Mounting of Embryos, Larvae, and Pupae for Live Drosophila Dendritic Arborization Neuron Imaging

Fangke Xu; Jason Y Tann; Oliver R Wilkes; Minami Kimura; Li-Foong Yoong; Adrian W Moore

doi:10.1101/pdb.prot108149

Mounting of Embryos, Larvae, and Pupae for Live Drosophila Dendritic Arborization Neuron Imaging

Cold Spring Harb Protoc. 2023 Dec 26. doi: 10.1101/pdb.prot108149. Online ahead of print.

Authors

Fangke Xu¹, Jason Y Tann¹, Oliver R Wilkes^{1

2}, Minami Kimura¹, Li-Foong Yoong¹, Adrian W Moore³

Affiliations

¹ Laboratory for Neurodiversity, RIKEN Center for Brain Science, Wako-shi, 350-0106, Japan.
² Department of Cellular and Molecular Biology, Institute for Translational Medicine, University of Liverpool, Liverpool L69 3BX, United Kingdom.
³ Laboratory for Neurodiversity, RIKEN Center for Brain Science, Wako-shi, 350-0106, Japan adrian.moore@riken.jp.

PMID: 38148167
DOI: 10.1101/pdb.prot108149

Abstract

Live imaging approaches are essential for monitoring how neurons go through a coordinated series of differentiation steps in their native mechanical and chemical environment. These imaging approaches also allow the study of dynamic subcellular processes such as cytoskeleton remodeling and the movement of organelles. Drosophila dendritic arborization (da) neurons are a powerful experimental system for studying the dendrite arbor in live animals. da neurons are located on the internal surface of the body wall and, therefore, are easily accessible for imaging. Moreover, many genetic tools target da neurons to disrupt genes or proteins of interest and allow the investigator to visualize fluorescent markers and endogenously tagged proteins in the neurons. This protocol introduces methods for preparing and mounting intact Drosophila embryos, larvae, and pupae, allowing live imaging of dynamic cellular processes in da neurons.