Difference between revisions of "Main Page"

Revision as of 13:05, 2 February 2007

The Tol2kit

Tol2kit v1.0, released February 2007

Generating stable transgenic zebrafish lines has historically been laborious, for three reasons:

• Building transgenesis constructs by conventional subcloning can be difficult, especially when using long coding or regulatory sequences
• Injecting plasmid DNA yields mosaic transient expression and low germline transgenesis rates
• When screening for stable integrations, transgenes that express fluorescent proteins (e.g. GFP) are easy to detect, but other transgenes are not.

The Tol2kit uses site-specific recombination-based cloning (multisite Gateway technology) to allow quick, modular assembly of promoter-coding sequence-3' tag constructs in a Tol2 transposon backbone.

It includes a variety of widely-useful entry clones, including hsp70 and beta-actin promoters; cytoplasmic, nuclear, and membrane-localized fluorescent proteins; and IRES-driven GFP cassettes for bicistronic expression. It includes two Tol2-based destination vector, one with a cmlc2:egfp transgenesis marker.

About this site

This wiki provides the documentation for the Tol2kit; it is maintained by the Chien lab. Please bear with us; it went live on 28 January and there are still many sections that are under construction.

• Basic Gateway principles
• List of entry and destination vectors
• Protocols
• Components used for the Tol2kit
• Sample results with the Tol2kit
• References

We are currently preparing a methods paper describing the Tol2kit. If you have questions or comments, please post them on the Tol2kit blog.

Links

• Tol2kit blog for discussion and questions about the system
• Lawson lab Gateway site
• Invitrogen multisite Gateway manual 11/29/04

Wiki help

Consult the User's Guide for information on using the wiki software.

• Configuration settings list
• MediaWiki FAQ