Gradient force leading to trapping, mass transfer by local heating, and molecular reorientation following laser polarization are intimately coupled with molecular cluster and aggregate formation due to their intermolecular interactions, which depend on whether the trapping position is at the interface/surface or in solution.
In this Account, we summarize our systematic BI 6727 studies on laser Inhibitors,Modulators,Libraries trapping chemistry and present some new advances and our future perspectives. We describe the laser trapping of nanoparticles, polymers, and amino acid clusters in solution by focusing a continuous wave 1064 nm laser beam on the molecules of interest and consider their dynamics and mechanism.
In dilute solution, nanoparticles with weak mutual interactions are individually trapped Inhibitors,Modulators,Libraries at the focal point, while laser trapping of nanoparticles in concentrated solution assembles and confines numerous particles at Inhibitors,Modulators,Libraries the focal spot. The assembly of polymers during their laser trapping extends Inhibitors,Modulators,Libraries out from the focal point because of the interpolymer interactions, heat transfer, and solvent flow. When the trapping laser is focused at an interface between a thin heavy water solution film of glycine and a glass substrate, the assembled molecules nucleate and evolve to a liquid liquid phase separation, or they will crystallize Entinostat if the trapping laser is focused on the solution surface. Laser trapping can induce spatiotemporally the liquid and solid nucleation of glycine, and the dense liquid droplet or crystal formed can grow to a bulk scale. We can control the polymorph of the formed glycine crystal selectively by tuning trapping laser polarization and power.
These results provide a new approach to elucidate dynamics and mechanism of crystallization and are the fundamental basis for studying not only enantioselective crystallization but also confined polymerization, trapping dynamics by ultrashort laser pulses, and resonance effect in laser trapping.”
“Single-molecule fluorescence measurements allow researchers to study asynchronous dynamics inhibitor manufacture and expose molecule-to-molecule structural and behavioral diversity, which contributes to the understanding of biological macromolecules. To provide measurements that are most consistent with the native environment of biomolecules, researchers would like to conduct these measurements in the solution phase if possible. However, diffusion typically limits the observation time to approximately 1 ms in many solution-phase single-molecule assays. Although surface immobilization is widely used to address this problem, this process can perturb the system being studied and contribute to the observed heterogeneity.