2. Academic Validation
  3. High-Resolution Confocal Fluorescence Imaging of Serine Hydrolase Activity in Cryosections - Application to Glioma Brain Unveils Activity Hotspots Originating from Tumor-Associated Neutrophils

High-Resolution Confocal Fluorescence Imaging of Serine Hydrolase Activity in Cryosections - Application to Glioma Brain Unveils Activity Hotspots Originating from Tumor-Associated Neutrophils

  • Biol Proced Online. 2020 Mar 15:22:6. doi: 10.1186/s12575-020-00118-4.
Niina Aaltonen # 1 Prosanta K Singha # 1 Hermina Jakupović 1 Thomas Wirth 2 Haritha Samaranayake 2 Sanna Pasonen-Seppänen 1 Kirsi Rilla 1 Markku Varjosalo 3 Laura E Edgington-Mitchell 4 5 6 Paulina Kasperkiewicz 7 Marcin Drag 7 Sara Kälvälä 1 Eemeli Moisio 1 Juha R Savinainen 1 Jarmo T Laitinen 1
Affiliations

Affiliations

  • 1 1Institute of Biomedicine, University of Eastern Finland (UEF), POB 1627, FI-70211 Kuopio, Finland.
  • 2 Aurealis Pharma, Kuopio, Finland.
  • 3 3Institute of Biotechnology & HiLIFE, University of Helsinki, Helsinki, Finland.
  • 4 4Department of Biochemistry and Molecular Biology, Bio21 Molecular Science and Biotechnology Institute, The University of Melbourne, Parkville, VIC Australia.
  • 5 5Drug Discovery Biology, Monash Institute of Pharmaceutical Sciences, Monash University, Parkville, VIC Australia.
  • 6 6Department of Oral and Maxillofacial Surgery, New York University College of Dentistry, Bluestone Center for Clinical Research, New York, NY USA.
  • 7 7Department of Bioorganic Chemistry, Wroclaw University of Science and Technology, Wroclaw, Poland.
  • # Contributed equally.
PMID: 32190011 DOI: 10.1186/s12575-020-00118-4
Abstract

Background: Serine hydrolases (SHs) are a functionally diverse family of Enzymes playing pivotal roles in health and disease and have emerged as important therapeutic targets in many clinical conditions. Activity-based protein profiling (ABPP) using fluorophosphonate (FP) probes has been a powerful chemoproteomic approach in studies unveiling roles of SHs in various biological systems. ABPP utilizes cell/tissue proteomes and features the FP-warhead, linked to a fluorescent reporter for in-gel fluorescence imaging or a biotin tag for streptavidin enrichment and LC-MS/MS-based target identification. Existing ABPP approaches characterize global SH activity based on mobility in gel or MS-based target identification and cannot reveal the identity of the cell-type responsible for an individual SH activity originating from complex proteomes.

Results: Here, by using an activity probe with broad reactivity towards the SH family, we advance the ABPP methodology to glioma brain cryosections, enabling for the first time high-resolution confocal fluorescence imaging of global SH activity in the tumor microenvironment. Tumor-associated cell types were identified by extensive immunohistochemistry on activity probe-labeled sections. Tissue-ABPP indicated heightened SH activity in glioma vs. normal brain and unveiled activity hotspots originating from tumor-associated neutrophils (TANs), rather than tumor-associated macrophages (TAMs). Thorough optimization and validation was provided by parallel gel-based ABPP combined with LC-MS/MS-based target verification.

Conclusions: Our study advances the ABPP methodology to tissue sections, enabling high-resolution confocal fluorescence imaging of global SH activity in anatomically preserved complex native cellular environment. To achieve global portrait of SH activity throughout the section, a probe with broad reactivity towards the SH family members was employed. As ABPP requires no a priori knowledge of the identity of the target, we envisage no imaginable reason why the presently described approach would not work for sections regardless of species and tissue source.

Keywords

Activity-based protein profiling (ABPP); Brain cryosection; Glioblastoma multiforme (GBM); Immunohistochemistry; Neutrophil serine protease (NSP); Serine hydrolase activity; TAMRA-FP probe; Tumor-associated neutrophils.

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