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使用多重离子激活和质子转移电荷降低技术对重组腺相关病毒衣壳蛋白进行自上而下的质谱分析。

Top-down mass spectrometry analysis of capsid proteins of recombinant adeno-associated virus using multiple ion activations and proton transfer charge reduction.

作者信息

Kline Jake T, Huang Jingjing, Lieu Linda B, Srzentić Kristina, Bergen David, Mullen Christopher, McAlister Graeme C, Durbin Kenneth R, Melani Rafael D, Fornelli Luca

机构信息

University of Oklahoma, Norman, Oklahoma, USA.

Thermo Fisher Scientific, San Jose, California, USA.

出版信息

Proteomics. 2025 Mar;25(5-6):e2400223. doi: 10.1002/pmic.202400223. Epub 2024 Sep 5.

Abstract

Adeno-associated viruses (AAVs) are common vectors for emerging gene therapies due to their lack of pathogenicity in humans. Here, we present our investigation of the viral proteins (i.e., VP1, VP2, and VP3) of the capsid of AAVs via top-down mass spectrometry (MS). These proteins, ranging from 59 to 81 kDa, were chromatographically separated using hydrophilic interaction liquid chromatography and characterized in the gas-phase by high-resolution Orbitrap Fourier transform MS. Complementary ion dissociation methods were utilized to improve the overall sequence coverage. By reducing the overlap of product ion signals via proton transfer charge reduction on the Orbitrap Ascend BioPharma Tribrid mass spectrometer, the sequence coverage of each VP was significantly increased, reaching up to ∼40% in the case of VP3. These results showcase the improvements in the sequencing of proteins >30 kDa that can be achieved by manipulating product ions via gas-phase reactions to obtain easy-to-interpret fragmentation mass spectra.

摘要

腺相关病毒(AAV)因其对人类无致病性,是新兴基因治疗中常用的载体。在此,我们通过自上而下的质谱法(MS)对AAV衣壳的病毒蛋白(即VP1、VP2和VP3)进行了研究。这些蛋白质分子量在59至81 kDa之间,采用亲水相互作用液相色谱法进行色谱分离,并通过高分辨率轨道阱傅里叶变换质谱在气相中进行表征。使用互补离子解离方法提高整体序列覆盖率。通过在轨道阱Ascend生物制药三合一质谱仪上通过质子转移电荷减少来减少产物离子信号的重叠,每个VP的序列覆盖率显著提高,VP3的序列覆盖率高达约40%。这些结果展示了通过气相反应操纵产物离子以获得易于解释的碎片质谱,在大于30 kDa蛋白质测序方面取得的进展。

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