Name: 비디오: 염증 마우스 모델에서 혈액 세포-내피 상호 작용을 분석하기 위한 생체 내 현미경 검사 - 개념
Uploaded: 2023-09-29T11:21:23.000+00:00
Duration: 1 min 49 s
Description: 183 조회수. 출처: Herr, N. et al., 생쥐의 장간막 정맥에서 백혈구-내피 및 혈소판-백혈구 상호 작용의 생체 내 현미경 검사. J. Vis. 특급. (2015년) 이 비디오에서는 복강내에 지질다당류를 주입한 마우스 모델의 장간막 정맥에서 혈액 세포-내피 상호 작용의 실시간 시각화를 보여줍니다.

eoe sub articles

EoE Sub Articles

All procedures involving animal models have been reviewed by the local institutional animal care committee and the JoVE veterinary review board.
1. Animal Handling, Preparation and Induction of Inflammation
<ol>
	<li>Use 4 - 6 week-old male mice with a weight range of 16 - 20 g. Note: If the mice are older or heavier they present excessive fat surrounding the vessel, limiting the microscopic observation.</li>
	<li>Sterilize all tools and microscope table prior to surgery.</li>
	<li>Inject 20 mg/kg LPS (lipopolysaccharide) intraperitoneally 4 hr prior to microscopy into the living mouse to induce a bacterial inflammation.</li>
	<li>Prewarm a 0.9% saline solution in a water bath at 37 &#176;C to humidify the plastic chamber and the mesentery tissue.</li>
	<li>Anesthetize the mouse with an intraperitoneal injection of ketamine (100 mg/kg) and xylazine (5 mg/kg) right before the microscopy procedure. Alternative anesthesia can be used, e.g., 2% isoflurane inhalation. Confirm proper anesthetization by the loss of response to reflex stimulation (toe or tail pinch with firm pressure).</li>
	<li>Depilate the abdomen using a shaver and remove loose hair with gauze saturated with ethanol 70%.</li>
	<li>Apply vet ointment on the eyes of the mouse to prevent dryness, while under anesthesia.</li>
</ol>
2. Surgery
<ol>
	<li>Sterilize the abdomen using 70% ethanol. This method is not a sterile method and could be lethal at the end of the experiment.</li>
	<li>Perform a median laparotomy: Open the abdominal skin using small, curved forceps and small scissors. Identify the epigastric vessels and open the peritoneum in the region of the linea alba, to protect the vessels.</li>
	<li>Apply a few drops of prewarmed saline into the abdominal cavity to keep the tissue moist.</li>
	<li>Label leukocytes and platelets fluorescently by injecting 50 &#181;l rhodamine 6G (1 mg/ml) retro-orbitally.</li>
	<li>Exteriorize a loop of ileum and place it in a petri dish with a diameter of 10 cm; make sure to keep the tissue moist by applying the 37 &#176;C prewarmed saline solution (0.9%) every other minute.</li>
</ol>
3. Intravital Microscopy
<ol>
	<li>Place the Mouse underneath the microscope and bring the mesentery vein with a diameter of 200 - 300 &#181;m in the center of view. Choose a vessel with no visible fat surroundings.</li>
	<li>Do not touch the mesentery vessels thereby avoiding stimulation of the endothelium. Handle the ileum loop cautiously.</li>
	<li>Visualize blood cell-endothelial interactions with an inverted or upright microscope and a camera using microscope software. Record blood cell-endothelial interactions for 1 min in 4 different veins per mouse.</li>
	<li>Euthanize the mouse by cervical dislocation after the completion of imaging experiments.</li>
</ol>
4. Analysis
<ol>
	<li>Carry out the analysis offline and blind for all parameters. Carry out analysis using any suitable software program.</li>
	<li>Confirm stable and interindividual comparable blood flow conditions in high time-resolution cine-clips (maximal frame rate) focused on intraluminal blood cell flow.</li>
	<li>Quantify the number of rolling leukocytes. Therefore draw a vertical line through the vein and count all leukocytes crossing this line in 1 min.</li>
	<li>Determine rolling velocity by measuring the time one single leukocyte needs to pass a distance of 50 &#181;m while stably rolling on the endothelium. To do this, draw two vertical lines at a distance of 50 &#181;m through the vein.
	<ol>
		<li>Measure the time a representative leukocyte needs to get from one line to the other. Calculate the speed of the leukocytes by dividing 50 &#181;m through the time needed (&#181;m/s).</li>
	</ol>
	</li>
	<li>Measure leukocyte adhesion in a field of 0.04 mm2. To do this, draw a square with a side length of 200 &#181;m into the vein.
	<ol>
		<li>Count the firm adherent leukocytes, defined as no visible movement for 30 sec, within this square.</li>
	</ol>
	</li>
	<li>Count the number of platelets bound to one leukocyte to quantify platelet-leukocyte interactions.</li>
</ol>

<table border="1" fo:keep-together.within-page="1" fo:keep-with-next.within-page="always">
	<tbody>
		<tr>
			<td>Rhodamine 6G</td>
			<td>Sigma-Aldrich</td>
			<td>989-38-8</td>
			<td></td>
		</tr>
		<tr>
			<td>Lipopolysaccharides from Escherichia coli 055:B5</td>
			<td>Sigma-Aldrich</td>
			<td>L2637</td>
			<td></td>
		</tr>
	</tbody>
</table>

intravital microscopy to analyze blood cell-endothelial interactions in an inflammation mouse model

Source: Herr, N. et al., <a href="https://app.jove.com/v/53077">Intravital Microscopy of Leukocyte-endothelial and Platelet-leukocyte Interactions in Mesenterial Veins in Mice.</a> J. Vis. Exp. (2015)
In this video, we demonstrate the real-time visualization of blood cell-endothelial interactions in the mesenterial veins of a mouse model injected intraperitoneally with lipopolysaccharide.

Intravital Microscopy to Analyze Blood Cell-Endothelial Interactions in an Inflammation Mouse Model

Source: Herr, N. et al., Intravital Microscopy of Leukocyte-endothelial and Platelet-leukocyte Interactions in Mesenterial Veins in Mice. J. Vis. Exp. ...

Begin with an anesthetized mouse that has been injected intraperitoneally with lipopolysaccharide to induce inflammation.
Incise the abdomen to expose the abdominal cavity. Maintain organ hydration with saline. Inject rhodamine 6G retro-orbitally. The fluorescent dye molecules enter the circulation and label leukocytes and platelets for their visualization.
Now, exteriorize a loop of ileum with its mesentery vessels. Keep the tissue hydrated with pre-warmed saline for optimal imaging. Under a fluorescence microscope, focus on a mesentery vein for intravital microscopy.
The lipopolysaccharide injection causes endothelial cell activation with the upregulation of adhesion molecules, including selectins. Circulating platelets are recruited to the endothelium, where they bind via specific adhesion molecule-ligand interactions, forming adhesion complexes.
Owing to these interactions, platelets get activated and release granules containing molecules, including serotonin, promoting leukocyte recruitment.
Leukocytes move to the endothelial surface and bind to activated platelets. Further, leukocytes roll along the endothelium and bind to the endothelial cells through weak adhesive interactions. Rolling motion activates leukocyte integrins for firm adhesion to endothelial cells, crucial for leukocyte-endothelial transmigration.
Using intravital microscopy, visualize the fluorescent leukocytes and platelets to determine their real-time interactions with endothelial cells.

intravital-microscopy-to-analyze-blood-cell-endothelial-interactions

Research

JoVE Encyclopedia of Experiments

Immunology

Immunopathology

Host-Pathogen Interaction Models

183 조회수. 출처: Herr, N. et al., 생쥐의 장간막 정맥에서 백혈구-내피 및 혈소판-백혈구 상호 작용의 생체 내 현미경 검사. J. Vis. 특급. (2015년) 이 비디오에서는 복강내에 지질다당류를 주입한 마우스 모델의 장간막 정맥에서 혈액 세포-내피 상호 작용의 실시간 시각화를 보여줍니다. 

비디오: 염증 마우스 모델에서 혈액 세포-내피 상호 작용을 분석하기 위한 생체 내 현미경 검사 - 개념

Intravital Microscopy Imaging of the Liver following Leishmania Infection: An Assessment of Hepatic Hemodynamics

Intravital microscopy (IVM) is a powerful optical imaging technique that has made possible the visualization, monitoring and quantification of various biological events in real time and in live animals. This technology has greatly advanced our understanding of physiological processes and pathogen-mediated phenomena in specific organs.
In this study, IVM is applied to the mouse liver and protocols are designed to image in vivo the circulatory system of the liver and measure red blood cell (RBC) velocity in individual hepatic vessels. To visualize the different vessel subtypes that characterize the hepatic organ and perform blood flow speed measurements, C57Bl/6 mice are intravenously injected with a fluorescent plasma reagent that labels the liver-associated vasculature. IVM enables in vivo, real time, measurement of RBC velocity in a specific vessel of interest. Establishing this methodology will make it possible to investigate liver hemodynamics under physiological and pathological conditions. Ultimately, this imaging-based methodology will be important for studying the influence of L. donovani infection&#160;on hepatic hemodynamics.
This method can be applied to other infectious models and mouse organs and might be further extended to pre-clinical testing of a drug&#8217;s effect on inflammation by quantifying its effect on blood flow.

Intravital Microscopy Imaging of the Liver following Leishmania Infection: An Assessment of Hepatic Hemodynamics

This article reports on a detailed method for the dynamic measurement and quantification of blood flow velocity within individual blood vessels of the mouse liver vasculature using intravital microscopy imaging in combination with a specific methodology for image acquisition and analysis.

다음 간 생체 내에 현미경 이미징<em&gt; 슈만 편모충</em&gt; 감염 : 간 혈류의 평가

Intravital microscopy (IVM) is a powerful optical imaging technique that has made possible the visualization, monitoring and quantification of various ...

연구

JoVE Journal

면역학 및 감염병학

Long Term Intravital Multiphoton Microscopy Imaging of Immune Cells in Healthy and Diseased Liver Using CXCR6.Gfp Reporter Mice

Liver inflammation as a response to injury is a highly dynamic process involving the infiltration of distinct subtypes of leukocytes including monocytes, neutrophils, T cell subsets, B cells, natural killer (NK) and NKT cells. Intravital microscopy of the liver for monitoring immune cell migration is particularly challenging due to the high requirements regarding sample preparation and fixation, optical resolution and long-term animal survival. Yet, the dynamics of inflammatory processes as well as cellular interaction studies could provide critical information to better understand the initiation, progression and regression of inflammatory liver disease. Therefore, a highly sensitive and reliable method was established to study migration and cell-cell-interactions of different immune cells in mouse liver over long periods (about 6 hr) by intravital two-photon laser scanning microscopy (TPLSM) in combination with intensive care monitoring.
The method provided includes a gentle preparation and stable fixation of the liver with minimal perturbation of the organ; long term intravital imaging using multicolor multiphoton microscopy with virtually no photobleaching or phototoxic effects over a time period of up to 6 hr, allowing tracking of specific leukocyte subsets; and stable imaging conditions due to extensive monitoring of mouse vital parameters and stabilization of circulation, temperature and gas exchange.
To investigate lymphocyte migration upon liver inflammation CXCR6.gfp knock-in mice were subjected to intravital liver imaging under baseline conditions and after acute and chronic liver damage induced by intraperitoneal injection(s) of carbon tetrachloride (CCl4).
CXCR6 is a chemokine receptor expressed on lymphocytes, mainly on Natural Killer T (NKT)-, Natural Killer (NK)- and subsets of T lymphocytes such as CD4 T cells but also mucosal associated invariant (MAIT) T cells1. Following the migratory pattern and positioning of CXCR6.gfp+ immune cells allowed a detailed insight into their altered behavior upon liver injury and therefore their potential involvement in disease progression.

Stable intravital high-resolution imaging of immune cells in the liver is challenging. Here we provide a highly sensitive and reliable method to study migration and cell-cell-interactions of immune cells in mouse liver over long periods (about 6 hours) by intravital multiphoton laser scanning microscopy in combination with intensive care monitoring.

CXCR6.Gfp 기자 마우스를 사용하여 건강하고 병에 걸린 간에서 면역 세포의 장기 생체 내에 다중 광자 현미경 이미징

Liver inflammation as a response to injury is a highly dynamic process involving the infiltration of distinct subtypes of leukocytes including monocytes, ...

Imaging Neutrophils and Monocytes in Mesenteric Veins by Intravital Microscopy on Anaesthetized Mice in Real Time

Efficient immune response is dependent on rapid mobilization of blood leukocytes to the site of infection or injury. Investigating leukocyte migration in vivo is crucial for understanding the molecular basis of leukocyte transendothelial migration and interaction with vascular endothelium. One powerful approach involves intravital microscopy on transgenic mice expressing fluorescent proteins in cells of interest.
Here we present a protocol for imaging monocytes and neutrophils in the CX3CR1gfp/wt mouse i.v. injected with orange dye-labeled neutrophils with an inverted confocal microscope. Time-lapse movies gathered from 30 min&#160;to several hours of imaging allow the analysis of leukocyte behavior in mesenteric veins under both steady state and inflammatory conditions. We also describe the steps to locally induce blood vessel inflammation with TLR2/TLR1 agonist Pam3SK4 and monitor the subsequent recruitment of neutrophils and monocytes.
The presented technique can also be used to monitor other populations of leukocytes and investigate molecules implicated in leukocyte recruitment or trafficking using other stimuli or transgenic mice.

We detail a protocol to monitor the behavior of neutrophils and monocytes in mesenteric veins under steady state and inflammatory conditions using intravital confocal microscopy on anaesthetized mice.

실시간으로 마취 마우스에 생체 내에 현미경으로 장간막 혈관에서 호중구와 단핵구 이미징

Efficient immune response is dependent on rapid mobilization of blood leukocytes to the site of infection or injury. Investigating leukocyte migration in ...

Intravital Microscopy to Analyze Blood Cell-Endothelial Interactions in an Inflammation Mouse Model

내레이션 대본

Intravital Microscopy to Analyze Blood Cell-Endothelial Interactions in an Inflammation Mouse Model