eoe sub articles

EoE Sub Articles

1. Preparation of CXCL12, Assay Buffer, and Jurkat Cells for the Competition Binding Assay
<ol>
	<li>Prepare a stock solution of CXCL12AF647 (20 &#181;g/mL; see Table of Materials and Reagents) by dissolving the lyophilized reagent (stored at -80 &#176;C, in the dark) in ultrapure water supplemented with 0.01% (volume/volume) of Polysorbate 20. Store single-use aliquots from this stock solution at -80 &#176;C, protected from light.</li>
	<li>Prepare assay buffer by adding 40 mL HEPES (1 M, 20 mM final concentration) to 200 mL Hank&#39;s Balanced Salt Solution (HBSS, 10x, without phenol red and without sodium bicarbonate, 1x final concentration). Add ultrapure water to obtain a final volume of 2 L. Add 4 g (0.2% weight/volume) bovine serum albumin (BSA), and dissolve the BSA via magnetic stirring. Finally, adjust the pH to 7.4 (use NaOH for this) and filter the solution through 0.2 &#181;m pores (see Table of Materials and Reagents) using a vacuum manifold. 
	NOTE: This assay buffer will be used in all further steps of the protocol.</li>
	<li>Count the number and the viability of the Jurkat cells. For this, take a sample of the cell suspension and dilute it in phosphate-buffered saline (PBS). 
	NOTE: We routinely use an automated cell viability analyzer (see Table of Materials and Reagents) capable of counting cell suspensions at varying concentrations. For cell counting, dilute 0.5 mL of cell suspension in 1.5 mL PBS (other dilutions, e.g., 0.1 mL in 1.9 mL PBS, are also possible). Several other devices are commercially available for counting cell numbers and viability that should work equally well.</li>
	<li>Collect the desired number of cells (i.e., ~24 x 106 cells to run the assay with one complete 96-well plate) in a sterile 50 mL tube by centrifugation (see Table of Materials and Reagents for the type of centrifuge used) at 400 x g for 5 min at RT.</li>
	<li>Gently pour off the supernatant without disturbing the cell pellet. Add fresh assay buffer (e.g., 20 mL) and resuspend the cells by gently pipetting up and down.</li>
	<li>Centrifuge the cells again at 400 x g for 5 min at RT.</li>
	<li>Pour off the supernatant again and resuspend the cell pellet in fresh assay buffer to obtain a density of 5 x 106 cells/mL.</li>
</ol>
2. Competition Binding Assay
NOTE: The actual competition binding assay is performed at RT and can be performed under non-sterile conditions.
<ol>
	<li>Dilute the compounds under investigation in assay buffer (see 1.2) to obtain the desired concentration. Either prepare a fixed concentration of compound for initial screening (e.g., 10 &#181;M final concentration) or, alternatively, a serial dilution series of concentrations for more detailed characterization of the compounds (e.g., a 1/3, 1/4, or 1/5 dilution series starting at 1 &#181;M, final concentration). Keep in mind that the compound solution will ultimately become 2x diluted in the assay; therefore, prepare a 2x concentrated solution.</li>
	<li>Dispense 100 &#181;L of compound solution (2x concentrated) into a clear 96-well round bottom plate (see Table of Materials and Reagents) according to a pre-defined experimental layout (e.g., Figure 1C). 
	NOTE: At this stage, negative and positive control samples are included in the assay. In the negative control sample, 100 &#181;L of assay buffer is added instead of the compound to the wells of the 96-well plate. For the positive control sample, an assay buffer is also added during this step. See also Figure 1C for a typical experimental layout in which a dilution series of several compounds is tested.</li>
	<li>Add 50 &#181;L of cell suspension (see 1.7; 0.25 x 106 cells) from a reagent reservoir into the 96-well plate using a multichannel pipette. Incubate the plate for 15 min at RT in the dark.</li>
	<li>Add 50 &#181;L of fluorescently labeled CXCL12 (i.e., 100 ng/mL of CXCL12AF647 in assay buffer, 4x concentrated, 25 ng/mL final concentration) from a similar reagent reservoir to the wells of the 96-well plate. Incubate for 30 min at RT in the dark. 
	NOTE: For the negative control samples, add assay buffer instead. Hence, the fluorescent signal detected in the negative control samples will correspond to the autofluorescent background signal (Figure 1A). For the positive control samples, add 50 &#181;L/well of CXCL12AF647. The positive control samples will yield the maximal fluorescence signal detected since no potential inhibition by pre-incubation with compounds was included (Figure 1A).</li>
	<li>Centrifuge the 96-well plate at 400 x g for 5 min at RT. Remove the supernatant from the pelleted cells by flipping over the plate. Dry the plate on a tissue.</li>
	<li>Add 200 &#181;L of fresh assay buffer from a reagent reservoir to the wells using a multichannel pipette. Immediately proceed.</li>
	<li>Centrifuge the plate again for 5 min at 400 x g at RT. Remove the supernatant by flipping over the plate and again dry it on a tissue.</li>
	<li>Gently resuspend the cell pellet in 200 &#181;L of 1% paraformaldehyde dissolved in PBS. This step will fix the cells.</li>
	<li>Continue the protocol immediately with the quantification of the fluorescence by flow cytometry.</li>
</ol>
3. Analysis of the samples by flow cytometry
CXCL12AF647 stained and fixated cells are now ready to be analyzed using flow cytometry. Several types of flow cytometers can be used, but they need to be equipped with the correct laser (i.e., a red laser, excitation range ~630 nm) for excitation and suitable filters for fluorophore detection (emission filters ~660 nm). They need to be capable of handling samples in a 96-well plate format. Examples of suitable flow cytometry devices are given in the Table of Materials and Reagents.
<ol>
	<li>Start up the device and open the corresponding software (see Table of Materials and Reagents).</li>
	<li>Select the following cellular parameters to be visualized in a dot blot format: forward scatter (FSC), side scatter (SSC), and the fluorophore (CXCL12AF647) detection channel. 
	NOTE: With the FSC parameter, cells are discriminated based on their size, since the detected light absorption is proportional to the cell&#39;s diameter. The SSC parameter, measuring light scattering at a 90&#176; angle, provides information about the granularity of the cells.</li>
	<li>Choose one sample (e.g., a negative control sample) to perform gating of a defined homogenous cell population based on the FSC and SSC parameters.
	<ol>
		<li>Select automatic injection of ~100 &#181;L of fixated cells from this negative control sample into the flow cytometer. Select the option &#34;mixing&#34; before injection and use a sample flow rate of 1.5 &#181;L/s.</li>
		<li>Run this sample by selecting &#34;Acquire Data.&#34; The FSC and SSC parameters for this sample will now appear on the screen.</li>
		<li>Select the software&#39;s gating tool. Based on the FSC and SSC dot blot visualization, pre-define a homogenous and viable cell population by gating. To do so, create a polygon (using the software&#39;s gating tool) that includes the homogenously distributed single cells (&#34;events&#34;) based on these two dimensions. 
		NOTE: The gating procedure aims to define a homogenous and viable cell population that will be used for further analysis. Gating relies on the assumption that the majority of viable cells will form a homogenous cell population based on the FSC and SSC parameters. By performing this step, cellular debris, dead cells, and cell aggregates can largely be excluded from further analysis. An illustration of the gating process is given in Figure 1B.</li>
	</ol>
	</li>
	<li>Select to analyze 20,000 &#34;events&#34; (i.e., single cells) per sample. 
	NOTE: This means that for each sample, 20,000 cells that fall within the pre-defined gate will eventually be analyzed. Data acquisition for each sample will continue until this number of events is analyzed.</li>
	<li>Start the run (select &#34;Record Data&#34;). The flow cytometry device will now analyze all samples one-by-one by recording the mean fluorescence intensity (MFI) for each sample. This MFI corresponds to the mean fluorescent signal corresponding to the 20,000 cells that fall within the pre-defined gate.</li>
</ol>

<table><tbody><tr><td>BD FACSCanto II</td><td>Becton Dickinson</td><td>Not applicable</td><td>Flow cytometry device</td></tr><tr><td>BD FACSDIVA Software</td><td></td><td></td><td></td></tr><tr><td>BD FACSArray</td><td>Becton Dickinson</td><td>Not applicable</td><td>Flow cytometry device</td></tr><tr><td>BD FACSArray System Software</td><td></td><td></td><td></td></tr><tr><td>Rapid flow filter: 0.2 &amp;mu;m aPES&amp;nbsp;</td><td>Thermo Scientific&amp;nbsp;</td><td>566-0020</td><td></td></tr><tr><td>FlowJo</td><td>FlowJo is now a wholly owned subsidiary of BD.</td><td></td><td></td></tr><tr><td>Vi-CELL</td><td>Beckman Coulter</td><td>Not applicable</td><td>Cell viability analyzer</td></tr><tr><td>Sigma 3-18 KS</td><td>Sigma</td><td>Not applicable</td><td>Centrifuge</td></tr><tr><td>AMD3100</td><td>Sigma</td><td>A5602-5mg</td><td>Specific CXCR4 antagonist</td></tr><tr><td>h-SDF1a (AF647)</td><td>ALMAC</td><td>CAF-11-B-01</td><td>Fluorescently-labeled CXCL12, CXCL12AF647</td></tr><tr><td>Sterilin microtiter plate, 96-well, U&lt;br/&gt; bottom, clear</td><td>Thermo Scientific</td><td>611U96</td><td></td></tr><tr><td>Bovine Serum Albumin (BSA)</td><td>Sigma</td><td>A1933-25G</td><td></td></tr><tr><td>HBSS (10x), calcium, magnesium, no phenol red</td><td>Gibco (Life Technologies)</td><td>14065-049</td><td></td></tr><tr><td>HEPES (1M)</td><td>Gibco (Life Technologies)</td><td>15630-056</td><td></td></tr><tr><td>Dulbecco&#039;s Phosphate Buffered Saline (DPBS)</td><td>Gibco (Life Technologies)</td><td>14190-094</td><td></td></tr><tr><td>Jurkat cells</td><td>ATCC</td><td></td><td></td></tr><tr><td>Reagent reservoir PP</td><td>Sigma</td><td>BR703411</td><td></td></tr><tr><td>Falcon tubes, 50ml</td><td>Greiner Bio-One</td><td>227 261</td><td></td></tr></tbody></table>

competitive binding assay to identify compounds disrupting receptor-ligand interactions

Source: Schoofs, G., et al. <a href="https://app-jove-com.remotexs.ntu.edu.sg/v/57271">A Flow Cytometry-based Assay to Identify Compounds That Disrupt Binding of Fluorescently-labeled CXC Chemokine Ligand 12 to CXC Chemokine Receptor 4.</a> J. Vis. Exp. (2018).
In this video, we describe a flow cytometry-based competitive binding assay to detect the interactions between the CXC Chemokine Receptor 4 (CXCR4) and its fluorescently-labeled natural ligand CXC Chemokine Ligand 12 (CXCL12), in the presence of a CXCR4-targeting small molecule. Incubating CXCR4-expressing cells with lower small molecule concentrations allows CXCR4-CXCL12 binding to some extent, which progressively declines upon a gradual increase in small molecule concentrations.

<img alt="Figure 1" src="/files/ftp_upload/21451/21451_Figure1.jpg" /> 
Figure 1: Overview of the workflow and illustration of the type of data obtained. (A). The main steps of the protocol are schematized for the negative and positive control samples, and compound-treated samples. Samples without compound pre-incubation and without addition of fluorescently labeled chemokine (CXCL12AF647) are included to determine the background (auto)fluorescence (negative control samples). Samples without compound pre-incubation, but with addition of a fixed amount of CXCL12AF647 are used to determine the maximal binding signal in the assay (positive control samples). In compound-treated samples, cells are pre-incubated with compound before addition of a fixed amount of CXCL12AF647. (B). The mean fluorescent binding signal is determined by flow cytometry analysis of Jurkat cells. From all events (i.e., Jurkat cells) analyzed (left panel) only the fluorescent signal from a gated subpopulation of cells is used for further analysis (middle panel). Pre-incubation of cells with small molecules (e.g., AMD3100) inhibits the binding of the fluorescently labeled receptor ligand and this will reduce the maximal binding signal (right panel, shown in a histogram representation). (C). A possible plate layout when performing the competitive binding assay in a 96-well plate format. In this case, six different compounds (cpd 1-&#160; 6) are tested in a 1/5 serial dilution series (in duplicate) ranging from 1,000 nM down to 0.32 nM.

Competitive Binding Assay to Identify Compounds Disrupting Receptor-Ligand Interactions

Source: Schoofs, G., et al. A Flow Cytometry-based Assay to Identify Compounds That Disrupt Binding of Fluorescently-labeled CXC Chemokine Ligand 12 to ...

The competitive binding assay identifies small molecules that disrupt receptor-ligand interactions by competitively binding to a target receptor, inhibiting natural ligand binding.
To identify a receptor&#39;s interactions with its natural ligand in the presence of a receptor-specific small molecule antagonist, begin with a suspension of human T-lymphocyte cells expressing the target receptor.
Add the cell suspension to the wells of a multi-well plate containing increasing antagonist concentrations. Incubate. The antagonist binds to the orthosteric binding site &#8212; the receptor&#39;s natural ligand-binding site.
Add a fixed concentration of fluorescently-labeled natural ligands to the wells. Incubate.
At low concentrations, the antagonists occupy few orthosteric binding sites, allowing natural ligand binding to the receptors. However, at higher concentrations, the antagonists occupy most of the orthosteric binding sites, allowing minimal natural ligand-receptor binding.
Centrifuge to pellet the cells. Discard the supernatant. Resuspend the cells in paraformaldehyde to fix them, preserving the cellular morphology.
Using a flow cytometer, analyze the fluorescence signals from individual T-lymphocytes expressing the antagonist- and fluorescent ligand-bound receptors.
A dose-dependent decrease in the mean fluorescence intensity with increasing receptor-specific antagonist concentrations indicates competitive binding of the antagonists to the orthosteric receptor-binding sites, inhibiting natural ligand-receptor interaction.

competitive-binding-assay-to-identify-compounds-disrupting-receptor

Nanyang Technological University

Research

JoVE Encyclopedia of Experiments

Biological Techniques

Biomolecular Interaction Detection Techniques

Protein-protein interactions

198 次观看. 来源:Schoofs， G. 等人。 一种基于流式细胞术的检测方法，用于鉴定破坏荧光标记的 CXC 趋化因子配体 12 与 CXC 趋化因子受体 4 结合的化合物。J. Vis. Exp.（2018 年）。 在本视频中，我们描述了一种基于流式细胞术的竞争性结合测定法，以检测 CXC 趋化因子受体 4 （CXCR4） 与其荧光标记的天然配体 CXC 趋化因子配体 12 （CXCL12） 之间的相互作用，在靶向 CXCR4 的小分子存在下。用较低...

视频: 竞争性结合测定，用于鉴定破坏受体-配体相互作用的化合物 - 概念

An ELISA Based Binding and Competition Method to Rapidly Determine Ligand-receptor Interactions

A comprehensive understanding of signaling pathways requires detailed knowledge regarding ligand-receptor interaction. This article describes two fast and reliable point-by-point protocols of enzyme-linked immunosorbent assays (ELISAs) for the investigation of ligand-receptor interactions: the direct ligand-receptor interaction assay (LRA) and the competition LRA. As a case study, the ELISA based analysis of the interaction between different lambda interferons (IFNLs) and the alpha subunit of their receptor (IL28RA) is presented: the direct LRA is used for the determination of dissociation constants (KD values) between receptor and IFN ligands, and the competition LRA for the determination of the inhibitory capacity of an oligopeptide, which was designed to compete with the IFNLs at their receptor binding site. Analytical steps to estimate KD and half maximal inhibitory concentration (IC50) values are described. Finally, the discussion highlights advantages and disadvantages of the presented method and how the results enable a better molecular understanding of ligand-receptor interactions.

The presented protocols describe two enzyme-linked immunosorbent assay (ELISA) based techniques for the rapid investigation of ligand-receptor interactions: The first assay allows the determination of dissociation constant between ligand and receptor. The second assay enables a rapid screening of blocking peptides for ligand-receptor interactions.

的ELISA基结合和竞争法快速测定配体 - 受体相互作用

A comprehensive understanding of signaling pathways requires detailed knowledge regarding ligand-receptor interaction. This article describes two fast and ...

科研

JoVE Journal

化学

Analyzing the Interaction of Fluorescent-Labeled Proteins with Artificial Phospholipid Microvesicles using Quantitative Flow Cytometry

In the human body, most of the major physiologic reactions involved in the immune response and blood coagulation proceed on the membranes of cells. An important first step in any membrane-dependent reaction is binding of protein on the phospholipid membrane. An approach to studying protein interaction with lipid membranes has been developed using fluorescently labeled proteins and flow cytometry. This method allows the study of protein-membrane interactions using live cells and natural or artificial phospholipid vesicles. The advantage of this method is the simplicity and availability of reagents and equipment. In this method, proteins are labeled using fluorescent dyes. However, both self-made and commercially available, fluorescently labeled proteins can be used. After conjugation with a fluorescent dye, the proteins are incubated with a source of the phospholipid membrane (microvesicles or cells), and the samples are analyzed by flow cytometry. The obtained data can be used to calculate the kinetic constants and equilibrium Kd. In addition, it is possible to estimate the approximate number of protein binding sites on the phospholipid membrane using special calibration beads.

Here, we describe a set of methods for characterizing the interaction of proteins with membranes of cells or microvesicles.

使用定量流式细胞术分析荧光标记蛋白与人工磷脂微泡的相互作用

In the human body, most of the major physiologic reactions involved in the immune response and blood coagulation proceed on the membranes of cells. An ...

生物化学

A BW Reporter System for Studying Receptor-Ligand Interactions

Interactions between receptors and ligands constitute a fundamental biological process. However, direct experiments with cells that express the native receptor and the ligand are challenging since the ligand of a specific receptor may be unknown and experimental procedures with the native ligand can be technically complicated. To address these obstacles, we describe a reporter system to detect the binding and activation of a specific receptor by a ligand of interest. In this reporter system, the extracellular domain of a specific receptor is conjugated to mouse CD3&#950; and this chimeric protein is then expressed in mouse BW cells. These transfected BW cells can then be incubated with different targets (e.g., cells or antibodies). Activation of a transfected receptor leads to the secretion of mouse interleukin-2 (mIL-2) which can be detected by enzyme-linked immunosorbent assay (ELISA). This reporter system has the advantages of being sensitive and specific to a single receptor. In addition, the activation level of a specific receptor can easily be quantified and can be used even in cases where the ligand of the receptor is unknown. This system has been implemented successfully in many of our studies to characterize receptor-ligand interactions. We have recently employed this system to study the activation of human Fc&#947; receptors (Fc&#947;Rs) by different monoclonal anti-CD20 antibodies in clinical use.

This protocol describes how to establish a reporter system that can be used to identify and quantify receptor-ligand interactions.

一种研究受体配体相互作用的 bw 报告系统

Interactions between receptors and ligands constitute a fundamental biological process. However, direct experiments with cells that express the native ...

Competitive Binding Assay to Identify Compounds Disrupting Receptor-Ligand Interactions

成績單

Competitive Binding Assay to Identify Compounds Disrupting Receptor-Ligand Interactions