Automated image analysis of stained cytospins to quantify Schwann cell purity and proliferation

Tamara Weiss; Lorenz Semmler; Flavia Millesi; Anda Mann; Maximilian Haertinger; Manuel Salzmann; Christine Radtke

doi:10.1371/journal.pone.0233647

Automated image analysis of stained cytospins to quantify Schwann cell purity and proliferation

PLoS One. 2020 May 22;15(5):e0233647. doi: 10.1371/journal.pone.0233647. eCollection 2020.

Authors

Tamara Weiss¹, Lorenz Semmler¹, Flavia Millesi¹, Anda Mann¹, Maximilian Haertinger¹, Manuel Salzmann², Christine Radtke^{1

3}

Affiliations

¹ Research Laboratory of the Division of Plastic and Reconstructive Surgery, Department of Surgery, Medical University of Vienna, Vienna, Austria.
² Institute of Vascular Biology and Thrombosis Research, Medical University of Vienna, Vienna, Austria.
³ Division of Plastic and Reconstructive Surgery, Department of Surgery, Medical University of Vienna, Vienna, Austria.

Abstract

In response to injury, adult Schwann cells (SCs) re-enter the cell cycle, change their expression profile, and exert repair functions important for wound healing and the re-growth of axons. While this phenotypical instability of SCs is essential for nerve regeneration, it has also been implicated in cancer progression and de-myelinating neuropathies. Thus, SCs became an important research tool to study the molecular mechanisms involved in repair and disease and to identify targets for therapeutic intervention. A high purity of isolated SC cultures used for experimentation must be demonstrated to exclude that novel findings are derived from a contaminating fibroblasts population. In addition, information about the SC proliferation status is an important parameter to be determined in response to different treatments. The evaluation of SC purity and proliferation, however, usually depends on the time consuming, manual assessment of immunofluorescence stainings or comes with the sacrifice of a large amount of SCs for flow cytometry analysis. We here show that rat SC culture derived cytospins stained for SC marker SOX10, proliferation marker EdU, intermediate filament vimentin and DAPI allowed the determination of SC identity and proliferation by requiring only a small number of cells. Furthermore, the CellProfiler software was used to develop an automated image analysis pipeline that quantified SCs and proliferating SCs from the obtained immunofluorescence images. By comparing the results of total cell count, SC purity and SC proliferation rate between manual counting and the CellProfiler output, we demonstrated applicability and reliability of the established pipeline. In conclusion, we here combined the cytospin technique, a multi-colour immunofluorescence staining panel, and an automated image analysis pipeline to enable the quantification of SC purity and SC proliferation from small cell aliquots. This procedure represents a solid read-out to simplify and standardize the quantification of primary SC culture purity and proliferation.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Biomarkers / metabolism
Cell Proliferation
Cells, Cultured
Female
Rats
Rats, Sprague-Dawley
Schwann Cells / cytology*

Substances

Biomarkers

Grants and funding

This work was supported by institutional funding.