miRCURY LNA dPCR Custom Assays for miRNA

For extremely sensitive and specific miRNA quantification using QIAcuity EvaGreen-based dPCR

S_1289_9_LS_dPCR_miRCURY_LNA_miRNA_Custom_PCR_Assay
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miRCURY LNA miRNA Custom PCR Assay

Cat. No. / ID:   339317

Contains forward and reverse primers for 200 SYBR® Green-based, real-time qPCR reactions, 166 EvaGreen-based digital PCR reactions for Nanoplate 8.5k or 50 EvaGreen-based digital PCR reactions for Nanoplate 26k
€267.00
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miRCURY LNA dPCR Custom Assays for miRNA are intended for molecular biology applications. These products are not intended for the diagnosis, prevention, or treatment of a disease.
Configure at GeneGlobe
Find or custom design the right target-specific assays and panels to research your biological targets of interest.

Features

  • Design your own LNA-enhanced digital PCR primer sets for any miRNA
  • Unmatched sensitivity allows miRNA quantification from just 1 pg total RNA
  • High specificity discriminates closely related miRNAs and mature miRNA from precursors
  • Fast and simple two-step dPCR protocol takes less than 3 hours
  • Absolute quantification of miRNA expression changes with dPCR using the QIAcuity instrument and the QIAcuity EG PCR Kit

Product Details

miRCURY LNA miRNA Custom PCR Assays are custom-designed miRNA PCR primer sets that enable extremely sensitive and specific miRNA quantification. Both forward and reverse PCR amplification primers are miRNA-specific and are optimized with LNA technology. The assays are provided in tube format and contain sufficient primers for 166 reactions in a Nanoplate 8.5k (12 μl per reaction) or 50 reactions in a Nanoplate 26k (40 μl per reaction). The upstream cDNA synthesis step is performed with the miRCURY LNA RT Kit, while the digital PCR amplification takes place on the QIAcuity instrument with the QIAcuity EG PCR Kit.

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Performance

Optimized digital PCR analysis with the QIAcuity EG PCR Kits and the QIAcuity instrument

miRCURY LNA miRNA PCR Assays were developed to provide high-specificity target amplification. This can be quantified by two PCR methods: qPCR with standard real-time thermocyclers and digital PCR using the QIAcuity instrument and the QIAcuity EG PCR Kit. After cDNA synthesis using the miRCURY LNA RT Kit, digital PCR provides highly precise target quantification, detecting even the smallest expression changes at the lowest concentrations. A subset of key miRNAs have been experimentally validated on the QIAcuity instrument.

LNA enhances PCR performance

miRCURY LNA miRNA PCR Assays have been developed using stringent design criteria and lab-validated algorithms. The rigorous assay selection process ensures that each primer set delivers the highest specificity and efficiency for the most reliable and accurate results. Tm-normalization and LNA enhancement give the primers a higher binding affinity than standard DNA primers, dramatically increasing assay sensitivity and specificity.

Compared with other miRNA PCR systems that use either stem-loop or standard DNA primers, the LNA-enhanced primers offer significantly increased sensitivity, especially for AT-rich miRNAs

Principle

The design process

The miRCURY LNA miRNA Custom PCR Assay design tool lets you easily design highly sensitive and specific LNA-enhanced PCR primer sets for any miRNA not available as a predesigned product. The advanced algorithm evaluates approximately 3,000 primer pair designs based on more than 60 different criteria to find LNA optimal primer sets for your miRNA within a few minutes. The tool has been designed for miRNAs but can also be used for other small RNAs 14–27 nucleotides in length.
The design criteria include:

  • Optimization of melting temperatures by varying the LNA distribution of the primers to ensure high amplification efficiency and specificity.
  • Calculations and adjustments of self-hybridization and cross-hybridization scores for efficient PCR reactions.
  • Adjustments to avoid potential primer–dimer formation in the PCR reaction.
  • Intelligent positioning of LNA bases in the primers based on our vast knowledge of LNA oligonucleotide design.
  • miRBase searches to identify potential miRNAs with high sequence similarity. This ensures that the primer sets are highly specific for the small RNA for which they were designed.
A unique system for miRNA profiling

miRCURY LNA miRNA PCR Assays offer the best combination of performance and ease-of-use on the microRNA PCR market by combining universal RT with LNA PCR amplification (see figure  Schematic outline of the miRCURY LNA miRNA digital PCR system). Universal RT makes it possible to use one first-strand cDNA synthesis reaction as the template for multiple miRNA real-time PCR assays. This saves precious samples, reduces technical variation and saves time in the laboratory. Plus, both the forward and reverse PCR amplification primers are miRNA specific and optimized with LNA. This provides 1) exceptional sensitivity and extremely low background, enabling accurate quantitation of very low miRNA levels and 2) highly specific assays that allow discrimination between closely related miRNA sequences.

The principle of the dPCR reaction in the QIAcuity Nanoplates is described here.

Reference gene assays for normalization

Five validated reference gene primer sets are available for dPCR, enabling high-quality data normalization and generation of reliable data from many different sample types (see table below). These control primer sets target endogenous, small non-coding RNAs that are constitutively and relatively stably expressed across different human tissues (see figure  Expression levels of reference genes in different human tissues). The control reference genes offer the possibility to accurately and reliably normalize across a range of miRNA expression levels. For more information refer to the miRCURY PCR Controls page.

List of available reference gene assays

Product name Target organism Alternative names NCBI reference
Control primer set, SNORD38B (hsa)* hsa U38B; RNU38B NR_001457
Control primer set, SNORD44 (hsa) hsa U44; RNU44 NR_002750
Control primer set, SNORD48 (hsa) hsa U48; RNU48 NR_002745
Control primer set, SNORD49A (hsa)* hsa U49; U49A; RNU49 NR_002744
Control primer set, SNORA66 (hsa) hsa U66; RNU66 NR_002444
Control primer set, 5S rRNA (hsa) hsa, mmu V00589
Control primer set, U6 snRNA (hsa, mmu)* hsa, mmu, rno U6 X59362
Control primer set, RNU5G snRNA (mmu, hsa)* mmu, hsa, rno Rnu5a; U5a; Rnu5g NR_002852
Control primer set, RNU1A1 (mmu, hsa)* mmu, hsa, rno Rnu1a-1; Rnu1a1 NR_004411
Control primer set, SNORD65 (mmu) mmu U65; RNU65 NR_028541
Control primer set, SNORD68 (mmu) mmu U68; RNU68 NR_028128
Control primer set, SNORD110 (mmu) mmu U110; RNU110 NR_028547

* Validated for use in digital PCR.

See figures

Procedure

A simple and rapid plate-based workflow

Partitioning, thermocycling and imaging are all integrated into a single fully automated instrument, delivering results in under two hours. Nanoplate formats are amenable to front-end automation for sample preparation, further reducing hands-on time.
Just like in qPCR experiments, sample preparation includes the transfer of diluted samples and the addition of master mix and primers to a 96- or 24-well nanoplate. The system integrates partitioning, thermocycling and imaging into a single fully automated instrument that takes users from the sample to result in under 3 hours. One can perform remote analysis on the Suite Software, which provides the concentration in copies per microliter of your target sequences as well as in-built quality control options.

Applications

miRCURY LNA miRNA PCR Assays, in combination with the QIAcuity Digital PCR System, enable digital PCR analysis for mature miRNA quantification.

Supporting data and figures

Resources

Safety Data Sheets (1)
Scientific Posters (1)
Poster for download
Kit Handbooks (2)
For highly sensitive detection of miRNA using EvaGreen
For highly sensitive, real-time RT-PCR detection of miRNAs using SYBR Green
Certificates of Analysis (1)