JoVE Journal > Biology
Summary
Abstract
Protocol
Discussion
Acknowledgements
Materials
Referências
Tadução automática
Please note that all translations are automatically generated. Click here for the English version.
Biologia

Microinjection of mRNA and Morpholino Antisense Oligonucleotides in Zebrafish Embryos.

Published: May 07, 2009
doi:
10.3791/1113
,
1Department of Genetics,Yale University School of Medicine

Summary

Microinjection is a well-established and effective method for introducing foreign substances into fertilized zebrafish embryos. Here, we demonstrate a robust microinjection technique for performing mRNA overexpression, and morpholino oligonucleotide gene knockdown studies in zebrafish.

Abstract

An essential tool for investigating the role of a gene during development is the ability to perform gene knockdown, overexpression, and misexpression studies. In zebrafish (Danio rerio), microinjection of RNA, DNA, proteins, antisense oligonucleotides and other small molecules into the developing embryo provides researchers a quick and robust assay for exploring gene function in vivo. In this video-article, we will demonstrate how to prepare and microinject in vitro synthesized EGFP mRNA and a translational-blocking morpholino oligo against pkd2, a gene associated with autosomal dominant polycystic kidney disease (ADPKD), into 1-cell stage zebrafish embryos. We will then analyze the success of the mRNA and morpholino microinjections by verifying GFP expression and phenotype analysis. Broad applications of this technique include generating transgenic animals and germ-line chimeras, cell-fate mapping and gene screening. Herein we describe a protocol for overexpression of EGFP and knockdown of pkd2 by mRNA and morpholino oligonucleotide injection.

Protocol

Part 1: Preparation of micropipettes, and microinjection chamber plates Fabricate micropipettes by heating and pulling borosilicate glass capillary tubes (World Precision Instruments, Inc., 1B100-4) in a micropipette puller device (Sutter Instruments Inc., Flaming/Brown P-97). Store in a Petri dish on top of small amount of clay or adhesive tape. Pour 1.5% agarose (American Bioanlytical, Inc., AB00972-00500) in 1x E3 medium plates molded with wedge-shaped troughs that will serve as an easy method fo…

Discussion

Microinjection into zebrafish embryos is a well-established and robust technique for exploring the role of a particular gene in development. Applications include overexpression, misexpression, and knockdown assays of your gene of interest as well as epistatic analysis between multiple genes. Microinjection in zebrafish has been widely used for generating transgenic animals, and mapping cell fate in early blastula embryos5,6,7,8,9. In addition, the application of this technique serves as a key step in generatin…

Acknowledgements

This work was supported by the NIH and PKD foundation to ZS. All animal experiments were conducted according to Yale Animal Resources Center (YARC) and Institutional Animal Care and Use Committee (IACUC) guidelines.

Materials

Material Name Tipo Company Catalogue Number Comment
1x E3 Medium Reagent     5 mM NaCl
0.17 mM KCl
0.33 mM CaCl2
0.33 mM MgSO2
0.1% Methylene blue
All other materials are listed in the protocol.
DOWNLOAD MATERIALS LIST

Referências

  1. Westerfield, M. . The zebrafish book. A guide for the laboratory use of zebrafish (Danio rerio). , (2000).
  2. Nasevicius, A., Ekker, S. Effective targeted gene ‘knockdown’ in zebrafish. Nat Genet. 26, 216-220 (2000).
  3. Draper, B., Morcos, P., Kimmel, C. Inhibition of zebrafish fgf8 pre-mRNA splicing with morpholino oligos: a quantifiable method for gene knockdown. Genesis. 30, 154-156 (2001).
  4. Sun, Z., et al. A genetic screen in zebrafish identifies cilia genes as a principal cause of cystic kidney. Development. 131, 4085-4093 (2004).
  5. Stuart, G., McMurray, J., Westerfield, M. Replication, integration and stable germ-line transmission of foreign sequences injected into early zebrafish embryos. Development. 103, 403-412 (1988).
  6. Stuart, G., Vielkind, J., McMurray, J., Westerfield, M. Stable lines of transgenic zebrafish exhibit reproducible patterns of transgene expression. Development. 109, 577-584 (1990).
  7. Culp, P., Nüsslein-Volhard, C., Hopkins, N. High-frequency germ-line transmission of plasmid DNA sequences injected into fertilized zebrafish eggs. Proc Natl Acad Sci U S A. 88, 7953-7957 (1991).
  8. Strehlow, D., Heinrich, G., Gilbert, W. The fates of the blastomeres of the 16-cell zebrafish embryo. Development. 120, 1791-1798 (1994).
  9. Helde, K., Wilson, E., Cretekos, C., Grunwald, D. Contribution of early cells to the fate map of the zebrafish gastrula. Science. 265, 517-520 (1994).
  10. Lin, S., Long, W., Chen, J., Hopkins, N. Production of germ-line chimeras in zebrafish by cell transplants from genetically pigmented to albino embryos. Proc Natl Acad Sci U S A. 89, 4519-4523 (1992).
  11. Long, Q., et al. GATA-1 expression pattern can be recapitulated in living transgenic zebrafish using GFP reporter gene. Development. 124, 4105-4111 (1997).
  12. Murphey, R., Zon, L. Small molecule screening in the zebrafish. Methods. 39, 255-261 (2006).

Tags

MicroinjectionMRNAMorpholino Antisense OligonucleotidesZebrafish EmbryosGene KnockdownOverexpression StudiesMisexpression StudiesGene FunctionIn Vivo AssayEGFP MRNATranslational-blocking Morpholino OligoAutosomal Dominant Polycystic Kidney Disease (ADPKD)1-cell Stage EmbryosGFP ExpressionPhenotype AnalysisTransgenic AnimalsGerm-line ChimerasCell-fate MappingGene Screening
check_url/pt/1113?article_type=t

Play Video
PDF
DOI
DOWNLOAD MATERIALS LIST
Citar este artigo
Yuan, S., Sun, Z. Microinjection of mRNA and Morpholino Antisense Oligonucleotides in Zebrafish Embryos.. J. Vis. Exp. (27), e1113, doi:10.3791/1113 (2009).
Baixar citação
Reimpressões e Permissões

View Video

To prove you're not a robot, please enter the text in the image below

CAPTCHA Image
Play CAPTCHA Audio
Refresh Image