Neat plasma proteomics: getting the best out of the worst

Ines Metatla; Kevin Roger; Cerina Chhuon; Sara Ceccacci; Manuel Chapelle; Pierre-Olivier Schmit; Vadim Demichev; Ida Chiara Guerrera

doi:10.1186/s12014-024-09477-6

Neat plasma proteomics: getting the best out of the worst

Clin Proteomics. 2024 Mar 12;21(1):22. doi: 10.1186/s12014-024-09477-6.

Authors

Ines Metatla^#¹, Kevin Roger^#¹, Cerina Chhuon¹, Sara Ceccacci¹, Manuel Chapelle², Pierre-Olivier Schmit², Vadim Demichev³, Ida Chiara Guerrera⁴

Affiliations

¹ Proteomics Platform Necker, Université Paris Cité-Structure Fédérative de Recherche Necker, INSERM US24/CNRS UAR3633, 75015, Paris, France.
² Bruker Daltonique SA, 34 Rue de l'Industrie, 67166, Wissembourg Cedex, France.
³ Department of Biochemistry, Charité-Universitätsmedizin Berlin, 10117, Berlin, Germany.
⁴ Proteomics Platform Necker, Université Paris Cité-Structure Fédérative de Recherche Necker, INSERM US24/CNRS UAR3633, 75015, Paris, France. chiara.guerrera@inserm.fr.

^# Contributed equally.

Abstract

Plasma proteomics holds immense potential for clinical research and biomarker discovery, serving as a non-invasive "liquid biopsy" for tissue sampling. Mass spectrometry (MS)-based proteomics, thanks to improvement in speed and robustness, emerges as an ideal technology for exploring the plasma proteome for its unbiased and highly specific protein identification and quantification. Despite its potential, plasma proteomics is still a challenge due to the vast dynamic range of protein abundance, hindering the detection of less abundant proteins. Different approaches can help overcome this challenge. Conventional depletion methods face limitations in cost, throughput, accuracy, and off-target depletion. Nanoparticle-based enrichment shows promise in compressing dynamic range, but cost remains a constraint. Enrichment strategies for extracellular vesicles (EVs) can enhance plasma proteome coverage dramatically, but current methods are still too laborious for large series. Neat plasma remains popular for its cost-effectiveness, time efficiency, and low volume requirement. We used a test set of 33 plasma samples for all evaluations. Samples were digested using S-Trap and analyzed on Evosep One and nanoElute coupled to a timsTOF Pro using different elution gradients and ion mobility ranges. Data were mainly analyzed using library-free searches using DIA-NN. This study explores ways to improve proteome coverage in neat plasma both in MS data acquisition and MS data analysis. We demonstrate the value of sampling smaller hydrophilic peptides, increasing chromatographic separation, and using library-free searches. Additionally, we introduce the EV boost approach, that leverages on the extracellular vesicle fraction to enhance protein identification in neat plasma samples. Globally, our optimized analysis workflow allows the quantification of over 1000 proteins in neat plasma with a 24SPD throughput. We believe that these considerations can be of help independently of the LC-MS platform used.

Keywords: DIA-NN; Extracellular vesicles (EVs); Neat plasma; Plasma proteomics; diaPASEF.