•与RT-PCR 系统兼容:RNasin®Plus RNase Inhibitor 已被证明可与Access and Access Quick™ RT-PCR Systems、ImPromII™ Reverse Transcription System 和Reverse Transcription System 兼容。同样也被证明可与基于TaqMan®的RT-PCR systems 兼容。
RNasin® Plus RNase Inhibitor is a recombinant mammalian RNase inhibitor that is expressed as a soluble protein inE. coli, allowing easy purification through a combination of ion exchange and hydrophobic interaction chromatography. The protein is capable of inhibiting eukaryotic RNases (e.g., RNase A and RNase B) similarly to human placental RNase inhibitor. RNasin® Plus RNase Inhibitor is tested in RT-PCR and is compatible with enzymes such as AMV, M-MLV and ImProm-II™ Reverse Transcriptases orTaqandTflDNA Polymerases. RNasin® Plus RNase Inhibitor also is tested and compatible with quantitative, real-time RT-PCR in a TaqMan® assay.
The inhibitor offers increased resistance to oxidation over the human version of the protein. Two cysteines in the human protein have been identified as especially sensitive to oxidation and react by forming a disulfide bond that can block the active site of the inhibitor. RNasin® Plus, through natural amino acid diversity, lacks the ability to form this site-blocking disulfide. In addition, the new protein has characteristics never before realized, including continued inhibition of RNases above 50°C. Heating solutions of RNasin® Plus and RNase followed by cooling does not result in the reappearance of RNase activity—even when the solution is heated above the denaturation temperature of the RNasin® Plus protein alone. This allows RNasin® Plus to protect RNA species prior to, during and after heating, even at temperatures normally used during first-strand DNA synthesis in RT-PCR. We have taken solutions up to 70°C for 15 minutes and did not see RNase reactivation.
Features - Benefits
Improved Resistance to Oxidation:Due to natural amino acid diversity, RNasin® Plus lacks the capability to form the active site-blocking disulfide bond that can form in the human protein under oxidative conditions.
Improved Purification:RNasin® Plus is expressed byE. colias a soluble protein, allowing easy purification by a combination of ion exchange and hydrophobic interaction chromatography. No direct affinity chromatography required. The new process yields a >90% pure protein with noE. coliRNase carryover.
Proven Compatibility with RT-PCR Systems:RNasin® Plus has proven compatible with the Access and AccessQuick™ RT-PCR Systems, ImProm-II™ Reverse Transcription System and the Reverse Transcription System. Also proven compatible with TaqMan®-based RT-PCR Systems.
Protection During RNA Template Denaturation:Heating mixtures of RNasin® Plus and RNase does not lead to reactivation of the RNase at temperatures even as high as 70°C for 15 minutes. Many RT-PCR protocols call for RNA template denaturation (e.g., 65–70°C for 5–10 minutes) in the presence of the RT primers prior to full RT reaction assembly for maximum sensitivity. You can now include RNasin® Plus at this step.
Protection During Higher Temperature RT Reactions:Add RNasin® Plus during RT reaction assembly and take the reaction to temperatures above 50°C with enzymes like the ImProm-II™ and AMV Reverse Transcriptases. RNases that may be present will not be reactivated at the higher temperature.
Choose Your Configuration:Learn more about our custom options for this product at:www.promega.com/custom/
Applications
RT-PCR.
Quantitative, real-time RT-PCR.
In vitro transcription.
In vitro translation.
Coupled transcription/translation.
Useful in any applications where eukaryotic RNase contamination is a potential problem.
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