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1. Analysis of Vitronectin, Vn as a Bacterial Surface Protein-Ligand
<ol>
	<li>Detection of Vn-binding at the bacterial surface using flow cytometry 
	NOTE: In flow cytometry, we used side scatter and forward scatter to gate positive events. To examine the interactions with Vn, Haemophilus influenzae&#160;type f, Hif clinical isolates (n=10)&#160;were selected together with&#160;E. coli&#160;BL21 (DE3) as a negative control (Figure 1A).
	<ol>
		<li>Culture Hif clinical isolates in brain-heart infusion (BHI) medium supplemented with 10 &#181;g/mL nicotinamide adenine dinucleotide (NAD) and hemin at 37 &#176;C with shaking at 200 rpm. Use Luria-Bertani medium to culture&#160;E. coli. Harvest Hif at mid-log phase (Optical density, OD600&#160;= 0.3), and resuspend the bacteria in phosphate-buffered saline (PBS), pH 7.2, containing 1% (w/v) bovine serum albumin (BSA) (blocking buffer; PBS-BSA). Adjust the suspension to 109&#160;colony-forming units, CFU/mL.</li>
		<li>Transfer the aliquots containing 5 x 106&#160;CFU to 5 mL polystyrene round-bottom tubes (12 x 75 mm2) and add 1 mL of blocking buffer. Centrifuge the suspension at 3,500 &#215;&#160;g&#160;at room temperature (RT) for 5 min to pellet the bacteria, then carefully aspirate to remove the supernatant without disturbing the pellet.</li>
		<li>Resuspend the bacterial pellets with 50 &#956;L of blocking buffer containing 250 nM Vn and incubate the samples for 1 h at RT without shaking. After incubation, pellet the bacteria by centrifugation at 3,500 x&#160;g&#160;for 5 min, then wash the pellets three times using PBS and similar centrifugation steps.</li>
		<li>To the bacterial pellet, add 50 &#956;L of primary sheep anti-human Vn polyclonal antibodies (pAbs) at 1:100 dilution in PBS-BSA. Incubate the suspension for 1 h at RT, then wash the bacteria three times with PBS to remove unbound antibodies (as described in step 1.1.3).</li>
		<li>Next, add 50 &#956;L of PBS-BSA containing fluorescein isothiocyanate (FITC)-conjugated donkey anti-sheep pAbs (1:100 dilution) and incubate at RT for 1 h in the dark.</li>
		<li>Prepare a blank control by incubating bacteria with blocking buffer only and pAbs without Vn.</li>
		<li>Wash bacteria three times with 1 mL of blocking buffer and pellet the suspension by centrifugation, as described in section 1.1.2. Finally, resuspend the bacterial pellet with 300 &#181;L of PBS and analyze it by flow cytometry.</li>
	</ol>
	</li>
</ol>

<table border="1" fo:keep-together.within-page="1" fo:keep-with-next.within-page="always">
	<tbody>
		<tr>
			<td>5 mL polystyrene round-bottom tube&#160;</td>
			<td>BD Falcon</td>
			<td>60819-138</td>
			<td>12 &#215; 75 mm style</td>
		</tr>
		<tr>
			<td>Bovine Serum Albumins (BSA)</td>
			<td>Sigma-Aldrich</td>
			<td>A2058</td>
			<td>Suitable for cell culture</td>
		</tr>
		<tr>
			<td>Flow cytometer&#160;</td>
			<td>BD Biosciences</td>
			<td>651154</td>
			<td>Cell analysis grade for research applications&#160;</td>
		</tr>
		<tr>
			<td>Vitronectin (Vn) from human plasma</td>
			<td>Sigma-Aldrich</td>
			<td>V8379-50UG</td>
			<td>Cell culture grade</td>
		</tr>
		<tr>
			<td>E. coli host (E. Coli BL21)</td>
			<td>Novagen</td>
			<td>69450-3</td>
			<td>Protein expression host</td>
		</tr>
		<tr>
			<td>FITC-conjugated donkey anti-sheep antibodies&#160;</td>
			<td>AbD Serotec</td>
			<td>STAR88F</td>
			<td>Polyclonal</td>
		</tr>
		<tr>
			<td>Sheep anti-human Vn antibodies</td>
			<td>AbD Serotec</td>
			<td>AHP396</td>
			<td>Polyclonal</td>
		</tr>
	</tbody>
</table>

detection of vitronectin binding to bacterial surfaces using flow cytometry

Source: Singh, B. et al., <a href="https://app.jove.com/v/54653">Assays for Studying the Role of Vitronectin in Bacterial Adhesion and Serum Resistance.</a>&#160;J. Vis. Exp.&#160;(2018)
This video demonstrates the detection of vitronectin&#39;s interaction with bacterial surface proteins. The flow-cytometry analysis measures the fluorescence signal of fluorescently labeled antibodies bound to vitronectin, confirming its presence at the bacterial surface. This technique provides insights into host-pathogen interactions and potential bacterial infection therapies.

<img alt="Figure 1" src="/files/ftp_upload/21806/21806_Figure1.jpg" /> 
Figure 1:&#160;Haemophilus influenzae&#160;serotype f binds Vn via surface-expressed PH.&#160;(A) Flow cytometry results showing binding of Vn to cells of Hif clinical isolates. Each clinical isolate (5 x 106&#160;CFU) was incubated with 250 nM human Vn. The bound ligand was detected using sheep anti-Vn pAbs and FITC-conjugated donkey anti-she...

Detection of Vitronectin Binding to Bacterial Surfaces using Flow Cytometry

1. Analysis of Vitronectin, Vn as a Bacterial Surface Protein-Ligand

	Detection of Vn-binding at the bacterial surface using flow cytometry
	NOTE: In ...

Take flow cytometer tubes containing wild-type and mutant strains of Haemophilus influenzae, type f.
Pipette a buffer containing blocking proteins and vitronectin. Incubate.
The blocking proteins reduce non-specific interactions on the bacterial surface, while vitronectin molecules bind to protein H, a vitronectin-binding protein, on wild-type bacterial surfaces. In the mutant strain, vitronectin does not bind due to the absence of protein H.
Centrifuge. Remove unbound vitronectin and blocking proteins.
Add a buffer containing primary anti-vitronectin antibodies, which specifically bind to vitronectin attached to the wild-type bacterial surfaces.
Next, introduce fluorophore-conjugated secondary antibodies, which bind to the primary antibodies on vitronectin and facilitate vitronectin detection.
Centrifuge. Remove unbound secondary antibodies. Resuspend bacteria in the buffer.
Perform flow cytometry to determine vitronectin binding to the bacterial surface.
Compare the fluorescence signals of wild-type and mutant strains. A shift in the fluorescence signal in wild-type bacteria confirms vitronectin binding to the bacterial surface.

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Research

JoVE Encyclopedia of Experiments

Immunology

Immunodiagnostics

Cellular Immunodiagnostics

95 Views. מקור: Singh, B. et al., Assays for Study the role of Vitronectin in Bacterial Adfusion and Serum Resistance.J. Vis. Exp.(2018) סרטון זה מדגים את זיהוי האינטראקציה של ויטרונקטין עם חלבוני פני השטח של חיידקים. ניתוח ציטומטריית הזרימה מודד את האות הפלואורסצנטי של נוגדנים המסומנים באופן פלואורסצנטי הקשורים לויטרונקטין, ומאשר את נ...

Video: איתור קישור ויטרונקטין למשטחים חיידקיים באמצעות ציטומטריית זרימה - Concept

Flow Cytometry-based Assay for the Monitoring of NK Cell Functions

Natural killer (NK) cells are an important part of the human tumor immune surveillance system. NK cells are able to distinguish between healthy and virus-infected or malignantly transformed cells due to a set of germline encoded inhibitory and activating receptors. Upon virus or tumor cell recognition a variety of different NK cell functions are initiated including cytotoxicity against the target cell as well as cytokine and chemokine production leading to the activation of other immune cells. It has been demonstrated that accurate NK cell functions are crucial for the treatment outcome of different virus infections and malignant diseases. Here a simple and reliable method is described to analyze different NK cell functions using a flow cytometry-based assay. NK cell functions can be evaluated not only for the whole NK cell population, but also for different NK cell subsets. This technique enables scientists to easily study NK cell functions in healthy donors or patients in order to reveal their impact on different malignancies and to further discover new therapeutic strategies.

A simple and reliable method is described here to analyze a set of NK cell functions such as degranulation, cytokine and chemokine production within different NK cell subsets.

Flow Cytometry מבוסס Assay עבור הניטור של פונקציות תא NK

Natural killer (NK) cells are an important part of the human tumor immune surveillance system. NK cells are able to distinguish between healthy and ...

JoVE Journal

Immunology and Infection

Quantifying Human Norovirus Virus-like Particles Binding to Commensal Bacteria Using Flow Cytometry

Commensal bacteria are well established to impact infection of eukaryotic viruses. Direct binding between the pathogen and the host microbiome is responsible for altering infection for many of these viruses. Thus, characterizing the nature of virus-bacteria binding is a foundational step needed for elucidating the mechanism(s) by which bacteria alter viral infection. For human norovirus, commensal bacteria enhance B cell infection. The virus directly binds to these bacteria, indicating that this direct interaction is involved in the mechanism of infection enhancement. A variety of techniques can be used to quantify interactions between bacteria and viruses including scintillation counting of radiolabeled viruses and polymerase chain reaction (PCR). Both methods require the use of live virus, which may need to be generated in the laboratory. Currently, none of the established in vitro culture systems available for human norovirus are robust enough to allow for generation of highly concentrated viral stocks. In lieu of live virus, virus-like particles (VLPs) have been used to characterize the interactions between norovirus and bacteria. Herein a flow cytometry method is described with uses virus specific antibodies to quantify VLP binding to gram-negative and gram-positive bacteria. Inclusion of both bacteria only and isotype controls allowed for optimization of the assay to reduce background antibody binding and accurate quantification of VLP attachment to the bacteria tested. High VLP:bacterium ratios result in VLPs binding to large percentages of the bacterial population. However, when VLP quantities are decreased, the percent of bacteria bound also decreases. Ultimately, this method can be employed in future experiments elucidating the specific conditions and structural components that regulate norovirus:bacterial interactions.

The goal of this protocol is to quantify binding of the eukaryotic pathogen human norovirus to bacteria. After performing an initial virus-bacterium attachment assay, flow cytometry is used to detect virally-bound bacteria within the population.

כימות האדם Norovirus וירוס כריכת כריכה של חיידקים קומנדסאל באמצעות זרימה Cy, לנסות

Commensal bacteria are well established to impact infection of eukaryotic viruses. Direct binding between the pathogen and the host microbiome is ...

Polarization of M1 and M2 Human Monocyte-Derived Cells and Analysis with Flow Cytometry upon Mycobacterium tuberculosis Infection

Human macrophages are primary host cells of intracellular Mycobacterium tuberculosis (Mtb) infection and thus have a central role in immune control of tuberculosis (TB). We have established an experimental protocol to follow immune polarization of myeloid-derived cells into M1 (classically activated) or M2 (alternatively activated) macrophage-like cells through assessment with a 10-color flow cytometry panel that allows visualization and deep-characterization of green-fluorescent-protein (GFP)-labeled Mtb in diverse macrophages subsets. Monocytes obtained from healthy blood donors were polarized into M1 or M2 cells using differentiation with granulocyte macrophage-colony-stimulating factor (GM-CSF) or macrophage-colony stimulating factor (M-CSF) followed by polarization with IFN-&#947; and lipopolysaccharide (LPS) or IL-4, respectively. Fully polarized M1 and M2 cells were infected with Mtb-GFP for 4 hours before detached Mtb-infected macrophages were stained with flow cytometry at 4- or 24-hours post-infection. Sample acquisition was performed with flow cytometry and the data was analyzed using a flow cytometry analysis software. Manual gating as well as dimensionality reduction with Uniform Manifold Approximation and Projection (UMAP) and phenograph analysis was performed. This protocol resulted in effective M1/M2 polarization characterized by elevated levels of CD64, CD86, TLR2, HLA-DR and CCR7 on uninfected M1 cells, while uninfected M2 cells exhibited a strong up-regulation of the M2 phenotype markers CD163, CD200R, CD206 and CD80. M1-polarized cells typically contained fewer bacteria compared to M2-polarized cells. Several M1/M2 markers were downregulated after Mtb infection, which suggests that Mtb can modulate macrophage polarization. In addition, 24 different cell clusters of different sizes were found to be uniquely distributed among the M1 and M2 uninfected and Mtb-infected cells at 24-hours post-infection. This M1/M2 flow cytometry protocol could be used as a backbone in Mtb-macrophage research and be adopted for special needs in different areas of research.

Polarization of M1 and M2 Human Monocyte-Derived Cells and Analysis with Flow Cytometry upon Mycobacterium tuberculosis Infection

This protocol provides a method to study Mycobacterium tuberculosis infection in human M1- or M2-polarized macrophages based on differentiation of peripheral-blood-monocytes to macrophage-like cells that are infected with the GFP-labeled virulent strain H37Rv, and analyzed with flow cytometry using a 10-color panel including expression of selected M1/M2 markers.

קיטוב של M1 ו M2 תאים נגזרים מונוציט אנושי וניתוח עם Cytometry זרימה על זיהום שחפת Mycobacterium

Human macrophages are primary host cells of intracellular Mycobacterium tuberculosis (Mtb) infection and thus have a central role in immune control of ...

Detection of Vitronectin Binding to Bacterial Surfaces using Flow Cytometry

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Detection of Vitronectin Binding to Bacterial Surfaces using Flow Cytometry