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Immunofluorescence Staining of Drosophila Brains for the Single-Cell Imaging of Glial Cells

作者：

简介：

Overview

This article details a protocol for imaging glial cells in transgenic Drosophila brains using immunofluorescence techniques. The method emphasizes the importance of preserving tissue architecture and minimizing background staining for accurate visualization of cell interactions.

Key Study Components

Area of Science

Neuroscience
Cell Biology
Immunology

Background

Transgenic Drosophila models are valuable for studying glial cell types.
Cell-specific recombinase systems enable targeted expression of proteins.
Immunofluorescence is a key technique for visualizing cellular structures.
Proper fixation and blocking are crucial for reducing non-specific binding.

Purpose of Study

To visualize interactions between different glial cells in Drosophila brains.
To develop a reliable protocol for immunofluorescence imaging.
To enhance understanding of glial cell functions in the nervous system.

Methods Used

Preparation of transgenic Drosophila brains with specific glial cell markers.
Fixation of tissue to preserve architecture and protein integrity.
Blocking non-specific binding sites to improve staining specificity.
Sequential incubation with primary and secondary antibodies for visualization.

Main Results

Successful labeling of different glial cell types with distinct fluorophores.
Clear visualization of cell-cell interactions within the tissue.
Demonstration of the effectiveness of the immunofluorescence protocol.
Preservation of three-dimensional structure during imaging.

Conclusions

The protocol provides a robust method for studying glial cells in Drosophila.
Immunofluorescence can reveal important insights into glial cell interactions.
Future studies can build on this method to explore glial cell functions.

Frequently Asked Questions

What are transgenic Drosophila used for?

Transgenic Drosophila are used to study specific gene functions and cellular interactions in the nervous system.

Why is fixation important in this protocol?

Fixation preserves tissue architecture and stabilizes proteins for accurate imaging.

What role do blocking proteins play?

Blocking proteins reduce non-specific binding, enhancing the specificity of antibody staining.

How are antibodies used in this method?

Primary antibodies bind to specific epitopes, while secondary antibodies conjugated with fluorophores enable visualization.

What is the significance of using fluorophore-conjugated antibodies?

Fluorophore-conjugated antibodies allow for the visualization of specific proteins under a fluorescence microscope.

How does the imaging spacer help in the protocol?

The imaging spacer maintains the three-dimensional structure of the tissue during imaging.

Begin with brains from transgenic Drosophila flies, containing different glial cell types harboring a cell-specific recombinase system.

It drives the expression of a cell surface protein fused to different antigenic epitopes on the same type of cells.

Treat the tissue with a fixative to cross-link proteins and preserve the tissue architecture.

Wash to remove excess fixative.

Add blocking proteins to mask non-specific binding sites to reduce background staining.

Incubate the tissue with a primary antibody cocktail that binds to the different epitopes expressed on glial cells.

Wash to remove unbound primary antibodies.

Incubate with fluorophore-conjugated secondary antibodies that bind to the primary antibodies.

Wash to remove unbound secondary antibodies.

Mount the brain inside an imaging spacer and place a coverslip. The spacer creates a chamber for the tissue, preserving its three-dimensional structure.

Different cells of the same glial type labeled with different fluorophore-conjugated antibodies allow an understanding of cell-cell interactions.

Transfer the isolated brains using a P10 pipette tip into a 200-microliter microcentrifuge tube with fixative solution. Never handle the brains using forceps. Incubate the tissues protected from light. Avoid aspirating the brains during solution transfers.

To remove the fixative, use three or more 15-minute washes with washing solution. Then, block the tissues with blocking solution for 30 minutes or longer. Next, replace the blocking solution with primary antibodies diluted in wash solution, and incubate the brains overnight at 4 degrees Celsius.

To remove the primary antibodies, use three 1-hour washes in wash solution. Next, add secondary fluorophore conjugated antibodies in wash solution, and incubate the brains overnight at 4 degrees Celsius, or for 4 hours at room temperature. To completely wash off the unbound antibodies, use three 1-hour washes in wash solution, followed by a longer wash with PBS.

Then, mount the brains. Prepare two coverslips with an imaging spacer. In the spacer, and on the extra coverslip, apply 10 microliters of mounting medium with an anti-fade agent. Next, using a P10 pipette, transfer the brains to the coverslip, depositing them next to the medium along with some PBS. Do not let the tissue dry out.

Now, carefully move the brains into the mounting medium, using the pipette. And finally, move them to the medium in the spacer and arrange them with forceps. Then, remove the adhesive liner on the spacers and attach a coverslip. Secure the coverslip with a little pressure using forceps and proceed immediately with imaging.

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