QuantiFast Pathogen +IC Kits

바이러스 RNA/DNA와 박테리아 DNA의 안정적인 고감도 검출용, 내부 대조물질 포함

S_2537_GEF_QFPatho

✓ 연중무휴 하루 24시간 자동 온라인 주문 처리

✓ 풍부한 지식과 전문성을 갖춘 제품 및 기술 지원

✓ 신속하고 안정적인 (재)주문

QuantiFast Pathogen RT-PCR +IC Kit (400)

Cat. No. / ID:   211454

400 x 25µL 반응용: 마스터 믹스, RT 혼합물, 동결건조 내부 대조군 분석, 동결건조 내부 대조군 RNA, ROX 염료 용액, High-ROX 염료 용액, RNase 불포함수, 핵산 희석 완충액, 완충액 TE
US$1,526.00
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키트대조물질
QuantiFast Pathogen Kit
Internal Control
유형
RT-PCR
PCR
QuantiFast Pathogen +IC Kits은/는 분자생물학 분야에 사용하기 위한 것입니다. 이 제품들은 질병의 진단, 예방, 또는 치료 목적으로 사용할 수 없습니다.

✓ 연중무휴 하루 24시간 자동 온라인 주문 처리

✓ 풍부한 지식과 전문성을 갖춘 제품 및 기술 지원

✓ 신속하고 안정적인 (재)주문

특징

  • 병원체 표적과 내부 대조물질 동시 검출
  • 더 많은 샘플 투입이 가능한 더 뛰어난 민감도의 5x 마스터 믹스
  • 프로세스 안전성 향상을 위한 음성 결과의 정확한 해석
  • 약한 양성 표적 신호의 명확한 검출
  • 표준 및 고속 사이클러 모두에서 빠르고 범용적인 프로토콜 지원

제품 세부 정보

QuantiFast Pathogen +IC Kits는 서열 특이적 프로브를 사용하여 병원체 핵산의 민감하고 신속한 real-time PCR 또는 원스텝 RT-PCR 검출을 위해 고안되었습니다. 음성 검출 결과의 정확한 해석을 통한 뛰어난 프로세스 안전성을 위해 각 키트에는 최대 4개의 사용자 지정 병원체 표적(예: 바이러스, 박테리아, 곰팡이 등)을 실시간 멀티플렉스 검출할 수 있는 시약과 내부 대조물질(Internal Control, IC) 시약이 포함되어 있습니다. 두 가지 키트 형식이 있습니다. 내부 RNA 대조물질 템플릿이 포함된 바이러스 RNA 검출용 QuantiFast Pathogen RT-PCR +IC Kit와 내부 대조물질 프라이머/프로브 세트 또는 내부 DNA 대조물질 템플릿이 포함된 바이러스, 박테리아, 곰팡이 DNA 검출용 QuantiFast PCR +IC Kit와 내부 대조물질 프라이머/프로브 세트입니다. 두 키트 모두 농도가 다른 ROX가 2개의 튜브에 담겨 제공되므로 거의 모든 real-time기기에서 사용할 수 있습니다. 편의를 위해 마스터 믹스는 2~8°C에서 보관할 수 있습니다.

성능

QuantiFast Pathogen +IC Kits는 멀티플렉싱 시 민감도 손실 없이 넓은 선형 범위에서 바이러스 RNA 또는 DNA 표적과 제공된 내부 대조물질을 동시에 검출할 수 있습니다(그림  Rotor-Gene Q에서의 노로바이러스 고감도 검출 싱글플렉스 및 듀플렉스 검출의 높은 선형성 및 정밀도 참고). 이 프로토콜은 대부분의 사이클러에서 고속 사이클링 실험을 높은 신뢰도로 실행할 수 있도록 개발되었습니다(그림 ' Rotor-Gene Q에서 BHV-1의 고감도 검출' 및 ' ABI 7500에서 BHV-1의 고감도 검출' 참고). QuantiFast Pathogen +IC Kits를 사용하여 병원체 표적을 증폭하고 내부 대조물질을 함께 사용하면 음성 결과의 올바른 해석을 보장하여 병원체 검출 워크플로우의 프로세스 안전성이 향상됩니다(그림 ' 음성 결과의 정확한 해석' 참고).

키트와 함께 제공되는 QuantiTect 핵산 희석 완충액은 희석 및 반응 셋업 중에 RNA 및 DNA 표준물질을 안정화시키고 튜브나 피펫 팁과 같은 플라스틱 표면에서 핵산의 손실을 방지합니다. 바이러스 핵산을 정량화하는 데 사용되는 표준물질을 안정적으로 희석하여 낮은 CT 값부터 높은 CT 값까지 넓은 선형 범위를 제공합니다. 완충액은 품질 저하 없이 표준물질을 더 오래 보관할 수 있게 해줍니다(그림 ' RNA 표준물질의 안정적인 희석 및 보관' 참고).

그림 참조

원리

음성 결과의 정확한 해석을 통해 프로세스 안전성을 높이기 위해, 각 QuantiFast Pathogen _IC Kit에는 내부 대조물질을 통해 사용자 지정 병원체 표적을 멀티플렉스로 실시간 검출할 수 있는 시약이 포함되어 있습니다. 대조물질과 표적 유전자를 별도의 반응이 아닌 동일한 반응에서 증폭하면 취급 오류를 최소화하여 유전자 정량화의 신뢰성을 높일 수 있습니다.

QuantiFast Pathogen +IC Kits를 통해 한 번의 시도로 병원체 핵산을 민감하고 신속하게 real-time 멀티플렉스 PCR 또는 원스텝 RT-PCR로 검출할 수 있습니다(순서도 ' QIAGEN 멀티플렉스 키트' 참고). 최적화된 마스터 믹스는 멀티플렉스 반응의 PCR 생성물이 대응하는 단일 증폭 반응의 PCR 산물과 동일한 효율과 민감도로 증폭되도록 보장합니다. 특별히 개발된 고속 PCR 완충액에는 변성, 어닐링 및 연장 시간을 크게 줄여주는 새로운 첨가제 Q-Bond가 함유되어 있습니다(그림 ' 고속 프라이머 어닐링' 참고). K+ 및 NH4+ 이온의 균형 잡힌 조성과 독자적인 합성 인자 MP는 프라이머와 프로브를 핵산 템플릿에 안정적이고 효율적으로 어닐링하여 높은 PCR 효율을 가능하게 합니다(그림  독자적인 PCR 완충액 참고). 또한 Sensiscript 역전사 효소의 독자적인 배합으로 바이러스 RNA의 고감도 역전사를 보장하며, HotStarTaq Plus DNA Polymerase는 엄격한 hot start를 제공하여 비특이적 생성물의 형성을 방지합니다.

QuantiFast Pathogen +IC Kit의 구성품
키트 구성품특징이점
5x QuantiFast Pathogen PCR 마스터 믹스농축 마스터 믹스고감도 병원체 검출에 최적화된 고농축 제품민감도 향상을 위해 더 많은 양의 템플릿을 분석에 추가할 수 있음
HotStarTaq Plus DNA Polymerase95ºC에서 5분 활성화실온에서 qPCR 반응 셋업
QuantiFast Pathogen 완충액NH4+와 K+ 이온의 균형 잡힌 조성특이적 프라이머 어닐링으로 신뢰할 수 있는 PCR 결과 보장
합성 인자 MP같은 튜브에서 최대 4개의 유전자를 안정적으로 멀티플렉싱 분석
독자적인 Q-Bond 첨가제더 빠른 PCR 실행 시간으로 신속한 결과 도출 및 하루 반응 횟수 증가
내부 대조군 분석내부 대조물질 템플릿QuantiFast Pathogen PCR +IC Kit의 내부 대조물질 DNA 템플릿다양한 병원체 분석에 사용할 수 있는 범용 DNA 증폭 대조물질
QuantiFast Pathogen RT-PCR +IC Kit의 내부 대조물질 RNA다양한 병원체 분석에 사용할 수 있는 범용 RNA 증폭 대조물질
내부 대조군 분석사전 혼합 프라이머/프로브 세트(TaqMan® 프로브), MAX 라벨링됨(HEX, VIC 등과 동등)병원체 표적에 대한 프라이머를 간섭하지 않음
추가 키트 구성품QuantiFast Pathogen RT 혼합물*Sensiscript 역전사 효소의 독자적인 배합 함유병원체 RNA의 고감도 검출에 최적화됨
ROX 염료 용액Applied Biosystems 7500 real-time PCR 시스템에서 형광 신호의 정규화를 위한 별도의 패시브 기준 염료 튜브. 선택 사항: Agilent의 Stratagene 기기에서 사용 가능ROX 염료가 필요한 사이클러에서 정확한 정량화. 모든 real-time 사이클러에서 PCR을 간섭하지 않음
High-ROX 염료 용액Applied Biosystems 7900 및 StepOne real-time PCR 시스템에서 형광 신호의 정규화를 위한 별도의 패시브 기준 염료 튜브
QuantiTect 핵산 희석 완충액핵산 표준물질의 희석 및 보관을 위한 독점적 배합의 완충액희석 및 반응 셋업 중에 RNA 및 DNA 표준물질을 안정화시키고 튜브나 피펫 팁과 같은 플라스틱 표면에서 핵산의 손실을 방지
그림 참조

절차

QuantiFast Pathogen +IC Kits는 사용자 지정 병원체 및 내부 대조물질 검출을 위한 간단한 절차를 제공합니다. 여기에는 바이러스 RNA(원스텝 RT-PCR) 또는 바이러스, 박테리아, 곰팡이 DNA(PCR)의 실시간 검출을 위한 즉시 사용 가능한 마스터 믹스가 포함되어 있습니다. 반응 및 사이클링 조건을 최적화할 필요가 없습니다. 제공된 마스터 믹스를 병원체 분석(프라이머 및 프로브), 제공된 내부 대조군 분석 및 내부 대조군 DNA 또는 RNA와 혼합하기만 하면 됩니다. 또는 샘플 정제 절차에 내부 대조물질을 추가한 경우, 반응 혼합물에 내부 대조물질 DNA 또는 RNA 대신 RNase 불포함수를 첨가합니다. 그런 다음 샘플 DNA 또는 RNA를 추가하고 사이클러에서 반응을 시작합니다. 키트 안내서에는 다양한 사이클러에서 TaqMan® 프로브와 함께 사용할 수 있도록 최적화된 프로토콜이 포함되어 있습니다. 또한 염료 조성 선택에 대한 권장 사항도 포함되어 있습니다.

각 QuantiFast Pathogen +IC Kit에는 반응 혼합물에 직접 추가하여 증폭 대조군으로 사용할 수 있는 내부 대조군 분석과 내부 대조군 DNA 또는 RNA가 함유되어 있습니다. 또는 IC를 정제 절차에 추가하여 정제 과정과 증폭을 모두 대조 관리할 수 있습니다. 정제 절차에 내부 대조물질을 추가하기 위해 고농축 내부 대조물질 DNA 또는 RNA(고농도)를 별도로 주문할 수 있습니다(그림 ' QIAGEN 내부 대조물질' 참고).

그림 참조

응용 분야

QuantiFast Pathogen +IC Kits는 내부 대조물질을 포함한 병원체 DNA 및/또는 RNA를 검출하기 위해 서열 특이적 프로브를 사용하여 민감한 real-time PCR 또는 원스텝 RT-PCR을 제공합니다. 이 키트는 QIAGEN, Applied Biosystems, Bio-Rad, Roche(capillary 사이클러 제외), Agilent의 사이클러를 포함한 다양한 real-time 사이클러에서 사용할 수 있습니다.

지원되는 데이터 및 수치

Specifications

FeaturesSpecifications
Applications병원체 검출: 바이러스, 박테리아, 곰팡이 DNA의 real-time PCR(QuantiFast Pathogen PCR +IC Kit) 또는 바이러스 RNA 검출을 위한 원스텝 RT-PCR(QuantiFast Pathogen RT-PCR +IC Kit)
Sample/target typeQuantiFast Pathogen PCR +IC Kit: 바이러스, 박테리아, 곰팡이 DNA; QuantiFast Pathogen RT-PCR +IC Kit: 바이러스 RNA
Single or multiplex듀플렉스
Reaction type내부 대조물질(IC)을 포함한 real-time PCR 또는 원스텝 RT-PCR
Real-time or endpointReal-time
SYBR Green I or sequence-specific probes서열 특이적 프로브
Thermal cycler듀플렉스 PCR/RT-PCR과 호환되는 대부분의 표준 및 고속 사이클러(예: Rotor-Gene Q 또는 Agilent, Applied Biosystems, BioRad, Roche의 사이클러)용
With or without ROX마스터 믹스는 ROX 염료 없이 제공되지만, 별도의 ROX 용액 2개가 포함되어 있음: ABI 7500을 제외한 ABI 사이클러와 함께 사용하기 위한 High-ROX 염료 용액, ABI 7500 및 기타 공급업체 기기와 함께 사용하기 위한 ROX 염료 용액(낮은 ROX 농도)

FAQ

What is the detection limit for the QuantiFast Pathogen + IC kits?
The detection limit for the QuantiFast Pathogen RT-PCR and PCR kits is < 10 copies.
FAQ ID -2453
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
What is the nature of the Internal Control in the QuantiFast Pathogen + IC kit?
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
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
Do the QuantiFast Pathogen PCR +IC Kit and the QuantiFast Pathogen RT-PCR +IC Kit contain ROX in the master mix?
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
How long does a QuantiFast Pathogen + IC run take on the Rotor-Gene Q?

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
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
On which cyclers can the QuantiFast Pathogen PCR +IC Kit or the QuantiFast Pathogen RT-PCR +IC Kit be used?
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
What should the cycler set-up be for a duplex reaction with the pathogen assay (FAM) and the Internal Control assay (MAX) on ABI instruments, when using the QuantiFast Pathogen PCR +IC Kit or the QuantiFast Pathogen RT-PCR +IC Kit?
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
What should the Rotor-Gene Q cycler settings be for a duplex reaction with the pathogen assay (FAM) and the Internal Control assay (MAX), when using the QuantiFast Pathogen PCR +IC Kit or the QuantiFast Pathogen RT-PCR +IC Kit?
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
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 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
When performing the Internal Control assay for the QuantiFast Pathogen PCR +IC Kit and the QuantiFast Pathogen RT-PCR +IC Kit, what channel or filter can be used to detect MAX?
MAX can be detected using the same channels or filters as for HEX, JOE, or VIC.
FAQ ID -2597
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
Are the Internal Controls used in the QuantiFast Pathogen PCR +IC Kit and the QuantiFast Pathogen RT-PCR +IC Kit homologous to a known target?
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
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
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
Can the QuantiFast Pathogen PCR +IC Kit or the QuantiFast Pathogen RT-PCR +IC Kit be used with hybridization probes?

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
When using the QuantiFast Pathogen PCR +IC Kit or the QuantiFast Pathogen RT-PCR +IC Kit, what should the fluorescent label of the probe be for the customer-defined assay to detect the pathogen?
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
Can the Internal Control DNA or RNA be added directly to the sample?
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
What should the cycler set-up be for a duplex reaction with the pathogen assay (FAM) and the Internal Control assay (MAX) on Mx instruments from Stratagene (Agilent), when using the QuantiFast Pathogen PCR +IC Kit or the QuantiFast Pathogen RT-PCR +IC Kit?
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
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 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
Which DNA/RNA extraction kits were tested in combination with the QuantiFast Pathogen PCR +IC Kit and the QuantiFast Pathogen RT-PCR +IC Kit?
FAQ ID -2606
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
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
Does the amount of Internal Control to be spiked into the lysis buffer or lysate depend on the elution volume only?

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
During data analysis, how should the threshold be set in the Yellow channel on the Rotor-Gene Q cycler to analyze the Internal Control from the QuantiFast Pathogen PCR +IC Kit or the QuantiFast Pathogen RT-PCR +IC Kit
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
What is the difference between QuantiTect Virus Kit and the new QuantiFast Pathogen +IC Kits?
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
What are the labels of the probe which is used in the Internal Control Assay for detection of the IC?
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
Can the Internal Controls be ordered separately in the QuantiFast Pathogen + IC kit for use during purification?

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
Why do the Internal Control templates for extraction (Internal Control DNA or RNA [High conc.]) have a 10x higher concentration than the IC templates provided with the QuantiFast Pathogen PCR +IC Kit and the QuantiFast Pathogen RT-PCR +IC Kit?

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
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 many times can the Internal Controls used in the QuantiFast Pathogen PCR +IC Kit and the QuantiFast Pathogen RT-PCR +IC Kit be freeze-thawed?
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
What is the difference between adding the Internal Control (IC) template used in the QuantiFast Pathogen PCR +IC Kit and the QuantiFast Pathogen RT-PCR +IC Kit to the amplification reaction versus adding the IC template at the extraction step?
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
For the QuantiFast Pathogen RT-PCR +IC kit, does the Internal Control also control for the reverse transcription reaction?
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