High-performance peptide and disulfide mapping by direct injection of intact proteins using on-line coupled UV-liquid chromatography microdroplet mass spectrometry (UVLC-MMS)

Chin-Ming Kuo; Hung-Hsiang Jen; Fung-Yu Chen; Mohsen Akbarian; Tai-Hong Ou; Kang-Yu Liu; Jung-Lee Lin; Shu-Hui Chen

doi:10.1016/j.aca.2023.341790

High-performance peptide and disulfide mapping by direct injection of intact proteins using on-line coupled UV-liquid chromatography microdroplet mass spectrometry (UVLC-MMS)

Anal Chim Acta. 2023 Oct 23:1279:341790. doi: 10.1016/j.aca.2023.341790. Epub 2023 Sep 11.

Authors

Chin-Ming Kuo¹, Hung-Hsiang Jen¹, Fung-Yu Chen¹, Mohsen Akbarian¹, Tai-Hong Ou¹, Kang-Yu Liu¹, Jung-Lee Lin², Shu-Hui Chen³

Affiliations

¹ Department of Chemistry, National Cheng Kung University, Tainan, 701, Taiwan.
² Genomics Research Center, Academia Sinica, Taipei, 115, Taiwan.
³ Department of Chemistry, National Cheng Kung University, Tainan, 701, Taiwan. Electronic address: shchen@mail.ncku.edu.tw.

PMID: 37827684
DOI: 10.1016/j.aca.2023.341790

Abstract

Microdroplet mass spectrometry (MMS), achieving ultra-fast enzyme digestion in the ionization source, holds great promises for innovating protein analysis. Here, in-depth protein characterization is demonstrated by direct injection of intact protein mixtures via on-line coupling MMS with capillary C4 liquid chromatography (LC) containing UV windows (UVLC-MMS) through an enzyme introduction tee. We showed complete sets of peptides of individual proteins (hemoglobin, bovine serum albumin, and ribonuclease A) in a mixture could be obtained in one injection. Such full (100%) sequence coverage, however, could not be achieved by conventional nanoLC-MS method using bottom-up approach with single enzyme. Moreover, direct injection of a chaperone α-crystalline (α-Cry) complex yielded identification of post-translational modifications including novel sites and semi-quantitative characterization including 3:1 stoichiometry ratio of αA- and αB-Cry sub-units and ∼1.4 phosphorylation/subunit on S45 (novel site) and S122 (main site) of αA-Cry, ∼0.7 phosphorylation/subunit on S19 (main site) and S45 of αB-Cry, as well as 100% acetylation on both N-termini of each subunits by matching the mass and retention time of the intact and its digested peptides. Furthermore, trifluoroacetic acid was able to be used in the mobile phase with UVLC-MMS to improve the separation of differentially reduced intact species and detectability of the droplet-digested products. This allowed us to completely map four disulfide linkages of ribonuclease A based on collision-induced dissociation of disulfide clusters, some of which would otherwise not be detected, preventing scrambling or shuffling errors arising from lengthy bulk solution digestion by the bottom-up approach. Integration of UVLC and MMS greatly improves droplet digestion efficiency and MS detection, enabling highly efficient workflow for in-depth and accurate protein characterization.

Keywords: Electrosonic spray; Mass spectrometry; Microdroplet digestion; Reverse liquid chromatography; Top-down analysis.

MeSH terms

Amino Acid Sequence
Chromatography, Liquid / methods
Disulfides* / chemistry
Mass Spectrometry / methods
Peptides / analysis
Proteins
Ribonuclease, Pancreatic*
Ribonucleases

Substances

Disulfides
Ribonuclease, Pancreatic
Peptides
Proteins
Ribonucleases