Optimized Protocol for Accurate Titration of Adeno-Associated Virus Vectors

腺相关病毒 病毒定量 病毒学 滴定法 效价 分子生物学 病毒 色谱法 生物 载体(分子生物学) 重组DNA 化学 基因 生物化学 无机化学
作者
Tuisku Suoranta,Nihay Laham-Karam,Seppo Ylä‐Herttuala
出处
期刊:Human Gene Therapy [Mary Ann Liebert, Inc.]
卷期号:32 (19-20): 1270-1279 被引量:15
标识
DOI:10.1089/hum.2020.318
摘要

Adeno-associated virus (AAV) is currently the most popular gene delivery vector for in vivo gene therapy. However, variability in titration methods between different laboratories affects the reproducibility of experiments and evaluation of safety and efficacy in clinical trials. We describe an optimized protocol for AAV titration, including quantitative PCR (qPCR) standard preparation and quantitation and treatment of AAV samples before qPCR and droplet digital PCR (ddPCR) titration. During the protocol development, we observed that quantitation of the qPCR standard was dependent on its conformation and that A260-based quantitation overestimated the plasmid copy numbers, introducing significant error. Linearized, free inverted terminal repeat (free-ITR), and supercoiled standards were compared with enhanced green fluorescent protein (EGFP), SV40p(A), and AAV2-ITR qPCR assays and we found that using the AAV2-ITR assay together with either linearized or supercoiled standard led to overestimation of the titers, while EGFP and SV40p(A) assays were more accurate with the linearized standard. Finally, we compared extraction of AAV1, AAV2, AAV5, AAV6, AAV8, and AAV9 genomes by heat denaturation, proteinase K treatment, and kit extraction. Kit extraction, which contained proteinase K treatment in denaturing buffer before spin-column purification, significantly increased the titers acquired for all the serotypes in both qPCR and ddPCR. These improvements resulted in an accurate quantitation of the ATCC reference standard and in a robust and reliable protocol for AAV titration.
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