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The assays can be used with gDNA extracted from FFPE tissues, fresh frozen tissues, and cell line samples.
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Mutant allele assays target key somatic mutations in oncogenes and tumor suppressor genes. All mutation targets are from the comprehensive Sanger COSMIC database (www.sanger.ac.uk/genetics/CGP/cosmic/). Target selection was based on frequency of occurrence and input from leading cancer researchers.
Each mutant allele assay (Figure 1) detects specific or multiple mutant alleles. Each assay contains:
Gene reference assays detect the genes that the target mutations reside in. They are designed to amplify a mutation-free and polymorphism-free region of the target gene. Each assay contains:
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For each real-time PCR reaction, the gDNA is combined with:
TaqMan® Genotyping Master Mix
The TaqMan® Genotyping Master Mix is optimized for somatic mutation detection using TaqMan® Mutation Detection Assays.
Optional Use of Internal Positive Control (IPC)
You can duplex IPC reagents with any TaqMan® Mutation Detection Assay to distinguish true target negatives from PCR failure or inhibition.
Reactions are run on an Applied Biosystems® real-time PCR system using a universal mutation detection thermal cycling protocol. After amplification, the Ct values are determined by the real-time PCR system analysis software.
TaqMan® Mutation Detection Assays are compatible with the following instruments: QuantStudio™ 3D, 3, 5, 6 Flex, 7 Flex, & 12K Flex, ViiA™ 7, 7900HT, 7500, 7500 Fast, and StepOnePlus® Real-Time PCR Systems.
Data files containing the sample Ct values can be exported from instrument software and imported into Mutation Detector™ Software for post-PCR data analysis of mutation detection experiments. In mutation analysis calculations, the difference between the Ct for each mutant allele assay and the Ct for the gene reference assay is calculated. This ΔCt value represents the quantity of the specific mutant allele detected within the sample.
The assays can be used with gDNA extracted from FFPE tissues, fresh frozen tissues, and cell line samples.
Recommended Products for DNA Isolation
DNA Isolation Kits
Mutant allele assays target key somatic mutations in oncogenes and tumor suppressor genes. All mutation targets are from the comprehensive Sanger COSMIC database (www.sanger.ac.uk/genetics/CGP/cosmic/). Target selection was based on frequency of occurrence and input from leading cancer researchers.
Each mutant allele assay (Figure 1) detects specific or multiple mutant alleles. Each assay contains:
Gene reference assays detect the genes that the target mutations reside in. They are designed to amplify a mutation-free and polymorphism-free region of the target gene. Each assay contains:
Order products using our Assay search tool
Order Custom plating services
For each real-time PCR reaction, the gDNA is combined with:
TaqMan® Genotyping Master Mix
The TaqMan® Genotyping Master Mix is optimized for somatic mutation detection using TaqMan® Mutation Detection Assays.
Optional Use of Internal Positive Control (IPC)
You can duplex IPC reagents with any TaqMan® Mutation Detection Assay to distinguish true target negatives from PCR failure or inhibition.
Reactions are run on an Applied Biosystems® real-time PCR system using a universal mutation detection thermal cycling protocol. After amplification, the Ct values are determined by the real-time PCR system analysis software.
TaqMan® Mutation Detection Assays are compatible with the following instruments: QuantStudio™ 3D, 3, 5, 6 Flex, 7 Flex, & 12K Flex, ViiA™ 7, 7900HT, 7500, 7500 Fast, and StepOnePlus® Real-Time PCR Systems.
Data files containing the sample Ct values can be exported from instrument software and imported into Mutation Detector™ Software for post-PCR data analysis of mutation detection experiments. In mutation analysis calculations, the difference between the Ct for each mutant allele assay and the Ct for the gene reference assay is calculated. This ΔCt value represents the quantity of the specific mutant allele detected within the sample.
All Applied Biosystems TaqMan Mutation Detection Assays have undergone extensive testing to ensure high sensitivity and specificity. The first set of released assays, covering 14 KRAS, 29 EGFR, and the BRAF V600E mutations, underwent additional testing, including determination of (a) the difference in inherent amplification efficiency between mutant allele assays and corresponding reference assays, to enable quantitative analysis of percent mutation in a sample, and (b) assay detection ΔCt cutoff values using spiked cell line gDNA samples.
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For research use only. Not for use in diagnostic procedures.