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Invitrogen™
Platinum™ SuperFi II DNA Polymerase
Invitrogen Platinum SuperFi II DNA Polymerase is a proofreading DNA polymerase that combines superior fidelity with an innovative buffer, enabling universal primer annealing for the highest success in PCR.
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| Catalog Number | No. of Reactions |
|---|---|
| 12361010 | 100 Reactions |
| 12361050 | 500 Reactions |
| 12361250 | 5 x 500 Reactions |
Catalog number 12361010
Price (EUR)
247,65
Online Exclusive
266,00Save 18,35 (7%)
Each
In stock
No. of Reactions:
100 Reactions
Price (EUR)
247,65
Online Exclusive
266,00Save 18,35 (7%)
Each
Invitrogen Platinum SuperFi II DNA Polymerase is a proofreading DNA polymerase that combines superior fidelity with an innovative buffer, enabling universal primer annealing for the highest success in PCR. Due to the unique composition of the SuperFi II PCR buffer, the annealing temperature is 60°C for most primer pairs designed following the general design rules.
Features of Platinum SuperFi II DNA Polymerase include:
- Exceptional >300X Taq fidelity
- Universal primer annealing at 60°C
- Superior specificity, sensitivity, and yields
- Robust amplification of difficult-to-amplify targets
Platinum SuperFi II DNA Polymerase is an engineered enzyme with high processivity and increased resistance to PCR inhibitors. It also enables fast-cycling protocols and amplification of long targets (up to 20 kb). Platinum hot-start technology is based on proprietary antibodies that inhibit enzyme activity until the initial PCR denaturation step, preventing non-specific amplification and primer degradation. This technology also enables reaction setup at room temperature and provides increased sensitivity and yield.
Isostabilizing molecules in the buffer increase primer-template duplex stability during the annealing step and contribute to enhanced specificity without the need to optimize the annealing temperature for each primer pair. With Platinum SuperFi II DNA Polymerase, different PCR assays can be cycled together using the same protocol with a universal primer annealing temperature and an extension step selected for the longest fragment to be amplified.
Applications
- High-fidelity PCR
- Cloning and sub-cloning
- Site-directed mutagenesis
- Amplification of GC-rich templates
- Template generation for sequencing
- High-throughput PCR
- Amplification of samples with suboptimal purity
- Long PCR
Specifications
Fidelity (vs. Taq)>300X
Hot StartBuilt-In Hot Start
No. of Reactions100 Reactions
OverhangBlunt
PolymerasePlatinum SuperFi II DNA Polymerase
Quantity100 reactions
Reaction FormatStandalone
Shipping ConditionDry Ice
Size (Final Product)20 kb or less
For Use With (Application)Hot-start PCR, High-fidelity PCR
GC-Rich PCR PerformanceHigh
Reaction SpeedFast
Unit SizeEach
Contents & Storage
• Platinum SuperFi II DNA Polymerase (100 μL)
• 5X SuperFi II Buffer (1.25 mL)
Store at –20°C.
• 5X SuperFi II Buffer (1.25 mL)
Store at –20°C.
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Lot #Certificate TypeDateCatalog Number(s)
3273461Certificate of AnalysisJul 03, 202512361050
3271105Certificate of AnalysisJun 30, 202512361050
3271086Certificate of AnalysisJun 30, 202512361050
3260106Certificate of AnalysisJun 13, 202512361010
3257509Certificate of AnalysisJun 10, 202512361050
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Product Information
Frequently asked questions (FAQs)
Platinum SuperFi II DNA Polymerase enables amplification of long targets (up to 20 kb).
Find additional tips, troubleshooting help, and resources within our PCR and cDNA Synthesis Support Center.
You may want to consider using our Platinum SuperFi II DNA Polymerase (Cat. No. 12361010) and try optimizing your PCR conditions if needed. The Platinum SuperFi II DNA Polymerase demonstrates a superior detection sensitivity with as little as 0.4 ng of genomic DNA. It is also a good idea to include a positive control reaction in parallel to your test PCR to ensure there are no issues with your reagents during handling or use over time. Please note that control templates may be ordered through our GeneArt Gene Synthesis (de novo sequence with 100% guarantee delivered in a vector) or Strings (up to 3 Kb, blunt-ended dsDNA pools, cloned into ZeroBlunt TOPO vector, convenient for multiple controls) services.
Good lab practices are important for long fragment amplification. These include using high-quality templates (pure, fresh, and intact) and fresh primer solutions. Reducing primer concentration to 0.2 µM may also improve the results.
Yes, Platinum SuperFi II DNA Polymerase works at both universal 60 degrees C annealing temperature and at annealing temperatures calculated with a Tm calculator.
Platinum SuperFi II DNA Polymerase produces blunt-ended PCR products that can be cloned directly into blunt-ended cloning vectors. TA cloning is also possible if 3' dA-overhangs are added after PCR. We recommend purifying the PCR products of Platinum SuperFi DNA Polymerase before adding the overhangs. The procedure for adding 3' dA-overhangs (TA cloning) includes the following steps:
- Purify the PCR product (e.g., with a PCR purification kit or phenol extraction/DNA precipitation). Before adding the overhangs, PCR product must be purified, as the strong proofreading activity of any remaining Platinum SuperFi DNA Polymerase will degrade the added 3' dA-overhangs.
- Perform 3' dA addition with a Taq DNA polymerase.
Reaction components:
Purified PCR product
0.2 mM dATP
1x Taq Buffer
1 U Taq DNA Polymerase
Incubate the reaction for 20 min at 72 degrees C.
- Proceed to TA cloning. For optimal ligation efficiency, we recommend using fresh PCR products, since 3' dA-overhangs can be lost during storage
Citations & References (14)
Search citations by name, author, journal title or abstract text
Citations & References
Abstract
A PCR amplicon-based SARS-CoV-2 replicon for antiviral evaluation.
Journal:Sci Rep
PubMed ID:33500537
'The development of specific antiviral compounds to SARS-CoV-2 is an urgent task. One of the obstacles for the antiviral development is the requirement of biocontainment because infectious SARS-CoV-2 must be handled in a biosafety level-3 laboratory. Replicon, a non-infectious self-replicative viral RNA, could be a safe and effective tool for
Engineering SARS-CoV-2 using a reverse genetic system.
Journal:Nat Protoc
PubMed ID:33514944
'Reverse genetic systems are a critical tool for studying viruses and identifying countermeasures. In response to the ongoing COVID-19 pandemic, we recently developed an infectious complementary DNA (cDNA) clone for severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2). The reverse genetic system can be used to rapidly engineer viruses with desired
The analysis of GSTA1 promoter genetic and functional diversity of human populations.
Journal:Sci Rep
PubMed ID:33658540
'GSTA1 encodes a member of a family of enzymes that function to add glutathione to target electrophilic compounds, including carcinogens, therapeutic drugs, environmental toxins, and products of oxidative stress. GSTA1 has several functional SNPs within its promoter region that are responsible for a change in its expression by altering promoter
Epigallocatechin-3-gallate Alleviates Vanadium-Induced Reduction of Antioxidant Capacity via Keap1-Nrf2-sMaf Pathway in the Liver, Kidney, and Ovary of Laying Hens.
Journal:Biol Trace Elem Res
PubMed ID:33405082
'This study evaluated the effect of epigallocatechin-3-gallate (EGCG) alleviating the reduction of antioxidant capacity induced by dietary vanadium (V) in the liver, kidney, and ovary of laying hens. Furthermore, Kelch-like ECH-associated protein 1(Keap1)-nuclear factor erythroid 2-related factor 2 (Nrf2)-small Maf proteins (sMaf) pathway was explored to reveal the molecular mechanism.
Human Ubiquitin-Specific Peptidase 18 Is Regulated by microRNAs
Journal:Front Genet
PubMed ID:33633774
'Ubiquitin-specific peptidase 18 (USP18) acts as gatekeeper of type I interferon (IFN) responses by binding to the IFN receptor subunit IFNAR2 and preventing activation of the downstream JAK/STAT pathway. In any given cell type, the level of USP18 is a key determinant of the output of IFN-stimulated transcripts. How the
14 total citations