromatography and sucrose gradient ultracentrifugation, which were used as comparative purification methods. The 3-stage purification of HPV-LPs from silkworm fat bodies described here was a proof of concept and is a scalable method, but the overall yield remains to be improved.
机译:开发了一种三级色谱方案,用于纯化来自基于家蚕的Bombyx Mori核心核细胞核表达系统的人乳头瘤病毒样颗粒(HPV-LPS)。对于宿主细胞DNA分离,在筛选合适的固定相后使用阴离子交换色谱。利用阳离子交换色谱和陶瓷羟基磷灰石(CHT)的金属亲和力的两个分离原理作为第二阶段,将样品中的杆状病毒量降低至小于QPCR的检测限。相对于使用的洗脱缓冲液优化CHT分离;磷酸钠pH7.2钠150-600mm,导致HPV-LP的恢复最高。使用肝素色谱法,可以减少样品体积,并在污染蛋白的分离过程中高度浓缩靶蛋白。在第二纯化阶段,除去超过99.3%的DNA,并且没有残留感染性杆状病毒。通过肝素柱色谱浓缩后,已去除超过99.9%的DNA和蛋白质。通过该方法实现的纯度超过基于DDDDK标签的亲和层析和蔗糖梯度超速离心,用作比较纯化方法。这里描述的蚕脂肪体的HPV-LPS的3阶段纯化是概念的证据,是一种可扩展的方法,但总收益率仍有待改善。

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