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Cell-specific microarray profiling experiments reveal a comprehensive picture of gene expression in the C. elegans nervous system

BACKGROUND: With its fully sequenced genome and simple, well-defined nervous system, the nematode Caenorhabditis elegans offers a unique opportunity to correlate gene expression with neuronal differentiation. The lineal origin, cellular morphology and synaptic connectivity of each of the 302 neurons...

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Autores principales: Von Stetina, Stephen E, Watson, Joseph D, Fox, Rebecca M, Olszewski, Kellen L, Spencer, W Clay, Roy, Peter J, Miller, David M
Formato: Texto
Lenguaje:English
Publicado: BioMed Central 2007
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2323220/
https://www.ncbi.nlm.nih.gov/pubmed/17612406
http://dx.doi.org/10.1186/gb-2007-8-7-r135
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author Von Stetina, Stephen E
Watson, Joseph D
Fox, Rebecca M
Olszewski, Kellen L
Spencer, W Clay
Roy, Peter J
Miller, David M
author_facet Von Stetina, Stephen E
Watson, Joseph D
Fox, Rebecca M
Olszewski, Kellen L
Spencer, W Clay
Roy, Peter J
Miller, David M
author_sort Von Stetina, Stephen E
collection PubMed
description BACKGROUND: With its fully sequenced genome and simple, well-defined nervous system, the nematode Caenorhabditis elegans offers a unique opportunity to correlate gene expression with neuronal differentiation. The lineal origin, cellular morphology and synaptic connectivity of each of the 302 neurons are known. In many instances, specific behaviors can be attributed to particular neurons or circuits. Here we describe microarray-based methods that monitor gene expression in C. elegans neurons and, thereby, link comprehensive profiles of neuronal transcription to key developmental and functional properties of the nervous system. RESULTS: We employed complementary microarray-based strategies to profile gene expression in the embryonic and larval nervous systems. In the MAPCeL (Microarray Profiling C. elegans cells) method, we used fluorescence activated cell sorting (FACS) to isolate GFP-tagged embryonic neurons for microarray analysis. To profile the larval nervous system, we used the mRNA-tagging technique in which an epitope-labeled mRNA binding protein (FLAG-PAB-1) was transgenically expressed in neurons for immunoprecipitation of cell-specific transcripts. These combined approaches identified approximately 2,500 mRNAs that are highly enriched in either the embryonic or larval C. elegans nervous system. These data are validated in part by the detection of gene classes (for example, transcription factors, ion channels, synaptic vesicle components) with established roles in neuronal development or function. Of particular interest are 19 conserved transcripts of unknown function that are also expressed in the mammalian brain. In addition to utilizing these profiling approaches to define stage-specific gene expression, we also applied the mRNA-tagging method to fingerprint a specific neuron type, the A-class group of cholinergic motor neurons, during early larval development. A comparison of these data to a MAPCeL profile of embryonic A-class motor neurons identified genes with common functions in both types of A-class motor neurons as well as transcripts with roles specific to each motor neuron type. CONCLUSION: We describe microarray-based strategies for generating expression profiles of embryonic and larval C. elegans neurons. These methods can be applied to particular neurons at specific developmental stages and, therefore, provide an unprecedented opportunity to obtain spatially and temporally defined snapshots of gene expression in a simple model nervous system.
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spelling pubmed-23232202008-04-19 Cell-specific microarray profiling experiments reveal a comprehensive picture of gene expression in the C. elegans nervous system Von Stetina, Stephen E Watson, Joseph D Fox, Rebecca M Olszewski, Kellen L Spencer, W Clay Roy, Peter J Miller, David M Genome Biol Research BACKGROUND: With its fully sequenced genome and simple, well-defined nervous system, the nematode Caenorhabditis elegans offers a unique opportunity to correlate gene expression with neuronal differentiation. The lineal origin, cellular morphology and synaptic connectivity of each of the 302 neurons are known. In many instances, specific behaviors can be attributed to particular neurons or circuits. Here we describe microarray-based methods that monitor gene expression in C. elegans neurons and, thereby, link comprehensive profiles of neuronal transcription to key developmental and functional properties of the nervous system. RESULTS: We employed complementary microarray-based strategies to profile gene expression in the embryonic and larval nervous systems. In the MAPCeL (Microarray Profiling C. elegans cells) method, we used fluorescence activated cell sorting (FACS) to isolate GFP-tagged embryonic neurons for microarray analysis. To profile the larval nervous system, we used the mRNA-tagging technique in which an epitope-labeled mRNA binding protein (FLAG-PAB-1) was transgenically expressed in neurons for immunoprecipitation of cell-specific transcripts. These combined approaches identified approximately 2,500 mRNAs that are highly enriched in either the embryonic or larval C. elegans nervous system. These data are validated in part by the detection of gene classes (for example, transcription factors, ion channels, synaptic vesicle components) with established roles in neuronal development or function. Of particular interest are 19 conserved transcripts of unknown function that are also expressed in the mammalian brain. In addition to utilizing these profiling approaches to define stage-specific gene expression, we also applied the mRNA-tagging method to fingerprint a specific neuron type, the A-class group of cholinergic motor neurons, during early larval development. A comparison of these data to a MAPCeL profile of embryonic A-class motor neurons identified genes with common functions in both types of A-class motor neurons as well as transcripts with roles specific to each motor neuron type. CONCLUSION: We describe microarray-based strategies for generating expression profiles of embryonic and larval C. elegans neurons. These methods can be applied to particular neurons at specific developmental stages and, therefore, provide an unprecedented opportunity to obtain spatially and temporally defined snapshots of gene expression in a simple model nervous system. BioMed Central 2007 2007-07-05 /pmc/articles/PMC2323220/ /pubmed/17612406 http://dx.doi.org/10.1186/gb-2007-8-7-r135 Text en Copyright © 2007 Von Stetina et al.; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an open access article distributed under the terms of the Creative Commons Attribution License ( (http://creativecommons.org/licenses/by/2.0) ), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Research
Von Stetina, Stephen E
Watson, Joseph D
Fox, Rebecca M
Olszewski, Kellen L
Spencer, W Clay
Roy, Peter J
Miller, David M
Cell-specific microarray profiling experiments reveal a comprehensive picture of gene expression in the C. elegans nervous system
title Cell-specific microarray profiling experiments reveal a comprehensive picture of gene expression in the C. elegans nervous system
title_full Cell-specific microarray profiling experiments reveal a comprehensive picture of gene expression in the C. elegans nervous system
title_fullStr Cell-specific microarray profiling experiments reveal a comprehensive picture of gene expression in the C. elegans nervous system
title_full_unstemmed Cell-specific microarray profiling experiments reveal a comprehensive picture of gene expression in the C. elegans nervous system
title_short Cell-specific microarray profiling experiments reveal a comprehensive picture of gene expression in the C. elegans nervous system
title_sort cell-specific microarray profiling experiments reveal a comprehensive picture of gene expression in the c. elegans nervous system
topic Research
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2323220/
https://www.ncbi.nlm.nih.gov/pubmed/17612406
http://dx.doi.org/10.1186/gb-2007-8-7-r135
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