Name: 视频: 感染的人体组织来源细胞中炎症介质的定量 - 概念
Uploaded: 2023-09-29T11:21:20.000+00:00
Duration: 1 min 56 s
Description: 112 次观看. 来源:Dousha， L. et al.， 评估对流感嗜血杆菌的呼吸免疫反应。J. Vis. Exp.（2021 年） 该视频演示了通过将人肺组织来源的免疫细胞与流感嗜血杆菌一起孵育来定量感染过程中的炎症介质。流式细胞术用于测量标记淋巴细胞中的细胞因子荧光，与细菌感染后促炎细胞因子的产生相关。

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All procedures involving human participants have been performed in compliance with the institutional, national, and international guidelines for human welfare and have been reviewed by the local institutional review board.
1. Antigenic preparation
<ol>
	<li>Live bacteria
	<ol>
		<li>First, characterize live bacteria. Obtain the bacteria from the appropriate sample (e.g., sputum or bronchoscopy). Confirm the strain as&#160;Haemophilus influenzae&#160;using an appropriate microbiology laboratory. Perform typing of the&#160;H. influenzae&#160;samples to confirm they are nontypeable (by a specialist microbiology laboratory). Use one well-characterized strain. Ensure that the strain is also stored in glycerol broth at -70 &#176;C as a reserve.</li>
		<li>Grow the bacteria on enriched media such as chocolate agar plates or in broth.
		<ol>
			<li>To use chocolate agar plates, spread the bacteria for a minimum of every 3-4 days with sterile spreaders.</li>
			<li>Alternatively, use Brain Heart Infusion (BHI) broth enriched with factors X (hemin) and V (&#946;-nicotinamide adenine dinucleotide) to grow the bacteria. Inoculate non-typeable H. influenzae (NTHi) from overnight plates in 5-10 mL of BHI broth supplemented with both hemin and &#946;-nicotinamide adenine dinucleotide (both 10 &#181;g/mL) and culture overnight at 37 &#176;C in a 5% carbon dioxide, CO2&#160;incubator.&#160;&#160;&#160;&#160;&#160;&#160;&#160; 
			NOTE: This has the advantage of reproducibility, higher colony-forming units (CFU) counts, and all bacteria being at a similar phase of log growth (on plates, bacterial viability can be greater depending on the position in the culture).</li>
		</ol>
		</li>
		<li>Use a multiplicity of infection (MOI) of 100 bacteria in one cell to elicit a strong immune response while maintaining cellular viability. Use MacFarland Standard&#160;or spectrophotometer&#160;to assess the number of bacteria.</li>
		<li>Ensure that the media used for live NTHi assays is free of any human serum, as this will kill the bacteria. Animal serum samples (e.g., fetal calf serum) do not generally cause any problems.&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160; 
		&#8203;NOTE: Use the methods described below to analyze standard tissue samples such as peripheral blood, bronchoscopy samples (particularly bronchoalveolar lavage (BAL)), and resected lung tissue. Incubate the samples with Hi antigen from 10 min to 24 h or more.</li>
	</ol>
	</li>
</ol>
2. Assessment of lymphocyte function/inflammatory mediators in lung tissue
<ol>
	<li>It is not usually possible to obtain enough lymphocytes from bronchoscopy; therefore, use the lung tissue from lobectomy samples. The optimization of lung tissue samples requires close liaison with the anatomical pathology service. Ensure the tissue has a margin of at least 3 cm from the tumor and is the cellular tissue without significant emphysema (as determined by the pathologist).</li>
	<li>Break the lung tissue into a cellular suspension before it can be used for flow cytometry assays. Digest the lung tissue chemically (e.g., with collagenase) or disaggregate it mechanically.&#160;&#160;&#160;&#160;&#160;&#160;&#160; 
	NOTE: The mechanical disaggregation of tissue may be preferred as this is associated with better surface staining of cells (e.g., CD3/4 labeling).
	<ol>
		<li>Obtain lobectomy samples from a pathologist (usually obtained from patients undergoing treatment of lung cancer). Slice about 20-40 g of the sample into 3-5 mm3&#160;sections. Place them inside a sterile 50 &#181;L chamber before being mechanically fragmented using an appropriate disaggregator.</li>
		<li>After tissue disaggregation, lyse the erythrocytes with 10:1 (i.e., 5 mL) of 0.8% ammonium chloride (150 mM ammonium chloride (NH4Cl), 1 mM sodium bicarbonate (NaHCO3), and 0.1 mM ethylenediaminetetraacetic acid (EDTA) solution.&#160;&#160;&#160;&#160;&#160; 
		NOTE: Alternatively, an automated system such as Q-prep may be used.</li>
		<li>Resuspend the cells in sterile RPMI (the volume will depend on the cell numbers and generally is 10-20 mL), and then filter them through a 100 &#181;m sterile nylon mesh. Count the number of viable cells using the trypan blue exclusion method.</li>
	</ol>
	</li>
</ol>
3. NTHi infection assay
<ol>
	<li>Resuspend the lung cells to a final cell concentration of 4 x 106&#160;cells/mL per tube (control and stimulated samples).</li>
	<li>Use a suspension of 4 x 106-6 x 106&#160;cells in 1 mL of RPMI for the (negative) control tube. Use the same amount for the NTHi tube (any additional sample may be used as a positive control with Staphylococcal superantigen E (SEB). Infect the cells in the NTHi tube at an MOI of 100 bacteria per cell. Loosen the cap half a rotation to allow gas transfer in the tubes.</li>
	<li>Place the cells in a tube rotator and incubate them at 37 &#176;C while rotating at 12 rpm.</li>
	<li>To prevent the extracellular export of cytokines, add a Golgi blocker (Brefeldin A) to the cell suspensions 1 h after stimulation to a final concentration of 10 &#181;g/mL. Return the cell suspensions for a further 16-22 h incubation on rotation.</li>
	<li>Wash the cell suspension with 500 &#956;L of phosphate-buffered saline (PBS) containing 1% bovine serum albumin (BSA) and 0.01% sodium azide, NaN3.</li>
	<li>Add the antibodies for intracellular cytokine staining (the choice of antibodies is to be determined by the investigator). Stain the cell suspension for specific human lymphocyte cell-surface markers (e.g., CD45, CD3, etc.) for 1 h. Wash the cells with PBS, fix and permeabilize them.</li>
	<li>Fix the cells using 500 &#956;L of 1%-2% paraformaldehyde for 1 h.</li>
	<li>Count the cells by hemocytometer, permeabilize 106&#160;cells with 100 &#956;L of 0.1% saponin for 15 min, and incubate the cells with fluorescent-labeled antibodies. Wash the cells and analyze them using a flow cytometer. 
	NOTE: The quantity of fluorescent-labeled antibodies will be specific for each cytokine. Follow the manufacturer&#39;s instructions. Typically, 106&#160;cells in 100 &#956;L of solution will be stained for 1 h. Most commercially obtained antibodies will be enough to perform 25-100 tests.</li>
	<li>Incubate the cells with intracellular cytokine staining antibodies (e.g., interferon-gamma, IFN-&#947; and tumor necrosis factor beta, TNF-&#945; or interleukin, IL-13, and IL-17A) for 1 h. 
	NOTE: It is recommended to stain surface markers first, then intracellular as fixation can cause conformational changes in the surface proteins to which antibodies bind.</li>
	<li>Wash the cells with 500 &#956;L of PBS and resuspend in 100 &#956;L of PBS before data acquisition on a flow cytometer.</li>
</ol>

<table border="1" fo:keep-together.within-page="1" fo:keep-with-next.within-page="always">
	<tbody>
		<tr>
			<td>Ammonium chloride</td>
			<td>Sigma Aldrich</td>
			<td>213330</td>
			<td></td>
		</tr>
		<tr>
			<td>Brefeldin</td>
			<td>Sigma Aldrich</td>
			<td>B6542</td>
			<td></td>
		</tr>
		<tr>
			<td>Filcon sterile nylon mesh</td>
			<td>Becton Dickinson</td>
			<td>340606</td>
			<td></td>
		</tr>
		<tr>
			<td>Gelatin substrate, Enzchek</td>
			<td>Molecular probes</td>
			<td>E12055</td>
			<td></td>
		</tr>
		<tr>
			<td>MACS mix tube rotater</td>
			<td>Miltenyi Biotec</td>
			<td>130-090-753</td>
			<td></td>
		</tr>
		<tr>
			<td>Medimachine</td>
			<td>Becton Dickinson</td>
			<td></td>
			<td>Catalogue number not available</td>
		</tr>
		<tr>
			<td>Saponin</td>
			<td>Sigma Aldrich</td>
			<td>8047152</td>
			<td></td>
		</tr>
	</tbody>
</table>

quantification of inflammatory mediators in infected human tissue-derived cells

Source: Dousha, L. et al., <a href="https://app.jove.com/v/62572">Assessing Respiratory Immune Responses to Haemophilus Influenzae.</a>&#160;J. Vis. Exp.&#160;(2021)
This video demonstrates the quantification of inflammatory mediators during infection by incubating human lung-tissue-derived immune cells with Haemophilus influenzae. Flow cytometry is used to measure cytokine fluorescence in labeled lymphocytes, correlating with the production of pro-inflammatory cytokines in response to bacterial infection.

Quantification of Inflammatory Mediators in Infected Human Tissue-Derived Cells

Source: Dousha, L. et al., Assessing Respiratory Immune Responses to Haemophilus Influenzae.&#160;J. Vis. Exp.&#160;(2021)
This video demonstrates the ...

During an infection, activated lymphocytes release inflammatory mediators &#8212; cytokines &#8212; to elicit an immune response.
To quantify inflammatory mediators in an infected tissue, begin with a cell suspension containing human lung-tissue-derived immune cells.
Incubate the cells with Haemophilus influenzae &#8212; a respiratory pathogenic bacterium. The bacteria&#39;s surface antigens interact with pattern recognition receptors on phagocytic immune cells. This initiates bacterium internalization, processing into smaller peptides, and the presentation of the peptide by the major histocompatibility complex molecule.
The antigen-MHC-II molecule on phagocytic cells binds to T lymphocytes through the T cell receptors, along with co-stimulatory receptor interactions, resulting in T lymphocyte activation and the production of pro-inflammatory cytokines.
Treat the cells with Golgi blockers, impairing cytokine release &#8212; causing their accumulation inside the cells. Wash the cells with a blocking buffer to block non-specific binding sites.
Stain the cell suspension with a mix of fluorophore-labeled antibodies that bind specifically to human T lymphocyte-surface markers, enabling lymphocytes&#39; labeling.
Fix the cells, and permeabilize them with a pore-forming surfactant. Incubate the permeabilized cells with fluorophore-labeled anti-cytokine antibodies, which enter the cells and interact with specific cytokines.
Using flow cytometry, measure the cytokine fluorescence signal within labeled lymphocytes, correlating with inflammatory mediator production due to bacterial infection.&#160;

quantification-inflammatory-mediators-infected-human-tissue-derived

Research

JoVE Encyclopedia of Experiments

Immunology

Immune Response

Host Defense Mechanism

112 次观看. 来源:Dousha， L. et al.， 评估对流感嗜血杆菌的呼吸免疫反应。J. Vis. Exp.（2021 年） 该视频演示了通过将人肺组织来源的免疫细胞与流感嗜血杆菌一起孵育来定量感染过程中的炎症介质。流式细胞术用于测量标记淋巴细胞中的细胞因子荧光，与细菌感染后促炎细胞因子的产生相关。 

视频: 感染的人体组织来源细胞中炎症介质的定量 - 概念

Implementation of a Permeable Membrane Insert-based Infection System to Study the Effects of Secreted Bacterial Toxins on Mammalian Host Cells

Many bacterial pathogens secrete potent toxins to aid in the destruction of host tissue, to initiate signaling changes in host cells or to manipulate immune system responses during the course of infection. Though methods have been developed to successfully purify and produce many of these important virulence factors, there are still many bacterial toxins whose unique structure or extensive post-translational modifications make them difficult to purify and study in in vitro systems. Furthermore, even when pure toxin can be obtained, there are many challenges associated with studying the specific effects of a toxin under relevant physiological conditions. Most in vitro cell culture models designed to assess the effects of secreted bacterial toxins on host cells involve incubating host cells with a one-time dose of toxin. Such methods poorly approximate what host cells actually experience during an infection, where toxin is continually produced by bacterial cells and allowed to accumulate gradually during the course of infection. This protocol describes the design of a permeable membrane insert-based bacterial infection system to study the effects of Streptolysin S, a potent toxin produced by Group A Streptococcus, on human epithelial keratinocytes. This system more closely mimics the natural physiological environment during an infection than methods where pure toxin or bacterial supernatants are directly applied to host cells. Importantly, this method also eliminates the bias of host responses that are due to direct contact between the bacteria and host cells. This system has been utilized to effectively assess the effects of Streptolysin S (SLS) on host membrane integrity, cellular viability, and cellular signaling responses. This technique can be readily applied to the study of other secreted virulence factors on a variety of mammalian host cell types to investigate the specific role of a secreted bacterial factor during the course of infection.

Here, a method using a permeable membrane insert-based infection system to study the effects of Streptolysin S, a secreted toxin produced by Group A Streptococcus, on keratinocytes is described. This system can be readily applied to the study of other secreted bacterial proteins on various host cell types during infection.

基于插入渗透膜感染系统的实现研究分泌细菌病毒对哺乳动物宿主细胞的作用

Many bacterial pathogens secrete potent toxins to aid in the destruction of host tissue, to initiate signaling changes in host cells or to manipulate ...

科研

JoVE Journal

免疫与感染

Experimental Infection with Listeria monocytogenes as a Model for Studying Host Interferon-&#947; Responses

L. monocytogenes is a gram-positive bacterium that is a cause of food borne disease in humans. Experimental infection of mice with this pathogen has been highly informative on the role of innate and adaptive immune cells and specific cytokines in host immunity against intracellular pathogens. Production of IFN-&#947; by innate cells during sublethal infection with L. monocytogenes is important for activating macrophages and early control of the pathogen1-3. In addition, IFN-&#947; production by adaptive memory lymphocytes is important for priming the activation of innate cells upon reinfection4. The L. monocytogenes infection model thus serves as a great tool for investigating whether new therapies that are designed to increase IFN-&#947; production have an impact on IFN-&#947; responses in vivo and have productive biological effects such as increasing bacterial clearance or improving mouse survival from infection. Described here is a basic protocol for how to conduct intraperitoneal infections of C57BL/6J mice with the EGD strain of L. monocytogenes and to measure IFN-&#947; production by NK cells, NKT cells, and adaptive lymphocytes by flow cytometry. In addition, procedures are described to: (1) grow and prepare the bacteria for inoculation, (2) measure bacterial load in the spleen and liver, and (3) measure animal survival to endpoints. Representative data are also provided to illustrate how this infection model can be used to test the effect of specific agents on IFN-&#947; responses to L. monocytogenes and survival of mice from this infection.

This protocol describes how to inoculate C57BL/6J mice with the EGD strain of Listeria monocytogenes (L. monocytogenes) and to measure interferon-&#947; (IFN-&#947;) responses by natural killer (NK) cells, natural killer T (NKT) cells, and adaptive T lymphocytes post-infection. This protocol also describes how to conduct survival studies in mice after infection with a modified LD50 dose of the pathogen.

实验性感染<em&gt;李斯特菌</em&gt;作为研究主机干扰素γ响应模型

L. monocytogenes is a gram-positive bacterium that is a cause of food borne disease in humans. Experimental infection of mice with this pathogen has been ...

Imaging of In Situ Interferon Gamma Production in the Mouse Spleen following Listeria monocytogenes Infection

Cytokines are small proteins secreted by cells, mediating cell-cell communications that are crucial for effective immune responses. One characteristic of cytokines is their pleiotropism, as they are produced by and can affect a multitude of cell types. As such, it is important to understand not only which cells are producing cytokines, but also in which environment they do so, in order to define more specific therapeutics. Here, we describe a method to visualize cytokine production in situ following bacterial infection. This technique relies on imaging cytokine-producing cells in their native environment by confocal microscopy. To do so, tissue sections are stained for markers of multiple cell types together with a cytokine stain. Key to this method, cytokine secretion is blocked directly in vivo before harvesting the tissue of interest, allowing for detection of the cytokine that accumulated inside the producing cells. The advantages of this method are multiple. First, the microenvironment in which cytokines are produced is preserved, which could ultimately inform on the signals required for cytokine production and the cells affected by those cytokines. In addition, this method gives an indication of the location of the cytokine production in vivo, as it does not rely on artificial in vitro re-stimulation of the producing cells. However, it is not possible to simultaneously analyze cytokine downstream signaling in cells that receive the cytokine. Similarly, the cytokine signals observed correspond&#160;only to the time-window during which cytokine secretion was blocked. While we describe the visualization of the cytokine Interferon (IFN) gamma in the spleen following mouse infection by the intracellular bacteria Listeria monocytogenes, this method could potentially be adapted to the visualization of any cytokine in most organs.

Imaging of In Situ Interferon Gamma Production in the Mouse Spleen following Listeria monocytogenes Infection

Here, we describe a simple confocal imaging method to visualize the in situ localization of cells secreting the cytokine Interferon gamma in murine secondary lymphoid organs. This protocol can be extended for the visualization of other cytokines in diverse tissues.

李斯特菌单细胞基因感染后小鼠脾脏原位干扰素伽马生产的成像

Cytokines are small proteins secreted by cells, mediating cell-cell communications that are crucial for effective immune responses. One characteristic of ...

Quantification of Inflammatory Mediators in Infected Human Tissue-Derived Cells

成績單

Quantification of Inflammatory Mediators in Infected Human Tissue-Derived Cells