ValidPrime® - Control for genomic DNA background in RNA preps
Description
ValidPrime® replaces the need to perform no reverse transcriptase
(RT(-)) controls to test for the presence of genomic DNA (gDNA) for all
samples in your reverse transcriptase quantitative PCR (RT-qPCR) profiling.
In an expression profiling experiment based on m samples and n
assays, traditional set up requires m RT(-) reactions plus m x n qPCR
controls.
When using ValidPrime® only m n 1 controls are needed.
ValidPrime® will minimize the amount of control reactions and hence your costs as well as your efforts.
Features
- Offers a cost-efficient alternative to RT(-) controls
- Accurately validates qPCR assays in terms of their sensitivity to gDNA
- Allows correction for gDNA-derived signals
- Reduces the need for DNase treatment
Use ValidPrime®
- as a control for gDNA background in qPCR
- for normalization of samples to cell copy number
- as an endogenous control for CNV applications
ValidPrime® is an assay to test for the presence of gDNA in test
samples and when combined with a gDNA control sample, replaces all RT(-)
controls. ValidPrime® is highly optimised and specific to a
non-transcribed locus of gDNA that is present in exactly one copy per
haploid normal genome. The sequence detected by the ValidPrime® assay
has no transcriptional activity and is not present in pure cDNA
preparations. Therefore, ValidPrime® measures the number of genomic
copies present in a sample.
In an expression profiling experiment the ValidPrime® assay is added
to the list of assays and the gDNA control is added to the list of
samples. From the combined measurements of the ValidPrime® assay and the
gene of interest (GOI) assays on all samples and on the gDNA control,
the genomic background contribution to all RT-qPCR measurements can be
assessed. ValidPrime® replaces the need to perform RT(-) controls for
all reactions and makes RT-qPCR profiling easier and substantially
cheaper.
The assay has very high PCR efficiency (E > 90% in tested
commercial master mixes) and produces negligible amount of primer dimer
products. Limit of detection (LOD) is estimated to 4 copies of DNA (0.01
ng of DNA) and limit of quantification (LOQ) is estimated to 32 copies
of DNA (0.08 ng of DNA).
For ValidPrime® Human, ValidPrime® Mouse, and ValidPrime® Rat, a gDNA
standard is provided which can be used to test the sensitivity of qPCR
assays for gDNA background. ValidPrime® Vertebrate does not include a
gDNA standard, since the standard needs to be specific for the species
analysed and arranged by the user.