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[공식 대리점] Jena Bioscience-Taq Polymerase,탑 폴리메라제( PCR-420-1KU)
- AI바이오허브 오래 전 2025.01.24 21:56 Bulletin Board 인기
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Taq Polymerase
Thermostable DNA Polymerase without buffer
Thermus aquaticus, recombinant, E. coli
PCR-420-1KU
For general laboratory use.
Unit Definition: One unit is defined as the amount of the enzyme required to catalyze the incorporation of 10 nmoles of dNTP's into an acid-insoluble form in 30 minutes at 70 °C using hering sperm DNA as substrate.
Shipping: shipped on gel packs
Shelf Life: 12 months
Form: liquid
Concentration: 5 units/μl
| component | final assay conc. |
| PCR-grade Water | fill up to final amount |
| Reaction Buffer | 1 x |
| dNTP Mix | 200 μM |
| Taq Polymerase | 0.025-0.05 units/μl |
| primer mix or each primer | 200-400 nM each primer |
| template/sample DNA | < 10 ng DNA/assay |
| initial denaturation | 95 °C | 2 min | 1 x |
| denaturation annealing 1) elongation 2) | 95 °C 50-68 °C 72 °C | 10-20 sec 10-20 sec 20 sec - 4 min | 25-30 x |
Crystal Buffer (#PCR-271) is recommended for down-stream applications such as DNA sequencing, ligation, restriction digestion or where an analysis of the PCR product by absorbance or fluorescence excitation is required. For gel electrophoresis add gel loading buffer and fluorescent DNA stain (e.g. Gel Loading Buffer with DNA Stain, #PCR-274 - #PCR-276) before loading the PCR into the gel. Using pre-stained gels or post-run staining protocols is also possible.,
KCl Buffer (#PCR-262) is recommended for use in routine PCR reactions. The buffer is optimized for highest specificity but may require additional fine-tuning of assay parameters like MgCl2 concentration and annealing temperature.,
Labeling Buffer (#PCR-263) is recommended for DNA labeling or mutagenesis applications. The buffer is specially optimized for incorporation of labeled or modified nucleotides into DNA. It gives superior results in a broad range of reaction conditions with most primer-template pairs but amplification may also tend to an increased inaccuracy.
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