live imaging of the drosophila pupal eye using fluorescence microscopy

Live Imaging of the Drosophila Pupal Eye Using Fluorescence Microscopy

Using forceps, carefully lift and remove the operculum to expose the pupal head. Next, tear along the side of the pupal case to expose the area around one eye. Gently remove the pupa from the adhesive tape.Construct a small 15-square-millimeter frame from blotting paper, and punch a 5-millimeter hole in the middle. Immerse the frame in distilled water and place it in the center of a microscope slide. With a 30-cc syringe, squeeze out a uniform ring of petroleum jelly to surround the blotting paper frame.Next, add a small bead of petroleum jelly directly onto the slide. Carefully arrange the pupa on its side, and support it with the petroleum jelly bead. Place a coverslip on top of the petroleum jelly ring so that it contacts the epithelium above the eye. Gently compress the preparation to seal the coverslip against the petroleum jelly, and generate a small, flat contact surface between the pupil eye region and the coverslip.Image the pupal preparation using a fluorescent microscope. Capture serial sections through the apical domain of the eye neuroepithelium in the region of the adherens junction every seven minutes. Use appropriate deconvolution software to reduce background and enhance contrast of the serial section images.For each z stack file in LAS AF software, navigate to the Tools panel, select 3D Deconvolution, and click Apply. Generate a maximum projection, or MP image, for each deconvoluted stack file. Align each MP image to highlight individual cell behaviors and reduce distractions caused by organismal growth, using the built-in algorithms in Photoshop CS5.From the File tab of the Main menu, open Scripts, and select Load Files into Stack. Next, import the MP image files into the Load Layers panel. Make sure that the Attempt to Automatically Align Source Images option is not selected, otherwise the image data may be distorted. Once all MP files have loaded into the layers pane, check that all images are in chronological order, and that the earliest time point is at the top of the layer stack. Drag and drop them until they are ordered correctly if needed.Then select Auto-Align Layers. Choose Reposition and click OK.

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&#160;<figure class='table'><table class='ck-table-resized'><colgroup><col style='width:33.33%;'><col style='width:33.33%;'><col style='width:33.34%;'></colgroup><tbody><tr><td>GMR-GAL4; UAS-a-cat:GFP, ubi-DE-Cadherin:GFP ; + / SM5-TM6b</td><td>&#160;</td><td>&#160;</td></tr><tr><td>UAS-dcr-2; UAS-a-cat:GFP, ubi-DE-Cadherin:GFP; + / SM5-TM6b</td><td>&#160;</td><td>&#160;</td></tr><tr><td>25 x 75 x 1 mm glass microscope slide</td><td>Fisher Scientific</td><td>12-550-413</td></tr><tr><td>22 x 40 mm glass coverslip</td><td>VWR</td><td>48393-172</td></tr><tr><td>Forceps</td><td>Fine Science Tools</td><td>91150-20</td></tr><tr><td>Whatman 3 mm chromatography paper</td><td>Fisher Scientific</td><td>05-713-336</td></tr><tr><td>Vaseline</td><td>Fisher Scientific</td><td>19-086-291</td></tr><tr><td>30 ml syringe</td><td>Fisher Scientific</td><td>S7510-30</td></tr><tr><td>Adobe Photoshop CS5</td><td>Adobe</td><td>&#160;</td></tr><tr><td>Leica TCS SP5 DM microscope</td><td>Leica Microsystems</td><td>&#160;</td></tr><tr><td>LAS AF Version 2.6.0.7266 microscope software</td><td>Leica Microsystems</td><td>&#160;</td></tr></tbody></table></figure>

Source:&#160;<a href='https://app-jove-com.bdigitaluss.remotexs.co/v/52120/live-imaging-of-the-drosophila-pupal-eye'>Hellerman, M. B.,&#160;et al.&#160;Live-imaging of the&#160;Drosophila Pupal Eye.&#160;J. Vis. Exp.&#160;(2015)</a>The video demonstrates a live-imaging technique to study eye patterning in a&#160;Drosophila melanogaster pupa. Green fluorescent protein (GFP)-tagged markers enable visualization of cellular organization and differentiation during the formation of the developing eye structure.

Source:&#160;Hellerman, M. B.,&#160;et al.&#160;Live-imaging of the&#160;Drosophila Pupal Eye.&#160;J. Vis. Exp.&#160;(2015)The video demonstrates a ...

Begin with a transgenic&#160;Drosophila pupa with an exposed eye.Place the pupa on a jelly bead within a hydrated paper frame, surrounded by a jelly ring.The pupa&#8217;s eye contains GFP-tagged junction proteins that highlight cell boundaries in the developing eye&#8217;s neuroepithelium.Gently press a coverslip onto the pupal eye region.Under a fluorescent microscope, GFP-tagged junctions fluoresce, displaying the neuroepithelium organization.Take images at regular intervals across different depths and process the images to enhance contrast and minimize background noise.&#160;Align these images with increasing time intervals to track the developing neuroepithelium.Initially, primary cells form boundaries around photoreceptor cell clusters, while interommatidial cells or ICs arrange into a single layer.Later, the ICs differentiate into secondary and tertiary cells near photoreceptors.Finally, excess ICs are removed via programmed cell death, forming a hexagonal lattice that structures the organized eye.&#160;

13 Views. Live Imaging of the Drosophila Pupal Eye Using Fluorescence Microscopy

Video: Live Imaging of the Drosophila Pupal Eye Using Fluorescence Microscopy - Experiment

Long-term Live Imaging of Drosophila Eye Disc

Live imaging provides the ability to continuously track dynamic cellular and developmental processes in real time. Drosophila larval imaginal discs have been used to study many biological processes, such as cell proliferation, differentiation, growth, migration, apoptosis, competition, cell-cell signaling, and compartmental boundary formation. However, methods for the long-term ex vivo culture and live imaging of the imaginal discs have not been satisfactory, despite many efforts. Recently, we developed a method for the long-term ex vivo culture and live imaging of imaginal discs for up to 18 h. In addition to using a high insulin concentration in the culture medium, a low-melting agarose was also used to embed the disc to prevent it from drifting during the imaging period. This report uses the eye-antennal discs as an example. Photoreceptor R3/4-specific m&#948;0.5-Ga4 expression was followed to demonstrate that photoreceptor differentiation and ommatidial rotation can be observed during a 10 h live imaging period. This is a detailed protocol describing this simple method.

Long-term Live Imaging of Drosophila Eye Disc

This protocol describes a detailed method for the long-term ex vivo culture and live imaging of a Drosophila imaginal disc. It demonstrates photoreceptor differentiation and ommatidial rotation within the 10 h period of live imaging of the eye disc. The protocol is simple and does not require expensive setup.

A lungo termine Imaging in diretta di<em&gt; Drosophila</em&gt; Disco Eye

Live imaging provides the ability to continuously track dynamic cellular and developmental processes in real time. Drosophila larval imaginal discs have ...

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JoVE Journal

Biologia dello sviluppo

The Tomato/GFP-FLP/FRT Method for Live Imaging of Mosaic Adult Drosophila Photoreceptor Cells

The Drosophila eye is widely used as a model for studies of development and neuronal degeneration. With the powerful mitotic recombination technique, elegant genetic screens based on clonal analysis have led to the identification of signaling pathways involved in eye development and photoreceptor (PR) differentiation at larval stages. We describe here the Tomato/GFP-FLP/FRT method, which can be used for rapid clonal analysis in the eye of living adult Drosophila. Fluorescent photoreceptor cells are imaged with the cornea neutralization technique, on retinas with mosaic clones generated by flipase-mediated recombination. This method has several major advantages over classical histological sectioning of the retina: it can be used for high-throughput screening and has proved an effective method for identifying the factors regulating PR survival and function. It can be used for kinetic analyses of PR degeneration in the same living animal over several weeks, to demonstrate the requirement for specific genes for PR survival or function in the adult fly. This method is also useful for addressing cell autonomy issues in developmental mutants, such as those in which the establishment of planar cell polarity is affected.

The Tomato/GFP-FLP/FRT Method for Live Imaging of Mosaic Adult Drosophila Photoreceptor Cells

The Tomato/GFP-FLP/FRT method involves visualizing mosaic photoreceptor cells in living Drosophila. It can be used to follow individual photoreceptor cell fates in the retina for days or weeks. This method is ideal for studies of retinal degeneration and neurodegenerative diseases or photoreceptor cell development.

Il pomodoro / GFP-FLP / FRT Metodo per Live Imaging del Mosaico adulti<em&gt; Drosophila</em&gt; cellule fotorecettrici

The Drosophila eye is widely used as a model  for studies of development and neuronal degeneration. With the powerful mitotic  recombination technique, ...

Biologia

Studying Membrane Protein Trafficking in Drosophila Photoreceptor Cells Using eGFP-Tagged Proteins

Membrane protein trafficking regulates the incorporation and removal of receptors and ion channels into the plasma membrane. This process is fundamentally important for cell function and cell integrity of neurons. Drosophila photoreceptor cells have become a model for studying membrane protein trafficking. Besides rhodopsin, which upon illumination becomes internalized from the photoreceptor membrane and is degraded, the transient receptor potential-like (TRPL) ion channel in Drosophila exhibits a light-dependent translocation between the rhabdomeral photoreceptor membrane (where it is located in the dark) and the photoreceptor cell body (to which it is transported upon illumination). This intracellular transport of TRPL can be studied in a simple and non-invasive way by expressing eGFP-tagged TRPL in photoreceptor cells. The eGFP fluorescence can then be observed either in the deep pseudopupil or by water immersion microscopy. These methods allow detection of fluorescence in the intact eye and are therefore useful for high-throughput assays and genetic screens for Drosophila mutants defective in TRPL translocation. Here, the preparation of flies, the microscopic techniques, as well as quantification methods used to study this light-triggered translocation of TRPL are explained in detail. These methods can be applied also for trafficking studies on other Drosophila photoreceptor proteins, for example, rhodopsin. In addition, by using eGFP-tagged rhabdomeral proteins, these methods can be used to assess the degeneration of photoreceptor cells.

Studying Membrane Protein Trafficking in Drosophila Photoreceptor Cells Using eGFP-Tagged Proteins

Here, non-invasive methods are described for localization of photoreceptor membrane proteins and assessment of retinal degeneration in the Drosophila compound eye using eGFP fluorescence.

Studio del traffico proteico di membrana nelle cellule fotorecettrici di Drosophila utilizzando proteine con tag eGFP

Membrane protein trafficking regulates the incorporation and removal of receptors and ion channels into the plasma membrane. This process is fundamentally ...

Live Imaging of the Drosophila Pupal Eye Using Fluorescence Microscopy

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Live Imaging of the Drosophila Pupal Eye Using Fluorescence Microscopy