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RT2 SYBR® Green FAST Mastermixes 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。
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RT² SYBR Green ROX FAST Mastermix (2)

Cat. No. / ID:   330620

Contains 2 x 1.35 ml tubes: for 12 x 100-well ring discs on the QIAGEN Rotor-Gene Q or 250 x 20 µl reactions
MX$6,370.00
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RT² SYBR Green FAST Mastermix (8)

Cat. No. / ID:   330601

Contains 8 x 1.35 ml tubes: for 8 x 100-well ring discs on the QIAGEN Rotor-Gene Q or 1000 x 20 µl reactions
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RT² SYBR Green ROX FAST Mastermix (24)

Cat. No. / ID:   330623

Contains 24 x 1.35 ml tubes: for 24 x 100-well ring discs on the QIAGEN Rotor-Gene Q or 3000 x 20 µl reactions
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RT² SYBR Green ROX FAST Mastermix (25 ml)

Cat. No. / ID:   330629

Contains 1 bottle of 25 ml mastermix: for 24 x 100-well ring discs on the QIAGEN Rotor-Gene Q or 2500 x 20 µl reactions
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RT² SYBR Green FAST Mastermix (12)

Cat. No. / ID:   330602

Contains 12 x 1.35 ml tubes: for 12 x 100-well ring discs on the QIAGEN Rotor-Gene Q or 1500 x 20 µl reactions
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RT² SYBR Green ROX FAST Mastermix (8)

Cat. No. / ID:   330621

Contains 8 x 1.35 ml tubes: for 8 x 100-well ring discs on the QIAGEN Rotor-Gene Q or 1000 x 20 µl reactions
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RT² SYBR Green FAST Mastermix (2)

Cat. No. / ID:   330600

Contains 2 x 1.35 ml tubes: for 2 x 100-well ring discs on the QIAGEN Rotor-Gene Q or 250 x 20 µl reactions
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RT² SYBR Green ROX FAST Mastermix (12)

Cat. No. / ID:   330622

Contains 12 x 1.35 ml tubes: for 12 x 100-well ring discs on the QIAGEN Rotor-Gene Q or 1500 x 20 µl reactions
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RT² SYBR Green FAST Mastermix (24)

Cat. No. / ID:   330603

Contains 24 x 1.35 ml tubes: for 24 x 100-well ring discs on the QIAGEN Rotor-Gene Q or 3000 x 20 µl reactions

特点

  • 特异性扩增,引物二聚体较少
  • 一体化混合物,适用于特定仪器
  • 可选含有ROX、荧光素或不含染料的规格
  • 实验步骤比常规SYBR Green预混液的步骤少
  • 灵敏度高、解离曲线好

产品详情

RT2 SYBR Green FAST Mastermixes非常适合使用SYBR Green进行real-time PCR分析,可选含有或不含参比染料的规格。RT2 SYBR Green FAST Mastermixes经优化后具有更快的PCR操作流程,而不影响灵敏度和特异性。RT2 SYBR Green FAST Mastermixes应与RT2 qPCR Primer Assays和RT2 Profiler PCR Arrays配合使用。

绩效

RT² SYBR Green FAST Mastermixes包含所有优化的试剂和缓冲液,可在各种real-time PCR分析仪上配合RT2 qPCR Primer Assays和RT2 Profiler PCR Arrays进行SYBR Green real-time PCR分析。

RT² SYBR Green FAST Mastermixes进行的高性能real-time PCR具有较高的扩增效率(参见" High amplification efficiency over a wide dynamic range")和高灵敏度及特异性(参见" Tighter control of polymerase activity yields greater specificity")。

此外,与常规方法获得的分离曲线相比,使用RT2 SYBR Green FAST Mastermixes得到的分离曲线有更低的背景和更明显的曲线(参见" Sharper dissociation curves with RT2 SYBR Green Fast Mastermix")。

查看图表

原理

RT2 SYBR Green FAST Mastermixes包含real-time PCR缓冲液、高性能的HotStart DNA Taq聚合酶、核苷酸和SYBR Green染料。有些预混液包含fluorescein荧光素或ROX染料,用于优化real-time PCR分析仪的光学元件。化学修饰并严格控制的HotStart酶可避免扩增引物二聚体和其他非特异性产物,提供准确的SYBR Green结果。RT2 SYBR Green FAST Mastermixes经优化后使用10s变性和30s退火/延伸的PCR实验方案,而不影响特异性和灵敏度。

不含ROX或荧光素的预混液

RT2 SYBR Green FAST Mastermix非常适合在不需要参比染料的仪器上进行基于SYBR Green的real-time PCR应用,仪器包括Bio-Rad models CFX96、CFX384;Bio-Rad/MJ Research Chromo4、DNA Engine Opticon、DNA Engine Opticon 2;Roche LightCycler 480(96孔和384孔);无ROX滤过装置的Eppendorf Mastercycler ep realplex以及Cepheid SmartCycler。

含有荧光素的预混液

RT2 SYBR Green Fluor FAST Mastermix非常适合在需要fluorescein荧光素作为参比染料的仪器上进行基于SYBR Green的real-time PCR应用,仪器包括Bio-Rad models iCycler、iQ5、MyiQ和MyiQ2。

含有ROX的预混液 

RT2 SYBR Green ROX FAST Mastermix非常适合在需要ROX作为参比染料的仪器上进行基于SYBR Green的real-time PCR应用,仪器包括QIAGEN的Rotor-Gene Q实时荧光定量PCR分析仪;Applied Biosystems models 5700、7000、7300、7500(标准和快速)、7700、7900HT(标准和快速的96-well block,384-well block)、StepOnePlus和ViiA 7(标准和快速的96-well block,384-well block);含有或无ROX滤过装置的Eppendorf Mastercycler ep realplex;Stratagene models Mx3000P、Mx3005P、Mx4000以及Takara TP-800。

应用

RT2 SYBR Green FAST Mastermixes适合用于real-time PCR分析。

辅助数据和图表

资源

安全数据表 (1)
Download Safety Data Sheets for QIAGEN product components.
试剂盒操作手册 (1)
For pathway-focused gene expression profiling using real-time RT-PCR
Safety Data Sheets (1)
Certificates of Analysis (1)

FAQ

Are primers available that only detect mitochondrial DNA encoded genes and not nuclear genomic DNA encoded genes?
There are less than a dozen genes encoded by the mitochondrial genome (all other mitochondrial proteins are encoded by nuclear genes), and they are all transcribed as one transcript (just like any prokaryote), so distinguishing the expression of individual genes by real-time RT-PCR is not possible.
FAQ ID -2680
How can I ensure that reaction volume is not lost due to evaporation during thermal cycling?
Be sure to carefully and completely seal the qPCR assay plate with fresh, optical, thin-wall, 8-cap strips or adhesive optical film before the plate is placed into the real-time cycler. In addition, refer to your instrument's user's manual to determine whether the real-time cycler manufacturer recommends use of a plate compression pad during the run.
FAQ ID -2679
How do I create a workspace that is free of DNA contamination, prior to carrying out a qPCR experiment?

Any DNA contamination will artificially inflate the SYBR Green signal, yielding skewed gene expression profiles and false-positive signals. The most common source of DNA contamination is from PCR products generated during previous experiments. Such contamination is most often due to the improper disposal of tubes, tips, and gels that previously came into contact with PCR products. Additionally, PCR products may also contaminate pipettors, racks, work pads, and commonly used reagents such as water and buffers. To minimize the risk of contaminating your experiment with extraneous DNA, the following steps should be taken:

 

  • Remove a single aliquot of water from your PCR-grade stock, sufficient to complete the experiment. This minimizes the number of times that the stock container is opened, thereby minimizing contamination risks.
  • Use only fresh PCR-grade reagents and disposable labware.
  • Treat any labware (tubes, tips, and tip boxes) used in PCR with 10% bleach, before discarding.
  • Maintain a dedicated workspace for PCR setup (perhaps a PCR-only hood), away from areas of the lab where post-PCR work is done, such as running gels, enzyme digestions, and cloning.
  • Change the lab bench pads/papers often and decontaminate lab benches and labware (racks, pipettors, etc.) before each use by washing with 10% bleach, and/or exposing to UV light for at least 10 minutes. This serves to degrade and/or inactivate contaminating DNA.
  • Before, during, and after the experiment, minimize the opening and closing of any tubes or plates used during the experiment.  
FAQ ID -2654
What is a dissociation curve, and why is it important to run a dissociation curve, following qPCR using SYBR Green chemistry?

Dissociation curves are carried out at the end of a PCR experiment by following a 3-step procedure.

First, all the components are denatured at 95°C, followed by complete annealing at a set temperature (based on the primer Tm values), followed by a gradual increase in temperature up to 95°C. Fluorescence intensity is monitored during this final temperature increase, resulting in the generation of a melting curve or dissociation curve.

By analyzing the first derivative of such a curve, you can readily assess the homogeneity of the PCR products, including the presence of primer–dimers, thereby determining the specificity of the PCR reaction. It is important to carry out such post-PCR analyses when using SYBR Green probe chemistry due to this reagent's lack of sequence specificity.

FAQ ID -2678
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