| Literature DB >> 33604853 |
Helle Sedighi Frandsen1, Martina Štampar2, Joel Mario Vej-Nielsen1, Bojana Žegura2, Adelina Rogowska-Wrzesinska3.
Abstract
Cells cultured in a monolayer have been a central tool in molecular and cell biology, toxicology, biochemistry, and so on. Therefore, most methods for adherent cells in cell biology are tailored to this format of cell culturing. Limitations and disadvantages of monolayer cultures, however, have resulted in the ongoing development of advanced cell culturing techniques. One such technique is culturing cells as multicellular spheroids, that had been shown to mimic the physiological conditions found in vivo more accurately. This chapter presents a novel method for separation of the spheroid rim and core in mature spheroids (>21 days) for further analysis using advanced molecular biology techniques such as flow cytometry, viability estimations, comet assay, transcriptomics, proteomics and lipidomic. This fast and gentle disassembly of intact spheroids into rim and core fractions, and further into viable single-cell suspension provides an opportunity to bridge the gap from 3D cell culture to current state-of-the-art analysis methods.Entities:
Keywords: 3D cell culture; Comet assay; Flow cytometry; HepG2/C3A; Lipidomic; Proteomics; Rim and core; Spheroids; Transcriptomics
Mesh:
Year: 2021 PMID: 33604853 DOI: 10.1007/978-1-0716-1246-0_12
Source DB: PubMed Journal: Methods Mol Biol ISSN: 1064-3745