Our broad portfolio consists of multiplex panels that allow you to choose, within the panel, analytes that best meet your needs. On a separate tab you can choose the premixed cytokine format or a single plex kit.
Cell Signaling Kits & MAPmates™
Choose fixed kits that allow you to explore entire pathways or processes. Or design your own kits by choosing single plex MAPmates™, following the provided guidelines.
The following MAPmates™ should not be plexed together:
-MAPmates™ that require a different assay buffer
-Phospho-specific and total MAPmate™ pairs, e.g. total GSK3β and GSK3β (Ser 9)
-PanTyr and site-specific MAPmates™, e.g. Phospho-EGF Receptor and phospho-STAT1 (Tyr701)
-More than 1 phospho-MAPmate™ for a single target (Akt, STAT3)
-GAPDH and β-Tubulin cannot be plexed with kits or MAPmates™ containing panTyr
.
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Select A Species, Panel Type, Kit or Sample Type
To begin designing your MILLIPLEX® MAP kit select a species, a panel type or kit of interest.
Custom Premix Selecting "Custom Premix" option means that all of the beads you have chosen will be premixed in manufacturing before the kit is sent to you.
If you have chosen panel analytes and then choose a premix or single plex kit, you will lose that customization.
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Add Additional Reagents (Buffer and Detection Kit is required for use with MAPmates)
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48-602MAG
Buffer Detection Kit for Magnetic Beads
1 Kit
Space Saver Option Customers purchasing multiple kits may choose to save storage space by eliminating the kit packaging and receiving their multiplex assay components in plastic bags for more compact storage.
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Description
Overview
A rapid and sensitive method for detecting protein and nucleic acids fractionated by PAGE. Provides gels with clear backgrounds and sharp bands. Silver staining is about 100 times more sensitive than the standard Coomassie Blue protein staining and about 10 times more sensitive than ethidium bromide for DNA and RNA.
FASTsilver™ is one of the most rapid and sensitive methods for detecting proteins and nucleic acids fractionated by PAGE. Staining is about 100 times more sensitive than Coomassie Blue protein staining and about 10 times more sensitive than ethidium bromide for DNA and RNA. FASTsilver™ provides gels with exceptionally clear backgrounds and sharp protein or nucleic acid images. The protocol is simple and takes as little as 60 min to yield perfect results.
Storage and Shipping Information
Ship Code
Ambient Temperature Only
Toxicity
Standard Handling
Storage
+15°C to +30°C
Storage Conditions
Upon arrival store entire kit contents at room temperature (20°C).
Do not freeze
Ok to freeze
Packaging Information
Transport Information
Supplemental Information
Kit contains
Silver stain, developer, sensitizers I and II, and a user protocol. Note: one kit provides reagents sufficient for staining 25 mini gels.
FASTsilver™ Gel Staining Kit Certificates of Analysis
Title
Lot Number
341298
User Protocol
Revision
12-April-2011 RFH
Storage
Upon arrival store entire kit contents at room temperature (20°C).
Intended use
FASTsilver™ is one of the most rapid and sensitive methods for detecting proteins and nucleic acids fractionated by PAGE. Staining is about 100 times more sensitive than Coomassie Blue protein staining and about 10 times more sensitive than ethidium bromide for DNA and RNA. FASTsilver™ provides gels with exceptionally clear backgrounds and sharp protein or nucleic acid images. The protocol is simple and takes as little as 60 min to yield perfect results.
• Fixative I: Mix 30 ml 100% ethanol, 10 ml glacial acetic acid, and 60 ml ultra-pure water to obtain 100 ml Fixative I.
• Fixative II: Mix 10 ml 100% ethanol and 90 ml ultra-pure water to obtain 100 ml Fixative II.
• Sensitizer: Mix 5 ml silver stain, 65 µl sensitizer-I, and 45 ml ultra-pure water to obtain 50 ml Sensitizer.
• Developer: Mix 2.5 g developer, 32.5 µl sensitizer-I, 32.5 µl sensitizer-II, and 50 ml ultra-pure water to obtain 50 ml Developer.
• Stopper: Mix 11 ml glacial acetic acid and 39 ml ultra-pure water to obtain 50 ml Stopper.
Detailed protocol
1. After electrophoresis, fix the gel in 50 ml of the freshly prepared Fixative I. Use highly purified deionized water to make the solution. For isoelectric focusing gels, fix the gel first in 20% TCA for 60 min.
2. Fix the gel for 30 min to 3 h depending upon its thickness. For mini gels, (8 x 10 cm), 30 min is sufficient.
3. Wash twice, 10 min each, in 50 ml of the freshly prepared Fixative II.
4. Wash three times, 10 min each, in ultra-pure water. During washing Steps 2 and 3, use generous amounts of water (100 ml per 8 x 10 cm mini gels) and use gentle rocking or agitation.
5. Soak the gel in 50 ml of freshly prepared Sensitizer for 30 min, with gentle rocking of the gel, depending upon the thickness of the gel.
6. Rinse the gel only for 10-20 s with 50 ml of ultra-pure water.
7. Soak the gel in 50 ml of freshly prepared Developer. Gently rock the gel until bands are visible. Band intensity will develop quickly.
8. As soon as band intensity reaches an acceptable level, stop color development by adding 5 ml of the freshly prepared Stopper. Gently rock the gel for 10 min. Store the gel in ultra-pure water for subsequent analysis.
Sensitivity Notes
The lower detection limit of FASTsilver™ gel stain is 1 ng/band for proteins and nucleic acids.
Registered Trademarks
Calbiochem® is a registered trademark of EMD Chemicals, Inc. Interactive Pathways™ is a trademark of EMD Chemicals, Inc. FASTsilver™ is a trademark of Geno Technology, Inc.