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使用反相液相色谱法直接分析完整的腺相关病毒血清型 9 衣壳蛋白的脱酰胺作用。

Direct deamidation analysis of intact adeno-associated virus serotype 9 capsid proteins using reversed-phase liquid chromatography.

机构信息

Analytical Development & Operation, Novartis Pharmaceuticals, 10210 Campus Point Drive, SanDiego, CA92121, USA.

Analytical Development & Operation, Novartis Pharmaceuticals, 10210 Campus Point Drive, SanDiego, CA92121, USA.

出版信息

Anal Biochem. 2023 May 1;668:115099. doi: 10.1016/j.ab.2023.115099. Epub 2023 Mar 4.

DOI:10.1016/j.ab.2023.115099
PMID:36871622
Abstract

Recombinant adeno-associated viral (AAV) vectors have taken center stage as gene delivery vehicles for gene therapy. Asparagine deamidation of AAV capsid proteins has been reported to reduce vector stability and potency of AAV gene therapy products. Deamidation of asparagine residue is a common post-translational modification of proteins that is detected and quantified by liquid chromatography-tandem mass spectrometry (LC-MS)-based peptide mapping. However, artificial deamidation can be spontaneously induced during sample preparation for peptide mapping prior to LC-MS analysis. We have developed an optimized sample preparation method to reduce and minimize deamidation artifacts induced during sample preparation for peptide mapping, which typically takes several hours to complete. To shorten turnaround time of deamidation results and to avoid artificial deamidation, we developed orthogonal RPLC-MS and RPLC-fluorescence detection methods for direct deamidation analysis at the intact AAV9 capsid protein level to routinely support downstream purification, formulation development, and stability testing. Similar trends of increasing deamidation of AAV9 capsid proteins in stability samples were observed at the intact protein level and peptide level, indicating that the developed direct deamidation analysis of intact AAV9 capsid proteins is comparable to the peptide mapping-based deamidation analysis and both methods are suitable for deamidation monitoring of AAV9 capsid proteins.

摘要

重组腺相关病毒(AAV)载体已成为基因治疗的基因传递载体的核心。已有报道称,AAV 衣壳蛋白的天冬酰胺脱酰胺会降低载体的稳定性和 AAV 基因治疗产品的效力。天冬酰胺残基的脱酰胺是蛋白质的一种常见翻译后修饰,可通过基于液相色谱-串联质谱(LC-MS)的肽图分析进行检测和定量。然而,在进行 LC-MS 分析之前,肽图分析的样品制备过程中会自发诱导人工脱酰胺。我们开发了一种优化的样品制备方法,以减少和最小化肽图分析样品制备过程中诱导的脱酰胺假象,该方法通常需要数小时才能完成。为了缩短脱酰胺结果的周转时间并避免人工脱酰胺,我们开发了正交的 RPLC-MS 和 RPLC-荧光检测方法,用于直接在完整的 AAV9 衣壳蛋白水平上进行脱酰胺分析,以常规支持下游纯化、制剂开发和稳定性测试。在完整蛋白水平和肽水平上,稳定性样品中 AAV9 衣壳蛋白的脱酰胺趋势相似,表明所开发的完整 AAV9 衣壳蛋白的直接脱酰胺分析与基于肽图的脱酰胺分析相当,两种方法均适用于 AAV9 衣壳蛋白的脱酰胺监测。

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