RESUMEN
Scanning acoustic microscopy (SAM) is used to characterize welds in a thermoplastic polymer (ABS) manufactured by injection-molding, particularly at the locations of weld-lines known to form as unavoidable significant defects. Acoustic micrographs obtained at 420 MHz clearly resolve the weld lines with morphological deformations and microelastic heterogenity. This is also where terahertz (THz) measurements, carried out in support of the SAM study, reveal enhanced birefringence corresponding to the location of these lines enabling verification of the SAM results. Rayleigh surface acoustic waves (RSAW), quantified by V(z) curves (with defocusing distance of 85 µm), are found to propagate slower in regions close to the weld lines than in regions distant from these lines. The discrepancy of about 100 m/s in the velocity of RSAW indicates a large variation in the micro-elastic properties between areas close to and distant from the weld lines. The spatial variations in velocity (VR) of RSAWs indicate anisotropic propagation of the differently polarized ultrasonic waves.
RESUMEN
OBJECTIVE: Deletion of inducible nitric oxide synthase (iNOS) in apolipoprotein E knockout mice was shown to mitigate the extent of arteriosclerosis. Oxidized low density lipoprotein (oxLDL) inhibits macrophage migration and traps foam cells, possibly through a mechanism involving oxidative stress. Here, we addressed whether a reduction of iNOS-mediated oxidative stress remobilizes macrophage-derived foam cells and may reverse plaque formation. METHODS: Migration of RAW264.7 cells and bone marrow cells was quantified using a modified Boyden chamber. iNOS expression, phalloidin staining, focal adhesion kinase phosphorylation, lipid peroxides, nitric oxide (NO) and reactive oxygen species (ROS) production were assessed. RESULTS: oxLDL treatment significantly reduced cell migration compared to unstimulated cells (p < 0.05). This migratory arrest was reversed by co-incubation with a pharmacologic iNOS inhibitor 1400 W (p < 0.05) and iNOS-siRNA (p > 0.05). Furthermore, apoE/iNOS double knockout macrophages do not show migratory arrest in response to oxLDL uptake, compared to apoE knockout controls (p > 0.05). We documented significantly increased iNOS expression following oxLDL treatment and downregulation using 1400 W and small inhibitory RNA (siRNA). iNOS inhibition was associated with a reduction in NO and peroxynitrite (ONOO-)- and increased superoxide generation. Trolox treatment of RAW264.7 cells restored migration indicating that peroxynitrite mediated lipid peroxide formation is involved in the signaling pathway mediating cell arrest.. CONCLUSIONS: Here, we provide pharmacologic and genetic evidence that oxLDL induced iNOS expression inhibits macrophage-derived foam cell migration. Therefore, reduction of peroxynitrite and possibly lipid hydroperoxide levels in plaques represents a valuable therapeutic approach to reverse migratory arrest of macrophage-derived foam cells and to impair plaque formation.