Abstract

An abnormal increase in the number and distribution of SMCs is a key feature of the vascular remodelling that underlies cardiovascular disease. The predominant explanation for these changes is that medial SMCs undergo phenotypic modulation followed by migration to the intima and subsequent proliferation. However, there has been no direct demonstration of this dedifferentiation process by tracking the fate of contractile SMCs and the very existence of phenotypic plasticity has been questioned. We therefore employed high‐resolution, multi‐wavelength fluorescence and simultaneous phase contrast, time‐lapse microscopy to monitor the fate of unambiguously identified, freshly isolated, mature SMCs. Phenotypic modulation of the initially contractile SMCs was clearly observed in response to serum‐containing culture media. Extensive cellular remodelling occurred, though a consistent sequence of events was observed in which spindle‐shaped SMCs initially rounded up following exposure to media. The cells remained round for varying lengths of time (1‐3 days) before spreading outwards and, at this stage, repetitive contractions occurred (measured via bursts of high speed imaging). Finally, the cells flattened further and migration began. Surprisingly, after the onset of migration, the extrusion of subcellular structures (e.g. mitochondria) from one cell and their subsequent uptake by another cell was observed. The phenotypically modulated SMCs also formed direct connections with other cells (tunnelling nanotubes). These results highlight the complexity of the remodelling process, the highly dynamic cellular interactions involved and the significant cell‐cell variation in response and will enable a detailed picture of SMC remodelling to be built.Grant Funding Source: Supported by the Wellcome Trust (092292/Z/10/Z) and the British Heart Foundation (PG/11/70/29086)

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