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Human and Insect Cell-Produced Recombinant Adeno-Associated Viruses Show Differences in Genome Heterogeneity

九氟化硫 基因组 衣壳 生物 载体(分子生物学) HEK 293细胞 人口 计算生物学 转染 重组DNA 夜蛾 质粒 腺相关病毒 病毒 病毒学 遗传学 细胞培养 基因 医学 环境卫生
作者
Ngoc Tam Tran,Émilie Lecomte,Sylvie Saleün,Suk Namkung,Cécile Robin,Kristina Weber,Eric Devine,Véronique Blouin,Oumeya Adjali,Eduard Ayuso,Guangping Gao,Magalie Penaud‐Budloo,Phillip W.L. Tai
出处
期刊:Human Gene Therapy [Mary Ann Liebert]
卷期号:33 (7-8): 371-388 被引量:54
标识
DOI:10.1089/hum.2022.050
摘要

In the past two decades, adeno-associated virus (AAV) vector manufacturing has made remarkable advancements to meet large-scale production demands for preclinical and clinical trials. In addition, AAV vectors have been extensively studied for their safety and efficacy. In particular, the presence of empty AAV capsids and particles containing "inaccurate" vector genomes in preparations has been a subject of concern. Several methods exist to separate empty capsids from full particles; but thus far, no single technique can produce vectors that are free of empty or partial (non-unit length) capsids. Unfortunately, the exact genome compositions of full, intermediate, and empty capsids remain largely unknown. In this work, we used AAV-genome population sequencing to explore the compositions of DNase-resistant, encapsidated vector genomes produced by two common production pipelines: plasmid transfection in human embryonic kidney cells (pTx/HEK293) and baculovirus expression vectors in Spodoptera frugiperda insect cells (rBV/Sf9). Intriguingly, our results show that vectors originating from the same construct design that were manufactured by the rBV/Sf9 system produced a higher degree of truncated and unresolved species than those generated by pTx/HEK293 production. We also demonstrate that empty particles purified by cesium chloride gradient ultracentrifugation are not truly empty but are instead packaged with genomes composed of a single truncated and/or unresolved inverted terminal repeat (ITR). Our data suggest that the frequency of these "mutated" ITRs correlates with the abundance of inaccurate genomes in all fractions. These surprising findings shed new light on vector efficacy, safety, and how clinical vectors should be quantified and evaluated.

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