eoe sub articles

EoE Sub Articles

1. Purification of GST-tagged GTPase
<ol>
	<li>Culture an E. coli strain such as BL21 transformed with pGEX-Rac1 O/N at 37 &#176;C, shaking at 220 rpm, in 500 ml of autoinduction media (25 mM Na2HPO4, 25 mM KH2PO4, 50 mM NH4Cl, 5 mM Na2SO4, 2 mM MgSO4, 2 mM CaCl2, 0.5% Glycerol, 0.05% Glucose, 0.2% Lactose, 5 g Tryptone, 2.5 g Yeast Extract, 100 &#181;g/ml Ampicillin).</li>
	<li>Harvest bacteria by centrifugation for 10 min at 10,000 x g, 4 &#176;C.</li>
	<li>Resuspend bacterial pellet in 20 ml protein extraction reagent, 1x protease inhibitor, and incubate for 20 min at RT with inversion.</li>
	<li>Clarify the lysate by centrifugation at 40,000 x g for 30 min.</li>
	<li>Add 2 ml glutathione magnetic beads, washed with phosphate-buffered saline (PBS: 10 mM Na2HPO4, 1.8 mM KH2PO4, 137 mM NaCl, 2.7 mM KCl).</li>
	<li>Incubate for 2 hr, mixing by inversion at 4 &#176;C.</li>
	<li>Wash protein-loaded beads four times with 10 ml PBS, using a magnetic particle sorter to precipitate the beads at each step.</li>
	<li>Resuspend protein-loaded beads in 2 ml PBS and store at -80 &#176;C in 100 &#181;l aliquots until needed.</li>
</ol>
2. Expression of GTPase-binding proteins
<ol>
	<li>The day before the experiment, transfect plasmids encoding the green fluorescent protein (GFP)-tagged versions of each GTPase-binding protein into a separate 75-cm2 flask of HEK293T as follows. For validation of nucleotide loading, transfect GFP-tagged TrioD1 into a third 75-cm2 flask of HEK293T.
	<ol>
		<li>Dilute polyethylamine to 1 mg/ml in 100 &#181;l sterile 150 mM NaCl.</li>
		<li>Add 27 &#181;l diluted polyethylamine to 223 &#181;l reduced serum media.</li>
		<li>Add 12 &#181;g plasmid DNA to 250 &#181;l reduced serum media.</li>
		<li>Incubate each tube for 2 min at RT.</li>
		<li>Combine the polyethylamine and DNA mixes in a single tube and vortex for 2 min.</li>
		<li>Incubate for 15-20 min at RT.</li>
		<li>Replace the growth media (Dulbecco&#39;s Modified Eagle Media, 10% fetal bovine serum, 2 mM L-glutamine, no antibiotics) on 90% confluent HEK293T with 5 ml fresh growth media.</li>
		<li>Add the combined polyethylamine/DNA mix to the flask and incubate O/N at 37 &#176;C, 5% CO2.</li>
	</ol>
	</li>
</ol>
3. Purification of GTPase-binding proteins
<ol>
	<li>Rinse flasks of transfected cells in PBS and drain the flask for 5 min, aspirating free liquid.</li>
	<li>Scrape off cells in 500 &#181;l lysis buffer (50 mM Tris-HCl (pH 7.8), 1% Nonidet P-40, 1x protease inhibitor) into a microfuge tube.</li>
	<li>Lyse cells by mixing by inversion at 4 &#176;C for 30 min.</li>
	<li>During lysis, wash two lots of 40 &#181;l GFP-Trap beads three times with fresh lysis buffer, sedimenting beads at 2,700 x g for 2 min between washes.</li>
	<li>Clarify lysates by centrifugation at 21,000 x g for 10 min.</li>
	<li>Transfer clarified lysate of each of the competitor proteins to separate washed GFP-trap beads and allow GFP-fusion proteins to bind for 2 hr, mixing by inversion at 4 &#176;C. Keep lysate from GFP-TrioD1 cells on ice.</li>
	<li>Wash loaded GFP-Trap beads twice in 50 mM Tris-HCl (pH 7.8), 50 mM NaCl, 0.7% (w/v) Nonidet P-40 and twice in 50 mM Tris-HCl (pH 7.6), 20 mM MgCl2, sedimenting beads at 2,700 x g for 2 min between washes.</li>
	<li>Elute GFP-fusion proteins by adding 40 &#181;l 0.2 M glycine (pH 2.5) and pipetting up and down for 30 sec. Immediately sediment beads at 21,000 x g for 60 s and transfer liquid to a new microfuge tube containing 4 &#181;l 1 M Tris-HCl (pH 10.4). Do this quickly to limit damage to the purified protein.</li>
	<li>Analyze 1 &#181;l of each purified protein by Western blot and probe with an anti-GFP antibody to establish relative yield using a quantitative blotting system according to the manufacturer&#39;s protocol. Alternatively, determine protein concentrations by bicinchoninic acid (BCA) assay but this introduces errors if the proteins do not react with the assay in an identical fashion or if there are contaminant proteins.</li>
	<li>Equalize molar protein concentration by the addition of 50 mM Tris-HCl (pH 7.6) and 20 mM MgCl2.</li>
</ol>
4. Nucleotide loading of GTPase
<ol>
	<li>Thaw one aliquot of GST-Rac1 magnetic beads, prepared in step 1.</li>
	<li>Take 90 &#181;l of GST-Rac1 beads and wash three times with 20 mM Tris-HCl (pH 7.6), 25 mM NaCl, 0.1 mM DTT, and 4 mM EDTA, using a magnetic particle sorter to precipitate the beads at each step.</li>
	<li>Aspirate buffer from beads and add 100 &#181;l 20 mM Tris-HCl (pH 7.6), 25 mM NaCl, 0.1 mM DTT, and 4 mM EDTA.</li>
	<li>According to whether GDP, GTP, or no nucleotide loading is required for the competition experiment, add 12 &#181;l 100 mM GDP, 12 &#181;l 10 mM guanosine 5&#39;-[&#947;-thio]triphosphate (GTP&#947;S) or no nucleotide to 60 &#181;l GST-Rac1 beads.</li>
	<li>For the nucleotide-loading controls, split the remaining beads into three 10-&#181;l aliquots and add 2 &#181;l 100 mM GDP, 2 &#181;l 10 mM GTP&#947;S or no nucleotide to each tube.</li>
	<li>Incubate bead mixes for 30 min at 30 &#176;C with agitation.</li>
	<li>Stabilize nucleotide-bound Rac1 by addition of 1 M MgCl2: 3 &#181;l to the experimental mix (step 4.4), and 0.5 &#181;l to each of the control mixes (step 4.5).</li>
</ol>
5. Competition binding
<ol>
	<li>Set up 6 microfuge tubes, each containing: 
	200 &#181;l 50 mM Tris-HCl (pH 7.6), 20 mM MgCl2 
	10 &#181;l experimental nucleotide-loaded Rac1 beads (from step 4.7) 
	5 &#181;l Rac1-binding protein A (constant binding protein)</li>
	<li>To each tube, add 0, 1, 2.5, 5, 10, or 20 &#181;l Rac1-binding protein B (variable binding protein). These volumes assume approximately equal stock concentrations of the constant and variable binding proteins and may need to be adjusted.
	<ol>
		<li>Adjust volumes of binding proteins A and B if there are large differences in the binding affinities of the two proteins and this should be determined empirically through the experimental repeats. Make up the total volume of the binding mixture to 235 &#181;l by the addition of 50 mM Tris-HCl (pH 7.6), and 20 mM MgCl2.</li>
	</ol>
	</li>
	<li>Set up a microfuge tube containing: 
	200 &#181;l 50 mM Tris-HCl (pH 7.6), 20 mM MgCl2 
	10 &#181;l experimental nucleotide-loaded Rac1 beads (from step 4.7) 
	10 &#181;l Rac1-binding protein A (constant binding protein)</li>
	<li>Set up the GDP, GTP&#947;S, and no nucleotide control tubes: 
	200 &#181;l 50 mM Tris-HCl (pH 7.6), 20 mM MgCl2 
	10 &#181;l control Rac1 beads loaded in step 4.5 with GDP, GTP&#947;S, or no nucleotide and stabilized in step 4.7. 
	180 &#181;l HEK293T GFP-TrioD1 lysate, prepared as in step 3.6 
	4 &#181;l 1 M MgCl2</li>
	<li>Incubate the mixture for 2 hr, mixing by inversion at 4 &#176;C.</li>
	<li>Wash the beads three times with 50 mM Tris-HCl (pH 7.6), and 20 mM MgCl2.</li>
	<li>Elute bound proteins in 20 &#181;l reducing sample buffer (50 mM Tris-HCl (pH 7), 5% SDS, 20% glycerol, 0.02 mg/ml bromophenol blue, 5% &#946;-mercaptoethanol).</li>
</ol>

<table border="1" fo:keep-together.within-page="1" fo:keep-with-next.within-page="always">
	<tbody>
		<tr>
			<td>Bugbuster</td>
			<td>Novagen</td>
			<td>70584-3</td>
			<td></td>
		</tr>
		<tr>
			<td>COMPLETE protease inhibitor</td>
			<td>Roche</td>
			<td>05 056 489 001</td>
			<td></td>
		</tr>
		<tr>
			<td>Glutathione magnetic beads</td>
			<td>Pierce</td>
			<td>88821</td>
			<td></td>
		</tr>
		<tr>
			<td>Polyethylenimine, branched, average Mw ~ 25,000</td>
			<td>Sigma Aldrich</td>
			<td>408727-100ML</td>
			<td></td>
		</tr>
		<tr>
			<td>OPIMEM</td>
			<td>Life Technologies</td>
			<td>31985-047</td>
			<td></td>
		</tr>
		<tr>
			<td>Dulbecco&#39;s Modified Eagle Media</td>
			<td>Sigma Aldrich</td>
			<td>D5796</td>
			<td></td>
		</tr>
		<tr>
			<td>Fetal Bovine Serum</td>
			<td>Life Technologies</td>
			<td>10270-1-6</td>
			<td></td>
		</tr>
		<tr>
			<td>L-Glutamine</td>
			<td>Life Technologies</td>
			<td>25030-024</td>
			<td></td>
		</tr>
		<tr>
			<td>GFP-Trap_A</td>
			<td>Chromotec</td>
			<td>gta-20</td>
			<td></td>
		</tr>
		<tr>
			<td>GDP</td>
			<td>Sigma Aldrich</td>
			<td>G7127</td>
			<td>Highly unstable. Aliquot and store at -80 immediately upon reconstitution</td>
		</tr>
		<tr>
			<td>GTP&#947;S</td>
			<td>Sigma Aldrich</td>
			<td>G8634</td>
			<td>Highly unstable. Aliquot and store at -80 immediately upon reconstitution</td>
		</tr>
		<tr>
			<td>Blocking Buffer</td>
			<td>Sigma Aldrich</td>
			<td>B6429</td>
			<td></td>
		</tr>
		<tr>
			<td>Tween-20</td>
			<td>Sigma Aldrich</td>
			<td>P9416</td>
			<td></td>
		</tr>
		<tr>
			<td>Anti-GFP antibody</td>
			<td>Living Colors</td>
			<td>632592</td>
			<td>Use at 1/1000 dilution</td>
		</tr>
		<tr>
			<td>DyLight 800 conjugated goat anti-rabbit secondary antibody</td>
			<td>Fisher Scientific</td>
			<td>10733944</td>
			<td></td>
		</tr>
		<tr>
			<td>Odyssey SA Infrared Imaging System</td>
			<td>Li-cor</td>
			<td>9260-11PC</td>
			<td></td>
		</tr>
	</tbody>
</table>

competition binding assay to study competing gtpase-binding protein partners

Source: Williamson, R. C., et al.&#160; <a href="https://app.jove.com/v/53254">Comparing the Affinity of GTPase-binding Proteins using Competition Assays.</a> J. Vis. Exp. (2015)
This video demonstrates a competition assay to study GTPase-binding protein partners. Utilizing nucleotide-bound GTPase protein immobilized on magnetic beads, the competitive binding between two interacting protein partners for the same binding site on the GTPase can be studied to assess the binding affinities of the protein partners.

Competition Binding Assay to Study Competing GTPase-Binding Protein Partners

Source: Williamson, R. C., et al.&#160; Comparing the Affinity of GTPase-binding Proteins using Competition Assays. J. Vis. Exp. (2015)
This video ...

Guanine nucleotide-binding proteins &#8212; a category of GTPases &#8212; function as a molecular switch, cycling between a GTP-bound active form and a GDP-bound inactive form.
The active GTPases bind to specific protein partners. These partners compete for the same binding site on the GTPases.
To study competitive binding, begin by taking a suspension of GTP-bound GTPase immobilized on magnetic beads. Add the first interaction partner &#8212; fluorescently-tagged protein A. Incubate under agitation to keep the beads in suspension. Protein A binds and saturates the binding sites on all the GTPase molecules.
Partition this solution equally into multiple tubes. Add a second interaction partner &#8212; fluorescently-tagged protein B &#8212; to the tubes in increasing amounts. Incubate under agitation.
Protein B binds to the same binding site on the GTPases &#8212; competitively displacing protein A.
Expose the tubes to a magnetic field to collect the beads on one side. Discard the supernatant to remove unbound proteins. Resuspend the protein-complexed beads in a suitable buffer, and quantify the bound proteins.
Plot the relative intensities of proteins A and B bound to GTPase at each concentration of protein B.
Protein B reaches an equilibrium &#8212; occupying the binding sites of half of the GTPase molecules &#8212; at a relatively lower concentration than protein A, indicating the higher affinity of protein B for GTPase.

competition-binding-assay-to-study-competing-gtpase-binding-protein

Research

JoVE Encyclopedia of Experiments

Biological Techniques

Biomolecular Interaction Detection Techniques

Protein-protein interactions

106 ビュー. 出典:Williamson, R. C., et al. Comparing the Affinity of GTPase-binding Proteins using Competition Assays. J. Vis. Exp. (2015) このビデオでは、GTPase結合タンパク質パートナーを研究するための競合アッセイを実演しています。磁気ビーズに固定化されたヌクレオチド結合GTPaseタンパク質を利用すると、GTPase上の同じ結合部位に対する2つの相互作用タンパク質パートナー間の競合的結合を研究し、タン...

ビデオ: 競合するGTPase結合タンパク質パートナーを研究するための競合結合アッセイ - 概念

Oligopeptide Competition Assay for Phosphorylation Site Determination

Protein phosphorylation at specific sites determines its conformation and interaction with other molecules. Thus, protein phosphorylation affects biological functions and characteristics of the cell. Currently, the most common method for discovering phosphorylation sites is by liquid chromatography/mass spectrometry (LC/MS) analysis, a rapid and sensitive method. However, relatively labile phosphate moieties are often released from phosphopeptides during the fragmentation step, which often yields false-negative signals. In such cases, a traditional in vitro kinase assay using site-directed mutants would be more accurate, but this method is laborious and time-consuming. Therefore, an alternative method using peptide competition may be advantageous. The consensus recognition motif of 5&#39; adenosine monophosphate-activated protein kinase (AMPK) has been established1 and was validated using a positional scanning peptide library assay2. Thus, AMPK phosphorylation sites for a novel substrate could be predicted and confirmed by the peptide competition assays. In this report, we describe the detailed steps and procedures for the in vitro oligopeptide-competing kinase assay by illustrating AMPK-mediated nuclear factor erythroid 2-related factor 2 (Nrf2) phosphorylation. To authenticate the phosphorylation site, we carried out a sequential in vitro kinase assay using a site-specific mutant. Overall, the peptide competition assay provides a method to screen multiple potential phosphorylation sites and to identify sites for validation by the phosphorylation site mutants.

Peptide competition assays are widely used in a variety of molecular and immunological experiments. This paper describes a detailed method for an in vitro oligopeptide-competing kinase assay and the associated validation procedures, which may be useful to find specific phosphorylation sites.

リン酸化部位決定のためのオリゴペプチド競合アッセイ

Protein phosphorylation at specific sites determines its conformation and interaction with other molecules. Thus, protein phosphorylation affects ...

JoVE Journal

生化学

High Sensitivity Measurement of Transcription Factor-DNA Binding Affinities by Competitive Titration Using Fluorescence Microscopy

Accurate quantification of transcription factor (TF)-DNA interactions is essential for understanding the regulation of gene expression. Since existing approaches suffer from significant limitations, we have developed a new method for determining TF-DNA binding affinities with high sensitivity on a large scale. The assay relies on the established fluorescence anisotropy (FA) principle but introduces important technical improvements. First, we measure a full FA competitive titration curve in a single well by incorporating TF and a fluorescently labeled reference DNA in a porous agarose gel matrix. Unlabeled DNA oligomer is loaded on the top as a competitor and, through diffusion, forms a spatio-temporal gradient. The resulting FA gradient is then read out using a customized epifluorescence microscope setup. This improved setup greatly increases the sensitivity of FA signal detection, allowing both weak and strong binding to be reliably quantified, even for molecules of similar molecular weights. In this fashion, we can measure one titration curve per well of a multi-well plate, and through a fitting procedure, we can extract both the absolute dissociation constant (KD) and active protein concentration. By testing all single-point mutation variants of a given consensus binding sequence, we can survey the entire binding specificity landscape of a TF, typically on a single plate. The resulting position weight matrices (PWMs) outperform those derived from other methods in predicting in vivo TF occupancy. Here, we present a detailed guide for implementing HiP-FA on a conventional automated fluorescent microscope and the data analysis pipeline.

Here we present a novel method for determining binding affinities at equilibrium and in solution with high sensitivity on a large scale. This improves the quantitative analysis of transcription factor-DNA binding. The method is based on automated fluorescence anisotropy measurements in a controlled delivery system.

蛍光顕微鏡を使用して競争力のある滴定による転写因子の DNA 結合親和性の高感度測定

Accurate quantification of transcription factor (TF)-DNA interactions is essential for understanding the regulation of gene expression. Since existing ...

Exploring Biomolecular Interaction Between the Molecular Chaperone Hsp90 and Its Client Protein Kinase Cdc37 using Field-Effect Biosensing Technology

Biomolecular interactions play versatile roles in numerous cellular processes&#160;by regulating and coordinating functionally relevant biological events. Biomolecules such as proteins, carbohydrates, vitamins, fatty acids, nucleic acids, and enzymes are fundamental building blocks of living beings; they assemble into complex networks in biosystems to synchronize a myriad of life events. Proteins typically utilize complex interactome networks to carry out their functions; hence it is mandatory to evaluate such interactions to unravel their importance in cells at both cellular and organism levels. Toward this goal, we introduce a rapidly emerging technology, field-effect biosensing (FEB), to determine specific biomolecular interactions. FEB is a benchtop, label-free, and reliable biomolecular detection technique to determine specific interactions and uses high-quality electronic-based biosensors. The FEB technology can monitor interactions in the nanomolar range due to the biocompatible nanomaterials used on its biosensor surface. As a proof of concept, the protein-protein interaction (PPI) between heat shock protein 90 (Hsp90) and cell division cycle 37 (Cdc37) was elucidated. Hsp90 is an ATP-dependent molecular chaperone that plays an essential role in the folding, stability, maturation, and quality control of many proteins, thereby regulating multiple vital cellular functions. Cdc37 is regarded as a protein kinase-specific molecular chaperone, as it specifically recognizes and recruits protein kinases to Hsp90 to regulate their downstream signal transduction pathways. As such, Cdc37 is considered a co-chaperone of Hsp90. The chaperone-kinase pathway (Hsp90/Cdc37 complex) is hyper-activated in multiple malignancies promoting cellular growth; therefore, it is a potential target for cancer therapy. The present study demonstrates the efficiency of FEB technology using the Hsp90/Cdc37 model system. FEB detected a strong PPI between the two proteins (KD values of 0.014 &#181;M, 0.053 &#181;M, and 0.072 &#181;M in three independent experiments). In summary, FEB is a label-free and cost-effective PPI detection platform, which offers fast and accurate measurements.

Field-effect biosensing (FEB) is a label-free technique for detecting biomolecular interactions. It measures the electric current through the graphene biosensor to which the binding targets are immobilized. The FEB technology was used to evaluate biomolecular interactions between Hsp90 and Cdc37 and a strong interaction between the two proteins was detected.

電界効果バイオセンシング技術を用いた分子シャペロンHsp90とそのクライアントプロテインキナーゼCdc37との生体分子相互作用の探索

Biomolecular interactions play versatile roles in numerous cellular processes&#160;by regulating and coordinating functionally relevant biological events. ...

Competition Binding Assay to Study Competing GTPase-Binding Protein Partners

記録