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QuantiFast Probe RT-PCR Plus Kit

使用序列特异性探针进行一步法快速RT-PCR,并去除基因组DNA

Features

  • 含独有的基因组DNA去除缓冲液,确保准确的基因表达分析
  • 十分适合分析FFPE样本中降解的短RNA
  • 同步检测两个目标RNA,灵敏度高
  • 含有即用型一步法real-time RT-PCR预混液
  • 适用于多种PCR仪的快速通用型实验方案

Product Details

QuantiFast Probe RT-PCR Plus Kit非常适合用于对多种来源的RNA,包括短的RNA片段进行基因表达分析(如福尔马林固定、石蜡包埋样本中的RNA)。使用探针检测,该试剂盒能对单管中的1到2个RNA靶标进行快速、一步法real-time RT-PCR定量检测(例如,使用与QuantiFast Probe Assays相同类型的水解作用[TaqMan]探针)。在real-time RT-PCR开始前的孵育步骤可有效去除基因组DNA污染,避免出现假阳性信号。该试剂盒还含有两管不同浓度的ROX染料,使其适用于各种real-time PCR分析仪。为便于使用,预混液可保存在2–8°C。

Performance

QuantiFast Probe RT-PCR Plus Kit能进行快速、灵敏的定量,甚至包括含有高度降解RNA的样本(参见" Highly efficient real-time RT-PCR detection of degraded RNA"),其基因组DNA残留量较高(参见" Efficient genomic DNA removal for accurate gene expression analysis")。
See figures

Principle

QuantiFast Probe RT-PCR Plus Kit含有特异性探针(如QuantiFast Probe Assays中的水解作用[TaqMan]探针),可对目标RNA进行快速、灵敏的扩增。在real-time RT-PCR开始前的孵育步骤可有效去除基因组DNA污染,确保RNA测量数据的准确性。基因组DNA的存在会导致CT值比真阳性值低,而出现假阳性信号。

参照和目标基因同时扩增,而不是在不同反应中分别扩增,这减少了人工操作误差,增加了基因扩增的可靠性。QuantiFast Probe RT-PCR Plus Kit在标准及快速循环仪上宽动态范围内均可获得快速、高灵敏度结果(参见" QIAGEN multiplex kits")。专门研发的快速PCR缓冲液包含创新的添加剂Q-Bond,显著减少了变形、退火、延伸时间(参见" Fast primer annealing")。通过使用专门的RT-PCR缓冲液,可确保一步法RT-PCR的高特异性和灵敏度,且省去了进行优化的时间。该缓冲液包含了K+和NH4+平衡组合,可加快特定引物的退火过程,且独特的Factor MP成分可稳定已结合的引物(参见" Unique PCR buffer")。此外,HotStarTaq Plus DNA Polymerase在一定温度下才会活化,防止了非特异性产物的生成。该试剂盒含有优化的RT预混液,可在20分钟内完成cDNA合成。该试剂盒含有两管不同浓度的ROX校准染料。ROX的浓度为优化浓度,因此可通过自动数据分析,实现对低拷贝RNA的检测。

QuantiFast Probe RT-PCR Plus Kit的组份
组份 特点 优势
QuantiFast RT-Mix 特殊的逆转录酶混合物对RNA有高亲和力,即使有复杂的次级结构 RNA可以在20分钟内转录,即使有复杂的次级结构
2x QuantiFast Mix 1
gDNA Wipeout Buffer 有效去除基因组DNA 只在qRT-PCR反应中检测RNA
2x QuantiFast Mix 2*
HotStarTaq Plus DNA Polymerase 95ºC孵育5分钟即可快速活化 在室温下启动qPCR反应
QuantiFast Probe RT-PCR Plus Reagents NH4+和K+的平衡组合 特异性引物退火确保可靠的PCR结果
合成的Factor MP 在同一管中对4个基因进行可靠的多通路分析
独特的Q-Bond添加剂 快速的PCR运行时间,获得较快的结果,每天进行较多的反应
* 还包含dNTP混合液(dATP、dCTP、dGTP和dTTP)。
See figures

Procedure

QuantiFast Probe RT-PCR Plus Kit含有即用型预混液,可减少优化试剂和反应条件的时间。按照操作手册中的实验方案进行操作,即可快速获得可靠结果(参见" QuantiFast Probe RT-PCR Plus Kit procedure")。

QuantiFast Probe Assays是初步设计的使用水解作用探针检测的全基因分析。QuantiFast Probe Assays与QuantiFast Probe RT-PCR Plus Kit联合应用于单重或多重一步法qRT-PCR,以获得可靠结果。

See figures

Applications

QuantiFast Probe RT-PCR Plus Kit非常适合用于对多种来源的样本包括FFPE组织样本和降解的RNA样本进行基因表达分析。该试剂盒可用于快速实时定量PCR分析仪和标准实时定量PCR分析仪,包括QIAGEN、Applied Biosystems、Bio-Rad、Cepheid、Eppendorf、Roche和Agilent的仪器。

Supporting data and figures

Resources

安全数据表 (1)
Download Safety Data Sheets for QIAGEN product components.
Safety Data Sheets (1)

FAQ

How many freeze-thaw cycles can the master mix contained in the QuantiFast Probe RT-PCR Plus Kit tolerate?
The master mixes of the QuantiFast Probe RT-PCR Plus Kit can undergo up to 10 freeze-thaw cycles without any reduction in performance. For optimal long-term storage, aliquot the master mix, and store it at -20°C in sterile, polypropylene tubes.
FAQ ID -2357
What are important points regarding the genomic DNA wipeout buffer in the QuantiFast Probe RT-PCR Plus Kit?
  • The gDNA removal should be performed at room temperature from 15-30°C.
  • Perform the gDNA removal step for 5 minutes. However, the incubation can be prolonged to 15 minutes. An incubation longer than 15 minutes is not recommended.
  • The gDNA elimination reaction is efficiently stopped by adding the QuantiFast Mix 2.

 

 

 

FAQ ID -2359
I would like to order the QuantiFast Probe Assays without master mix. Is this possible?

QuantiFast Probe Assays are only sold in combination with optimized real-time RT-PCR master mixes and cannot be sold as stand-alone assays.

 

FAQ ID -2360
Do you have any information or guidelines regarding the choice of reference genes for real-time PCR?

Yes, please visit our website section 'Using endogenous control genes in real-time RT-PCR' for general information. It provides a list of relative gene expression levels for commonly used human and mouse reference genes.

We offer a set of ready-to-order control genes for use in SYBR Green based as well as probe based real-time RT-PCR.

In addition, you may want to refer to the following citations on reference gene selection for quantitative real-time PCR:

• Vandesompele J, De Preter K, Pattyn F, Poppe B, Van Roy N, DePaepe A, Speleman F [2002]: Accurate normalization of real-time quantitative RT-PCR data by geometric averaging of multiple internal control genes. Genome Biol 2002, 3:0034.

• Radonic A, Thulke S, Mackay IM, Landt O, Siegert W, Nitsche A., 2004. Guideline to reference gene selection for quantitative real-time PCR. Biochem Biophys Res Commun. 313(4): 856-62.

• Katrien Smits,Karen Goossens, Ann Van Soom, Jan Govaere, Maarten Hoogewijs, Emilie Vanhaesebrouck,Cesare Galli, Silvia Colleoni, Jo Vandesompele, and Luc Peelman [2009]Selection of reference genes for quantitative real-time PCR in equine in vivo and fresh and frozen-thawed in vitro blastocysts. BMC Res Notes. Dec 11;2:246.

FAQ ID -2371
How does the QuantiFast Probe RT-PCR Plus Kit eliminate genomic DNA contamination?
Genomic DNA contamination is effectively eliminated through an optimized incubation step prior to real-time RT-PCR step.
FAQ ID -2354
Why do replicates in real-time PCR have different plateau heights?

Replicates in real-time PCR may have different plateau heights due to differences in the reaction kinetics for each sample. Even though replicates start out with identical template amounts, the rate at which reagents are being depleted, and the point when exponential accumulation of PCR product stops and becomes linear, differ between replicates. This will result in different plateau heights, the stage where PCR reactions have come to a halt, and little or no additional PCR product is being amplified. You can find further information in Chapter 'Quantification of target amounts' of our Brochure "Critical Factors for Successful Real-Time PCR".

 

FAQ ID -539
How should fluorescent labeled probes be stored?

Fluorescent oligonucleotides should be stored in the dark, as light can slowly degrade the fluorescent moieties. For optimal long-term storage of fluorescent dye-labeled probes (except Cyanine 570, Cy3.5, Cyanine 670, and Cy5.5), the oligos should be resuspended in a slightly basic solution (e.g., TE buffer at pH 8.0). If resuspended below pH 7.0, the probe can degrade. We recommend to aliquot the sample, and store the aliquots at -20°C.

Note that Cyanine 570, Cy3.5, Cyanine 670, and Cy5.5 begin to degrade at a pH above pH 7.0. For best results, resuspend Cy-labeled oligos at pH 7.0, aliquot, lyophilize, and store at -20°C.

FAQ ID -784
Do you have information on the use of recombinant DNA and RNA as absolute standards for realtime RT-PCR?

Recombinant DNA (recDNA) is very stable and represents the average size of mRNA. Due to the cloning and purification processes, obtaining recDNA can lengthen the overall process of generating standards.

Recombinant RNA (recRNA) and native RNA undergo reverse transcription as well as PCR, and mimic the natural process for mRNA in RT-PCR. Complicated cloning and purification of recRNA and instability of recRNA are two disadvantages for using recRNA as a standard. For further details please refer to the section "Generating Standard Curves" in Appendix D of the QuantiTect SYBR Green PCR Handbook.

FAQ ID -729
What are the differences between the existing QuantiFast Probe RT-PCR Kit and the new Plus Kit?
QuantiFast Mix 1 is delivered with the QuantiFast Probe RT-PCR Plus kit which contains genomic DNA Wipeout Buffer to eliminate residual gDNA. The rest of the procedure is comparable to the existing QuantiFast Probe RT-PCR Kit.
FAQ ID -2358
Can I do singleplex PCR with the QuantiFast Probe Assays?
Yes, for 2-step RT-PCR, the QuantiFast Probe PCR Kit can be used, for 1-step RT-PCR, the QuantiFast Probe RT-PCR Plus Kit is combined with the assays.
FAQ ID -2362
How important is the RNA purification process, for obtaining reliable qRT-PCR results?

The most important prerequisite for any gene expression analysis experiment is the preparation of consistently high-quality RNA from every experimental sample. Contamination by DNA, protein, polysaccharide, or organic solvents can jeopardize the success of an experiment.

Genomic DNA contamination in an RNA sample compromises the quality of gene expression analysis results. The contaminating DNA inflates the OD reading of the RNA concentration. It is also a source of false positive signals in RT-PCR experiments.

RNase contamination degrades RNA samples whichcauses low signal and false-negative results in PCR.

Residual polysaccharides, collagen, other macromolecules, and organic solvents in an RNA sample can inhibit the activity of DNase, which may interfere with DNase treatment for genomic DNA removal. These contaminants may also inhibit reverse transcriptase and DNA polymerase, leading to lower reverse transcription efficiency and reduced PCR sensitivity.

For fast purification of high-quality RNA we recommend QIAGEN’s RNeasy Kits like the RNeasy Mini Kit, the RNeasy Plus Universal Kit, or the RNeasy FFPE Kit.

FAQ ID -2655
What is the threshold cycle or Ct value?
The Ct or threshold cycle value is the cycle number at which the fluorescence generated within a reaction crosses the fluorescence threshold, a fluorescent signal significantly above the background fluorescence. At the threshold cycle, a detectable amount of amplicon product has been generated during the early exponential phase of the reaction. The threshold cycle is inversely proportional to the original relative expression level of the gene of interest.
FAQ ID -2682
Why does my realtime PCR assay quality decrease over time?
Make sure that template, primers, probes, and amplification reagents are stored correctly and avoid multiple freeze–thaw cycles for oligonucleotides and template. Check the performance of your real-time instrument as some instruments require the halogen lamp to be frequently replaced. Lasers must also be replaced occasionally.
FAQ ID -589
What are the recommended storage conditions of the QuantiFast Probe RT-PCR Plus Kit components?
The QuantiFast Probe RT-PCR Plus kit should be stored immediately upon receipt at –20°C in a constant-temperature freezer and protected from light. The 2x QuantiFast Mix 2 (Probe) can also be stored protected from light at 2–8°C for up to 1 month without showing any reduction in performance.
FAQ ID -2355
Why should DNA or cDNA targets be less than 250 bp long for real-time PCR?

Shorter amplification products facilitate high PCR efficiencies. Ideally, amplicon length should be less than 150 bp for optimal amplification efficiency. PCR efficiencies close to 100% are a crucial prerequisite for accurate quantification of target copy numbers in real-time PCR.

FAQ ID-751
What should I use as a standard for absolute quantification in real-time PCR?

For quantification of RNA, we strongly recommend using RNA molecules as standards. Use of in vitro transcripts as standards takes into account the variable efficiency of the RT reaction. An alternative to the use of in vitro transcripts as RNA standards is the use of a defined RNA preparation (e.g., from a cell line or virus preparation), for which the absolute concentration of the target has already been determined.

For quantification of DNA, several types of DNA can be used, such as plasmids, PCR products, or genomic DNA.

For more information, see Appendix E 'Generating Standard Curves' in the QuantiTect Probe PCR Handbook.

FAQ ID -1085
Is it necessary to perform calibration steps for the use of the MAX dye in duplex RT-PCR experiments on different cyclers?

It is not necessary to perform calibration steps with MAX dye.  For instruments from Applied Biosystems, simply use the VIC channel/filter for the detection of MAX. The emission maxima of MAX and VIC are very similar (557nm and 554nm), respectively. On the Rotor-Gene Q, use the yellow channel. On the BioRad CFX, use channel 2 for MAX detection. On the LightCycler 480, use the combination 523 nm (Excitation) / 568 nm (Emission).  MAX was chosen as a second dye label because VIC label is protected by ABI and HEX showed more crosstalk in our experiments.

FAQ ID -2373
How can I adjust the ROX concentration in the QuantiFast Probe RT-PCR Plus master mix?
The master mix supplied with the QuantiFast Probe RT-PCR Plus Kit contains no ROX dye. In order to adjust the reaction for instruments from Applied Biosystems (models 7000, 7300, 7700, 7900HT, StepOne™, and StepOnePlus™ Real-Time PCR Systems), it is necessary to add High-ROX Dye Solution to the master mix. For Applied Biosystems 7500 and instruments from Stratagene, ROX dye is required at a lower concentration. This requires the user to add the supplied ROX Dye Solution to the master mix during reaction setup (see the kit handbook for details).
FAQ ID -2356
What do I do if no fluorescent signal is detected in a real-time PCR assay?

Check the template quality and integrity by amplifying an endogenous control gene. Check the amplicon by QIAxcel Advanced system or agarose gel electrophoresis to show that amplification was successful.

 

Determine whether the gene of interest is expressed in your sample. See How can I find out if my gene of interest is express in a specific tissue type or cell line.  Ensure the assay setup and cycling conditions are correct, and that the data collection channel matches the emission wavelength of the fluorescent dye used. Use a control sample in which the gene of interest is definitely expressed.

 

If the issue persists, please send the original run file to QIAGEN Technical Services.

FAQ ID -9091
Can I use uracil-N-glycosylase (UNG) with the QuantiFast and Rotor-Gene PCR kits?

No. UNG treatment does not provide any advantage for the QuantiFast and Rotor-Gene PCR kits because the mastermixes do not contain dUTP. Use the QuantiTect kits if you intend to use the UNG treatment.

FAQ ID -9092
How do I setup and validate a multiplex PCR assay with QIAGEN PCR kits?

Ensure PCR amplicons are as short as possible, ideally 60–150 bp. Always use the same algorithm or software to design the primers and probes. For optimal results, only combine assays that have been designed using the same parameters.

 

Check the functionality of each set of primers and probes in individual assays before combining the different sets in the multiplex assay. Choose compatible reporters and quenchers based on a specific instrument. See How do I select appropriate reporter and quencher combinations for multiplex PCR.

 

FAQ ID -9093
How do I select appropriate reporter and quencher combinations for multiplex PCR?

For duplex analysis, using non-fluorescent quenchers (e.g., Black Hole Quencher®) is preferred over fluorescent quenchers (e.g., TAMRA fluorescent dye). For triplex and 4-plex analysis, QIAGEN strongly recommends using non-fluorescent quenchers. Generally, use the green channel, the yellow channel, and the orange and crimson channels to detect the least abundant target, the second least abundant target, and the two most abundant targets, respectively. For instrument-specific recommendations, please see the handbooks for the QuantiTect Multiplex PCR kit, QuantiFast Multiplex kit or Rotor-Gene Multiplex kit.

 

FAQ ID -9094
How do I quantify gene expression levels if the amplification efficiencies are different between the genes of interest and endogenous reference gene?

The REST 2009 (Relative Expression Software Tool) software applies mathematic models that compensate for the different PCR efficiencies of the gene of interest and reference genes. In addition, the software can use multiple reference gene normalization to improve the reliability of result, as well as provides statistical information suitable for robust comparison of expression in groups of treated and untreated. QIAGEN offers the REST 2009 software free of charge.

FAQ ID -9095
How do I avoid collecting a fluorescence reading from primer-dimer with the QuantiTect SYBR Green PCR Kit?

Depending on primer design and copy number of target, primer-dimer may occur and its signal might be detected. Typical strategies against this are to optimize PCR conditions and/or redesign the assay.

 

Alternatively, an additional data-acquisition step can be added to the 3-step cycling protocol. First, determine the melting temperatures (Tm) for both the amplicon and the primer-dimer. Then, add a 15 second data-acquisition step with a temperature that is higher than the primer-dimer Tm, but approximately 3ºC lower than the specific amplicon Tm.

FAQ ID -9096
How do I ensure reliable results for High Resolution Melting (HRM) assays?

Reliable HRM analysis results depend on template quality, highly specific HRM PCR kit with a saturation dye, a real-time instrument with HRM capability, and powerful software package. Factors critical for successful HRM analysis are:

 

  • Use the same genomic DNA purification procedure for all samples being analyzed by HRM. This avoids variation due to differing composition of elution buffers.
  • DNA template concentrations should be normalized using the same dilution buffer. Ensure the CT values are below 30 and differ no more than 3 CT values across individual samples.
  • Design assays with amplicon length 70–350 bp. For SNP analysis, use amplicon length 70–150 bp.
  • Always start with 0.7 µM primer concentration

 

For more details, please refer to the HRM Technology – FAQs and the Critical Success Factor for HRM performance.

FAQ ID -9097
Can I skip the gDNA wipeout buffer treatment step for the QuantiTect Reverse Transcription Kit?

The gDNA wipeout buffer incubation step can be skipped when the total RNA is free from genomic DNA. However, the gDNA wipeout buffer is still required to be added because the reverse transcription step is optimized in the presence of components in the gDNA wipeout buffer.

FAQ ID -9098
Why do I see multiple high-intensity peaks in my qPCR dissociation curve at temperatures less than 70ºC?

If the extra peaks seem irregular or noisy, do not occur in all samples, and occur at temperatures less than 70 ºC, then these peaks may not represent real PCR products and instead may represent artifacts caused by instrument settings.

 

Usually extra peaks caused by secondary products are smooth and regular, occur reproducibly in most samples, and occur at temperatures greater than 70 ºC. Characterization of the product by agarose gel electrophoresis is the best way to distinguish between these cases. If only one band appears by agarose gel then the extra peaks in the dissociation curve are instrument artifacts and not real products. If this is the case, refer to the thermal cycler user manual, and confirm that all instrument settings (smooth factor, etc.) are set to their optimal values.

 

FAQ ID -90990
How should I handle and store absolute quantitation standards for real-time experiments?
Store the standards at a high concentration in aliquots at -20oC to -70oC. If using low concentrations, stabilize standards with carrier nucleic acid. It is always best to use freshly diluted standards for each experiment. If possible, use siliconized tubes for standard (and target) dilutions. This will prevent any unspecific binding of nucleic acids to the plastic.
FAQ ID -9099
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