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多剂量瞬时转染人胚肾 293 细胞可调节重组腺相关病毒 2/5 Rep 蛋白的表达,并影响填充衣壳的浓缩分数。

Multidose transient transfection of human embryonic kidney 293 cells modulates recombinant adeno-associated virus2/5 Rep protein expression and influences the enrichment fraction of filled capsids.

机构信息

Center for Biomedical Innovation, Massachusetts Institute of Technology, Cambridge, Massachusetts, USA.

Department of Chemical Engineering, Massachusetts Institute of Technology, Cambridge, Massachusetts, USA.

出版信息

Biotechnol Bioeng. 2024 Dec;121(12):3694-3714. doi: 10.1002/bit.28828. Epub 2024 Aug 23.

DOI:10.1002/bit.28828
PMID:39176568
Abstract

Recombinant adeno-associated virus (rAAV) is a commonly used in vivo gene therapy vector because of its nonpathogenicity, long-term transgene expression, broad tropism, and ability to transduce both dividing and nondividing cells. However, rAAV vector production via transient transfection of mammalian cells typically yields a low fraction of filled-to-total capsids (~1%-30% of total capsids produced). Analysis of our previously developed mechanistic model for rAAV2/5 production attributed these low fill fractions to a poorly coordinated timeline between capsid synthesis and viral DNA replication and the repression of later phase capsid formation by Rep proteins. Here, we extend the model by quantifying the expression dynamics of total Rep proteins and their influence on the key steps of rAAV2/5 production using a multiple dosing transfection of human embryonic kidney 293 (HEK293) cells. We report that the availability of preformed empty capsids and viral DNA copies per cell are not limiting to the capsid-filling reaction. However, optimal expression of Rep proteins (<240 ± 13 ag per cell) enables enrichment of the filled capsid population (>12% of total capsids/cell) upstream. Our analysis suggests increased enrichment of filled capsids via regulating the expression of Rep proteins is possible but at the expense of per cell capsid titer in a triple plasmid transfection. Our study reveals an intrinsic limitation of scaling rAAV2/5 vector genome (vg) production and underscores the need for approaches that allow for regulating the expression of Rep proteins to maximize vg titer per cell upstream.

摘要

重组腺相关病毒(rAAV)因其非致病性、长期转基因表达、广泛的嗜性以及能够转导分裂和非分裂细胞而被广泛应用于体内基因治疗载体。然而,通过瞬时转染哺乳动物细胞生产 rAAV 载体通常只能得到一小部分填充的完整衣壳(~产生的总衣壳的 1%-30%)。我们之前开发的 rAAV2/5 生产的机制模型分析将这些低填充分数归因于衣壳合成和病毒 DNA 复制之间时间安排不协调,以及 Rep 蛋白对后期衣壳形成的抑制。在这里,我们通过使用人胚肾 293(HEK293)细胞的多次剂量转染来定量总 Rep 蛋白的表达动态及其对 rAAV2/5 生产关键步骤的影响,从而扩展了该模型。我们报告称,每个细胞中预形成的空衣壳和病毒 DNA 拷贝的可用性不是限制衣壳填充反应的因素。然而,Rep 蛋白的最佳表达(<240±13 ag/细胞)可以在上游富集填充衣壳群体(>细胞中总衣壳的 12%/细胞)。我们的分析表明,通过调节 Rep 蛋白的表达,增加填充衣壳的富集是可能的,但代价是在三质粒转染中每细胞衣壳滴度降低。我们的研究揭示了 rAAV2/5 载体基因组(vg)生产规模的内在限制,并强调需要采用允许调节 Rep 蛋白表达的方法,在上游最大限度地提高每个细胞的 vg 滴度。

相似文献

1
Multidose transient transfection of human embryonic kidney 293 cells modulates recombinant adeno-associated virus2/5 Rep protein expression and influences the enrichment fraction of filled capsids.多剂量瞬时转染人胚肾 293 细胞可调节重组腺相关病毒 2/5 Rep 蛋白的表达,并影响填充衣壳的浓缩分数。
Biotechnol Bioeng. 2024 Dec;121(12):3694-3714. doi: 10.1002/bit.28828. Epub 2024 Aug 23.
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Recombinant adeno-associated virus type 2 replication and packaging is entirely supported by a herpes simplex virus type 1 amplicon expressing Rep and Cap.2型重组腺相关病毒的复制和包装完全由表达Rep和Cap的1型单纯疱疹病毒扩增子支持。
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Utilizing minimally purified secreted rAAV for rapid and cost-effective manipulation of gene expression in the CNS.利用最小纯化的分泌型 rAAV 在中枢神经系统中快速且经济有效地操纵基因表达。
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Adeno-associated virus type 2 protein interactions: formation of pre-encapsidation complexes.2型腺相关病毒的蛋白质相互作用:衣壳化前复合物的形成
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Efficient recombinant adeno-associated virus production by a stable rep-cap HeLa cell line correlates with adenovirus-induced amplification of the integrated rep-cap genome.稳定的rep-cap HeLa细胞系高效生产重组腺相关病毒与腺病毒诱导的整合rep-cap基因组扩增相关。
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Role for highly regulated rep gene expression in adeno-associated virus vector production.高度调控的rep基因表达在腺相关病毒载体生产中的作用。
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Perfusion-Based Production of rAAV via an Intensified Transient Transfection Process.通过强化瞬时转染过程基于灌注的重组腺相关病毒生产
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