protoarrayIRBP_short_protocol
ProtoArray? Human Protein Microarray v5.0 for Immune Response
BioMarker Profiling (IRBP)
IRBP Experienced Users Guide
Introduction
This quick reference contains brief instructions for using the ProtoArray? Human Protein Microarray v5.0 for the immune response biomarker profiling (IRBP) application. It is intended for experienced users of ProtoArray?Microarrays.
If you are a first time user, refer to the ProtoArray? Applications Guide available at https://www.wendangku.net/doc/da17850974.html,, for detailed instructions for performing the IRBP application, microarray specifications, ProtoArray? technology overview, troubleshooting, and license information.
Experimental Overview
1.Block the ProtoArray? Human Protein Microarray with Blocking Buffer.
2.Probe the array with diluted (1:500) human serum or plasma.
3.Perform detection using Alexa Fluor? 647 goat anti-human IgG.
4.Dry the array for scanning.
5.Scan the array with a fluorescent microarray scanner to obtain an array image.
6.Download the protein array lot specific information from ProtoArray? Central portal and acquire the image
data using microarray data acquisition software.
7.Analyze results using ProtoArray? Prospector data analysis software available from
https://www.wendangku.net/doc/da17850974.html,/protoarray.
Important Guidelines
To obtain the best results with the ProtoArray? Human Protein Microarray, follow these guidelines:
?The ProtoArray? Microarray can only be used once. Do not re-use or re-probe the array.
?Always wear clean gloves while handling microarrays. Take the appropriate precautions (wear a laboratory coat, disposable gloves, and eye protection) when handling serum or plasma, and dispose of used samples as biohazardous waste.
?Do not touch the surface of the array. Damage to the array surface can result in uneven or high background.
?Do not use LifterSlip? or any other coverslip for the IRBP application.
?Maintain the array and reagents at 2–8°C during the experiment.
?Avoid drying of the array during the experiment. Ensure the array is completely covered with the appropriate reagent during all steps of the protocol.
?Perform array experiments at a clean location to avoid dust or contamination. Filter solutions as needed (particles invisible to the eye can produce high background signals and cause irregular spot morphology).
?Dry the array by centrifugation prior to scanning. Do not dry the array using compressed air or commercial aerosol sprays. Scan the array immediately upon completion of the experiment.
?Avoid exposing the array to light after probing with a fluorescent detection reagent.
?Select the appropriate application from the Mode Selection Menu in ProtoArray? Prosepctor when performing analysis of microarray results. Use the Immune Response Profiling with Plasma application for plasma samples, and the Immune Response Profiling application for serum samples.
Continued on next page Part no. 25-1011MAN0000600Rev. Date: 18 May 2009
1 For technical support, email tech_support@https://www.wendangku.net/doc/da17850974.html,. For country-specific contact information, visit https://www.wendangku.net/doc/da17850974.html,.
Materials Needed
?Human serum or plasma sample (dilute the sample 1:500 in Washing Buffer, store on ice until use) ?ProtoArray? Human Protein Microarray v5.0 and buffers (see recipes below)
?Alexa Fluor? 647 Goat Anti-Human IgG (Invitrogen, Cat. no. A21445)
?10X Synthetic Block (Invitrogen, Cat. no. PA017)
?Clean, 4-chamber incubation tray with cover (Greiner, Cat. no. 96077307 or ISC Bioexpress, Cat. no. T-2896-1), chilled on ice
?Forceps and deionized water
?Shaker (capable of circular shaking at 50 rpm, place the shaker at 4oC)
?Microarray slide holder and centrifuge equipped with a plate holder (Optional)
?Fluorescence microarray scanner (refer to the ProtoArray? Applications Guide for recommended microarray scanners)
?Microarray data acquisition software (e.g. GenePix? Pro from Molecular Devices; refer to the ProtoArray?Applications Guide for details and optional software packages)
?Data analysis software (ProtoArray? Prospector recommended, available from
https://www.wendangku.net/doc/da17850974.html,/protoarray)
Sample Preparation
The IRBP application has been optimized for use with human serum and plasma samples (fresh or frozen).
Avoid repeated freeze-thaw cycles with samples. Prior to use, process the sample to remove any aggregates by centrifugation (12,000 × g for 30 seconds in a microcentrifuge), if needed.
We recommend using a 1:500 dilution of the serum or plasma sample in Washing Buffer to maximize signals while minimizing false positive and false negative results. Based on your initial results, you may need to optimize the serum dilution to obtain optimal performance.
Preparing Buffers
Prepare buffers fresh for best results. Mix buffers using the Blocking Buffer Kit (Invitrogen, Cat. no. PA055), or from scratch as described below. Mix stocks in a glass bottle. Cool buffers to 4°C before use.
Blocking Buffer*
(50 mM HEPES, pH 7.5, 200 mM NaCl, 0.08% Triton? X-100, 25% Glycerol, 20 mM Reduced glutathione, 1X Synthetic Block, 1 mM DTT)
5 ml buffer required per microarray.Washing Buffer
(1X PBS, 0.1% Tween 20, 1X Synthetic Block)
60 ml buffer required per microarray.
1.Prepare 50 ml Blocking Buffer fresh as follows:
1 M HEPES, pH 7.5 2.5 ml
5 M NaCl 2 ml
10% Triton? X-100 0.4 ml
50% Glycerol 25 ml
Reduced glutathione 305 mg
10X Synthetic Block 5 ml
Deionized water to 50 ml
2.Adjust pH to 7.5 with NaOH.
3.Mix reagents, chill to 4°C and add 50 μl of 1 M DTT prior to use.
https://www.wendangku.net/doc/da17850974.html,e buffer immediately. Store any remaining buffer at 4oC for <24 hours. 1.Prepare 600 ml Washing Buffer
fresh as follows:
10X PBS 60 ml
10% Tween 20 6 ml
10X Synthetic Block 60 ml
Deionized water to 600 ml
2.Mix reagents and cool to 4°C.
https://www.wendangku.net/doc/da17850974.html,e buffer immediately. Store any
remaining buffer at 4oC for <24
hours.
* Blocking Buffer without 10X Synthetic Block and DTT may be prepared the day before the assay. Store stock at 4°C for no more than 24 hrs.
Continued on next page 2
Blocking the Microarray
1.Remove the mailer containing the ProtoArray? Human Protein Microarray v5.0 from
storage and place immediately at 4°C. Equilibrate the mailer at 4°C for at least 15 minutes prior to blocking. Not doing so may result in condensation on the array which can reduce protein activity or alter spot morphology.
2.Place one microarray with the barcode facing up into each well of a chilled 4-chamber
incubation tray (see previous page) such that the barcoded end of the microarray is near the end of the tray marked with an indented numeral (see figure 1a). The indentation in the tray bottom is used as the site for buffer removal (see figure 1b, arrow).
https://www.wendangku.net/doc/da17850974.html,ing a sterile pipette, add 5 ml Blocking Buffer equilibrated to 4°C into each chamber
with an array. Avoid pipetting buffer directly onto the array surface.
4.Incubate the tray for 1 hour at 4°C on a shaker set at 50 rpm (circular shaking).
5.After incubation, aspirate Blocking Buffer using vacuum or a pipette. Position the tip of
the aspirator or pipette into the indentation at the end of the tray (see figure 1b, arrow) and aspirate the buffer from each well (see figure 2). Tilt the tray so that any remaining buffer accumulates at the base of the well at the numbered end of the tray and aspirate.
Important: Do not position the tip on, or aspirate from the microarray surface as this can cause scratches. Immediately proceed to adding the next solution to prevent any part of the array surface from drying.
6.Proceed immediately to the Probing the Microarray. 1a 1b 2
Probing the Microarray
1.Add 5 ml Washing Buffer at the numbered end of the 4-chamber incubation tray without touching the array
surface. Incubate the tray for 5 minutes at 4oC on a shaker set at 50 rpm (circular shaking).
2.Aspirate the buffer using vacuum or pipette as described on the previous page (Step 5).
3.Add 5 ml serum or plasma sample diluted (1:500) in Washing Buffer at the numbered end of the 4-chamber
incubation tray without touching the array surface. Allow the sample to flow across the array surface. Avoid pipetting sample directly onto the array surface.
4.Incubate the tray for 90 minutes at 4oC on a shaker set at 50 rpm (circular shaking).
5.Aspirate the sample using vacuum or pipette as described on the previous page (Step 5).
6.Wash each array with 5 ml Washing Buffer with gentle shaking on a shaker set at 50 rpm for 5 minutes at
room temperature. Aspirate the Washing Buffer as described on the previous page (Step 5).
7.Repeat wash step four more times using fresh Washing Buffer each time to obtain a total of 5 washes.
8.During the wash steps, mix 2.5 μl Alexa Fluor? 647 goat anti-human IgG antibody with 5 ml Washing Buffer
per array to obtain a final antibody concentration of 1 μg/ml. Store on ice until use. Optional: if using
exogenous anti-V5 antibody for serum-independent normalization, see detailed instructions in the
ProtoArray? Applications Guide.
9.Add 5 ml Alexa Fluor? 647 antibody solution from Step 8 to the incubation tray at the numbered end of the
tray without touching the array surface. Allow the solution to flow across the array surface. Avoid pipetting solution directly onto the array surface.
10.Incubate the tray for 90 minutes at 4oC on a shaker set at 50 rpm (circular shaking).
11.Aspirate the antibody solution as described on the previous page (Step 5).
12.Wash each array with 5 ml Washing Buffer with gentle shaking on a shaker set at 50 rpm for 5 minutes at
room temperature. Aspirate the Washing Buffer as described on the previous page (Step 5).
13.Repeat wash step four more times using fresh Washing Buffer each time to obtain a total of 5 washes.
14.Proceed immediately to Drying and Scanning the Microarray, next page.
Continued on next page
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Drying and Scanning the Microarray
1.To remove array from the 4-chamber incubation tray, insert the tip of the forceps into the
indentation at the numbered end of the tray and gently pry the array upward (see
3 figure 3). Using a gloved hand, pick up the array by holding the array by its edges
only.
2.Insert arrays into a slide holder and quickly rinse by submerging arrays into a large
beaker filled with deionized water three times. Ensure the array is properly placed
and is secure in the holder to prevent damage to the array during centrifugation.
3.Centrifuge the array in the slide holder or 50 ml conical tube at 200 × g for 1 minute
in a centrifuge (equipped with a plate rotor, if you are using the slide holder) at
room temperature. Ensure the array is completely dry.
4.After drying, store the arrays vertically or horizontally in a slide box protected from light and avoid
prolonged exposure to light. To obtain the best results, scan the array within 24 hours of probing.
5.To scan the array, start the appropriate array acquisition and analysis software on the computer connected to
the fluorescence microarray scanner.
6.Insert the array into the fluorescent microarray scanner such that the nitrocellulose-coated side faces the laser
source and barcode on the array is closest to the outside of the instrument.
7.Adjust scanner settings as follows:
?Wavelength: 635 nm ?Pixel Size: 10 μm
?PMT Gain: 600 ?Lines to Average: 1.0
?Laser Power: 100% ?Focus Position: 0 μm
8.Preview the microarray. Adjust PMT Gain, if needed. Scan the microarray in detail and include the barcode
for record.
9.Save the image to a suitable location as ‘multi-image TIFF’ file. Remove the microarray from the scanner.
10.Proceed to Data Acquisition and Analysis, below.
Data Acquisition and Analysis
1.Connect to the portal at https://www.wendangku.net/doc/da17850974.html,/protoarray and then click on the ProtoArray? Lot Specific
Information link that can be found under BioMarker Discovery Resources.
2.Enter the array barcode in the Input Barcode Number box and click on the Search button.
3.For each input barcode, various lot specific files are displayed.
4.Start the GenePix? Pro microarray data acquisition software on the computer. Open the saved image (.tiff)
from Step 9 (Drying and Scanning the Microarray) and open the .GAL files downloaded from ProtoArray?Central. The .GAL file defines the array grid required by the data acquisition software.
Important: Make sure you download the latest files for the specific barcode on your array. Lot specific
information files are updated frequently based on recently available sequence or protein information.
5.Adjust the subarray grid to ensure the grid is in proper location for each subarray. After the grid is properly
adjusted and all features are aligned, acquire the pixel intensity data for each feature by clicking the Analyze button in GenePix? Pro, and save/export the results as a .GPR (GenePix? Results) file.
https://www.wendangku.net/doc/da17850974.html,e the files from Step 5, above, for data analysis using ProtoArray? Prospector (available through the
Online Tools link under BioMarker Discovery Resources at https://www.wendangku.net/doc/da17850974.html,/protoarray).
7.Install ProtoArray? Prospector on your computer.
8.Start ProtoArray? Prospector from the desktop icon. Set the Application to Immune Response Profiling (for
serum samples), or Immune Response Profiling with Plasma (for plasma samples).
9.Select the Analyze button from the Tool Bar.
10.Select the .GPR files from the “Files of type” pull-down list and navigate to your data file(s). Select the file(s)
for analysis and click the Open button.
11.After analysis, ProtoArray? Prospector generates a list of human proteins showing significant interactions
with the sample. The proteins that score as positive, are proteins that satisfy the basic program options. We recommend validating the interactions as described in the ProtoArray? Applications Guide.
Continued on next page 4
Expected Results
Use controls printed on the ProtoArray? Human Protein Microarray v5.0 in verifying the probing, detection, and scanning protocols. Refer to the ProtoArray? Applications Guide for details.
An example of control spots obtained with the ProtoArray? Human Protein Microarray v5.0 probed with 1:500 diluted human serum and Alexa Fluor? 647 goat anti-human IgG antibody are shown below.
Alexa
Fluor? Ab
Human IgG
Alexa
Fluor? Ab
Anti-human IgG
Alexa
Fluor? Ab
Alexa
Fluor? Ab
V5 Control Protein
Additional Products
The table below lists additional products available separately from Invitrogen. For more information about these products, visit https://www.wendangku.net/doc/da17850974.html, or contact Technical Support.
Product Quantity Catalog
no. ProtoArray? Products
ProtoArray? Human Protein Microarray v5.0 1 array
20 arrays PAH052501 PAH0525020
ProtoArray? Control Protein Microarray v5.0 1 array PA10057
10X Synthetic Block 75 ml PA017
Blocking Buffer Kit 1 kit PA055
Array Control Protein 40 μl 451096
Alexa Fluor? 647 Goat Anti-Human IgG 500 μl A21445 Phosphate Buffered Saline (PBS), 1X 500 ml 10010-023
?2009 Life Technologies Corporation. All rights reserved.
For research use only. Not intended for any animal or human therapeutic or diagnostic use.
Trademarks referenced herein are registered trademarks or trademarks of Life Technologies Corporation. Any registration or trademark symbols used herein denote the registration status of trademarks in the United States. Trademarks may or may not be registered in other countries.
GenePix? is a registered trademark of Molecular Devices Corporation.
ScanArray? is a registered trademark of PerkinElmer, Inc.
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