In this mini-symposium, our special guest-experts discuss the role OT can play in the search for new and innovative analysis and characterization methods, and how the technique can contribute towards a more in-depth understanding of nanomechanical processes.
The Nobel Prize winning Optical Tweezers (OT) technique enables the non-invasive, nanometer-precise manipulation of molecules and nanoparticles and the simultaneous application and recording of the piconewton forces acting on them. OT can be used to perform optical, thermodynamic or nanomanipulation experiments, to trigger, visualize, and quantify molecular interactions, and to characterize mechanical properties such as adhesion, viscoelasticity, or deformation.
Presentations in this symposium include an introduction to Novel Applications of Optical Tweezers in the Physical and Life Sciences, as well as individual sessions focused on how OT can be used to study:
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Dr. Julie Goyon and Antoine Aubel, Laboratoire Navier, Université Gustave Eiffel - ENPC - CNRS, France
While the ageing behavior of dense suspensions or pastes at rest is almost exclusively attributed to structural dynamics, a set of experiments conducted on dense aqueous silica suspensions allowed us to identify another ageing process: contact-controlled ageing. We have investigated the origin of shear modulus and yield strength ageing in dense aqueous silica suspensions at moderate ionic forces. By combining rheometry and confocal microscopy, we first showed that the elastic modulus and yield stress of these suspensions at rest grow logarithmically with time, while their structural evolution is rapidly arrested by the formation of interparticle contacts [[i]]. So these suspensions age in the absence of structural rearrangement. Then, by performing three-point optical tweezer (OT) bending tests on particle rods, we showed that both the rolling stiffness and rolling threshold grow logarithmically in time. By comparing the results of the measurements on the particle contact properties with the results of the rheometry tests, we were able to show that ageing of interparticle contacts governs both shear modulus ageing and yield stress ageing of these dense aqueous silica suspensions [[ii]-[iii]].
REFERENCES:
Dr. Soma Dhakal, Virginia Commonwealth University, USA
DNA Double-strand breaks (DSBs) are among the most detrimental types of DNA damage. The repair of DSBs occurs via a process called homologous recombination (HR), which involves several DNA-binding proteins. Therefore, to have a better insight into the repair mechanism and origin of repair defects, we need a better understanding of how these proteins interact with DNA and DNA intermediates such as Holliday junctions (HJs). Using dual-trap optical tweezers, we recently studied the biomechanics of HJ and a prokaryotic protein RuvA and showed that the RuvA protein not only stabilizes the HJ but also assists in its refolding.
Dr. Pierre-Henri Puech, INSERM, Adhesion & Inflammation, Marseille, France
In our labs, we use a collection of force based biophysical techniques to study early T cell mechanotransduction (Atomic Force Microscopy (AFM)1,2, Biomembrane Force Probe (BFP), Flow Chamber3, Traction Force Microscopy, Optical Tweezers), smart decorated substrates, and advanced quantitative surface microscopies4–6. We focus on the particular moment where the ligation of the T cell receptors (TCR) with antigens displayed on partner substrates (antigen-presenting cell - APC) is the very first step in triggering the T cells response. It has been demonstrated that this passes through the formation of the so called 'immune synapse' (IS) that involves additional molecules like integrins and CD45 7.
The mechanosensitive nature of the T-cell/APC and the mechanics of the TCR-complex is currently being studied extensively, but the question of the existence, if any, of a direct physical interaction between the TCR and the cytoskeleton is still not known8. Such an interaction could have a profound impact on the motion and recruitment of TCR at the interface between the T cell and the partner cell or substrate. In particular, it may explain complex behaviour, like biphasic response to substrate elasticity. The proposed mechanism crucially depends on this coupling9,10.
To explore this link, we used optical tweezers to pull membrane tubes from T cells using different antibodies as a handle, each targeting a given protein present at the IS, here, TCR/CD3, LFA1, CD45. We also pulled nanotubes after disrupting the actin cytoskeleton using Latrunculin. We then developed a theoretical mechanical model that retains the key biophysical properties of the coupled system, consisting of the T cell and the bound receptor/ligand pair on one hand and the force transducer on the other.
The model provides a fine description of the force curves and the fitting strategy we developed allowed us to extract information on cellular and molecular viscoelastic parameters. Our model also enables the estimation of key viscoelastic parameters, which account for the stiffness of the ligand/receptor complex, the cell rigidity, and viscosity. To process our large datasets, composed of both membrane tube pulling and handle/protein detachment events, we developed a refined post-fit data processing strategy to recover molecular information from the latter in the frame of our model to strengthen our statistics.
Our results suggest that the mechanical link with the cytoskeleton is modulated for the different molecules in the immune synapse such as TCR, LFA-1 and CD45. Finally, our model allows us to propose a quantitative description of the intra-cellular molecular bonds, which are usually quite difficult to infer or impossible to measure, from externally pulling nano-tubes, a rather easy experimental method adaptable to other force-based techniques such as AFM or BFP.
REFERENCES:
Dr. Julie Goyon
Laboratoire Navier, Université Gustave Eiffel - ENPC - CNRS, France
Antoine Aubel
Laboratoire Navier, Université Gustave Eiffel - ENPC - CNRS, France
Dr. Soma Dhakal
Virginia Commonwealth University, USA
Dr. Pierre-Henri Puech
INSERM, Adhesion & Inflammation, Marseille, France