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Published April 1, 2017 | Published
Journal Article Open

Live Confocal Imaging of Developing Arabidopsis Flowers

Abstract

The study of plant growth and development has long relied on experimental techniques using dead, fixed tissues and lacking proper cellular resolution. Recent advances in confocal microscopy, combined with the development of numerous fluorophores, have overcome these issues and opened the possibility to study the expression of several genes simultaneously, with a good cellular resolution, in live samples. Live confocal imaging provides plant biologists with a powerful tool to study development, and has been extensively used to study root growth and the formation of lateral organs on the flanks of the shoot apical meristem. However, it has not been widely applied to the study of flower development, in part due to challenges that are specific to imaging flowers, such as the sepals that grow over the flower meristem, and filter out the fluorescence from underlying tissues. Here, we present a detailed protocol to perform live confocal imaging on live, developing Arabidopsis flower buds, using either an upright or an inverted microscope.

Additional Information

© 2017 JoVE. Creative Commons Attribution-NonCommercial-NoDerivs 3.0 Unported License. Date Published: 4/01/2017. The author wish to thank Prof. Elliot M. Meyerowitz for his support, and comments on the manuscript, as well as Ann Lavanway at Dartmouth College and Dr. Andres Collazo at the Biological Imaging Facility at Caltech for their help in solving technical issues with the live confocal imaging. Nathanaël Prunet's work is supported by the US National Institutes of Health through Grant R01 GM104244 to Elliot M. Meyerowitz. The author has nothing to disclose.

Attached Files

Published - jove-protocol-55156-live-confocal-imaging-of-developing-arabidopsis-flowers.pdf

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jove-protocol-55156-live-confocal-imaging-of-developing-arabidopsis-flowers.pdf

Additional details

Created:
August 19, 2023
Modified:
October 25, 2023