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通过阴离子交换色谱法从1型腺相关病毒载体储备液中去除空衣壳可增强转基因表达。

Removal of empty capsids from type 1 adeno-associated virus vector stocks by anion-exchange chromatography potentiates transgene expression.

作者信息

Urabe Masashi, Xin Ke-Qin, Obara Yoko, Nakakura Takayo, Mizukami Hiroaki, Kume Akihiro, Okuda Kenji, Ozawa Keiya

机构信息

Division of Genetic Therapeutics, Jichi Medical School, 3311-1 Yakushiji, Tochigi 329-0498, Japan.

出版信息

Mol Ther. 2006 Apr;13(4):823-8. doi: 10.1016/j.ymthe.2005.11.024. Epub 2006 Feb 13.

DOI:10.1016/j.ymthe.2005.11.024
PMID:16473554
Abstract

Production of recombinant adeno-associated virus (rAAV) results in substantial quantities of empty capsids or virus-like particles (VLPs), virus protein shells without the vector genome. The contaminating VLPs would interfere with transduction by competing for cell-surface receptors and, when administered in vivo, contribute to antigen load, which may elicit a stronger immune response. Density-gradient ultracentrifugation provides a means to separate VLPs from rAAV particles, but is not feasible for large-scale preparations of vectors. Since the compositions of the VLP and vector differ by the single-stranded DNA genome, we hypothesized that the isoelectric point of the vector may differ from that of the VLP. In an attempt to separate type 1 rAAV particles from VLPs by ion-exchange chromatography, we tested a number of buffer systems and found that trimethylammonium sulfate, or [(CH3)4N]2SO4, effectively separated rAAV1 particles from VLPs. The rAAV1-GFP chromatographically separated from VLPs induced stronger GFP expression in HEK293 cells than rAAV1-GFP contaminated with VLPs. The transduction of mouse muscles with rAAV1-SEAP (secreted form of alkaline phosphatase) isolated from VLPs also showed higher serum SEAP levels than rAAV1-SEAP with VLPs. These results suggest that chromatographic separation of rAAV1 from empty capsids increased the efficacy of rAAV1.

摘要

重组腺相关病毒(rAAV)的生产会产生大量空衣壳或病毒样颗粒(VLP),即没有载体基因组的病毒蛋白外壳。污染的VLP会通过竞争细胞表面受体干扰转导,并且在体内给药时会增加抗原负荷,这可能引发更强的免疫反应。密度梯度超速离心提供了一种从rAAV颗粒中分离VLP的方法,但对于大规模制备载体来说并不可行。由于VLP和载体的组成因单链DNA基因组而不同,我们推测载体的等电点可能与VLP的等电点不同。为了通过离子交换色谱从VLP中分离出1型rAAV颗粒,我们测试了多种缓冲系统,发现硫酸三甲基铵,即[(CH3)4N]2SO4,能有效地从VLP中分离出rAAV1颗粒。经色谱分离从VLP中分离出的rAAV1-GFP在HEK-29细胞中诱导的GFP表达比受VLP污染的rAAV1-GFP更强。用从VLP中分离出的rAAV1-SEAP(碱性磷酸酶的分泌形式)转导小鼠肌肉,其血清SEAP水平也高于含有VLP的rAAV1-SEAP。这些结果表明,从空衣壳中色谱分离rAAV1可提高rAAV1的效力。

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