QuantiFast Pathogen +IC Kits

灵敏、可靠的检测病毒RNA/DNA和细菌DNA，含有内参

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QuantiFast Pathogen RT-PCR +IC Kit (400)

Cat. No. / ID: 211454

For 400 x 25 µl reactions: Master Mix, RT Mix, lyophilized Internal Control Assay, lyophilized Internal Control RNA, ROX Dye Solution, High-ROX Dye Solution, RNase-Free Water, Nucleic Acid Dilution Buffer, Buffer TE

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KitControl

QuantiFast Pathogen Kit

Internal Control

Type

RT-PCR

PCR

See trademarks.

QuantiFast Pathogen +IC Kits 旨在用于分子生物学应用。这些产品不能用于疾病诊断、预防和治疗。

✓ 24/7 automatic processing of online orders

✓ Knowledgeable and professional Product & Technical Support

✓ Fast and reliable (re)-ordering

Features

同时检测目标病原体和内参
5x预混液具有更高的灵敏度，且起始样本量更大
正确解读阴性信号，检测灵敏度更高
清晰检测微弱的阳性信号
快速的通用型实验方案适用于标准和快速PCR仪

Product Details

QuantiFast Pathogen +IC Kits使用序列特异性探针，可灵敏、快速的对病原体核酸进行real-time PCR或一步法RT-PCR检测。该试剂盒含有检测4个用户定义的病原体核酸（如：病毒、细菌、真菌等）所需的试剂和内参，可对阴性结果进行正确解读，提高了检测灵敏度。该试剂盒有两种规格。QuantiFast Pathogen RT-PCR +IC Kit含有RNA内参模板和内参引物/探针对，用于检测病毒RNA。QuantiFast Pathogen PCR +IC Kit含有DNA内参模板和内参引物/探针对，用于检测病毒、细菌或真菌DNA。这两种试剂盒均提供分装在两个管中的不同浓度的ROX染料，因此适用于多种real-time PCR仪。为便于使用，预混液可存放在2–8°C。

Performance

QuantiFast Pathogen +IC Kits可通过多重扩增，同时检测病毒RNA或DNA、以及自带的内参（参见"Sensitive detection of Norovirus on the Rotor-Gene Q"和"High linearity and precision of singleplex and duplex detection"）。实验方案专为快速PCR设计，适用于多数PCR仪，具有极高的可靠性（参见"Sensitive detection of BHV-1 on the Rotor-Gene Q"和"Sensitive detection of BHV-1 on the ABI 7500"）。使用QuantiFast Pathogen +IC Kits同时扩增目标病原体和内参，提高了检测的可靠性，能够确保正确解读阴性结果（参见"Correct interpretation of negative results"）。

该试剂盒提供QuantiTect Nucleic Acid Dilution Buffer，可在稀释和反应体系构建时稳定RNA和DNA标准品，避免核酸损失。能够可靠的稀释标准品，进而用于核酸的定量检测，检测范围广，覆盖从低至高的C_T值。该缓冲液能够确保标准品长期保存不降解（参见"Reliable dilution and storage of RNA standards"）。

Principle

为避免假阴性结果，所有QuantiFast Pathogen +IC Kit都含有必须的试剂，可real-time检测病原体和内参。在同一反应中扩增内参和靶基因，提高了定量检测的可靠性，减少了手动操作可能产生的错误。

QuantiFast Pathogen +IC Kits可通过多重PCR灵敏、快速的进行real-time检测，或通过一步法RT-PCR检测病原体（参见"QIAGEN multiplex kits"）。优化的预混液可确保PCR产物在多重扩增反应中以相同的效率和灵敏度扩增。特别研制的快速PCR缓冲液含有新型的添加剂Q-Bond，能够大幅度缩短变性、退火和延伸的时间（参见"Fast primer annealing"）。浓度平衡的K⁺和NH₄⁺离子、以及独特的Factor MP能够促进引物和探针与核酸模板特异性结合，确保PCR效率高（参见"Unique PCR buffer"）。此外，配方独特的Sensiscript Reverse Transcriptase能确保病毒RNA的高度灵敏的逆转录，HotStarTaq Plus DNA Polymerase则提供严格的热启动，防止非特异性产物的形成。

QuantiFast Pathogen +IC Kit的组分
	试剂盒组分	特点	优势
5x QuantiFast Pathogen PCR Master Mix	浓缩的预混液	浓度高，专为灵敏的检测病原体而设计	可加入的模板体积更多，增加了灵敏度
	HotStarTaq Plus DNA Polymerase	95ºC孵育5分钟激活	在室温进行qPCR反应体系构建
	QuantiFast Pathogen Buffer	浓度平衡的NH₄⁺和K⁺离子	引物探针的特异性结合确保获得可靠结果
		合成的Factor MP	在单管中对至多4个基因进行多重分析
		独特的Q-Bond添加物	PCR运行时间缩短，更快获得结果，一天内可完成更多PCR反应
Internal Control Assay	Internal Control 模板	QuantiFast Pathogen PCR +IC Kit含有内参DNA模板	通用的DNA扩增对照能用于分析不同的病原体
	Internal Control 模板	QuantiFast Pathogen RT-PCR +IC Kit含有内参RNA	通用的RNA扩增对照能用于分析不同的病原体
	Internal Control Assay	引物探针预混液（TaqMan探针）标记有MAX（相当于HEX、VIC等）	不会干扰引物
Additional kit components	QuantiFast Pathogen RT Mix*	含有配方独特的Sensiscript Reverse Transcriptase	专为灵敏检测病原体RNA而设计
	ROX Dye Solution	参照染料可用于Applied Biosystems 7500 real-time PCR仪的荧光信号校准。可选：可用于Stratagene仪器	准确定量检测需要使用ROX染料。不会干扰PCR反应
	High-ROX Dye Solution	参照染料可用于Applied Biosystems 7900 PCR仪和StepOne real-time PCR仪的荧光信号校准	准确定量检测需要使用ROX染料。不会干扰PCR反应
	QuantiTect Nucleic Acid Dilution Buffer	缓冲液为专有配方，用于稀释和储存核酸标准品	在稀释和反应体系构建时稳定RNA和DNA标准品，避免核酸损失

Procedure

QuantiFast Pathogen +IC Kits通过简单的流程，即可检测病原体和内参。试剂盒含有即用型预混液，可real-time检测病毒RNA（一步法RT-PCR）或病毒、细菌和真菌DNA（PCR）。无需优化反应条件。只需将预混液与检测试剂（引物与探针）、Internal Control Assay和Internal Control DNA或RNA 混合。也可在样本纯化步骤中加入内参，然后加入不含RNase的纯水至反应混合液。将样本DNA或RNA加入后即可开始反应，适用于各种PCR仪。试剂盒使用手册含有优化的实验方案，适用于TaqMan探针和多种PCR仪。使用手册中还推荐了可用的染料。

所有QuantiFast Pathogen +IC Kit都含有Internal Control Assay和Internal Control DNA或RNA，可直接加入反应混合液，用作扩增对照。此外，也可在纯化过程中加入内参，作为纯化和扩增的对照。如需在纯化过程中加入内参，可另外订购高浓度的Internal Control DNA或RNA (High conc.) （参见"QIAGEN Internal Control"）。

Applications

QuantiFast Pathogen +IC Kits利用序列特异性探针进行灵敏的real-time PCR或一步法RT-PCR，检测病原体DNA和/或RNA，以及内参。该试剂盒适用于多种real-time PCR仪，包括QIAGEN、Applied Biosystems、Bio-Rad、Roche和Agilent的仪器。

Supporting data and figures

Correct interpretation of negative results.

Duplicates of two concentrations of a viral RNA target were co-amplified with the Internal Control in the presence of different amounts of a PCR inhibitory substance (humic acid) on the Rotor-Gene Q. [A] No template controls (NTCs) serve as a reference for Internal Control signal. [B] Amplification of viral RNA target and Internal Control confirms successful amplification. [C] The Internal Control indicates the presence of a low amount of inhibitors. [D] Failure to detect the Internal Control shows the failure of the amplification reaction through presence of inhibitors.

Sensitive detection of BHV-1 on the ABI 7500.

Sensitive detection of BHV-1 on the Rotor-Gene Q.

High linearity and precision of singleplex and duplex detection.

Reliable dilution and storage of RNA standards.

Specifications

Features	Specifications
Applications	Pathogen Detection: Real-time PCR of viral, bacterial or fungal DNA (QuantiFast Pathogen PCR +IC Kit) or one-step RT-PCR for detection of viral RNA (QuantiFast Pathogen RT-PCR +IC Kit)
Sample/target type	QuantiFast Pathogen PCR +IC Kit: viral, bacterial or fungal DNA; QuantiFast Pathogen RT-PCR +IC Kit: viral RNA
Single or multiplex	Duplex
Reaction type	Real-time PCR or one-step RT-PCR including of an internal control (IC)
Real-time or endpoint	Real-time
SYBR Green I or sequence-specific probes	Sequence-specific probes
Thermal cycler	For most standard and fast real-time cylcers compatible with duplex PCR/RT-PCR, e.g. Rotor-Gene Q or cyclers from Agilent, Applied Biosystems, BioRad, Roche
With or without ROX	Master Mix is provided without ROX dye, but 2 separate ROX solutions are included: High-ROX Dye Solution for use with ABI cyclers except ABI 7500, ROX Dye Solution (low ROX conc.) for use with ABI 7500 and other suppliers

Resources

Download Safety Data Sheets for QIAGEN product components.

Now with even more applications!

FAQ

The detection limit for the QuantiFast Pathogen RT-PCR and PCR kits is < 10 copies.

FAQ ID -2453

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

The DNA IC is a non-linearized plasmid. The RNA IC is an in vitro transcript. Both are naked nucleic acids. The size (base pair length) of both templates is sufficient to allow for efficient purification with standard methods for nucleic acid extraction.

FAQ ID -2450

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

The QuantiFast Pathogen PCR +IC Kit and the QuantiFast Pathogen RT-PCR +IC Kit are supplied with master mixes that do not contain ROX. Instead, 2 different ROX concentrations are supplied in separate tubes. “High-ROX Dye Solution” is suitable for use with all ABI cyclers except ABI 7500, and “ROX Dye Solution” is suitable for use with ABI 7500 and, optionally, instruments from Stratagene (Agilent). Recommendations are provided in the handbook.

FAQ ID -2605

Using the QuantiFast Pathogen + IC kits on the Rotor-Gene Q:

RT-PCR
40 cycles	~95 minutes
45 cycles	~100 minutes

PCR
40 cycles	~75 minutes
45 cycles	~80 minutes

FAQ ID -2452

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

The QuantiFast Pathogen PCR + RT-PCR +IC Kits can be used on all leading block cycler platforms, but not on capillary systems (e.g., LightCycler 2.0).

FAQ ID -2596

No calibration for MAX is needed if the instrument is calibrated for VIC. Use the FAM/SYBR Green filter for the pathogen assay and the VIC/JOE filter for the IC assay. To detect the Internal Control (MAX) in the VIC/JOE filter, create a new detector (e.g., “MAX/IowaBlack”). Assign “VIC” as the reporter dye and “None” for the quencher dye.

FAQ ID -2610

Please follow the instructions in the handbook. Briefly, use gain optimization “Before First Acquisition” for the pathogen assay (FAM) in the Green channel, and use a fixed gain of 9 for the Internal Control Assay (MAX) in the Yellow channel.

FAQ ID -2608

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

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

MAX can be detected using the same channels or filters as for HEX, JOE, or VIC.

FAQ ID -2597

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

No, the Internal Controls used in the QuantiFast Pathogen PCR +IC Kit and the QuantiFast Pathogen RT-PCR +IC Kit are an artificial sequence that is not present in biological sample material.

FAQ ID -2598

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

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

No, the QuantiFast Pathogen PCR +IC kits are designed for use with hydrolysis probes (also known as TaqMan® probes) only.

See trademarks.

FAQ ID -2595

Typically, the target-specific probe should be labeled with FAM as the reporter dye and a non-fluorescent quencher (e.g., Dark Quencher, Black Hole Quencher [BHQ] or Iowa Black Quencher). Other reporter dyes than FAM, detected in a different detection channel than MAX, may also be suitable. It is not recommended to use fluorescent quenchers (e.g., TAMRA fluorescent dye). Due to their own native fluorescence, fluorescent quenchers contribute to an overall increase in background and reduce the signal-to-noise ratio.

FAQ ID -2594

No, the Internal Control template DNA or RNA must be added to the lysis buffer or to the lysate in order to prevent the loss of Internal Control template thorough matrix effects.

FAQ ID -2602

In the “Filter Gain Settings” dialog box, set the filter gain to a value of 4 for both the FAM/SYBR Green and HEX/JOE/VIC filters. See the Mx instrument/software manual for details.

FAQ ID -2609

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

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

Both membrane and magnetic bead-based kits have been tested (e.g., QIAamp MinElute Virus Kit, QIAamp Viral RNA Kit, DNeasy kits, RNeasy kits, QIAsymphony Virus/Bacteria kits, QIAxtractor Vx Reagents).

FAQ ID -2606

Store the standards at a high concentration in aliquots at -20^oC to -70^oC. 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

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 C_T values are below 30 and differ no more than 3 C_T 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

Principally, yes. However, additional factors influencing the CT are:

1. Extraction efficiency, which depends on extraction method and sample material.

2. Volume of the eluate used for PCR.

Examples: Use of the Internal Control according to handbook instructions (0.1µl per 1µl elution volume) for two different workflows.

Workflow 1: High extraction efficiency: use of 5 µl of the eluate for PCR results in a CT value of 29-30.
Workflow 2: High extraction efficiency: use of 10 µl of the eluate for PCR results in a CT of 28-29.

Depending on the workflow, the amount of Internal Control to be added to the extraction might have to be adjusted to more than 0.1 µl per 1 µl elution volume, or to less than 0.1 µl per 1 µl elution volume, in order to achieve a CT value within the expected range.

Running the Internal Control DNA/RNA provided with the QuantiFast Pathogen +IC Kit in a separate reaction can serve as a reference for adjusting the amount of Internal Control DNA/RNA (High conc.) to be added to the extraction.

FAQ ID -2604

On the Rotor-Gene Q, setting the threshold in the Yellow channel to an absolute value of 0.05 will give satisfactory results in most cases.

FAQ ID -2607

The QuantiTect Virus Kit and the new QuantiFast Pathogen +IC Kits are based on similar reaction chemistry and show identical sensitivity but as a new feature, the QuantiFast Pathogen kits include an Internal Control template and the corresponding primer/probe set for duplex amplification of a user-defined pathogen target with the provided Internal Control. Additional new features are pack size, kit variants, ROX variants, and speed.

FAQ ID -2448

In the QuantiFast Pathogen + IC kit, the probe is labeled with MAX-NHS ester (MAX) as the reporter dye which has a spectrum equivalent to HEX, JOE or VIC dyes. IowaBlack is used as the quencher dye. IowaBlack is a non-fluorescent quencher (dark quencher).

FAQ ID -2449

Yes, the Internal Control RNA (High conc.) and Internal Control DNA (High conc.) templates are available under a separate catalog number. After reconstitution according to the description in the handbook, these IC templates have a 10x higher concentration than the Internal Control templates provided in the kits. They are sufficiently concentrated to be spiked into the sample prep without replacing too much of the sample input volume.

**Please note that there is no assay (primer/probe set) for amplification of the IC included in these separate catalog numbers. The assay is only included in the QuantiFast Pathogen PCR +IC Kit and QuantiFast Pathogen RT-PCR +IC Kit. The ICs cannot be used with the QuantiTect Virus kits because the assay (primer/probe set) for the detection of the IC is provided with the QuantiFast Pathogen Kits only.

FAQ ID -2451

After reconstitution according to handbook instructions, the Internal Control (IC) templates provided with the kits have a ready-to-use concentration for direct use as an amplification control in PCR or RT-PCR. For each 25 µl reaction, 2.5 µl of the IC are added, resulting in an expected CT value of approximately 29-30.

In order to achieve the same CT value when using the IC as an extraction control, more IC template has to be spiked in before extraction. The exact amount depends mainly on the elution volume. For each 1 µl of elution volume, 0.1 µl of the IC High conc. should be added to each of the extraction samples. This should result in a CT value in the PCR or RT-PCR reactions of approximately 29-30.

Examples: For 100 µl of elution volume, 10 µl of the IC, per sample, should be added to the lysis buffer or lysate. For 50 µl of elution volume, 5 µl of the IC, per sample, should be added to the lysis buffer or lysate.

FAQ ID -2603

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 (T_m) 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 T_m, but approximately 3ºC lower than the specific amplicon T_m.

FAQ ID -9096

The Internal Control templates can be freeze-thawed for up to 6 times without decrease in performance. However, great care should be taken to avoid inadvertently introducing RNAses/DNAses into the Internal Control template solutions. In general, in order to avoid repeated freeze-thaw cycles, we recommend preparing aliquots of the Internal Control templates.

FAQ ID -2599

When the IC is added to the amplification reaction mix, the IC signal confirms that PCR amplification has been successful. When it is added at the extraction step to the lysis buffer or lysate, the IC signal confirms that nucleic acid purification and PCR amplification have been successful.

FAQ ID -2600

Yes, the Internal Control RNA will only give the expected signal when both the reverse transcription and the PCR reactions have been successful.

FAQ ID -2601