Unique blend of highly-efficient MyTaq™ HS DNA Polymerase and a proprietary proofreading enzyme that combine to give increased target affinity for use with challenging templates and
A 525 bp fragment of the 62% GC-rich human epidermal growth factor receptor (EGFR) gene (A), a 750 bp fragment of the 64% GC-rich translation factor p64 (myc) gene (B), a 900 bp fragment of 43% GC-rich angiotensin II receptor type I (AGTR1) gene (C), a 1.2 kb fragment of 62% GC-rich EGFR gene (D) were amplified using MyFi™ DNA Polymerase and similar polymerases from other suppliers. A five-fold serial dilution of human genomic DNA (25 ng – 8 pg, 1.6 pg and 0 pg, lanes 1-8 respectively) was used as template. Marker is HyperLadder 1kb (M). The results demonstrate that that MyFi delivers more reliable amplification of challenging targets.
A 3.9 kb fragment of a-1-antitrypsin (AT-R3) gene (A), and a 7.0 kb (B), 9.0 kb (C) and 10.0 kb (D) fragment of human (ß-globin) HbG gene, were amplified using MyFi™ DNA Polymerase and similar DNA Polymerases from other suppliers. A serial dilution of human genomic DNA (5 ng, 1 ng, 200 pg, 40 pg, 8 pg, 1.6 pg, 0.32 pg and 0 pg, Lanes 1-8 respectively) was used as template. Marker is HyperLadder 1kb (M). The results demonstrate that MyFi can be used to amplify targets up to 10 kb from even very challenging templates.
MyFi™ has been developed to give reliable amplification of targets up to 10 kb from challenging and complex targets. MyFi™ shows improved tolerance to PCR inhibitors, thereby enabling reliable detection from samples from which DNA is difficult to purify. Furthermore a unique buffer system and enzyme blend promote highly sensitive amplification, ideal for low-copy number targets. The inclusion of MyFi™ HS means MyFi™ generates PCR products with 3’-A overhangs making it suitable for TA cloning. MyFi™ has the added convenience of room temperature reaction assembly, to avoid non-specific amplification and primer-dimer formation.
An advanced buffer system and enzyme blend combine to give increased target affinity, ideal for amplification of cDNA libraries, complex genomic fragments and GC-rich targets.
| Presentation | BIO-21117 250 Units (Polymerase 125 µL, Buffer 625 µL) BIO-21118 500 Units (Polymerase 250 µL, Buffer 1.25 mL) BIO-21119 2,500 Units (Polymerase 2x 625 µL, Buffer 5x 1.25 mL) |
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| Appearance | Clear, colorless solutions | ||
| Hot start | Antibody mediated | ||
| Application | Amplification of challenging and complex templates, Robust PCR, Longer PCR (up to 10 kb), Low-copy PCR, TA cloning | ||
| Sample type | DNA, cDNA | ||
| Presentation | 2 vials / 2 vials / 7 vials | ||
| Storage | -20 °C | ||
| Mix stability | See outer label | ||
| Specific Activity | 2 u/µL | ||
| Functional | Single bands of PCR product on an agarose gel, size and sensitivity | ||
| DNA Contamination | No detectable product in a qPCR assay | ||
| DNase Contamination | No detectable degradation | ||
Cat. No. Size
BIO-21117 250 Units
BIO-21118 500 Units
BIO-21119 2500 Units
Hiroshi Shinozuka, AgriBio, Bundoora, Australia
Maiko Shi, AgriBio, Bundoora, Australia
Duke University, USA
McMaster University, USA
Keele University, Life Sciences, Staffs, UK
University of Birmingham, UK
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