ex vivo calcium imaging to study drosophila brain responses to neuropeptides

Ex Vivo Calcium Imaging to Study Drosophila Brain Responses to Neuropeptides

To acquire calcium fluorescence images, place the imaging chamber containing the brain explant under the microscope. Lower the objective lens until it touches the PBS. And under brightfield illumination, position the brain and bring it into focus.Switch to fluorescent light and adjust the focus on the GCaMP6 labeled cells. Start the acquisition at 250 milliseconds per frame at a resolution of 512 by 512 pixels in water-cooled mode. Then, adjust the exposure time to obtain the fluorescence values within the CCD camera dynamic range, but not lower than 1,000 arbitrary units with 16-bit images.Once the imaging parameters are determined, take the images for one minute before peptide administration to detect baseline signal intensities. Subsequently, apply the test peptide directly by pipetting 100 microliters of the prepared peptide solution into the larval bath. Record the GCaMP6 emission for a few minutes.

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filter</td></tr><tr style='height:20px;'><td style='background-color:#ffffff;color:#1a202c;font-family:Arial;font-size:10pt;font-weight:normal;overflow:hidden;padding:0px 3px;vertical-align:bottom;white-space:normal;word-wrap:break-word;wrap-strategy:4;'>&#181;Manager</td><td style='background-color:#ffffff;color:#1a202c;font-family:Arial;font-size:10pt;font-weight:normal;overflow:hidden;padding:0px 3px;text-align:center;vertical-align:bottom;white-space:normal;word-wrap:break-word;wrap-strategy:4;'>Open Imaging, Inc.</td><td style='background-color:#ffffff;color:#1a202c;font-family:Arial;font-size:10pt;font-weight:normal;overflow:hidden;padding:0px 3px;text-align:center;vertical-align:bottom;white-space:normal;word-wrap:break-word;wrap-strategy:4;'>N/A</td><td style='background-color:#ffffff;color:#1a202c;font-family:Arial;font-size:10pt;font-weight:normal;overflow:hidden;padding:0px 3px;vertical-align:bottom;white-space:normal;word-wrap:break-word;wrap-strategy:4;'><a class='in-cell-link' href='https://micro-manager.org' target='_blank'>https://micro-manager.org</a></td></tr></tbody></table></figure>

Source:&#160;<a style='text-decoration:none;' href='https://appjove.unicartagenaproxy.elogim.com/v/57701/ex-vivo-calcium-imaging-for-visualizing-brain-responses-to-endocrine-signaling-in-drosophila'><span style='-webkit-text-decoration-skip:none;font-family:Arial,sans-serif;font-size:12pt;font-style:normal;font-variant:normal;font-weight:400;text-decoration-skip-ink:none;vertical-align:baseline;white-space:pre-wrap;'>Ishimoto, H.&#160;et. al.,<span style='-webkit-text-decoration-skip:none;font-family:Arial,sans-serif;font-size:12pt;font-style:normal;font-variant:normal;font-weight:400;text-decoration-skip-ink:none;vertical-align:baseline;white-space:pre-wrap;'> Ex Vivo Calcium Imaging for Visualizing Brain Responses to Endocrine Signaling in Drosophila.&#160;J. Vis. Exp.<span style='-webkit-text-decoration-skip:none;font-family:Arial,sans-serif;font-size:12pt;font-style:normal;font-variant:normal;font-weight:400;text-decoration-skip-ink:none;vertical-align:baseline;white-space:pre-wrap;'> (2018)</a> &#160;This video demonstrates calcium imaging to study&#160;Drosophila brain responses to neuropeptides. Neurons expressing a fluorescent calcium indicator reveal intracellular calcium dynamics and functional responses to signaling molecules.

Source:&#160;Ishimoto, H.&#160;et. al., Ex Vivo Calcium Imaging for Visualizing Brain Responses to Endocrine Signaling in Drosophila.&#160;J. Vis. Exp. ...

Begin with an imaging chamber containing an immobilized Drosophila brain explant submerged in a buffer to maintain cellular function.The neurons in the brain express cytoplasmic fluorescent calcium indicators, which bind to calcium ions and fluoresce.Place the imaging chamber under a fluorescence microscope equipped with a water-immersion lens.Lower the lens, and under bright-field illumination, focus on the brain.Switch to fluorescence mode and capture the image.Next, introduce a neuropeptide into the buffer and initiate time-lapse recording.The neuropeptide binds to its receptor on neurons, triggering intracellular signaling. This opens the calcium channels and allows the calcium ion influx.These calcium ions bind to the indicators and increase fluorescence intensity.Recapture the image after neuropeptide stimulation.Compare the images before and after neuropeptide stimulation.An increase in fluorescence intensity after neuropeptide stimulation reflects the Drosophila brain's response to neuropeptide signaling.

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视频: Ex Vivo Calcium Imaging to Study Drosophila Brain Responses to Neuropeptides - 实验

In Vivo Functional Brain Imaging Approach Based on Bioluminescent Calcium Indicator GFP-aequorin

Functional in vivo imaging has become a powerful approach to study the function and physiology of brain cells and structures of interest. Recently a new method of Ca2+-imaging using the bioluminescent reporter GFP-aequorin (GA) has been developed. This new technique relies on the fusion of the GFP and aequorin genes, producing a molecule capable of binding calcium and&#160;&#8212; with the addition of its cofactor coelenterazine &#8212; emitting bright light that can be monitored through a photon collector. Transgenic lines carrying the GFP-aequorin gene have been generated for both mice and Drosophila. In Drosophila, the GFP-aequorin gene has been placed under the control of the GAL4/UAS binary expression system allowing for targeted expression and imaging within the brain. This method has subsequently been shown to be capable of detecting both inward Ca2+-transients and Ca2+-released from inner stores. Most importantly it allows for a greater duration in continuous recording, imaging at greater depths within the brain, and recording at high temporal resolutions (up to 8.3 msec). Here we present the basic method for using bioluminescent imaging to record and analyze Ca2+-activity within the mushroom bodies, a structure central to learning and memory in the fly brain.

In Vivo Functional Brain Imaging Approach Based on Bioluminescent Calcium Indicator GFP-aequorin

Here we present a novel Ca2+-imaging approach using a bioluminescent reporter. This approach uses a fused construct GFP-aequorin which binds to Ca2+ and emits light, eliminating the need for light excitation. Significantly this method permits long continuous imaging, access to deep brain structures and high temporal resolution.

在基于生物发光钙指标GFP的水母体内脑功能成像方法

Functional in vivo imaging has become a powerful approach to study the function and physiology of brain cells and structures of interest. Recently a new ...

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JoVE Journal

神经科学

Ex Vivo Imaging of Cell-specific Calcium Signaling at the Tripartite Synapse of the Mouse Diaphragm

The electrical activity of cells in tissues can be monitored by electrophysiological techniques, but these are usually limited to the analysis of individual cells. Since an increase of intracellular calcium (Ca2+) in the cytosol often occurs because of the electrical activity, or in response to a myriad of other stimuli, this process can be monitored by the imaging of cells loaded with fluorescent calcium-sensitive dyes.&#160; However, it is difficult to image this response in an individual cell type within whole tissue because these dyes are taken up by all cell types within the tissue. In contrast, genetically encoded calcium indicators (GECIs) can be expressed by an individual cell type and fluoresce in response to an increase of intracellular Ca2+, thus permitting the imaging of Ca2+ signaling in entire populations of individual cell types. Here, we apply the use of the GECIs GCaMP3/6 to the mouse neuromuscular junction, a tripartite synapse between motor neurons, skeletal muscle, and terminal/perisynaptic Schwann cells. We demonstrate the utility of this technique in classic ex vivo tissue preparations. Using an optical splitter, we perform dual-wavelength imaging of dynamic Ca2+ signals and a static label of the neuromuscular junction (NMJ) in an approach that could be easily adapted to monitor two cell-specific GECI or genetically encoded voltage indicators (GEVI) simultaneously. Finally, we discuss the routines used to capture spatial maps of fluorescence intensity. Together, these optical, transgenic, and analytic techniques can be employed to study the biological activity of distinct cell subpopulations at the NMJ in a wide variety of contexts.

Ex Vivo Imaging of Cell-specific Calcium Signaling at the Tripartite Synapse of the Mouse Diaphragm

Here we present a protocol to image calcium signaling in populations of individual cell types at the murine neuromuscular junction.

前体小鼠膈肌三方突触细胞特异性钙信号的影像学研究

The electrical activity of cells in tissues can be monitored by electrophysiological techniques, but these are usually limited to the analysis of ...

Time-Resolved In Vivo Measurement of Neuropeptide Dynamics by Capacitive Immunoprobe in Porcine Heart

The ability to measure biomarkers in vivo relevant to the assessment of disease progression is of great interest to the scientific and medical communities. The resolution of results obtained from current methods of measuring certain biomarkers can take several days or weeks to obtain, as they can be limited in resolution both spatially and temporally (e.g., fluid compartment microdialysis of interstitial fluid analyzed by enzyme-linked immunosorbent assay [ELISA], high-performance liquid chromatography [HPLC], or mass spectrometry); thus, their guidance of timely diagnosis and treatment is disrupted. In the present study, a unique technique for detecting and measuring peptide transmitters in vivo through the use of a capacitive immunoprobe biosensor (CI probe) is reported. The fabrication protocol and in vitro characterization of these probes are described. Measurements of sympathetic stimulation-evoked neuropeptide Y (NPY) release in vivo are provided. NPY release is correlated to the sympathetic release of norepinephrine for reference. The data demonstrate an approach for the fast and localized measurement of neuropeptides in vivo. Future applications include intraoperative real-time assessment of disease progression and minimally invasive catheter-based deployment of these probes.

Time-Resolved In Vivo Measurement of Neuropeptide Dynamics by Capacitive Immunoprobe in Porcine Heart

Established immunochemical methods to measure peptide transmitters in vivo rely on microdialysis or bulk fluid draw to obtain the sample for offline analysis. However, these suffer from spatiotemporal limitations. The present protocol describes the fabrication and application of a capacitive immunoprobe biosensor that overcomes the limitations of the existing techniques.

Ex Vivo Calcium Imaging to Study Drosophila Brain Responses to Neuropeptides

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Ex Vivo Calcium Imaging to Study Drosophila Brain Responses to Neuropeptides