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. 2023 Nov 15;14(11):1002-1014.e5.
doi: 10.1016/j.cels.2023.10.003. Epub 2023 Oct 30.

A framework for ultra-low-input spatial tissue proteomics

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Free article

A framework for ultra-low-input spatial tissue proteomics

Anuar Makhmut et al. Cell Syst. .
Free article

Abstract

Spatial proteomics combining microscopy-based cell phenotyping with ultrasensitive mass-spectrometry-based proteomics is an emerging and powerful concept to study cell function and heterogeneity in (patho)physiology. However, optimized workflows that preserve morphological information for phenotype discovery and maximize proteome coverage of few or even single cells from laser microdissected tissue are currently lacking. Here, we report a robust and scalable workflow for the proteomic analysis of ultra-low-input archival material. Benchmarking in murine liver resulted in up to 2,000 quantified proteins from single hepatocyte contours and nearly 5,000 proteins from 50-cell regions. Applied to human tonsil, we profiled 146 microregions including T and B lymphocyte niches and quantified cell-type-specific markers, cytokines, and transcription factors. These data also highlighted proteome dynamics within activated germinal centers, illuminating sites undergoing B cell proliferation and somatic hypermutation. This approach has broad implications in biomedicine, including early disease profiling and drug target and biomarker discovery. A record of this paper's transparent peer review process is included in the supplemental information.

Keywords: FFPE; deep visual proteomics; histopathology; mass spectrometry; proteomics; single-cell proteomics; spatial proteomics.

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Conflict of interest statement

Declaration of interests The authors declare no competing interests.

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