The proteome of the blood-brain barrier in rat and mouse: highly specific identification of proteins on the luminal surface of brain microvessels by in vivo glycocapture

Tammy-Lynn Tremblay; Wael Alata; Jacqueline Slinn; Ewa Baumann; Christie E Delaney; Maria Moreno; Arsalan S Haqqani; Danica B Stanimirovic; Jennifer J Hill

doi:10.1186/s12987-024-00523-x

The proteome of the blood-brain barrier in rat and mouse: highly specific identification of proteins on the luminal surface of brain microvessels by in vivo glycocapture

Fluids Barriers CNS. 2024 Mar 4;21(1):23. doi: 10.1186/s12987-024-00523-x.

Authors

Tammy-Lynn Tremblay¹, Wael Alata^{1

2}, Jacqueline Slinn¹, Ewa Baumann¹, Christie E Delaney¹, Maria Moreno¹, Arsalan S Haqqani¹, Danica B Stanimirovic¹, Jennifer J Hill³

Affiliations

¹ Human Health Therapeutics, National Research Council Canada, 100 Sussex Dr., Ottawa, ON, K1A 0R6, Canada.
² Biology Program, New York University Abu Dhabi, Saadiyat Island Campus, P.O. Box 129188, Abu Dhabi, United Arab Emirates.
³ Human Health Therapeutics, National Research Council Canada, 100 Sussex Dr., Ottawa, ON, K1A 0R6, Canada. Jennifer.Hill@nrc-cnrc.gc.ca.

Abstract

Background: The active transport of molecules into the brain from blood is regulated by receptors, transporters, and other cell surface proteins that are present on the luminal surface of endothelial cells at the blood-brain barrier (BBB). However, proteomic profiling of proteins present on the luminal endothelial cell surface of the BBB has proven challenging due to difficulty in labelling these proteins in a way that allows efficient purification of these relatively low abundance cell surface proteins.

Methods: Here we describe a novel perfusion-based labelling workflow: in vivo glycocapture. This workflow relies on the oxidation of glycans present on the luminal vessel surface via perfusion of a mild oxidizing agent, followed by subsequent isolation of glycoproteins by covalent linkage of their oxidized glycans to hydrazide beads. Mass spectrometry-based identification of the isolated proteins enables high-confidence identification of endothelial cell surface proteins in rats and mice.

Results: Using the developed workflow, 347 proteins were identified from the BBB in rat and 224 proteins in mouse, for a total of 395 proteins in both species combined. These proteins included many proteins with transporter activity (73 proteins), cell adhesion proteins (47 proteins), and transmembrane signal receptors (31 proteins). To identify proteins that are enriched in vessels relative to the entire brain, we established a vessel-enrichment score and showed that proteins with a high vessel-enrichment score are involved in vascular development functions, binding to integrins, and cell adhesion. Using publicly-available single-cell RNAseq data, we show that the proteins identified by in vivo glycocapture were more likely to be detected by scRNAseq in endothelial cells than in any other cell type. Furthermore, nearly 50% of the genes encoding cell-surface proteins that were detected by scRNAseq in endothelial cells were also identified by in vivo glycocapture.

Conclusions: The proteins identified by in vivo glycocapture in this work represent the most complete and specific profiling of proteins on the luminal BBB surface to date. The identified proteins reflect possible targets for the development of antibodies to improve the crossing of therapeutic proteins into the brain and will contribute to our further understanding of BBB transport mechanisms.

Keywords: Blood–brain barrier; Endothelial; Luminal; Proteomics; Vessel.

MeSH terms

Animals
Blood-Brain Barrier*
Brain
Endothelial Cells
Membrane Proteins
Mice
Microvessels
Polysaccharides
Proteome*
Proteomics
Rats

Substances

Proteome
Membrane Proteins
Polysaccharides