 two-photon microscopy for in vivo imaging of mouse brain microvasculature 

 Two-Photon Microscopy for In Vivo Imaging of Mouse Brain Microvasculature 

In this procedure, remove the skin on the medial left thigh of the mouse. Next, locate the femoral vein. Using a 1-milliliter syringe and a 30-gauge needle, draw up 130 microliters of the fluorescent dye solution. Inject 100 microliters of the dye slowly into the femoral vein.After removing the needle, apply steady, gentle pressure to the injection site to stop any bleeding, and allow the dye to circulate for five minutes. Then, close the surgical site with sutures. Carefully flip the mouse onto its stomach and place it into the mouse head plate harness. For in vivo two-photon imaging, move the surgical apparatus to the two-photon microscope, and make sure to maintain the animal's anesthesia level.Next, place a small amount of 0.9% saline into the head plate reservoir, and lower the microscope objective so that it comes into contact with the saline. Then, locate the area of interest, using the bright field viewing objective. Afterward, begin two-photon imaging. Locate a capillary bed on the view screen, and magnify this area using the optical zoom 2. Acquire images of the capillaries using the two-photon imaging software.

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Universidad de Cartagena UDEC

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Neurovascular & Blood Flow Imaging

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<figure class='table'><table class='ck-table-resized' style='border-collapse:collapse;font-family:Calibri;font-size:11pt;table-layout:fixed;' cellspacing='0' cellpadding='0' dir='ltr' border='1' data-sheets-root='1' data-sheets-baot='1'><colgroup><col style='width:25%;' width='416'><col style='width:25%;' width='293'><col style='width:25%;' width='249'><col style='width:25%;' width='279'></colgroup><tbody><tr style='height:20px;'><td style='border:1px solid #000000;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>T/PUMP</td><td style='border-bottom:1px solid #000000;border-right:1px solid #000000;border-top:1px solid #000000;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Gaymar Industries, Inc.</td><td style='border-bottom:1px solid #000000;border-right:1px solid #000000;border-top:1px solid #000000;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>TP-500</td><td style='border-bottom:1px solid #000000;border-right:1px solid #000000;border-top:1px solid 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Source:<a style='text-decoration:none;' href='https://appjove.unicartagenaproxy.elogim.com/v/53582/quantification-of-cerebral-vascular-architecture-using-two-photon-microscopy-in-a-mouse-model-of-hiv-induced-neuroinflammation'><span style='-webkit-text-decoration-skip:none;font-family:Roboto,sans-serif;font-size:10pt;font-style:normal;font-variant:normal;font-weight:400;text-decoration-skip-ink:none;vertical-align:baseline;white-space:pre-wrap;'>&#160;<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;'>Nishimura, C.&#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;'> Quantification of Cerebral Vascular Architecture using Two-photon Microscopy in a Mouse Model of HIV-induced Neuroinflammation.&#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;'> (2016).</a> &#160;This video demonstrates the in vivo visualization of cortical capillaries in the mouse brain using two-photon microscopy. It outlines the steps for injecting a fluorescent dye into an anesthetized mouse with a thin-skull cortical window, preparing the setup for imaging, and acquiring detailed images of brain microvascular structures for analysis.

Source:&#160;Nishimura, C.&#160;et al. Quantification of Cerebral Vascular Architecture using Two-photon Microscopy in a Mouse Model of HIV-induced ...

Begin with an anesthetized mouse with a headplate secured over a surgically prepared thin-skull cortical window.Position the mouse supine. Remove the medial thigh skin to expose the femoral vein.Inject a fluorescent dye conjugate into the vein to label blood plasma, enabling blood vessel visualization.Suture the incision.Flip the mouse and secure the headplate in a harness to stabilize the mouse.Transfer the setup to a two-photon microscope stage.Add saline over the cortical window. Lower the objective lens until it contacts the saline.Using bright-field illumination, locate the imaging region.Switch to two-photon imaging.The microscope&#8217;s laser focuses low-energy near-infrared light into the brain.At the laser&#8217;s focal point, two photons combine their energy to excite the dye, making the blood vessels fluoresce.Identify a capillary bed&#8212;a network of small blood vessels connecting arteries to veins&#8212; and magnify it.Acquire images to analyze the brain&#8217;s microvasculature.

13 Görüntüleme.  Two-Photon Microscopy for In Vivo Imaging of Mouse Brain Microvasculature 

Video:  Two-Photon Microscopy for In Vivo Imaging of Mouse Brain Microvasculature  - Deney

Longitudinal In Vivo Imaging of the Cerebrovasculature: Relevance to CNS Diseases

Remodeling of the brain vasculature is a common trait of brain pathologies. In vivo imaging techniques are fundamental to detect cerebrovascular plasticity or damage occurring overtime and in relation to neuronal activity or blood flow. In vivo two-photon microscopy allows the study of the structural and functional plasticity of large cellular units in the living brain. In particular, the thinned-skull window preparation allows the visualization of cortical regions of interest (ROI) without inducing significant brain inflammation. Repetitive imaging sessions of cortical ROI are feasible, providing the characterization of disease hallmarks over time during the progression of numerous CNS diseases. This technique accessing the pial structures within 250 &#956;m of the brain relies on the detection of fluorescent probes encoded by genetic cellular markers and/or vital dyes. The latter (e.g., fluorescent dextrans) are used to map the luminal compartment of cerebrovascular structures. Germane to the protocol described herein is the use of an in vivo marker of amyloid deposits, Methoxy-O4, to assess Alzheimer&#39;s disease (AD) progression. We also describe the post-acquisition image processing used to track vascular changes and amyloid depositions. While focusing presently on a model of AD, the described protocol is relevant to other CNS disorders where pathological cerebrovascular changes occur.

Longitudinal In Vivo Imaging of the Cerebrovasculature: Relevance to CNS Diseases

This manuscript describes a procedure to track the remodeling of the cerebrovasculature during amyloid plaque accumulation in vivo using longitudinal two-photon microscopy. A thinned-skull preparation enables the visualization of fluorescent dyes to assess the progression of cerebrovascular damage in a mouse model of Alzheimer&#39;s disease.

uzunlamasına<em&gt; İn Vivo</em&gt; Cerebrovasculature Görüntüleme: MSS Hastalıkları uygunluk

Remodeling of the brain vasculature is a common trait of brain pathologies. In vivo imaging techniques are fundamental to detect cerebrovascular ...

JoVE Journal

Tıp

In Vivo Two-photon Imaging of Cortical Neurons in Neonatal Mice

Two-photon imaging is a powerful tool for the in vivo analysis of neuronal circuits in the mammalian brain. However, a limited number of in vivo imaging methods exist for examining the brain tissue of live newborn mammals. Herein we summarize a protocol for imaging individual cortical neurons in living neonatal mice. This protocol includes the following two methodologies: (1) the Supernova system for sparse and bright labeling of cortical neurons in the developing brain, and (2) a surgical procedure for the fragile neonatal skull. This protocol allows the observation of temporal changes of individual cortical neurites during neonatal stages with a high signal-to-noise ratio. Labeled cell-specific gene silencing and knockout can also be achieved by combining the Supernova with RNA interference and CRISPR/Cas9 gene editing systems. This protocol can, thus, be used for analyzing the developmental dynamics of cortical neurons, molecular mechanisms that control the neuronal dynamics, and changes in neuronal dynamics in disease models.

In Vivo Two-photon Imaging of Cortical Neurons in Neonatal Mice

We present an in vivo two-photon imaging protocol for imaging the cerebral cortex of neonatal mice. This method is suitable for analyzing the developmental dynamics of cortical neurons, the molecular mechanisms that control the neuronal dynamics, and the changes in neuronal dynamics in disease models.

Vivo Yenidoğan farelerde kortikal nöronların iki fotonlu görüntüleme

Two-photon imaging is a powerful tool for the in vivo analysis of neuronal circuits in the mammalian brain. However, a limited number of in vivo imaging ...

Nörobilim

In Vivo Wide-Field and Two-Photon Calcium Imaging from a Mouse Using a Large Cranial Window

Wide-field calcium imaging from the mouse&#39;s neocortex allows one to observe cortex-wide neural activity related to various brain functions. On the other hand, two-photon imaging can resolve the activity of local neural circuits at the single-cell level. It is critical to make a large cranial window to perform multiple-scale analysis using both imaging techniques in the same mouse. To achieve this, one must remove a large section of the skull and cover the exposed cortical surface with transparent materials. Previously, glass skulls and polymer-based cranial windows have been developed for this purpose, but these materials are not easily fabricated. The present protocol describes a simple method for making a large cranial window consisting of commercially available polyvinylidene chloride (PVDC) wrapping film, a transparent silicone plug, and a cover glass. For imaging the dorsal surface of an entire hemisphere, the window size was approximately 6 x 3 mm2. Severe brain vibrations were not observed regardless of such a large window. Importantly, the condition of the brain surface did not deteriorate for more than one month. Wide-field imaging of a mouse expressing a genetically-encoded calcium indicator (GECI), GCaMP6f, specifically in astrocytes, revealed synchronized responses in a few millimeters. Two-photon imaging of the same mouse showed prominent calcium responses in individual astrocytes over several seconds. Furthermore, a thin layer of an adeno-associated virus was applied to the PVDC film and successfully expressed GECI in cortical neurons over the cranial window. This technique is reliable and cost-effective for making a large cranial window and facilitates the investigation of the neural and glial dynamics and their interactions during behavior at the macroscopic and microscopic levels.

In Vivo Wide-Field and Two-Photon Calcium Imaging from a Mouse Using a Large Cranial Window

The present protocol describes making a large (6 x 3 mm2) cranial window using food wrap, transparent silicone, and cover glass. This cranial window allows in vivo wide-field and two-photon calcium imaging experiments in the same mouse.

İn Vivo Büyük Bir Kraniyal Pencere Kullanarak Bir Fareden Geniş Alan ve İki Foton Kalsiyum Görüntüleme

Wide-field calcium imaging from the mouse&#39;s neocortex allows one to observe cortex-wide neural activity related to various brain functions. On the ...

Two-Photon Microscopy for In Vivo Imaging of Mouse Brain Microvasculature

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Two-Photon Microscopy for In Vivo Imaging of Mouse Brain Microvasculature