eoe sub articles

EoE Sub Articles

1. Protein binding reaction and separation of bound RNA
<ol>
	<li>Carry out binding of protein and RNA in 10 mM Tris-HCl, pH 7.5 in a volume of 100 &#181;L by adding the following ingredients to these final concentrations: 50 mM KCl, 1 mM DTT, 0.09 &#181;g/&#181;L bovine serum albumin, 0.5 units/&#181;L RNasin, 0.15 &#181;g/&#181;L tRNA, 1 mM EDTA, and 30 &#181;L of appropriate recombinant protein (PTB) concentration. Add RNA from the appropriate pool. 
	NOTE: The splicing factor U2AF65 typically binds to the polypyrimidine-tract/3&#39; splice sites of model introns with a binding affinity (equilibrium dissociation constant or Kd) of approximately 1&#8211;10 nM. Therefore, the first two rounds of binding used protein concentration 10-fold above the Kd for U2AF65; for SXL and PTB proteins, the starting concentration in this range was only our best guess. This ensured that desired RNA species could bind, although lower affinity sequences were also potentially bound. In rounds 3 and 4 (transcription, binding, and amplification), the protein concentration was reduced three-fold. This was done to successfully eliminate low-affinity RNA species.</li>
	<li>Place the tubes containing the binding reactions for about 30 min at 25 &#176;C in a temperature block (or on ice).</li>
	<li>Fractionate the bound RNA from the unbound RNA for the first 4 rounds of selection-amplification using the following steps.
	<ol>
		<li>Filter the sample (100 &#181;L) at room temperature through a nitrocellulose filter attached to a vacuum manifold. 
		NOTE: The RNA-protein complex, but not the unbound RNA, remains on the filter.</li>
		<li>Chop the filter with retained RNA into fragments with a sterile razor blade; insert these into a centrifuge tube. Recover RNA by tumbling the tube gently for a minimum of 3 h (or overnight) with filter pieces immersed in the proteinase K (PK) buffer.</li>
		<li>Deproteinize the RNA sample by vortexing it in the presence of an equal volume of phenol-chloroform (1:1) and then of chloroform. Recover the aqueous phase each time by centrifuging the sample at high speed for 5 min at room temperature.</li>
		<li>Mix it with sodium acetate (0.1 volume of 3.0 M, pH 5.2) and ethanol (2&#8211;3 volumes of absolute ethanol, 200 proof). Leave the tube in a -80 &#176;C freezer for 30 min, centrifuge it at high speed for 10 min, and, following the washing and drying steps, solubilize the RNA in water treated with DEPC.</li>
	</ol>
	</li>
	<li>Separate the protein-bound RNA fractions from the unbound fractions for the last 2 rounds (rounds 5 and 6; transcription, binding, and amplification) as follows. Reduce the protein concentration in the binding reaction (step 1.1) by a further three-fold for additional selection pressure to enrich high-affinity binding sequences and preferentially remove low-affinity sequences.
	<ol>
		<li>Pre-cast a native polyacrylamide gel (5% with 60:1 acrylamide:bis-acrylamide ratio) in 0.5x TBE buffer (Tris-Borate-EDTA) prior to setting up the above RNA:protein-binding (step 1.1) reaction. Electrophorese this gel in a cold room (4 &#176;C) by applying 250 V for 15 min.</li>
		<li>Pipette the above RNA:protein binding reactions (step 1.1) into different wells of this gel. 
		NOTE: The protein is stored at -80 &#176;C and diluted prior to use in 20 mM 4-(2-Hydroxyethyl)piperazine-1-ethanesulfonic acid (HEPES), pH 8.0, 20% glycerol, 0.2 mM ethylenediaminetetraacetic acid (EDTA), 0.05% NP-40, and 1 mM dithiothreitol (DTT). The addition of 0.5&#8211;1.0 mM protease inhibitor phenylmethane sulfonyl fluoride (PMSF) is optional. In the binding reaction, this buffer contributes about 6% glycerol, which allows the direct loading of samples into the wells without the need for mixing them with a separate gel-loading buffer.</li>
		<li>Fractionate the bound RNA from the unbound RNA using gel electrophoresis in a cold room (4 &#176;C) at 250 V for 1 to 2 h. This process is also known as gel mobility shift assay. 
		NOTE: Duration of electrophoresis varies depending on features of the RNA and protein used for binding.</li>
		<li>Expose the gel to an X-ray film and identify the location of the bound RNA using autoradiography. Cut out the gel slice with the bound RNA and insert it into a tube.</li>
		<li>Incubate the crushed gel slice in the PK buffer used for elution for 3 h or overnight.</li>
		<li>Vortex the eluted RNA sample vigorously first with phenol-chloroform and then with chloroform.</li>
		<li>Mix sodium acetate and ethanol with the aqueous phase after chloroform extraction. Following incubation in a -80 &#176;C freezer, spin at 4 &#176;C for 5&#8211;10 min to collect the RNA pellet. Wash the RNA pellet with ethanol and air dry it by leaving the lid of the tube open. Dissolve the RNA in water treated with DEPC. 
		NOTE: Switching to the gel mobility shift assay for fractionation allows the elimination of unwanted RNA species that might have been enriched for binding, for example, to the nitrocellulose filter here (or any matrix) used in the initial rounds for fractionation.</li>
	</ol>
	</li>
</ol>
2. Reverse transcription and PCR amplification
<ol>
	<li>Synthesize cDNA from the dissolved RNA using reverse transcriptase and the reverse primer by incubating the 20 &#181;L reaction (2 &#181;L of 10x RT Buffer, 2 &#181;L of AMV reverse transcriptase, 1 &#181;M reverse primer, 10 &#181;L of RNA, RNase inhibitor optional) at 42 &#176;C for 60 min.</li>
	<li>Amplify the cDNA using 20&#8211;25 PCR cycles. Attach the T7 RNA polymerase promoter to the library by polymerase chain reaction (PCR) containing 1 &#181;M DNA random library template, 1 &#181;M of each primer, 20 mM Tris (pH 8.0), 1.5 mM MgCl2, 50 mM KCl, 0.1 &#181;g/&#181;L acetylated bovine serum albumin, 2 units of Taq polymerase, and 200 &#181;M each of dNTPs (deoxyguanosine, deoxyadenosine, deoxycytidine, and deoxythymidine triphosphate).</li>
</ol>
3. Transcription and protein binding
<ol>
	<li>Repeat the process of RNA synthesis, protein binding, and separation of protein-bound, and unbound fractions.</li>
</ol>

<table><tbody><tr><td>Gel Electrophoresis equipment</td><td>Standard</td><td>Standard</td><td></td></tr><tr><td>Nitrocellulose</td><td>Millipore</td><td>HAWP</td><td></td></tr><tr><td>Nitrocellulose</td><td>Schleicher &amp;amp; Schuell</td><td>PROTRAN</td><td></td></tr><tr><td>Polyacrylamide gel solutions</td><td>Standard</td><td>Standard</td><td></td></tr><tr><td>Proteinase K</td><td>NEB</td><td>P8107S</td><td></td></tr><tr><td>Recombinant PTB</td><td>Laboratory Preparation</td><td>Not applicable</td><td></td></tr><tr><td>Reverse Transcriptase</td><td>NEB</td><td>M0277S</td><td></td></tr><tr><td>Vacuum manifold</td><td>Fisher Scientific</td><td>XX1002500</td><td>Millipore 25mm Glass Microanalysis Vacuum Filter</td></tr><tr><td>Vacuum manifold</td><td>Millipore</td><td>XX2702552</td><td>1225 Sampling Vacuum Manifold</td></tr><tr><td>X-ray films</td><td>Standard</td><td>Standard</td><td></td></tr><tr><td>Glass Plates</td><td>Standard</td><td>Standard</td><td></td></tr></tbody></table>

selex-based in vitro binding assay to identify rna-protein interactions

Source: Singh, R. <a href="https://app.jove.com/v/59635">Exploring Sequence Space to Identify Binding Sites for Regulatory RNA-Binding Proteins.</a> J. Vis. Exp. ( (2019).
In this video, we describe the systematic evolution of ligands by the exponential enrichment (SELEX) method to identify specific RNA-binding sequences for a target protein of interest. The protein is incubated with a large pool of randomized RNA sequences, and the protein-binding RNA sequences are isolated, PCR-amplified, and sequenced to identify their protein-binding sites.

SELEX-Based In Vitro Binding Assay to Identify RNA-Protein Interactions

Source: Singh, R. Exploring Sequence Space to Identify Binding Sites for Regulatory RNA-Binding Proteins. J. Vis. Exp. ( (2019).
In this video, we ...

Systematic evolution of ligands by exponential enrichment, SELEX, allows the identification of protein-binding RNA sequences.
First, obtain a randomized RNA pool containing radiolabeled RNAs with randomized sequences that fold into highly-specific structures. Incubate with the target protein. The protein binds to RNA molecules with specific sequences and three-dimensional structures, while non-specific RNAs remain unbound.
Pass the mixture through a nitrocellulose filter. Unbound RNA passes through filter pores, while RNA-protein complexes remain retained.
Chop the RNA-protein complex-containing filter into fragments. Repeat RNA-protein interaction by incubating the RNA pool with reduced target protein concentration &#8212; allowing only high-affinity sequence binding, while low-affinity sequences fail to bind.
Load this mixture on a polyacrylamide gel and perform electrophoresis. The RNA-protein complexes migrate slowly through the gel compared to low-affinity, unbound RNAs. X-ray gel imaging shows a band shift corresponding to the RNA-protein complex location.
Slice the complex-containing gel portion. Add Proteinase K to the filter fragments and gel slices, digesting the proteins and releasing RNA from the complex. Add phenol-chloroform and centrifuge, separating the RNA from the digested proteins.
Mix the RNA-containing supernatant with sodium acetate and ethanol. Centrifuge to precipitate the RNA. Resuspend in RNase-free water. Reverse-transcribe the RNA to complementary DNA and PCR-amplify the DNA.
Repeat several rounds of filter-based and gel-based separation to obtain a pool of target protein-specific DNA sequences.

selex-based-vitro-binding-assay-to-identify-rna-protein

Research

JoVE Encyclopedia of Experiments

Biological Techniques

Biomolecular Interaction Detection Techniques

Protein-nucleic acid interactions

200 Views. Source: Singh, R. Exploring Sequence Space to Identify Binding Sites for Regulatory RNA-Binding Proteins. J. Vis. Exp. ( (2019). In this video, we describe the systematic evolution of ligands by the exponential enrichment (SELEX) method to identify specific RNA-binding sequences for a target protein of interest. The protein is incubated with a large pool of randomized RNA sequences, and the protein-binding RNA sequences are isolated, PCR-amplified, and sequenced to identify their protein-bindin...

Video: SELEX-Based In Vitro Binding Assay to Identify RNA-Protein Interactions - Concept

Desthiobiotin-Streptavidin-Affinity Mediated Purification of RNA-Interacting Proteins in Mesothelioma Cells

The in vitro RNA-pulldown is still largely used in the first steps of protocols aimed at identifying RNA-binding proteins that recognize specific RNA structures and motifs. In this RNA-pulldown protocol, commercially synthesized RNA probes are labeled with a modified form of biotin, desthiobiotin, at the 3' terminus of the RNA strand, which reversibly binds to streptavidin and thus allows elution of proteins under more physiological conditions. The RNA-desthiobiotin is immobilized through interaction with streptavidin on magnetic beads, which are used to pull down proteins that specifically interact with the RNA of interest. Non-denatured and active proteins from the cytosolic fraction of mesothelioma cells are used as the source of proteins. The method described here can be applied to detect the interaction between known RNA binding proteins and a 25-nucleotide (nt) long RNA probe containing a sequence of interest. This is useful to complete the functional characterization of stabilizing or destabilizing elements present in RNA molecules achieved using a reporter vector assay.

Desthiobiotin labeling of a synthetic 25-nucleotide RNA oligo, which contains an adenine-rich element (ARE) motif, allows specific binding of cytosolic ARE-binding protein.

The in vitro RNA-pulldown is still largely used in the first steps of protocols aimed at identifying RNA-binding proteins that recognize specific RNA ...

JoVE Journal

Cancer Research

A Novel Saturation Mutagenesis Approach: Single Step Characterization of Regulatory Protein Binding Sites in RNA Using Phosphorothioates

Gene regulation plays an important role in development. Numerous DNA- and RNA-binding proteins bind their target sequences with high specificity to control gene expression. These regulatory proteins control gene expression either at the level of DNA (transcription) or at the level of RNA (pre-mRNA splicing, polyadenylation, mRNA transport, decay, and translation). Identification of regulatory sequences helps understand not only how a gene is switched on or off, but also which downstream genes are regulated by a particular regulatory protein. Here, we describe a one-step approach that allows saturation mutagenesis of a protein binding site in RNA. It involves doping DNA template with non-wild-type nucleotides within the binding site, synthesis of separate RNAs with each phosphorothioate nucleotide, and isolation of the bound fraction following incubation with protein. Interference from non-wild-type nucleotides results in their preferential exclusion from the protein-bound fraction. This is monitored by gel electrophoresis following selective chemical cleavage with iodine of phosphodiester bonds containing phosphorothioates (phosphorothioate mutagenesis or PTM). This single-step saturation mutagenesis approach is applicable to the characterization of any protein binding site in RNA.

Proteins that bind specific RNA sequences play critical roles in gene expression. Detailed characterization of these binding sites is crucial for our understanding of gene regulation. Here, a single-step approach for saturation mutagenesis of protein-binding sites in RNA is described. This approach is relevant for all protein-binding sites in RNA.

Gene regulation plays an important role in development. Numerous DNA- and RNA-binding proteins bind their target sequences with high specificity to ...

Genetics

A Flow Cytometry-Based Cell Surface Protein Binding Assay for Assessing Selectivity and Specificity of an Anticancer Aptamer

A key challenge in developing an anticancer aptamer is to efficiently determine the selectivity and specificity of the developed aptamer to the target protein. Due to its several advantages over monoclonal antibodies, aptamer development has gained enormous popularity among cancer researchers. Systematic evolution of ligands by exponential enrichment (SELEX) is the most common method of developing aptamers specific for proteins of interest. Following SELEX, a quick and efficient binding assay accelerates the process of identification, confirming the selectivity and specificity of the aptamer. 
This paper explains a step-by-step flow cytometric-based binding assay of an aptamer specific for epithelial cellular adhesion molecule (EpCAM). The transmembrane glycoprotein EpCAM is overexpressed in most carcinomas and plays roles in cancer initiation, progression, and metastasis. Therefore, it is a valuable candidate for targeted drug delivery to tumors. To evaluate the selectivity and specificity of the aptamer to the membrane-bound EpCAM, EpCAM-positive and -negative cells are required. Additionally, a non-binding EpCAM aptamer with a similar length and 2-dimensional (2D) structure to the EpCAM-binding aptamer is required. The binding assay includes different buffers (blocking buffer, wash buffer, incubation buffer, and FACS buffer) and incubation steps. 
The aptamer is incubated with the cell lines. Following the incubation and washing steps, the cells will be evaluated using a sensitive flow cytometry assay. Analysis of the results shows the binding of the EpCAM-specific aptamer to EpCAM-positive cells and not the EpCAM-negative cells. In EpCAM-positive cells, this is depicted as a band shift in the binding of the EpCAM aptamer to the right compared to the non-binding aptamer control. In EpCAM-negative cells, the corresponding bands of EpCAM-binding and -non-binding aptamers overlap. This demonstrates the selectivity and specificity of the EpCAM aptamer. While this protocol is focused on the EpCAM aptamer, the protocol is applicable to other published aptamers.

A necessary step in anticancer aptamer development is to test its binding to the target. We demonstrate a flow cytometric-based assay to study this binding, emphasizing the importance of including a negative control aptamer and cancer cells that are positive or negative for that particular protein.&#160;

A key challenge in developing an anticancer aptamer is to efficiently determine the selectivity and specificity of the developed aptamer to the target ...