reverse phase protein arrays based protein expression analysis: a procedure for simultaneous quantification of expression of multiple proteins from cell lysate

Reverse Phase Protein Arrays Based Protein Expression Analysis: A Procedure for Simultaneous Quantification of Expression of Multiple Proteins from Cell Lysate

Prior to RPPA printing, a series of five twofold dilutions are made from each sample. One of the most time-consuming aspects of this procedure is making hundreds of dilutions. Successful outcome can be assured by double-checking prior to printing slides.
A MicroGrid II robotics spotter is then used to spot protein lysates onto nitrocellulose-coated glass slides. Each sample is spotted in triplicate, resulting in a total of 15 spots per sample. The slides used in this experiment contain two pads onto which the samples are spotted. Each pad was spotted with identical samples, in this case, 100 samples. Other available formats include 1, 8, and 16 pad slides. The higher the number of pads, the smaller the number of samples that can be spotted onto each.
To begin the procedure for protein detection, wet slides in excess blocking buffer and incubate at room temperature for 1 hour on a rocking platform. Prepare 800 microliters of primary antibodies in blocking buffer at the desired concentrations and keep on ice. After the one-hour incubation in blocking buffer, mount slides in either the single frame Chip Clip or the FastFrame four-bay slide holder so that a tight seal is formed between the slide and the incubation chamber.
Remove residual buffer from wells and add 600 microliters of primary antibody to the respective wells. Place the slides and chamber into a sealed wet box and incubate on a rocking platform overnight at 4 degrees Celsius. On the following morning, remove slides from the cold room. Carefully remove the primary antibodies from each well. Add 600 microliters of 0.1% PBS-Tween20 or PBS-T and wash slides on a rocking platform at room temperature for 5 minutes.
Replace the PBS-T with fresh PBS-T. In this way, wash slides a total of three times. Remove buffer from wells and add 600 microliters of fluorescently-labeled secondary antibodies at the appropriate dilution to the respective wells. Incubate with secondary antibodies at room temperature for 45 minutes with gentle shaking. It is important to protect the membrane from light until the time it is scanned. After 45 minutes, remove secondary antibodies from wells and briefly washed three times in 600 microliters PBS-T at room temperature.
Remove slides from the carrier, transfer to a suitable container, and wash in excess PBS-T for 15 minutes, keeping the membrane in the dark. Remove PBS-T and wash the membrane with PBS at room temperature for 15 minutes to remove residual Tween20, again keeping the membrane in the dark. Dry the Fastslides in a 50 degrees Celsius oven for 10 minutes. Finally, scan the slides at 680 nanometers and/or 800 nanometers, depending on the secondary antibodies used.

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1. RPPA Printing
<ol>
	<li>Protein lysates were spotted onto nitrocellulose-coated glass slides (Fastslides-Whatman) using a MicroGrid II robotic spotter. The slides used contained 2 pads onto which the samples were spotted. Each pad was spotted with identical samples, in this case, 100 samples. Other available formats include 1, 8, and 16 pad slides. The higher the number of pads the smaller the number of samples which can be spotted onto each.</li>
	<li>A series of five 2-fold dilutions were made from each sample and each was then spotted in triplicate (resulting in a total of 15 spots per sample).</li>
</ol>
2. RPPA Protein Detection
<ol>
	<li>Wet slides in excess LiCor Blocking Buffer (diluted 50:50 in PBS). Incubate at RT for 1 hr on a rocking platform.</li>
	<li>Prepare 800 &#956;L of primary antibodies in LiCor Blocking Buffer (diluted 50:50 in PBS) at the desired concentrations and keep on ice.</li>
	<li>Mount the slides in either (i) the single frame Chip Clip or (ii) the &#39;FastFrame&#39;&#160;four-bay slide holder so that a tight seal is formed between the slide and the incubation chamber.</li>
	<li>Remove residual buffer from wells and add 600 &#956;L primary antibody to respective wells.</li>
	<li>Place the slide and chamber into a sealed wet box and incubate on rocking platform overnight at 4 &#176;C.</li>
	<li>Make up 0.1% PBS-Tween20 (PBS-T; 100 &#956;L Tween 20/100 mL PBS).</li>
	<li>Remove slides from the cold room and carefully remove the primary antibodies from each well.</li>
	<li>Add 600 &#956;L of PBS-T and wash slides on rocking platform at RT for 5 min (X3).</li>
	<li>Prepare fluorescently labeled secondary antibodies by diluting in Odyssey Blocking Buffer (diluted 50:50 in PBS) 0.01% SDS at 1:2,000 dilution (1 &#956;L/2 mL) in the first instance.</li>
	<li>Remove buffer from wells and add 600 &#956;L fluorescently labeled secondary antibodies to respective wells. Incubate secondary antibodies at room temperature for 45 min with gentle shaking; it is important to protect the membrane from the light until such time as it has been finally scanned.</li>
	<li>Remove secondary antibodies from the well and briefly wash (x3) in 600 &#956;L PBS-T at room temperature. Remove slide from carrier, transfer to a suitable container and wash in excess PBS-T for 15 min, keeping the membrane in the dark.</li>
	<li>Remove PBS-T and further wash membrane with PBS at room temperature for 15 min to remove residual Tween-20, again keeping the membrane in the dark.</li>
	<li>Dry the Fastslide in 50 &#176;C oven for 10 min and then scan on the Li-Cor Odyssey scanner. Keep the slide in the dark until it has been scanned.</li>
	<li>Scan the slide at 680 nm and/or 800 nm depending on the secondary antibody/antibodies used. For two-color detection always use highly cross-adsorbed secondary antibodies to minimize cross-reactivity. Careful selection of primary and secondary antibodies is necessary for two-color detection. Of primary importance is the selection of different host species (e.g.&#160;rabbit and mouse) for the two primary antibodies. This allows discrimination by anti-rabbit and anti-mouse secondary antibodies which are labeled with dye with easily distinguishable emission spectra.</li>
	<li>Image files are saved as .tiff files.&#160;Figure 1 depicts the image of scanned files.</li>
</ol>

<table><tbody><tr><td>Triton X-100</td><td>Triton-X</td><td>T8787</td><td></td></tr><tr><td>Li-Cor Odyssey Blocking Buffer</td><td>Li-Cor</td><td>927-40000</td><td></td></tr><tr><td>MicroGrid II robotic spotter</td><td>Biorobotics</td><td></td><td></td></tr><tr><td>FastFrame&#039; four bay slide holder</td><td>Whatman</td><td>10486001</td><td></td></tr><tr><td>FAST Slide - 2-Pad</td><td>Whatman</td><td>10485317</td><td></td></tr><tr><td>IRDye 680LT Goat anti-Mouse IgG</td><td>Licor</td><td>926-68020</td><td></td></tr><tr><td>IRDye 800CW Goat anti-Rabbit IgG</td><td>Licor</td><td>926-32211</td><td></td></tr></tbody></table>

Source: O&#39;Mahony, F. C. et al. <a href="https://www.jove.com/video/50221" target="_blank">The Use of Reverse Phase Protein Arrays (RPPA) to Explore Protein Expression Variation within Individual Renal Cell Cancers.</a> J. Vis. Exp. (2013)
This video demonstrates the methodology for performing Reverse Phase Protein Arrays (RPPA) to study protein expression patterns from cell lysate.&#160;In RPPA, the lysate containing a mixture of proteins is printed on nitrocellulose slides and proteins of interest are analyzed using fluorescently labeled antibodies.

<img alt="Figure 1" src="/files/ftp_upload/20571/20571_Figure1.jpg" /> 
Figure 1.&#160;Flow diagram of RPPA scanning process.&#160;

Source: O&#39;Mahony, F. C. et al. The Use of Reverse Phase Protein Arrays (RPPA) to Explore Protein Expression Variation within Individual Renal Cell ...

A tumor sample contains a heterogeneous population of proteins. Using tumor lysate, multiple such proteins can be analyzed parallelly to identify the protein of interest. This high-throughput technique is called Reverse Phase Protein Arrays or RPPA.
To perform RPPA, begin by taking an immunoassay glass slide coated with nitrocellulose. Spot an array of tumor lysate proteins on the slide. Incubate to allow protein capture on nitrocellulose. Subsequently, treat the slide with a blocking buffer that blocks non-specific antibody binding sites on proteins.
Remove the excess blocking solution. Now, mount the protein-coated slide in a holder and seal it tightly. This creates temporary wells over the slide surface. Next, load the wells with a primary antibody solution. These antibodies recognize epitopes present on the corresponding target from a mixture of proteins on the array.
Finally, add fluorescently-labeled secondary antibodies. These antibodies attach to the pre-bound primary antibodies forming a complex. Wash the slide to remove any unbound secondary antibodies. Unfasten the slide from the holder and allow it to air dry.
Scan the slide using a fluorescent scanner. The antibody-tagged target proteins fluoresce at a specific wavelength and appear as colored spots on the slide surface.

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Reverse Phase Protein Arrays Based Protein Expression Analysis: A Procedure for Simultaneous Quantification of Expression of Multiple Proteins from Cell Lysate

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Reverse Phase Protein Arrays Based Protein Expression Analysis: A Procedure for Simultaneous Quantification of Expression of Multiple Proteins from Cell Lysate