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All procedures involving animal models have been reviewed by the local institutional animal care committee and the JoVE veterinary review board.Animal Model<ol><li>Intercross hemizygous Tg(Gfap-luc+/-) mice with hemizygous Tg(M83+/-) mice to generate hemizygous bigenic Tg(M83+/-:Gfap-luc+/-) mice.</li><li>Genotype the progeny with real-time PCR for the presence of the transgene encoding human alpha-synuclein and with standard PCR for firefly luciferase.</li><li>Inoculate the animals at the age of six to eight weeks.</li></ol>Inoculum Preparation<ol><li>Prepare monomeric recombinant human alpha-synuclein with the A53T mutation in Tris-buffered saline (TBS) buffer containing 150 mM NaCl in 20 mM Tris-HCl (pH 7.2).</li><li>Prepare fibrillar alpha-synuclein for inoculations by agitating 3 &#181;g/&#181;L of monomeric recombinant human alpha-synuclein in an orbital shaker at 800 rpm and 37 &#176;C for 5 days.</li><li>Dilute fibril assemblies in phosphate-buffered saline (PBS) to reach a final concentration of 1 &#181;g/&#181;L for intraperitoneal inoculations.</li><li>Fragment the alpha-synuclein fibrils with a rod sonicator for 1 min (40 pulses of 0.5 s duration with a one-second pause between each pulse and amplitude set to 50%) on ice. To avoid contamination by cross-seeding. Use clean sonication probes to prepare different inoculum.</li></ol>Intraperitoneal Injections<ol><li>For intraperitoneal injections, narcotize the animals shortly in an anesthesia chamber by inhalation with isoflurane/oxygen using a flow rate of 2 L/min and the vaporizer set to 2%. Pinch the animal's toe and confirm that it does not withdraw its hindlimb to ensure proper anesthesia.</li><li>Fill a 27 G disposable hypodermic syringe with 50 &#181;L of sonicated alpha-synuclein fibrils or PBS.</li><li>Directly inject into the peritoneum of the mouse and avoid penetrating the small intestine or cecum located behind the abdominal wall by holding the animal in a dorsal position with the head facing away from the investigator and downward at approximately 45&#176;. Monitor animals until they have recovered from the anesthesia.</li></ol>Bioluminescence Imaging<ol><li>Image Tg(M83+/-:Gfap-luc+/-) mice every 2-4 weeks using a bioluminescence imaging system.</li><li>Prior to imaging shortly anesthetize mice in an isoflurane/oxygen chamber with a flow rate of 2 L/min and the vaporizer set to 2%. Pinch the animal's toe and confirm that it does not withdraw its hindlimb to ensure proper anesthesia.</li><li>Shave and depilate the heads of the mice with a depilatory cream. Color the ears in black with a non-irritating marker to block unspecific bioluminescence.</li><li>Dilute D-luciferin potassium salt, the substrate of luciferase, in PBS to a 30 mg/mL stock solution. Store this in 1 mL aliquots at -20 &#176;C. Protect the dissolved D-luciferin from exposure to light.</li><li>Weigh the animals prior to injection. Calculate the exact volume of D-luciferin for injection of 150 mg/kg body weight. Intraperitoneally inject D-luciferin and return the animal to the anesthesia chamber.</li><li>Start the imaging software. After the imaging system has reached its operating temperature initialize the system by clicking on the 'Initialize' button in the control panel.</li><li>Select the buttons 'Luminescent' and 'Photograph'. Set the exposure time to 60 s, the binning to 'Medium', the F/Stop to '1', and the EM gain to 'Off'.</li><li>Confirm that the excitation filter is set to 'Block' and the emission filter to 'Open', and set the subject height to 1.50 cm.</li><li>Ten min after injection with D-luciferin, place the animals onto the heating plate in the imaging chamber and ensure that their muzzles are correctly placed in the anesthesia outlet. Close the isoflurane/oxygen flow from the inhalation chamber and open the flow for the imaging chamber with a flow rate of 0.25 L/min and an evaporation of 2%. Close the door of the imaging chamber properly.</li><li>Click on the 'Acquire' button to measure the bioluminescence, which takes 60 s.</li></ol>

<figure class='table' style='width:534pt;'><table class='ck-table-resized'><colgroup><col style='width:39.51%;'><col style='width:18.35%;'><col style='width:16.85%;'><col style='width:25.29%;'></colgroup><tbody><tr><td style='height:14.5pt;width:211pt;'>27-gauge syringe</td><td style='width:98pt;'>VWR</td><td style='width:90pt;'>613-4900</td><td style='width:135pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:211pt;'>Isoflurane</td><td style='width:98pt;'>Piramal Healthcare</td><td style='width:90pt;'>PZN 4831850</td><td style='width:135pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:211pt;'>Depilatory cream</td><td style='width:98pt;'>Veet</td><td style='width:90pt;'>&#160;</td><td style='width:135pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:211pt;'>Secureline lab marker</td><td style='width:98pt;'>Neolab</td><td style='width:90pt;'>25040</td><td style='width:135pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:211pt;'>D-luciferin potassium salt</td><td style='width:98pt;'>Acris</td><td style='width:90pt;'>LK10000</td><td style='width:135pt;'>30 mg/mL stock solution</td></tr><tr><td style='height:14.5pt;width:211pt;'>Thermomixer</td><td style='width:98pt;'>Eppendorf</td><td style='width:90pt;'>5776671</td><td style='width:135pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:211pt;'>Sonopuls Mini20 sonicator</td><td style='width:98pt;'>Bandelin</td><td style='width:90pt;'>3648</td><td style='width:135pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:211pt;'>IVIS Lumina II imaging system</td><td style='width:98pt;'>PerkinElmer</td><td style='width:90pt;'>&#160;</td><td style='width:135pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:211pt;'>Living Image 3.0 Software</td><td style='width:98pt;'>PerkinElmer</td><td style='width:90pt;'>&#160;</td><td style='width:135pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:211pt;'>Tg(M83+/-) mice or B6;C3-Tg(Prnp-SNCA*A53T)83Vle/J mice</td><td style='width:98pt;'>The Jackson Laboratory</td><td style='width:90pt;'>4479</td><td style='width:135pt;'>&#160;</td></tr></tbody></table></figure>

bioluminescence imaging of neuroinflammation in a transgenic mouse

<a href='https://app.jove.com/v/55503/bioluminescence-imaging-neuroinflammation-transgenic-mice-after'>Source: Breid, S., et. al. Bioluminescence Imaging of Neuroinflammation in Transgenic Mice After Peripheral Inoculation of Alpha-Synuclein Fibrils. J. Vis. Exp. (2017)</a>This video demonstrates the bioluminescence imaging of neuroinflammation in transgenic mice, showcasing luciferase-luciferin reactions in activated astrocytes. The protocol enables non-invasive quantification of astrocytic activation, aiding studies on CNS inflammation and therapeutic efficacy.

Bioluminescence Imaging of Neuroinflammation in a Transgenic Mouse

Source: Breid, S., et. al. Bioluminescence Imaging of Neuroinflammation in Transgenic Mice After Peripheral Inoculation of Alpha-Synuclein Fibrils. J. ...

Begin with an anesthetized transgenic mouse containing pathogenic protein aggregates, which cause neuroinflammation and astrocyte activation, leading to increased luciferase expression.Remove the fur from its head to prevent light scattering during imaging.Color the ears with a non-irritating marker to block nonspecific bioluminescence.Take an appropriate volume of luciferin based on the mouse's body weight and inject it intraperitoneally.Luciferin enters the bloodstream, reaches the brain, and is taken up by activated astrocytes.Within the astrocyte, the luciferase oxidizes luciferin, emitting a bioluminescent signal.Set the imaging parameters and precisely position the mouse on the bioluminescence imaging chamber's heating plate.&#160;Ensure proper anesthesia flow and capture the bioluminescent signal for the desired duration.Then, select the region of interest and quantify the targeted bioluminescent signal.&#160;The intensity of this signal corresponds to luciferase activity, reflecting astrocytic activation and providing a direct measure of neuroinflammation.

bioluminescence-imaging-of-neuroinflammation-in-a-transgenic-mouse

Nanyang Technological University

Research

JoVE Encyclopedia of Experiments

Neuroscience

Neuroimaging

Neurodegeneration & Disease Monitoring

44 Görüntüleme. Source: Breid, S., et. al. Bioluminescence Imaging of Neuroinflammation in Transgenic Mice After Peripheral Inoculation of Alpha-Synuclein Fibrils. J. Vis. Exp. (2017) This video demonstrates the bioluminescence imaging of neuroinflammation in transgenic mice, showcasing luciferase-luciferin reactions in activated astrocytes. The protocol enables non-invasive quantification of astrocytic activation, aiding studies on CNS inflammation and therapeutic efficacy. 

Video: Bioluminescence Imaging of Neuroinflammation in a Transgenic Mouse - Kavram

Bioluminescence Imaging to Detect Late Stage Infection of African Trypanosomiasis

Human African trypanosomiasis (HAT) is a multi-stage disease that manifests in two stages; an early blood stage and a late stage when the parasite invades the central nervous system (CNS). In vivo study of the late stage has been limited as traditional methodologies require the removal of the brain to determine the presence of the parasites.
Bioluminescence imaging is a non-invasive, highly sensitive form of optical imaging that enables the visualization of a luciferase-transfected pathogen in real-time. By using a transfected trypanosome strain that has the ability to produce late stage disease in mice we are able to study the kinetics of a CNS infection in a single animal throughout the course of infection, as well as observe the movement and dissemination of a systemic infection.
Here we describe a robust protocol to study CNS infections using a bioluminescence model of African trypanosomiasis, providing real time non-invasive observations which can be further analyzed with optional downstream approaches.

This manuscript describes the use of a bioluminescent strain of African trypanosomes to enable the tracking of late stage infection and demonstrates how in vivo live imaging can be used to visualize infections within the central nervous system in real-time.

Biyoparlaklık Görüntüleme Afrika Trypanosomiasis Geç Evre Enfeksiyon Algılama için

Human African trypanosomiasis (HAT) is a multi-stage disease that manifests in two stages; an early blood stage and a late stage when the parasite invades ...

JoVE Journal

İmmünoloji ve Enfeksiyon

Bioluminescence Imaging of an Immunocompetent Animal Model for Glioblastoma

In contrast to commonly reported human glioma xenograft animal models, GL261 murine glioma xenografts recapitulate nearly all relevant clinical and histopathologic features of the human disease. When GL261 cells are implanted intracranially in syngeneic C57BL/6 mice, the model has the added advantage of maintaining an intact immune microenvironment. Stable expression of luciferase in GL261 cells allows non-invasive cost effective bioluminescence monitoring of intracranial tumor growth. We have recently demonstrated that luciferase expression in GL261 cells does not affect the tumor growth properties, tumor cell immunomodulatory cytokine expression, infiltration of immune cells into the tumor, or overall survival of animals bearing the intracranial tumor. Therefore, it appears that the GL261 luciferase glioma model can be useful in the study of novel chemotherapeutic and immunotherapeutic modalities. Here we report the technique for generating stable luciferase expression in GL261 cells and how to study the in vitro and in vivo growth of the tumor cells by bioluminescence imaging.

GL261 glioma cells provide a useful immunocompetent animal model of glioblastoma. The goals of this protocol are to demonstrate proper techniques for monitoring intracranial tumor growth using in vivo bioluminescence imaging, and to verify the utility of luciferase-modified GL261 cells for studying tumor immunology and immunotherapeutic approaches for treating glioblastoma.

Glioblastoma&#39;nın için bir Immünkompetan Hayvan Modeli Biyoparlaklık Görüntüleme

In contrast to commonly reported human glioma xenograft animal models, GL261 murine glioma xenografts recapitulate nearly all relevant clinical and ...

Tıp

Bioluminescence and Near-infrared Imaging of Optic Neuritis and Brain Inflammation in the EAE Model of Multiple Sclerosis in Mice

Experimental autoimmune encephalomyelitis (EAE) in SJL/J mice is a model for relapsing-remitting multiple sclerosis (RRMS). Clinical EAE scores describing motor function deficits are basic readouts of the immune-mediated inflammation of the spinal cord. However, scores and body weight do not allow for an in vivo assessment of brain inflammation and optic neuritis. The latter is an early and frequent manifestation in about 2/3 of MS patients. Here, we show methods for bioluminescence and near-infrared live imaging to assess EAE evoked optic neuritis, brain inflammation, and blood-brain barrier (BBB) disruption in living mice using an in vivo imaging system. A bioluminescent substrate activated by oxidases primarily showed optic neuritis. The signal was specific and allowed the visualization of medication effects and disease time courses, which paralleled the clinical scores. Pegylated fluorescent nanoparticles that remained within the vasculature for extended periods of time were used to assess the BBB integrity. Near-infrared imaging revealed a BBB leak at the peak of the disease. The signal was the strongest around the eyes. A near-infrared substrate for matrix metalloproteinases was used to assess EAE-evoked inflammation. Auto-fluorescence interfered with the signal, requiring spectral unmixing for quantification. Overall, bioluminescence imaging was a reliable method to assess EAE-associated optic neuritis and medication effects and was superior to the near-infrared techniques in terms of signal specificity, robustness, ease of quantification, and cost.

We show a technique for in vivo live bioluminescence and near-infrared imaging of optic neuritis and encephalitis in the experimental autoimmune encephalomyelitis (EAE) model for multiple sclerosis in SJL/J mice.

Farelerde Multipl Skleroz EAE Modeli Optik Nörit ve Beyin Enflamasyon Biyoparlaklık ve Yakın-Kızılötesi Görüntüleme

Experimental autoimmune encephalomyelitis (EAE) in SJL/J mice is a model for relapsing-remitting multiple sclerosis (RRMS). Clinical EAE scores describing ...

Bioluminescence Imaging of Neuroinflammation in a Transgenic Mouse

TRANSKRIPT

Bioluminescence Imaging of Neuroinflammation in a Transgenic Mouse

Biyoparlaklık Görüntüleme Afrika Trypanosomiasis Geç Evre Enfeksiyon Algılama için

Glioblastoma'nın için bir Immünkompetan Hayvan Modeli Biyoparlaklık Görüntüleme

Farelerde Multipl Skleroz EAE Modeli Optik Nörit ve Beyin Enflamasyon Biyoparlaklık ve Yakın-Kızılötesi Görüntüleme