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One Step RT-qPCR Probe Kit
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One Step RT-qPCR Probe Kit
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One Step RT-qPCR Probe Kit

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One Step RT-qPCR Probe Kit Cat:P***2 Price: $**4 for **0T Storage conditions: Store at **0℃; avoid repeated freezing and thawing.   Product Introduction   One Step RT-qPCR Probe Kit v2 is a kit for multiple reverse transcription-fluorescence quantitative PCR reactions using RNA as a template. During the experiment, reverse transcription and quantitative PCR are performed in the same reaction tube, which simplifies the experimental operation and reduces the risk of contamination. This kit uses heat-resistant Reverse Transcriptase to efficiently synthesize the first-strand cDNA, and uses hot-start Ab-Taq DNA Polymerase for quantitative amplification, which is suitable for probe-based qPCR. This product contains all reverse transcription-fluorescence quantitative PCR components except primers and sample RNA, including RNase inhibitors, RTase, and Ab-Taq. It can reduce the number of operation steps, shorten the sample addition time, and reduce the chance of contamination.   Compatible models   Rox calibration is not required: Bio-Rad full series, Roche full series, Eppendorf full series, Takara full series, Qiagen full series, Hongshi full series, Tianlong full series, Biori full series, Yarui full series, etc.   High Rox needs to be added: ABI ***0, ***0, ***0, ***0, ***0HT Fast, StepOne™, StepOnePlus™, etc.; Low Rox needs to be added: ABI ***0, ***0 Fast, ViiA™7, QuantStudio™ 3 and 5, tratageneMX***0P™, MX***5P™, MX***0P™, etc.   Instructions   1. Precautions for use   â‘  Before use, it should be fully thawed at room temperature, mixed and centrifuged instantly;   â‘¡ Avoid bubbles in the reaction solution as much as possible;   â‘¢ The RNA to be tested should be as fresh as possible, and RNase contamination should be strictly prevented during the extraction process.
   
Reagents Amount of Usage Final concentration
RTQ Enzyme Mix μl /
2×RTQ Reaction Buffer *0 μl /
forward primer (*0 μM)a 0.4 μl 0.2 μM
reverse primer (*0 μM)a 0.4 μl 0.2 μM
TaqMan æŽ¢é’ˆ (5 μM)b μl 0.*5 μM
RNA æ¨¡æ¿c 1 pg~1 μg /
Nuclease-Free Water To *0 μl  
a. The recommended final concentration of primers is 0.2 μM. If the effect is not good, it can be adjusted to 0.1~1 μM; please set the primer length to *8~*5 bp and the GC content to *0%~*0%;   b. The recommended final concentration of probes is 0.*5 μM. If the effect is not good, it can be adjusted to 0.1~1 μM;   c. The recommended template loading volume is 1~5 μl. qPCR has extremely high sensitivity. It is recommended to dilute the template and control the Ct value between *0~*5;   d. Please prepare in a clean bench and use a gun tip and reaction tube without nuclease residue; it is recommended to use a gun tip with a filter. Avoid cross contamination and aerosol contamination.   2. Reaction procedure (can be adjusted appropriately according to the model)
procedure temperature time  
reverse transcription *0℃ *0min  
predegeneration *7℃ 1 min  
denaturation *7℃ 5 sec *0~*5
cycling
Annealing & Extension a *8℃ *0 sec
Notes Please use RNase free consumables during the experiment.

Pays: China
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Localité: China
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Groupe de produits : Molecular Biology

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