4.6 Article

Opto-Thermophoretic Attraction, Trapping, and Dynamic Manipulation of Lipid Vesicles

Journal

LANGMUIR
Volume 34, Issue 44, Pages 13252-13262

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/acs.langmuir.8b01979

Keywords

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Funding

  1. Beckman Young Investigator Program
  2. Army Research Office [W911NF-17-1-0561]
  3. National Aeronautics and Space Administration Early Career Faculty Award [80NSSC17K0520]
  4. National Institute of General Medical Sciences of the National Institutes of Health [DP2GM128446]
  5. German Academic Exchange Service (DAAD) from funds of the German Federal Ministry of Education and Research (BMBF) [57429511]

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Lipid vesicles are important biological assemblies, which are critical to biological transport processes, and vesicles prepared in the lab are a workhorse for studies of drug delivery, protein unfolding, biomolecular interactions, compartmentalized chemistry, and stimuli-responsive sensing. The current method of using optical tweezers for holding lipid vesicles in place for single-vesicle studies suffers from limitations such as high optical power, rigorous optics, and small difference in the refractive indices of vesicles and water. Herein, we report the use of plasmonic heating to trap vesicles in a temperature gradient, allowing long-range attraction, parallel trapping, and dynamic manipulation. The capabilities and limitations with respect to thermal effects on vesicle structure and optical spectroscopy are discussed. This simple approach allows vesicle manipulation using down to 3 orders of magnitude lower optical power and at least an order of magnitude higher trapping stiffness per unit power than traditional optical tweezers while using a simple optical setup. In addition to the benefit provided by the relaxation of these technical constraints, this technique can complement optical tweezers to allow detailed studies on thermophoresis of optically trapped vesicles and effects of locally generated thermal gradients on the physical properties of lipid vesicles. Finally, the technique itself and the large-scale collection of vesicles have huge potential for future studies of vesicles relevant to detection of exosomes, lipid-raft formation, and other areas relevant to the life sciences.

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