# Dual Electron-Based Fragmentation with Ion Mobility to Advance Native Top-Down Proteomics

> **NIH NIH R44** · E-MSION, INC. · 2021 · $746,325

## Abstract

The identification and quantification of biological macromolecules remain challenging despite major
advances in the speed, resolution and mass accuracy of modern mass spectrometers. A key weakness with
current instrumentation lies in the methods used to induce fragmentation. The reliance in particular on
collision-induced dissociation (CID) has limited such analyses to bottom-up workflows of trypsin-digested
peptides of 10-30 residues. At e-MSion, we have developed an efficient electron-fragmentation technology
called ExD now co-marketed with Agilent for their family of Q-TOFs and with Thermo for their QE
Orbitraps. We succeeded with our phase I feasibility question to raise the fragmentation efficiency for doubly
charged peptides from 1-3% to approaching 20%. This makes our ExD technology practical for peptide
characterization and PTM localization in bottom up workflows -- the bread and butter for most proteomics
laboratories. What has really captured the interest of the biopharma and the top-down communities in the
past year is the exceptional sequence coverage of native proteins we obtain with the same ExD cell. The
resulting spectra are less congested than those obtained with ETD/UVPD/CID fragmentation methodologies
and it works for larger macromolecular protein complexes than has ever been possible before. Even with our
simpler fragmentation patterns, the spectral congestion from proteoforms greater than ~30 kDa becomes too
complex for many fragments to be distinguished even the highest resolution mass spectrometers. Our ExD
technology is also faster than all other electron-based fragmentation methods. This speed allows entire
proteins to be sequenced even after Ion Mobility Separations (IMS), which allows for spectra to be better
resolved by adding a fourth dimension of resolution. Because of this unique capability, Waters recently
purchased a prototype of our ExD cell adapted to fit at the exit of the IMS in their Synapt G2 mass
spectrometer. Shortly after installation, we were able to sequence hemoglobin variants from native tetramers
directly sprayed from human red blood cell lysates, FAB antibody subunits, and alcohol dehydrogenase (150
kDa). Some complexes such as GroEL and viral capsids still resist dissociation. We propose to overcome the
challenges of both spectral congestion and dissociation of large native complexes by utilizing dual ExD cells
with IMS. We will optimize the entrance-ExD cell to dissociate native protein complexes and use the exit-
ExD cell to further fragment IMS-resolved subunits. We will develop the control electronics and software
needed to coordinate the behavior of the two ExD cells with the IMS operation. Success will make possible
characterization of larger proteoforms by top-down native proteomics than possible before. The adoption of
our technology offers an extremely cost-effective solution that will accelerate the ability of many NIH
investigators to probe disease mechanisms by characterizing complex ma...

## Key facts

- **NIH application ID:** 10136641
- **Project number:** 5R44GM134792-03
- **Recipient organization:** E-MSION, INC.
- **Principal Investigator:** Valery G. Voinov
- **Activity code:** R44 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2021
- **Award amount:** $746,325
- **Award type:** 5
- **Project period:** 2019-09-01 → 2022-09-30

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10136641

## Citation

> US National Institutes of Health, RePORTER application 10136641, Dual Electron-Based Fragmentation with Ion Mobility to Advance Native Top-Down Proteomics (5R44GM134792-03). Retrieved via AI Analytics 2026-05-24 from https://api.ai-analytics.org/grant/nih/10136641. Licensed CC0.

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