Long-term microfluidic cultures of myotube microarrays for high-throughput focal stimulation.

Nat Protoc

Department of Bioengineering, University of Washington, Box 355061, Seattle, Washington 98195-2255, USA.

Published: June 2007

We have developed a microfluidic cell culture method that allows for the formation of linear isolated myotubes organized in a parallel microarray. Attachment and spreading of cells are confined within microtracks of cell-adherent proteins separated by a protein-repellent coating. Signaling molecules or other molecules of interest can be focally delivered to the myotubes using heterogeneous microfluidic streams. We have used the method to focally deliver agrin (a molecule implicated as a postsynaptic organizer), which leads to localized acetylcholine receptor clustering. These techniques can be modified to accommodate other cell types and can be adapted to virtually any bioactive molecule such as signaling factors or drugs. This protocol features two major techniques that can be utilized simultaneously or independently to (i) micropattern cells using surface chemical modification and (ii) use a microfluidic platform for culturing and focal stimulation of cells with molecules of interest. Device design, fabrication and assembly can be completed in 3 days.

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http://www.ncbi.nlm.nih.gov/pmc/articles/PMC4393750PMC
http://dx.doi.org/10.1038/nprot.2006.123DOI Listing

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