4.7 Article

A multiple-channel, multiple-assay platform for characterization of full-range shear stress effects on vascular endothelial cells

Journal

LAB ON A CHIP
Volume 14, Issue 11, Pages 1880-1890

Publisher

ROYAL SOC CHEMISTRY
DOI: 10.1039/c3lc51304a

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Funding

  1. Utah Science Technology and Research Initiative (USTAR)

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Vascular endothelial cells (VECs), which line blood vessels and are key to understanding pathologies and treatments of various diseases, experience highly variable wall shear stress (WSS) in vivo (1-60 dyn cm(-2)), imposing numerous effects on physiological and morphological functions. Previous flow-based systems for studying these effects have been limited in range, and comprehensive information on VEC functions at the full spectrum of WSS has not been available yet. To allow rapid characterization of WSS effects, we developed the first multiple channel microfluidic platform that enables a wide range (similar to 15 Chi) of homogeneous WSS conditions while simultaneously allowing trans-monolayer assays, such as permeability and trans-endothelial electrical resistance (TEER) assays, as well as cell morphometry and protein expression assays. Flow velocity/WSS distributions between channels were predicted with COMSOL simulations and verified by measurement using an integrated microflow sensor array. Biomechanical responses of the brain microvascular endothelial cell line bEnd.3 to the full natural spectrum of WSS were investigated with the platform. Under increasing WSS conditions ranging from 0 to 86 dyn cm(-2), (1) permeabilities of FITC-conjugated dextran and propidium iodide decreased, respectively, at rates of 4.06 Chi 10(-8) and 6.04 Chi 10(-8) cm s(-1) per dyn cm(-2); (2) TEER increased at a rate of 0.8 Omega cm(2) per dyn cm(-2); (3) increased alignment of cells along the flow direction under increasing WSS conditions; and finally (4) increased protein expression of both the tight junction component ZO-1 (similar to 5 Chi) and the efflux transporter P-gp (similar to 6 Chi) was observed at 86 dyn cm(-2) compared to static controls via western blot. We conclude that the presented microfluidic platform is a valid approach for comprehensively assaying cell responses to fluidic WSS.

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