AI Article Synopsis

  • Mammosphere assays help identify cancer-initiating stem cells that can form spheres in a lab setting, but traditional methods lead to cell clumping, making it hard to measure true efficiency.
  • A new technique using lipid anchors was developed to reduce cell aggregation while allowing for free-floating growth, improving the accuracy of monitoring mammosphere formation.
  • This method resulted in a significantly higher percentage of clonal mammospheres and better size correlation compared to traditional low-attachment approaches, indicating more reliable assay outcomes.

Article Abstract

Mammosphere assays are widely used in vitro to identify prospective cancer-initiating stem cells that can propagate clonally to form spheres in free-floating conditions. However, the traditional mammosphere assay inevitably introduces cell aggregation that interferes with the measurement of true mammosphere forming efficiency. We developed a method to reduce tumor cell aggregation and increase the probability that the observed mammospheres formed are clonal in origin. Tethering individual tumor cells to lipid anchors prevents cell drift while maintaining free-floating characteristics. This enables real-time monitoring of single tumor cells as they divide to form mammospheres. Monitoring tethered breast cancer cells provided detailed size information that correlates directly to previously published single cell tracking data. We observed that 71% of the Day 7 spheres in lipid-coated wells were between 50 and 150 μm compared to only 37% in traditional low attachment plates. When an equal mixture of MCF7-GFP and MCF7-mCherry cells were seeded, 65% of the mammospheres in lipid-coated wells demonstrated single color expression whereas only 32% were single-colored in low attachment wells. These results indicate that using lipid tethering for mammosphere growth assays can reduce the confounding factor of cell aggregation and increase the formation of clonal mammospheres.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC7865010PMC
http://dx.doi.org/10.1038/s41598-021-81919-9DOI Listing

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