33 research outputs found
Spatiotemporally Super-Resolved Volumetric Traction Force Microscopy
Quantification of mechanical forces is a major challenge across biomedical sciences. Yet such measurements are essential to understanding the role of biomechanics in cell regulation and function. Traction force microscopy remains the most broadly applied force probing technology but typically restricts itself to single-plane two-dimensional quantifications with limited spatiotemporal resolution. Here, we introduce an enhanced force measurement technique combining 3D super-resolution fluorescence structural illumination microscopy and traction force microscopy (3D-SIM-TFM) offering increased spatiotemporal resolution, opening-up unprecedented insights into physiological three-dimensional force production in living cells
Spatiotemporally Super-resolved Volumetric Traction Force Microscopy
Quantification of mechanical forces is a major
challenge across biomedical sciences. Yet such measurements
are essential to understanding the role of biomechanics in cell
regulation and function. Traction force microscopy remains
the most broadly applied force probing technology but
typically restricts itself to single-plane two-dimensional
quantifications with limited spatiotemporal resolution. Here,
we introduce an enhanced force measurement technique
combining 3D super-resolution fluorescence structural illumination microscopy and traction force microscopy (3D-SIMTFM) offering increased spatiotemporal resolution, openingup unprecedented insights into physiological three-dimensional force production in living cells
Enhanced Lifetime Of Excitons In Nonepitaxial Au/cds Core/shell Nanocrystals
The ability of metal nanoparticles to capture light through plasmon excitations offers an opportunity for enhancing the optical absorption of plasmon-coupled semiconductor materials via energy transfer. This process, however, requires that the semiconductor component is electrically insulated to prevent a backward charge flow into metal and interfacial states, which causes a premature dissociation of excitons. Here we demonstrate that such an energy exchange can be achieved on the nanoscale by using nonepitaxial Au/CdS core/shell nanocomposites. These materials are fabricated via a multistep cation exchange reaction, which decouples metal and semiconductor phases leading to fewer interfacial defects. Ultrafast transient absorption measurements confirm that the lifetime of excitons in the CdS shell (tau approximate to 300 ps) is much longer than lifetimes of excitons in conventional, reduction-grown Au/CdS heteronanostructures. As a result, the energy of metal nanoparticles can be efficiently utilized by the semiconductor component without undergoing significant nonradiative energy losses, an important property for catalytic or photovoltaic applications. The reduced rate of exciton dissociation in the CdS domain of Au/CdS nanocomposites was attributed to the nonepitaxial nature of Au/CdS interfaces associated with low defect density and a high potential barrier of the interstitial phase
Extended mechanical force measurements using structured illumination microscopy
Quantifying cell generated mechanical forces is key to furthering our understanding of mechanobiology. Traction force microscopy (TFM) is one of the most broadly applied force probing technologies, but its sensitivity is strictly dependent on the spatio-temporal resolution of the underlying imaging system. In previous works, it was demonstrated that increased sampling densities of cell derived forces permitted by super-resolution fluorescence imaging enhanced the sensitivity of the TFM method. However, these recent advances to TFM based on super-resolution techniques were limited to slow acquisition speeds and high illumination powers. Here, we present three novel TFM approaches that, in combination with total internal reflection, structured illumination microscopy and astigmatism, improve the spatial and temporal performance in either two-dimensional or three-dimensional mechanical force quantification, while maintaining low illumination powers. These three techniques can be straightforwardly implemented on a single optical set-up offering a powerful platform to provide new insights into the physiological force generation in a wide range of biological studies.
This article is part of the Theo Murphy meeting issue ‘Super-resolution structured illumination microscopy (part 1)'
Label-Free Optical Nanoscopy of Single-Layer Graphene
The application of ultrafast pulsed laser sources and spectroscopic techniques enables label-free, deep-tissue optical microscopy. However, circumvention of the diffraction limit in this field is still an open challenge. Among such approaches, pump\u2013probe microscopy is of increasing interest thanks to its highly specific nonfluorescent-based contrast mechanisms for the imaging of material and life science samples. In this paper, a custom femtosecond-pulsed near-infrared pump\u2013probe microscope, which exploits transient absorption and stimulated Raman scattering interactions, is presented. The conventional pump\u2013probe configuration is combined with a spatially shaped saturation pump beam, which allows for the reduction of the effective focal volume exploiting transient absorption saturation. By optimizing the acquisition parameters, such as power and temporal overlap of the saturation beam, we can image single-layer graphene deposited on a glass surface at the nanoscale and with increased layer sensitivity. These results suggest that saturation pump\u2013probe nanoscopy is a promising tool for label-free high-resolution imaging
Exploring the potential of Airyscan microscopy for live cell imaging
Biological research increasingly demands the use of non-invasive and ultra-sensitive imaging techniques. The Airyscan technology was recently developed to bridge the gap between conventional confocal and super-resolution microscopy. This technique combines confocal imaging with a 0.2 Airy Unit pinhole, deconvolution and the pixel-reassignment principle in order to enhance both the spatial resolution and signal-to-noise-ratio without increasing the excitation power and acquisition time. Here, we present a detailed study evaluating the performance of Airyscan as compared to confocal microscopy by imaging a variety of reference samples and biological specimens with different acquisition and processing parameters. We found that the processed Airyscan images at default deconvolution settings have a spatial resolution similar to that of conventional confocal imaging with a pinhole setting of 0.2 Airy Units, but with a significantly improved signal-to-noise-ratio. Further gains in the spatial resolution could be achieved by the use of enhanced deconvolution filter settings, but at a steady loss in the signal-to-noise ratio, which at more extreme settings resulted in significant data loss and image distortion
Development of the pump-probe nanoscopy architecture
Although modern optical microscopy allows the achievement of sub-diffraction resolution, most of the current techniques rely on a fluorescence contrast mechanism. Moreover, deep tissue imaging remains a challenging task especially for thick and highly scattering biological objects. The infrared absorption/saturation microscopy method is designed to overcome these issues [1, 2], having InfraRed Nanoscopy (IRN) as an instrumental perspective. The main idea behind IRN is an absorption/saturation effect similar to conventional pump-probe in which the first pump beam modifies the carrier density inside the sample, followed by intensity changes in the transmitted probe beam
Plasmon Bleaching Dynamics in Colloidal Gold-Iron Oxide Nanocrystal Heterodimers
Colloidal nanocrystal heterodimers composed of a plasmonic and a magnetic domain have been widely studied as potential materials for various applications in nanomedicine, biology, and photocatalysis. One of the most popular nanocrystal heterodimers is represented by a structure made of a Au domain and a iron oxide domain joined together. Understanding the nature of the interface between the two domains in such type of dimer and how this influences the energy relaxation processes is a key issue. Here, we present the first broad-band transient absorption study on gold/iron oxide nanocrystal heterodimers that explains how the energy relaxation is affected by the presence of such interface. We found faster electron-electron and electron-phonon relaxation times for the gold "nested" in the iron oxide domain in the heterodimers with respect to gold "only" nanocrystals, that is, free-standing gold nanocrystals in solution. We relate this effect to the decreased electron screening caused by spill-out of the gold electron distribution at gold/iron oxide interface