Bioscience, Biotechnology, and Biochemistry
Online ISSN : 1347-6947
Print ISSN : 0916-8451

This article has now been updated. Please use the final version.

Development of Gateway Binary Vectors, R4L1pGWBs, for Promoter Analysis in Higher Plants
Shinya NAKAMURAAkihide NAKAOMakoto KAWAMUKAITetsuya KIMURASumie ISHIGUROTsuyoshi NAKAGAWA
Author information
Keywords: binary vector, Gateway cloning, plant transformation, promoter, reporter
JOURNAL FREE ACCESS Advance online publication

Article ID: 90720

The final version of this article is now available: Vol. 73 (2009) , No. 11 p.2556
Details
Download PDF (183K)
Download citation RIS

(compatible with EndNote, Reference Manager, ProCite, RefWorks)

BIB TEX

(compatible with BibDesk, LaTeX)

Text
How to download citation
Contact us
Abstract

We developed a new series of Gateway binary vectors for plant transformation, R4L1pGWBs, which allow easy construction of promoter:reporter clones. R4L1pGWBs contain a recombination attR4-attL1-reporter cassette, and thus an attL4-promoter-attR1 entry clone was efficiently incorporated by the Gateway LR reaction, resulting in the generation of an attB4-promoter-attB1-reporter construct. The reporters employed in R4L1pGWBs were β-glucuronidase (GUS), luciferase (LUC), enhanced yellow fluorescent protein (EYFP), enhanced cyan fluorescent protein (ECFP), G3 green fluorescent protein (G3GFP), G3GFP-GUS, and tag red fluorescent protein (TagRFP).

Content from these authors

This article cannot obtain the latest cited-by information.

© 2009 by Japan Society for Bioscience, Biotechnology, and Agrochemistry
Favorites & Alerts

Recently viewed articles
Predecessor

Bulletin of the Agricultural Chemical Society of Japan

Agricultural and Biological Chemistry

Share this page
feedback
 Top