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Platinum qPCR SuperMix for SNP Genotyping is a ready-to-use reaction mix for the amplification and identification of single-nucleotide polymorphisms (SNPs) in genomic DNA using PCR-based SNP genotyping technologies such as fluorescent primers or probes. The SuperMix has been specifically formulated for discrimination of alleles by real-time qPCR or end-point PCR followed by allelic-discrimination analysis on a real-time instrument or fluorescent microplate reader. It provides enhanced fluorescent signals for better discrimination of alleles and good separation with minimal scattering between replicate samples. The SuperMix format and integrated UDG carryover prevention make this reagent well suited for high-throughput applications.
This SuperMix has been developed using Applied Biosystems’ TaqMan®-based SNP genotyping products.
Platinum qPCR SuperMix for SNP Genotyping is supplied at 2X concentration and contains Platinum Taq DNA polymerase, Tris-HCl (pH 8.4), 6 mM MgCl2, 400 µM dGTP, 400 µM dATP, 400 µM dCTP, 800 µM dUTP, uracil DNA glycosylase (UDG), and PCR enhancer and proprietary stabilizers.
Platinum qPCR SuperMix for SNP Genotyping is supplied at 2X concentration to allow for the addition of template, primers, and probes. ROX Reference Dye is provided as a separate tube to normalize the fluorescent signal on instruments that are compatible with this option.
Reagents are provided for 250 or 1250 amplification reactions of 20 µl each.
Component | 250-rxn Kit | 1250-rxn Kit |
Platinum qPCR SuperMix for SNP Genotyping | 2 × 1.25 ml | 12.5 ml |
ROX Reference Dye | 500 µl | 500 µl |
Store components at –20ºC for long-term storage. After initial use, Platinum qPCR SuperMix for SNP Genotyping may be stored at 4ºC for up to one month to minimize freeze-thawing. For periodic use over several months, we recommend preparing aliquots of SuperMix to minimize freeze-thawing.
Store ROX Reference Dye in the dark.
The following protocol uses TaqMan® probes in a SNP genotyping assay on ABI real-time instruments or a standard thermal cycler. Note the separate cycling conditions for the ABI 7500 in Fast Mode, and the lower amount of ROX Reference Dye required for the ABI 7500 and 7500 Fast systems. This generic protocol may also be suitable with some modifications for other real-time instruments.
For additional information about specific instruments click here . Since PCR is a powerful technique capable of amplifying trace amounts of DNA, all appropriate precautions should be taken to avoid cross-contamination.
Standard Cycling Program | Fast Cycling Program (for the ABI 7500 in Fast Mode) |
---|---|
50°C for 2 minutes hold (UDG incubation) 95°C for 2 minutes hold 40 cycles of: 95°C, 15 seconds 65°C, 30 seconds (60 seconds for the | Select Fast Mode on the Thermal Profile tab 50°C for 2 minutes hold (UDG incubation) 95°C for 2 minutes hold 40 cycles of: 95°C, 3 seconds 65°C, 30 seconds |
Component | Single reaction |
---|---|
Platinum qPCR SuperMix for SNP Genotyping | 10 µl |
Forward primer, 10 µM | 0.4 µl |
Reverse primer, 10 µM | 0.4 µl |
Probe for SNP allele 1, 10 µM | 0.2 µl |
Probe for SNP allele 2, 10 µM | 0.2 µl |
Template (100 pg to 1 µg of genomic DNA) | 1 µl |
ROX Reference Dye, 25 µM (optional) | 0.4 µl/0.04 µl * |
DEPC-treated water | to 20 µl |
The target template for SNP genotyping is purified genomic DNA. For a 20-µl reaction, use 10 ng to 1 µg of purified genomic DNA in a 1µl volume. To purify genomic DNA, we recommend the PureLink or ChargeSwitch® genomic DNA purification kits from Invitrogen.
PlatinumqPCR SuperMix for SNP Genotyping includes magnesium chloride at a final concentration of 3 mM, which is optimal for SNP genotyping experiments.
ROX Reference Dye is included in each kit to normalize the fluorescent reporter signal for instruments that are compatible with this option. ROX is supplied at a 25 µM concentration, and is composed of a glycine conjugate of 5-carboxy-X-rhodamine, succinimidyl ester in 20 mM Tris-HCl (pH 8.4), 0.1 mM EDTA, and 0.01% Tween® 20. Use the following table to determine the amount of ROX to use with a particular real-time instrument per 20-µl reaction:
Instrument | ROX per 20-µl reaction* | Final Concentration |
---|---|---|
ABI 7000, 7300 7700, 7900HT, and 7900HT Fast | 0.4 µl | 500 nM |
ABI 7500; Stratagene Mx3000™, Mx3005P™, and Mx4000™ | 0.04 µl | 50 nM |
* To enable accurate pipetting, you can dilute the appropriate amount of ROX in DEPC-treated water immediately before use. For example, to add 0.4 µl per reaction, dilute 1:2.5 immediately before use and add 1 µl of the dilution to each reaction.
Platinum qPCR SuperMix for SNP Genotyping can be used with real-time qPCR instruments that can detect three colors (one for each SNP, plus one for ROX Reference Dye). Supported real-time instruments include the ABI PRISM® 7000, 7700, and 7900HT; the ABI 7300 and 7500 Real-Time PCR Systems; the Stratagene Mx3000P®, Mx3005P™, and Mx4000® the Corbett Research Rotor-Gene™ and the MJ Research DNA Engine Opticon® and Opticon® 2.
You can also perform end-point PCR on a standard thermal cycler and analyze the results using a fluorescent microplate reader capable of detecting in three channels.
Problem | Possible Cause | Solution |
No PCR product is evident in the qPCR graph or allelic-discrimination plot, or on a gel
|
The protocol was not followed correctly
|
Verify that all steps have been followed and the correct reagents, dilutions, volumes, and cycling parameters have been used.
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Template contains inhibitors, nucleases, or proteases, or has otherwise been degraded.
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Purify or re-purify your template.
| |
Primer and/or probe design is suboptimal
|
Verify your primer and probe selections. We recommend using validated pre-designed primers or designing primers or primer/probe combinations using dedicated software programs or primer databases.
| |
PCR product is evident in the gel, but not on the qPCR graph
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qPCR instrument settings are incorrect
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Confirm that you are using the correct instrument settings (dye selection, reference dye, filters, acquisition points, etc.) for your application.
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Problems with your specific qPCR instrument
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For instrument-specific information about probes, consult your instrument documentation and/or your probe technology documentation. For additional instrument-specific tips and troubleshooting, visit this
page.
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