Fully automated viability and toxicity screening—A reliable all‐in‐one attempt

Victoria Liedtke; Romano Weiss; Anastasia Skifov; Stefan Rödiger; Lysann Schenk

doi:10.1002/cam4.7392

Cancer Medicine (Jun 2024)

Fully automated viability and toxicity screening—A reliable all‐in‐one attempt

Victoria Liedtke,
Romano Weiss,
Anastasia Skifov,
Stefan Rödiger,
Lysann Schenk

Affiliations

Victoria Liedtke: Faculty of Natural Sciences Brandenburg University of Technology Cottbus‐Senftenberg Senftenberg Germany
Romano Weiss: Faculty of Natural Sciences Brandenburg University of Technology Cottbus‐Senftenberg Senftenberg Germany
Anastasia Skifov: Faculty of Natural Sciences Brandenburg University of Technology Cottbus‐Senftenberg Senftenberg Germany
Stefan Rödiger: Faculty of Natural Sciences Brandenburg University of Technology Cottbus‐Senftenberg Senftenberg Germany
Lysann Schenk: Faculty of Natural Sciences Brandenburg University of Technology Cottbus‐Senftenberg Senftenberg Germany

DOI: https://doi.org/10.1002/cam4.7392
Journal volume & issue: Vol. 13, no. 12
pp. n/a – n/a

Abstract

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Abstract Background The CRISPR/Cas9 technology is nowadays a common tool for genome editing to achieve new insights into, for example, diagnostics and therapeutics in cancer and genetic disorders. Cell proliferation and anticancer drug response studies are widely used to evaluate the impact of editing. However, these assays are often time‐consuming, expensive, and reproducibility is an issue. To overcome this, we developed a fast and cheap assay that combines a fully automated multispectral fluorescence microscopy platform with a nuclei staining and open‐source software analysis. Methods Here, we generated different LEDGF/p75 model cell lines to validate the effect on proliferation and chemosensitivity. Therefore, a fast protocol for an optimized all‐in‐one attempt for cytotoxicity screenings and proliferation analysis of adherent cells in a 96‐well plate format was established using differential staining with two fluorescent dyes (Hoechst 33342 and propidium iodide) for live/dead cell discrimination. Subsequently, an automated cell nuclei count and analysis were performed using bioimage informatics. Results With the new established assay technology, up to 50,000 cells/well can be detected and analyzed in a 96‐well plate, resulting in a fast and accurate verification of viability and proliferation with consistency of 98% compared to manual counting. Our screening revealed that LEDGF depletion using CRISPR/Cas9 showed a diminished proliferation and chemosensitivity independent of cell line origin. Moreover, LEDGF depletion caused a significant increase in 𝛾H2AX foci, indicating a substantial increase in DNA double strand breaks. LEDGF/p75 overexpression enhanced proliferation and chemoresistance underlining the role of LEDGF in DNA damage response. Conclusion Independent of cancer cell type, LEDGF/p75 is a central player in DNA damage repair and is implicated in chemoresistance. Moreover, our automated fluorescence biosensor technology allowed fast and reliable data acquisition without any fixation or additional washing steps. Additionally, data analysis was implemented using the modular open‐source software that can be adapted as needed.

Published in Cancer Medicine

ISSN: 2045-7634 (Online)
Publisher: Wiley
Country of publisher: United Kingdom
LCC subjects: Medicine: Internal medicine: Neoplasms. Tumors. Oncology. Including cancer and carcinogens
Website: https://onlinelibrary.wiley.com/journal/20457634

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