Native and compactly folded in-solution conformers of pepsin are revealed and distinguished by mass spectrometric ITEM-TWO analyses of gas-phase pepstatin A - pepsin complex binding strength differences

Cornelia Koy; Ursula M Glocker; Bright D Danquah; Michael O Glocker

doi:10.1177/14690667231178999

Native and compactly folded in-solution conformers of pepsin are revealed and distinguished by mass spectrometric ITEM-TWO analyses of gas-phase pepstatin A - pepsin complex binding strength differences

Eur J Mass Spectrom (Chichester). 2023 Oct;29(5-6):303-312. doi: 10.1177/14690667231178999. Epub 2023 May 31.

Authors

Cornelia Koy¹, Ursula M Glocker¹, Bright D Danquah¹, Michael O Glocker¹

Affiliation

¹ Proteome Center Rostock, Medical Faculty and Natural Science Faculty, University of Rostock, Rostock, Germany.

PMID: 37259551
DOI: 10.1177/14690667231178999

Abstract

Pepsin, because of its optimal activity at low acidic pH, has gained importance in mass spectrometric proteome research as a readily available and easy-to-handle protease. Pepsin has also been study object of protein higher-order structure analyses, but questions about how to best investigate pepsin in-solution conformers still remain. We first determined dependencies of pepsin ion charge structures on solvent pH which indicated the in-solution existence of (a) natively folded pepsin (N) which by nanoESI-MS analysis gave rise to a narrow charge state distribution with an 11-fold protonated most intense ion signal, (b) unfolded pepsin (U) with a rather broad ion charge state distribution whose highest ion signal carried 25 protons, and (c) a compactly folded pepsin conformer (C) with a narrow charge structure and a 12-fold protonated ion signal in the center of its charge state envelope. Because pepsin is a protease, unfolded pepsin became its own substrate in solution at pH 6.6 since at this pH some portion of pepsin maintained a compact/native fold which displayed enzymatic activity. Subsequent mass spectrometric ITEM-TWO analyses of pepstatin A - pepsin complex dissociation reactions in the gas phase confirmed a very strong binding of pepstatin A by natively folded pepsin (N). ITEM-TWO further revealed the existence of two compactly folded in-solution pepsin conformers (C^a and C^b) which also were able to bind pepstatin A. Binding strengths of the respective compactly folded pepsin conformer-containing complexes could be determined and apparent gas phase complex dissociation constants and reaction enthalpies differentiated these from each other and from the pepstatin A - pepsin complex which had been formed from natively folded pepsin. Thus, ITEM-TWO turned out to be well suited to pinpoint in-solution pepsin conformers by interrogating quantitative traits of pepstatin A - pepsin complexes in the gas phase.

Keywords: CID; ITEM-TWO; Pepstatin A – pepsin complex; complex binding strength; gas phase complex dissociation; in-solution protein conformers; intermediate analysis; nanoESI-MS; protein folding.

MeSH terms

Pepsin A* / chemistry
Pepsin A* / metabolism
Pepstatins / chemistry
Spectrometry, Mass, Electrospray Ionization* / methods

Substances

Pepsin A
pepstatin
Pepstatins