Single-site sonoporation disrupts actin cytoskeleton organization
Author(s) -
Xian Chen,
Ruen Shan Leow,
Yaxin Hu,
Jennifer M. F. Wan,
Alfred C. H. Yu
Publication year - 2014
Publication title -
journal of the royal society interface
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.655
H-Index - 139
eISSN - 1742-5689
pISSN - 1742-5662
DOI - 10.1098/rsif.2014.0071
Subject(s) - sonoporation , actin , cytoskeleton , cytochalasin d , biophysics , actin cytoskeleton , microbiology and biotechnology , cytoplasm , chemistry , actin remodeling , biology , cell , microbubbles , ultrasound , biochemistry , medicine , radiology
Sonoporation is based upon an ultrasound-microbubble cavitation routine that physically punctures the plasma membrane on a transient basis. Over such process, the actin cytoskeleton may be disrupted in tandem since this network of subcellular filaments is physically interconnected with the plasma membrane. Here, by performing confocal fluorescence imaging of single-site sonoporation episodes induced by ultrasound-triggered collapse of a single targeted microbubble, we directly observed immediate rupturing of filamentary actin (F-actin) at the sonoporation site (cell type: ZR-75-30; ultrasound frequency: 1 MHz; peak negative pressure: 0.45 MPa; pulse duration: 30 cycles; bubble diameter: 2-4 m). Also, through conducting a structure tensor analysis, we observed further disassembly of the F-actin network over the next 60 min after the onset of sonoporation. The extent of F-actin disruption was found to be more substantial in cells with higher uptake of sonoporation tracer. Commensurate with this process, cytoplasmic accumulation of globular actin (G-actin) was evident in sonoporated cells, and in turn the G:F-actin ratio was increased in a trend similar to drug-induced (cytochalasin D) actin depolymerization. These results demonstrate that sonoporation is not solely a membrane-level phenomenon: organization of the actin cytoskeleton is concomitantly perturbed
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