In experiments that involve contact with adhesion between two surfaces, as found in atomic force microscopy or nanoindentation, two distinct contact force (P) vs. indentation-depth (h) curves are often measured depending on whether the indenter moves towards or away from the sample. The origin of this hysteresis is not well understood and is often attributed to moisture, plasticity or viscoelasticity. Here we report experiments that show that hysteresis can exist in the absence of these effects, and that its magnitude depends on surface roughness. We develop a theoretical model in which the hysteresis appears as the result of a series of surface instabilities, in which the contact area grows or recedes by a finite amount. The model can be used to estimate material properties from contact experiments even when the measured P-h curves are not unique.
Mechanobiology relates cellular processes to mechanical signals, such as determining the effect of variations in matrix stiffness with cell tractions. Cell traction recorded via traction force microscopy (TFM) commonly takes place on materials such as polyacrylamideand polyethylene glycol-based gels. Such experiments remain limited in physiological relevance because cells natively migrate within complex tissue microenvironments that are spatially heterogeneous and hierarchical. Yet, TFM requires determination of the matrix constitutive law (stress-strain relationship), which is not always readily available. In addition, the currently achievable displacement resolution limits the accuracy of TFM for relatively small cells. To overcome these limitations, and increase the physiological relevance of in vitro experimental design, we present a new approach and a set of associated biomechanical signatures that are based purely on measurements of the matrix's displacements without requiring any knowledge of its constitutive laws. We show that our mean deformation metrics (MDM) approach can provide significant biophysical information without the need to explicitly determine cell tractions. In the process of demonstrating the use of our MDM approach, we succeeded in expanding the capability of our displacement measurement technique such that it can now measure the 3D deformations around relatively small cells (∼10 micrometers), such as neutrophils. Furthermore, we also report previously unseen deformation patterns generated by motile neutrophils in 3D collagen gels.traction force microscopy | confocal microscopy | large deformations | neutrophil M echanical cues within the cellular microenvironment regulate numerous fundamental functions including cell adhesion, deformation, and generation of traction (1-6). Analysis of cellular force generation, and its role in regulating homeostasis across a variety of cellular phenotypes and experimental platforms, has received much attention over the last three decades (7-13). Experimental quantification of cellular forces has produced several cell traction measurement techniques, ranging from surface wrinkle detection and flexure of micropillars to traction force microscopy (TFM) (12,(14)(15)(16)(17)(18)(19)(20). In TFM, measured cell-induced displacements are converted into tractions using various mathematical frameworks (14,15,17,18,21,22). Both twoand 3D TFM techniques have steadily increased in sophistication and now feature high-spatial displacement resolution and advanced computational formalisms to connect this displacement information to complex material constitutive laws (17,23,24).To successfully perform TFM, it is critical to know the stressstrain constitutive behavior of the matrix surrounding the cell. Although many TFM substrates feature relatively simple artificial gel constructs, such as polyacrylamide and polyethylene glycol, these constructs are impenetrable by cells and obviate measures obtained while cells are in a 3D setting (as would be the case within a bodily ...
Closed-form expressions for the stiffness and the damping coefficients of a squeeze film are derived for MEMS devices with perforated back plates. Two kinds of perforation configurations are considered-staggered and matrix or non-staggered configuration. The analytical solutions are motivated from the observation of repetitive pressure patterns obtained from numerical (FEM) solutions of the compressible Reynolds equation for the two configurations using ANSYS. A single pressure pattern is isolated and further subdivided into circular pressure cells. Circular geometry is used based on observed symmetry. Using suitable boundary conditions, the Reynolds equation is analytically solved over the pressure cells. The complex pressure obtained is used to identify the stiffness and damping offered by the pressure cells. The stiffness and damping forces due to pressure cells within a pattern are added up separately. In turn, the stiffness and damping due to all the patterns are summed up resulting in the stiffness and damping forces due to the entire squeeze film. The damping and spring forces thus obtained analytically are compared with those obtained from the FEM simulations in ANSYS. The match is found to be very good. The regime of validity and limitations of the analytical solutions are assessed in terms of design parameters such as pitch to air gap, hole length to diameter and pitch to hole radius ratios. The analysis neglects inertial effects. Hence, the results are presented for low values of Reynolds number.
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