Moving live dissociated neurons with an optical tweezer
- Creators
- Pine, Jerome
- Chow, Gary
Abstract
The use of an optical tweezer for moving dissociated neurons was studied. The main features of the tweezers are outlined as well as the general principles of its operation. Infrared beams at 980 and 1064 nm were used, focused so as to make a trap for holding neurons and moving them. Absorption by cells at those wavelengths is very small. Experiments were done to evaluate nonsticky substrate coatings, from which neurons could be easily lifted with the tweezers. The maximum speed of cell movement as a function of laser power was determined. Detailed studies of the damage to cells as a function of beam intensity and time of exposure were made. The 980 nm beam was much less destructive, for reasons that are not understood, and could be used to safely move cells through distances of millimeters in times of seconds. An illustrative application of the use of the tweezers to load neurons without damage into plastic cages on a glass substrate was presented. The conclusion is that optical tweezers are an accessible and practical tool for helping to establish neuron cultures of cells placed in specific locations.
Additional Information
© 2009 IEEE. Manuscript received May 23, 2008; revised August 14, 2008. First published October 31, 2008; current version published May 6, 2009. This work was supported in part by the National Institutes of Health under Grant NS-044134.Attached Files
Published - Pine2009p2570Ieee_T_Bio-Med_Eng.pdf
Files
| Name | Size | Download all |
|---|---|---|
|
md5:168440df290be3c6d6a5848ddbb6e9f6
|
328.6 kB | Preview Download |
Additional details
- Eprint ID
- 14349
- Resolver ID
- CaltechAUTHORS:20090601-153814029
- NS-044134
- NIH
- Created
-
2009-08-17Created from EPrint's datestamp field
- Updated
-
2021-11-08Created from EPrint's last_modified field