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The Preparation of Drosophila Embryos for Live-Imaging Using the Hanging Drop Protocol

Green fluorescent protein (GFP)-based timelapse live-imaging is a powerful technique for studying the genetic regulation of dynamic processes such as tissue morphogenesis, cell-cell adhesion, or cell death. Drosophila embryos expressing GFP are readily imaged using either stereoscopic or confocal mi...

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Detalles Bibliográficos
Autores principales: Reed, Bruce H., McMillan, Stephanie C., Chaudhary, Roopali
Formato: Texto
Lenguaje:English
Publicado: MyJove Corporation 2009
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2789762/
https://www.ncbi.nlm.nih.gov/pubmed/19287353
http://dx.doi.org/10.3791/1206
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author Reed, Bruce H.
McMillan, Stephanie C.
Chaudhary, Roopali
author_facet Reed, Bruce H.
McMillan, Stephanie C.
Chaudhary, Roopali
author_sort Reed, Bruce H.
collection PubMed
description Green fluorescent protein (GFP)-based timelapse live-imaging is a powerful technique for studying the genetic regulation of dynamic processes such as tissue morphogenesis, cell-cell adhesion, or cell death. Drosophila embryos expressing GFP are readily imaged using either stereoscopic or confocal microscopy. A goal of any live-imaging protocol is to minimize detrimental effects such as dehydration and hypoxia. Previous protocols for preparing Drosophila embryos for live-imaging analysis have involved placing dechorionated embryos in halocarbon oil and sandwiching them between a halocarbon gas-permeable membrane and a coverslip(1-3). The introduction of compression through mounting embryos in this manner represents an undesirable complication for any biomechanical-based analysis of morphogenesis. Our method, which we call the hanging drop protocol, results in excellent viability of embryos during live imaging and does not require that embryos be compressed. Briefly, the hanging drop protocol involves the placement of embryos in a drop of halocarbon oil that is suspended from a coverslip, which is, in turn, fixed in position over a humid chamber. In addition to providing gas exchange and preventing dehydration, this arrangement takes advantage of the buoyancy of embryos in halocarbon oil to prevent them from drifting out of position during timelapse acquisition. This video describes in detail how to collect and prepare Drosophila embryos for live imaging using the hanging drop protocol. This protocol is suitable for imaging dechorionated embryos using stereomicroscopy or any upright compound fluorescence microscope.
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spelling pubmed-27897622011-03-15 The Preparation of Drosophila Embryos for Live-Imaging Using the Hanging Drop Protocol Reed, Bruce H. McMillan, Stephanie C. Chaudhary, Roopali J Vis Exp Developmental Biology Green fluorescent protein (GFP)-based timelapse live-imaging is a powerful technique for studying the genetic regulation of dynamic processes such as tissue morphogenesis, cell-cell adhesion, or cell death. Drosophila embryos expressing GFP are readily imaged using either stereoscopic or confocal microscopy. A goal of any live-imaging protocol is to minimize detrimental effects such as dehydration and hypoxia. Previous protocols for preparing Drosophila embryos for live-imaging analysis have involved placing dechorionated embryos in halocarbon oil and sandwiching them between a halocarbon gas-permeable membrane and a coverslip(1-3). The introduction of compression through mounting embryos in this manner represents an undesirable complication for any biomechanical-based analysis of morphogenesis. Our method, which we call the hanging drop protocol, results in excellent viability of embryos during live imaging and does not require that embryos be compressed. Briefly, the hanging drop protocol involves the placement of embryos in a drop of halocarbon oil that is suspended from a coverslip, which is, in turn, fixed in position over a humid chamber. In addition to providing gas exchange and preventing dehydration, this arrangement takes advantage of the buoyancy of embryos in halocarbon oil to prevent them from drifting out of position during timelapse acquisition. This video describes in detail how to collect and prepare Drosophila embryos for live imaging using the hanging drop protocol. This protocol is suitable for imaging dechorionated embryos using stereomicroscopy or any upright compound fluorescence microscope. MyJove Corporation 2009-03-13 /pmc/articles/PMC2789762/ /pubmed/19287353 http://dx.doi.org/10.3791/1206 Text en Copyright © 2009, Journal of Visualized Experiments http://creativecommons.org/licenses/by/2.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Developmental Biology
Reed, Bruce H.
McMillan, Stephanie C.
Chaudhary, Roopali
The Preparation of Drosophila Embryos for Live-Imaging Using the Hanging Drop Protocol
title The Preparation of Drosophila Embryos for Live-Imaging Using the Hanging Drop Protocol
title_full The Preparation of Drosophila Embryos for Live-Imaging Using the Hanging Drop Protocol
title_fullStr The Preparation of Drosophila Embryos for Live-Imaging Using the Hanging Drop Protocol
title_full_unstemmed The Preparation of Drosophila Embryos for Live-Imaging Using the Hanging Drop Protocol
title_short The Preparation of Drosophila Embryos for Live-Imaging Using the Hanging Drop Protocol
title_sort preparation of drosophila embryos for live-imaging using the hanging drop protocol
topic Developmental Biology
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2789762/
https://www.ncbi.nlm.nih.gov/pubmed/19287353
http://dx.doi.org/10.3791/1206
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