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Letter

Nature 436, 370-372 (21 July 2005) | doi:10.1038/nature03831; Received 27 March 2005; Accepted 11 May 2005

Massively parallel manipulation of single cells and microparticles using optical images

Pei Yu Chiou1, Aaron T. Ohta1 & Ming C. Wu1

  1. Department of Electrical Engineering and Computer Sciences, and Berkeley Sensor and Actuator Centre (BSAC), University of California at Berkeley, California 94720, USA

Correspondence to: Ming C. Wu1 Correspondence and requests for materials should be addressed to M.C.W. (Email: wu@eecs.berkeley.edu).

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The ability to manipulate biological cells and micrometre-scale particles plays an important role in many biological and colloidal science applications. However, conventional manipulation techniques—including optical tweezers1, 2, 3, 4, 5, 6, electrokinetic forces (electrophoresis7, 8, dielectrophoresis9, travelling-wave dielectrophoresis10, 11), magnetic tweezers12, 13, acoustic traps14 and hydrodynamic flows15, 16, 17—cannot achieve high resolution and high throughput at the same time. Optical tweezers offer high resolution for trapping single particles, but have a limited manipulation area owing to tight focusing requirements; on the other hand, electrokinetic forces and other mechanisms provide high throughput, but lack the flexibility or the spatial resolution necessary for controlling individual cells. Here we present an optical image-driven dielectrophoresis technique that permits high-resolution patterning of electric fields on a photoconductive surface for manipulating single particles. It requires 100,000 times less optical intensity than optical tweezers. Using an incoherent light source (a light-emitting diode or a halogen lamp) and a digital micromirror spatial light modulator, we have demonstrated parallel manipulation of 15,000 particle traps on a 1.3 times 1.0 mm2 area. With direct optical imaging control, multiple manipulation functions are combined to achieve complex, multi-step manipulation protocols.

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