miScript PCR Controls

Human, mouse, rat의 miRNA를 real-time PCR로 정량 후 정량값을 표준화 할 수 있습니다

Features

Human, mouse, rat에 효율적
Highly efficient amplification
Constant expression levels across a variety of cells and tissues
Easy to order via GeneGlobe

Product Details

For accurate and reproducible results in miRNA quantification by real-time PCR, it is necessary to normalize the amount of target miRNA by using a suitable endogenous reference RNA. This is known as relative quantification. miScript PCR Controls are primers that enable normalization of real-time PCR results in miRNA quantification studies using the miScript PCR System. miScript PCR Controls are available for a panel of 5 snoRNAs (SNORD61, SNORD68, SNORD72, SNORD95, and SNORD96A) and the snRNA RNU6B (RNU6-2). These controls are designed taking into consideration sequence homologies in human, mouse, rat, and dog so that the same control can be used for all 4 species. They can be ordered individually at the GeneGlobe Web portal.

Performance

miScript Primer Assays designed for a large panel of ncRNAs were evaluated to determine their amplification efficiencies and the variability of expression levels of the target ncRNAs in various cell and tissue types. Sequence conservation between human, mouse, rat, and dog ncRNAs was also studied to design miScript PCR Controls that can be used in all 4 species. miScript Primer Assays for 6 ncRNAs were selected as miScript PCR Controls. They fulfilled the following criteria:

Endogenous reference ncRNA targets which show a relatively constant expression level across a variety of cells and tissue (see figure "Constant expression levels of RNAs targeted by miScript PCR Controls")
Amplification efficiencies close to 100% under standard conditions
Equal performance in human, mouse, rat, and dog providing flexibility to use the same control for all 4 species

Principle

For accurate and reproducible results in real-time PCR analysis, it is necessary to normalize the amount of target miRNA by using a suitable endogenous reference RNA. This is known as relative quantification and is an important control which corrects for factors that could otherwise lead to inaccurate quantification. These factors include variation in quantity of input RNA, possible RNA degradation or presence of inhibitors in the RNA samples, and differences in sample handling. Normalization also allows results from different experiments and samples to be compared directly.

Features of a good control

An ideal endogenous reference RNA for normalization of data in real-time PCR quantification of miRNA should have the following features:

A constant expression level across all samples in the study

A similar small size as the miRNA under study

A similar expression level in the sample as the miRNA under study

Should not be regulated under the experimental conditions

Primers for the endogenous reference RNA and the miRNA should have similar amplification efficiencies (close to 100%)

miScript PCR Controls meet the above criteria, enabling the ΔΔCT method of relative quantification of miRNA levels in human, mouse, rat, and dog using the miScript PCR System.

miScript PCR Controls target noncoding RNAs

QIAGEN provides a range of miScript Primer Assays targeting ncRNAs such as snoRNAs and snRNAs. Scientists at QIAGEN have systematically evaluated a wide panel of these miScript Primer Assays for various ncRNAs and selected 6 miScript PCR Controls for 5 snoRNAs and an snRNA (see table "miScript PCR Controls"). These controls are also found on every miScript miRNA PCR Array (see figure "miScript miRNA PCR Array layout for 96-well plates").

Table. miScript PCR Controls
miScript PCR Control name	ncRNA official symbol	ncRNA alternative name	ncRNA type	Expressed in human, mouse, rat, and dog
Hs_SNORD61_1 miScript Primer Assay	SNORD61		snoRNA	Yes
Hs_SNORD68_1 miScript Primer Assay	SNORD68		snoRNA	Yes
Hs_SNORD72_1 miScript Primer Assay	SNORD72		snoRNA	Yes
Hs_SNORD95_1 miScript Primer Assay	SNORD95		snoRNA	Yes
Hs_SNORD96A_1 miScript Primer Assay	SNORD96A		snoRNA	Yes
Hs_RNU6-2_1 miScript Primer Assay	RNU6-2	RNU6B	snRNA	Yes

Important Note: The miScript II RT Kit contains 2 buffers: miScript HiFlex Buffer and miScript HiSpec Buffer. The following, previously available miScript PCR Controls cannot be used with cDNA prepared using miScript HiSpec Buffer:
Hs_RNU1A_1 miScript Primer Assay
Hs_RNU5A_1 miScript Primer Assay
Hs_SNORD25_1 miScript Primer Assay
Hs_SCARNA17_1 miScript Primer Assay
Hs_SNORA73A_1 miScript Primer Assay
If using these miScript PCR Controls, ensure that cDNA is prepared using miScript HiFlex Buffer.

For cDNA prepared using miScript HiSpec Buffer or miScript HiFlex Buffer, we recommend use of any of the updated miScript PCR Controls listed in the table above.

Procedure

How to choose miScript PCR Controls

Choosing an appropriate miScript PCR Control for an miRNA quantification experiment is similar to choosing an appropriate housekeeping gene for normalization when quantifying mRNA. For each sample type or treatment under study, it is necessary to verify that the miScript PCR Control target ncRNA is not regulated under the experimental conditions. In addition, a miScript PCR Control for an ncRNA that shows a constant level of expression and similar abundance to the target miRNA should be chosen. miScript PCR Controls can be ordered individually at the GeneGlobe Web portal. In addition, they are provided on all miScript miRNA PCR Arrays and miScript miRNA QC PCR Arrays.

ΔΔC_T method for relative quantification

The ΔΔC_T method is commonly used for relative quantification when working with the miScript PCR System. This comparative method relies on comparing the differences in C_T values obtained with normal versus experimental samples. Real-time PCR is performed using a primer (miScript Primer Assay) for the miRNA of interest side by side with reactions using a miScript PCR Control, which detects a snoRNA or snRNA. The threshold cycle (C_T) obtained with the miScript PCR Control is used to normalize the data as shown below.

Firstly, the threshold cycle (C_T) for each sample is determined. Next, the ΔC_T value is calculated. The ΔC_T value is the difference between the C_T value of the target miRNA and the CT value of the endogenous reference ncRNA:

ΔC_T = C_T (target miRNA) - C_T (endogenous reference ncRNA)

In the next steps, the ΔΔC_T value and the normalized target expression are calculated:

ΔΔC_T = ΔC_T (sample [e.g., disease cells]) - ΔCT (calibrator [e.g., normal cells])

Normalized target miRNA expression in sample = 2^-ΔΔCT
Finally, the normalized level of expression in the calibrator is set to be 100%:

% change in expression = (Normalized target miRNA expression in sample x 100)% - 100%

miScript miRNA PCR Array data analysis

The miScript miRNA PCR Array data analysis tool automically performs quantification using the the ∆∆C_T method of relative quantification as well as interpretation of the control assays. Results are presented in a tabular format, a scatter plot, a three-dimensional profile, and a volcano plot (when replicates are included). The complimentary analysis tool is individually tailored for each miScript miRNA PCR Array and can be used in a Web-based or Excel format.

Applications

miRNA quantification and profiling

Supporting data and figures

miScript miRNA PCR Array layout for 96-well plates.

Wells H3 to H8 each contain an assay for a different snoRNA/snRNA that can be used as a normalization control for the array data (SN1=SNORD61 assay, SN2=SNORD68 assay, SN3=SNORD72 assay, SN4=SNORD95 assay, SN5=SNORD96A assay, SN6=RNU6B/RNU6-2 assay). Wells H1 and H2 contain replicate C. elegans miR-39 miScript Primer Assays that can be used as an alternative normalizer for array data (Ce). Wells H9 and H10 contain replicate reverse transcription controls (miRTC). Wells H11 and H12 contain replicate positive PCR controls (PPC). These controls are also included in 384-well plate and Rotor-Disc 100 format miScript miRNA PCR Arrays.

Constant expression levels of RNAs targeted by miScript PCR Controls.

Resources

FAQ

After reconstitution of the lyophilized primers in 550ul nuclease-free water or TE, the miScript Primer Assay and miScript Precursor Assay 100 reaction tubes will be at 10X stock concentration. They should be used at 1X concentration (0.5 uM) in the PCR/RT-PCR reaction (eg. for a 25ul reaction, 1/10^th of the total volume, or 2.5ul, should be primer). For Fluidigm^® BioMark^TM System related applications, please refer to the miScript Microfluidics Handbook for primer concentrations and reconstitution recommendations.

Yes, miScript Primer Assays included in miScript miRNA PCR Arrays are the same primers as the miScript Primer Assays available in individual tubes.

FAQ ID - 3441

In general, precursor miRNA (pre-miRNA) levels are lower than those of mature miRNAs. However this is not always the case. Sometimes the levels of both mature and pre-miRNA may be similar, or pre-miRNA levels may be higher. For this reason, researchers often want to quantify pre-miRNA as well as mature miRNA. QIAGEN offers miScript precursor miRNA assays as well as mature assays for many miRNAs.

FAQ ID -2807

Yes, miScript Primer Assays are available for plant miRNAs at www.qiagen.com/GeneGlobe.

FAQ ID - 3439

Assuming the use of good, consistent experimental technique, real-time PCR methods such as the miScript Primer Assays provide very reproducible results. To insure the reliability of your results and to reliably detect smaller fold changes in miRNA expression from the PCR Assays, the performance of replicate determinations (such as biological triplicates) is highly recommended.

FAQ ID -2730

Any plant miScript Primer Assay included on a plant miScript miRNA PCR Array has been bench validated.

FAQ ID - 3440