Most cellular functions are performed by large molecular assemblies and information about the structures and functions of these higher-order complexes can lead to an improved understanding of many biological processes, including how diseases progress, at the molecular level. The goal of the proposed research is to develop an integrated approach to determining detailed information about the higher-order structures of proteins and macromolecular assemblies that combines high-resolution ion mobility spectrometry (IMS) with solution-phase chemistry and hydrogen deuterium exchange (H/DX) with supercharging tandem mass spectrometry, and apply these methods to determine detailed information about the structures and structural transitions that occur in important macromolecular complexes where only limited information has been obtained using conventional high resolution structural methods. A low-pressure drift tube apparatus will be constructed and interfaced to a QTOF mass spectrometer to obtain absolute collision cross sections of large macromolecular complexes. These cross sections can provide information about structure/function relationships of the complex, as well as provide reference measurements for others using commercially available traveling wave IMS instruments that only provide relative cross section measurements. This IMS capability will be used to develop new H/DX methods that use supercharging reagents to unfold, dissociate, and highly charge the constituent molecules in the ms or sub-ms time frame of ion formation by electrospray, which eliminates any back exchange that can occur with conventional acid quenching methods. The goal is to obtain backbone amide exchange rates with close to individual amino acid resolution using electron transfer or electron capture dissociation tandem mass spectrometry, which have been shown to minimize gas-phase H/D scrambling and the concomitant loss of exchange rate information. The effect of increased charging obtained with these reagents on any gas-phase H/D scrambling that may occur will be investigated. A proteolytic 'nicking'strategy will be pursued to significantly increase the molecular size range where this top-down method can be used. A novel method to measure assembly kinetics at short times will be developed and used to find molecular frameworks that have the potential to be developed into effective drugs for treatment of anthrax infection and proteasome inhibitors in development for cancer therapy. These integrated approaches can potentially increase the speed, sensitivity, and molecular size range for which structural information can be obtained with high fidelity, and will provide complementary information to other structural methods, including electron microscopy, NMR, crystallography, and molecular modeling. These approaches will be applied to investigate the structures and structural transitions that occur in several complexes where limited information has been obtained, including Anthrax toxin complexes, and the 26S proteasome.

Public Health Relevance

This research is aimed at developing a fast and sensitive integrated approach for obtaining detailed information about the structure/function relationships of large molecular assemblies. This methodology can be used where conventional structural methods provide only limited information, and should be applicable to a wide range of areas of biomedical interest, including discovery of therapeutic agents aimed at regulating biomolecular complex formation, signal transduction, immune response, transcriptional regulation, protein translocation, apoptosis, and protein misfolding and aggregation that play a role in many diseases, including Alzheimer's disease, cystic fibrosis, spongiform encephalopathies (e.g., Mad Cow or Creutzfeldt Jakob disease), and even some cancers.

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM097357-03
Application #
8641395
Study Section
Enabling Bioanalytical and Imaging Technologies Study Section (EBIT)
Program Officer
Edmonds, Charles G
Project Start
2012-04-01
Project End
2016-03-31
Budget Start
2014-04-01
Budget End
2015-03-31
Support Year
3
Fiscal Year
2014
Total Cost
$250,008
Indirect Cost
$79,008
Name
University of California Berkeley
Department
Chemistry
Type
Schools of Arts and Sciences
DUNS #
124726725
City
Berkeley
State
CA
Country
United States
Zip Code
94704
Susa, Anna C; Lippens, Jennifer L; Xia, Zijie et al. (2018) Submicrometer Emitter ESI Tips for Native Mass Spectrometry of Membrane Proteins in Ionic and Nonionic Detergents. J Am Soc Mass Spectrom 29:203-206
Susa, Anna C; Xia, Zijie; Tang, Henry Y H et al. (2017) Charging of Proteins in Native Mass Spectrometry. J Am Soc Mass Spectrom 28:332-340
Susa, Anna C; Xia, Zijie; Williams, Evan R (2017) Native Mass Spectrometry from Common Buffers with Salts That Mimic the Extracellular Environment. Angew Chem Int Ed Engl 56:7912-7915
Mortensen, Daniel N; Susa, Anna C; Williams, Evan R (2017) Collisional Cross-Sections with T-Wave Ion Mobility Spectrometry without Experimental Calibration. J Am Soc Mass Spectrom 28:1282-1292
Mortensen, Daniel N; Williams, Evan R (2016) Electrothermal supercharging of proteins in native MS: effects of protein isoelectric point, buffer, and nanoESI-emitter tip size. Analyst 141:5598-606
Mortensen, Daniel N; Williams, Evan R (2016) Microsecond and nanosecond polyproline II helix formation in aqueous nanodrops measured by mass spectrometry. Chem Commun (Camb) 52:12218-12221
Mortensen, Daniel N; Williams, Evan R (2016) Ultrafast (1 ?s) Mixing and Fast Protein Folding in Nanodrops Monitored by Mass Spectrometry. J Am Chem Soc 138:3453-60
Mortensen, Daniel N; Williams, Evan R (2016) Surface-Induced Protein Unfolding in Submicron Electrospray Emitters. Anal Chem 88:9662-9668
Bhattacharyya, Moitrayee; Stratton, Margaret M; Going, Catherine C et al. (2016) Molecular mechanism of activation-triggered subunit exchange in Ca(2+)/calmodulin-dependent protein kinase II. Elife 5:
Going, Catherine C; Xia, Zijie; Williams, Evan R (2016) Real-time HD Exchange Kinetics of Proteins from Buffered Aqueous Solution with Electrothermal Supercharging and Top-Down Tandem Mass Spectrometry. J Am Soc Mass Spectrom 27:1019-27

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