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Characterization of Adeno-Associated Viral assemblies on an Ultra-High Mass Range Hybrid Quadrupole-Orbitrap Mass Spectrometer

Posters | 2021 | Thermo Fisher Scientific | ASMSInstrumentation
LC/HRMS, LC/MS, LC/MS/MS, LC/Orbitrap
Industries
Clinical Research
Manufacturer
Thermo Fisher Scientific

Summary

Significance of the Topic


Advancements in gene therapy hinge on precise characterization of viral delivery vehicles. Adeno-associated viruses (AAVs) are widely used capsid systems whose therapeutic efficacy and safety depend on detailed insights into capsid assembly, subunit composition, and post-translational modifications.

Study Objectives and Overview


This work assesses the Thermo Scientific Q Exactive UHMR hybrid quadrupole-Orbitrap mass spectrometer for two key applications:
  • Native MS of intact AAV capsids to determine empty versus genome-loaded particle ratios.
  • LC-MS/MS top-down analysis of denatured AAV capsid proteins (VP1, VP2, VP3) to characterize stoichiometry and proteoforms.


Methodology


Sample Preparation:
  • AAV serotypes 2 and 6 were expressed in HEK293 cells and buffer-exchanged into 100 mM ammonium acetate for native analysis.
  • AAV6 capsids were acid-treated to dissociate subunits for top-down investigation.

Chromatography and Mass Spectrometry:
  • Native MS: Static nanospray via coated emitters and NanoFlex source on the Q Exactive UHMR.
  • IEX-FLD: Ion-exchange separation with fluorescence detection to quantify empty versus full capsids.
  • RP LC-MS/MS: Denaturing reverse-phase UHPLC (Vanquish Horizon) coupled to UHMR for top-down fragmentation using All Ion Fragmentation (AIF) and higher-energy collisional dissociation (HCD).


Results and Discussion


1. Native Intact Capsid Analysis:
  • AAV6 empty : full ratio of approximately 64 : 36 was determined by IEX-FLD.
  • AAV2 displayed three distinct VP1 : VP2 : VP3 stoichiometries—5 : 5 : 50, 5 : 6 : 49, and 5 : 7 : 48—resolved in the m/z domain under native conditions.

2. Top-Down Subunit Characterization:
  • High-resolution MS confirmed N-terminal acetylation of VP1 and VP3 with mass accuracy < 0.1 Da.
  • Phosphorylation sites on VP2 at Ser-11 and Thr-56 were localized via HCD fragment ion series with < 10 ppm tolerance.
  • Relative quantitation based on integrated LC-MS peak areas yielded a VP1 : VP2 : VP3 ratio near 7 : 5 : 48 for AAV6.


Practical Benefits and Applications


  • Enables rapid quality control of AAV vector preparations by determining packaging efficiency and stoichiometry.
  • Provides detailed proteoform mapping to monitor critical PTMs that may affect capsid stability or immunogenicity.
  • Facilitates batch-to-batch comparability and compliance with regulatory requirements in gene therapy manufacturing.


Future Trends and Applications


Integration of UHMR-MS with automation and high-throughput workflows will accelerate vector development. Coupling native MS with ion mobility may further resolve assembly variants. Advanced top-down approaches could uncover new PTMs and proteoforms, supporting personalized gene therapy design.

Conclusion


The Orbitrap-based Q Exactive UHMR instrument demonstrated robust performance for both intact native analysis and top-down subunit characterization of AAV capsids, delivering high mass accuracy, sensitivity, and detailed proteoform insights essential for gene therapy vector development.

Instrumentation Used


  • Q Exactive UHMR hybrid quadrupole-Orbitrap mass spectrometer
  • Vanquish Horizon and Flex UHPLC systems
  • Static NanoFlex nanospray source with coated emitters
  • Ion-exchange fluorescence detector setup


References


No additional references cited.

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