PLoS ONE (Jan 2014)

Isolation of specific neurons from C. elegans larvae for gene expression profiling.

  • W Clay Spencer,
  • Rebecca McWhirter,
  • Tyne Miller,
  • Pnina Strasbourger,
  • Owen Thompson,
  • LaDeana W Hillier,
  • Robert H Waterston,
  • David M Miller

DOI
https://doi.org/10.1371/journal.pone.0112102
Journal volume & issue
Vol. 9, no. 11
p. e112102

Abstract

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The simple and well-described structure of the C. elegans nervous system offers an unprecedented opportunity to identify the genetic programs that define the connectivity and function of individual neurons and their circuits. A correspondingly precise gene expression map of C. elegans neurons would facilitate the application of genetic methods toward this goal. Here we describe a powerful new approach, SeqCeL (RNA-Seq of C. elegans cells) for producing gene expression profiles of specific larval C. elegans neurons.We have exploited available GFP reporter lines for FACS isolation of specific larval C. elegans neurons for RNA-Seq analysis. Our analysis showed that diverse classes of neurons are accessible to this approach. To demonstrate the applicability of this strategy to rare neuron types, we generated RNA-Seq profiles of the NSM serotonergic neurons that occur as a single bilateral pair of cells in the C. elegans pharynx. These data detected >1,000 NSM enriched transcripts, including the majority of previously known NSM-expressed genes.This work offers a simple and robust protocol for expression profiling studies of post-embryonic C. elegans neurons and thus provides an important new method for identifying candidate genes for key roles in neuron-specific development and function.