An optimized quantitative proteomics method establishes the cell type-resolved mouse brain secretome.

Abstract:

To understand how cells communicate in the nervous system, it is essential to define their secretome, which is challenging for primary cells because of large cell numbers being required. Here, we miniaturized secretome analysis by developing the "high-performance secretome protein enrichment with click sugars" (hiSPECS) method. To demonstrate its broad utility, hiSPECS was used to identify the secretory response of brain slices upon LPS-induced neuroinflammation and to establish the cell type-resolved mouse brain secretome resource using primary astrocytes, microglia, neurons, and oligodendrocytes. This resource allowed mapping the cellular origin of CSF proteins and revealed that an unexpectedly high number of secreted proteins in vitro and in vivo are proteolytically cleaved membrane protein ectodomains. Two examples are neuronally secreted ADAM22 and CD200, which we identified as substrates of the Alzheimer-linked protease BACE1. hiSPECS and the brain secretome resource can be widely exploited to systematically study protein secretion and brain function and to identify cell type-specific biomarkers for CNS diseases.

SEEK ID: http://lmmeisd-2.srv.mwn.de/publications/24

PubMed ID: 32954517

Projects: Published Datasets

Publication type: Journal

Journal: EMBO J

Citation: EMBO J. 2020 Oct 15;39(20):e105693. doi: 10.15252/embj.2020105693. Epub 2020 Sep 21.

Date Published: 15th Oct 2020

Registered Mode: by PubMed ID

Authors: J. Tushaus, S. A. Muller, E. S. Kataka, J. Zaucha, L. Sebastian Monasor, M. Su, G. Guner, G. Jocher, S. Tahirovic, D. Frishman, M. Simons, S. F. Lichtenthaler

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Created: 5th Jul 2024 at 09:33

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