| Literature DB >> 31015629 |
Ivan Pushkarsky1, Peter Tseng1,2, Dylan Black1, Bryan France3, Lyndon Warfe1, Cynthia J Koziol-White4, William F Jester4, Ryan K Trinh5, Jonathan Lin1, Philip O Scumpia6, Sherie L Morrison5, Reynold A Panettieri4, Robert Damoiseaux3,7, Dino Di Carlo8,9,10.
Abstract
As cells with aberrant force-generating phenotypes can directly lead to disease, cellular force-generation mechanisms are high-value targets for new therapies. Here, we show that single-cell force sensors embedded in elastomers enable single-cell force measurements with ~100-fold improvement in throughput than was previously possible. The microtechnology is scalable and seamlessly integrates with the multi-well plate format, enabling highly parallelized time-course studies. In this regard, we show that airway smooth muscle cells isolated from fatally asthmatic patients have innately greater and faster force-generation capacity in response to stimulation than healthy control cells. By simultaneously tracing agonist-induced calcium flux and contractility in the same cell, we show that the calcium level is ultimately a poor quantitative predictor of cellular force generation. Finally, by quantifying phagocytic forces in thousands of individual human macrophages, we show that force initiation is a digital response (rather than a proportional one) to the proper immunogen. By combining mechanobiology at the single-cell level with high-throughput capabilities, this microtechnology can support drug-discovery efforts for clinical conditions associated with aberrant cellular force generation.Entities:
Mesh:
Substances:
Year: 2018 PMID: 31015629 PMCID: PMC6619436 DOI: 10.1038/s41551-018-0193-2
Source DB: PubMed Journal: Nat Biomed Eng ISSN: 2157-846X Impact factor: 25.671