Horse-Power™ Taq DNA Polymerase with dNTPs
High-performance thermostable Taq polymerase with TruePure™ dNTPs for reliable PCR amplification.
Horse-Power™ Taq DNA Polymerase with TruePure™ dNTPs provides a high-performance DNA amplification system optimized for routine and demanding PCR applications. This thermostable polymerase delivers strong amplification efficiency, fidelity, and robustness across a broad range of DNA templates.
The inclusion of TruePure™ dNTPs, ultrapure nucleotides free of DNase, RNase, and phosphatase activity, ensures maximum reaction consistency and reproducibility. This combination is ideal for genotyping, colony PCR, fragment amplification, and diagnostic research workflows requiring dependable and consistent performance.
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Price: 82.30 €
Detailed information:
Advantages & Features
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High amplification efficiency: Produces strong yields across diverse templates.
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Thermostable Taq polymerase: Maintains activity through repeated thermal cycles.
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TruePure™ dNTP quality: Guarantees high-purity nucleotides for reliable PCR results.
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Reproducible performance: Minimizes variability and ensures consistent product yield.
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Versatile applications: Works efficiently with genomic, plasmid, and cDNA templates.
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Optimized buffer system: Supports robust and specific amplification.
Specifications
Assay conditions:
25 mM Tris-HCl pH 9.0 at 25 °C, 50 mM KCl, 2 mM MgCl2, 0.1 mg/mL gelatine, 200 µM dATP, dGTP, dTTP, 100 µM [α32-P] dCTP (0.05 µCi/nmol) and 12.5 µg activated salmon sperm DNA.
Unit definition:
One unit is defined as the amount of enzyme required to catalyse the incorporation of 10 nanomoles of dNTPs into acid-insoluble material in 30 minutes at 74 °C.
Includes
– 100 μL Horse-Power™ Taq Polymerase (5 U/μL)
– 25 mM MgCl2 (1.5 mL)
– 1.5 mL Buffer (10x)
– 1 mL TruePure™ Ultrapure dNTPs (2 mM each)
Applications
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Routine PCR.
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Genotyping and colony screening.
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DNA fragment amplification.
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Cloning and sequencing template generation.
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High-throughput PCR workflows.
Tables & Figures
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Quality Control
- Each batch is tested for purity, activity, specificity, and absence of DNase/RNase contamination, ensuring reproducible amplification results.
Advice
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Use 1–2.5 U per 50 µL PCR reaction.
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Thaw reagents on ice and mix gently before use.
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For GC-rich templates, optimize annealing temperature or Mg²⁺ concentration.
Storage, Shipping & Guarantee
- Shipped in: Gel pack.
- Storage: -20 °C (NON Frost-Free Freezer).
Citations
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- Núñez Delegido, E. (2017). Caracterización funcional de los genes CRD de Arabidopsis thaliana.
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- Demyda-Peyrás, S., Anaya, G., Bugno-Poniewierska, M., Pawlina, K., Membrillo, A., Valera, M., & Moreno-Millán, M. (2014). The use of a novel combination of diagnostic molecular and cytogenetic approaches in horses with sexual karyotype abnormalities: a rare case with an abnormal cellular chimerism. Theriogenology, 81(8), 1116-1122.
- Navarro-Domínguez, B., Cabrero, J., Camacho, J. P. M., & López-León, M. D. (2016). B-chromosome effects on Hsp70 gene expression does not occur at transcriptional level in the grasshopper Eyprepocnemis plorans. Molecular Genetics and Genomics, 291(5), 1909-1917.
- ALMENDROS, V. M. T. (2016). Identificación de especies de Dactylonectria e Ilyonectria asociadas al pie negro de la vid en Castilla la Mancha.
- Martínez-Miguel, P., Valdivielso, J. M., Medrano-Andrés, D., Román-García, P., Cano-Peñalver, J. L., Rodríguez-Puyol, M., … & López-Ongil, S. (2014). The active form of vitamin D, calcitriol, induces a complex dual upregulation of endothelin and nitric oxide in cultured endothelial cells. American Journal of Physiology-Endocrinology and Metabolism, 307(12), E1085-E1096.
- Daddaoua, A., Molina-Santiago, C., de la Torre, J., Krell, T., & Ramos, J. L. (2014). GtrS and GltR form a two-component system: the central role of 2-ketogluconate in the expression of exotoxin A and glucose catabolic enzymes in Pseudomonas aeruginosa. Nucleic acids research, 42(12), 7654-7665.
- Nieves-Morión, M., Lechno-Yossef, S., López-Igual, R., Frías, J. E., Mariscal, V., Nürnberg, D. J., … & Flores, E. (2017). Specific glucoside transporters influence septal structure and function in the filamentous, heterocyst-forming cyanobacterium Anabaena sp. strain PCC 7120. Journal of Bacteriology, JB-00876.
- Sierra, A. M. P., Sala, B. M., Santana, M. L., Jiménez, J. G., & Campos, P. A. (2012). Enfermedades causadas por en viveros de plantas ornamentales. In Boletin de Sanidad Vegetal: Plagas (Vol. 38, No. 1, pp. 143-156). Ministerio de Agricultura, Pesca y Alimentacion, Gobierno de España.
- Pérez-Sierra, A., Landeras, E., León, M., Berbegal, M., García-Jiménez, J., & Armengol, J. (2007). Characterization of Fusarium circinatum from Pinus spp. in northern Spain. Mycological research, 111(7), 832-839.
- Valverde-Tercedor, C., Montalbán-López, M., Perez-Gonzalez, T., Sanchez-Quesada, M. S., Prozorov, T., Pineda-Molina, E., … & Jimenez-Lopez, C. (2015). Size control of in vitro synthesized magnetite crystals by the MamC protein of Magnetococcus marinus strain MC-1. Applied microbiology and biotechnology, 99(12), 5109-5121.
- Mohammadi, H., Banihashemi, Z., Gramaje, D., & Armengol, J. (2012). Fungal pathogens associated with grapevine trunk diseases in Iran. Journal of Agricultural Science and Technology, 15(1), 137-150.
- Hernández-Hernández, J., Espino, A., Rodríguez-Rodríguez, J. M., Pérez-Sierra, A., León, M., Abad-Campos, P., & Armengol, J. (2010). Survey of diseases caused by Fusarium spp. on palm trees in the Canary Islands. Phytopathologia Mediterranea, 49(1), 84-88.
- Boughalleb, N., Salem, I. B., Beltrán, R., Vicent, A., Sierra, A. P., Abad‐Campos, P., … & Armengol, J. (2010). Occurrence of Monosporascus cannonballus in watermelon fields in Tunisia and factors associated with ascospore density in soil. Journal of phytopathology, 158(3), 137-142.
- Soto, E. C., Yáñez-Ruiz, D. R., Cantalapiedra-Hijar, G., Vivas, A., & Molina-Alcaide, E. (2012). Changes in ruminal microbiota due to rumen content processing and incubation in single-flow continuous-culture fermenters. Animal production science, 52(9), 813-822.
- Jroundi, F., Fernández-Vivas, A., Rodriguez-Navarro, C., Bedmar, E. J., & González-Muñoz, M. T. (2010). Bioconservation of deteriorated monumental calcarenite stone and identification of bacteria with carbonatogenic activity. Microbial ecology, 60(1), 39-54.
- Macias, M. I., Grande, J., Moreno, A., Domínguez, I., Bornstein, R., & Flores, A. I. (2010). Isolation and characterization of true mesenchymal stem cells derived from human term decidua capable of multilineage differentiation into all 3 embryonic layers. American journal of obstetrics and gynecology, 203(5), 495-e9.
- Clemente, A., Marín-Manzano, M. C., Jiménez, E., Arques, M. C., & Domoney, C. (2012). The anti-proliferative effect of TI1B, a major Bowman–Birk isoinhibitor from pea (Pisum sativum L.), on HT29 colon cancer cells is mediated through protease inhibition. British Journal of Nutrition, 108(S1), S135-S144.
- Alvarez, L. A., León, M., Abad-Campos, P., García-Jiménez, J., & Vicent, A. (2011). Genetic variation and host specificity of Phytophthora citrophthora isolates causing branch cankers in Clementine trees in Spain. European journal of plant pathology, 129(1), 103-117.
- Pérez-Sierra, A., León, M., Álvarez, L. A., Alaniz, S., Berbegal, M., García-Jiménez, J., & Abad-Campos, P. (2010). Outbreak of a new Phytophthora sp. associated with severe decline of almond trees in eastern Spain. Plant Disease, 94(5), 534-541.
- Jiménez-Hidalgo, M., Kurz, C. L., Pedrajas, J. R., Naranjo-Galindo, F. J., González-Barrios, M., Cabello, J., … & Fierro-González, J. C. (2014). Functional characterization of thioredoxin 3 (TRX-3), a Caenorhabditis elegans intestine-specific thioredoxin. Free Radical Biology and Medicine, 68, 205-219.
- Berbegal, M., Pérez-Sierra, A., Armengol, J., & Grünwald, N. J. (2013). Evidence for multiple introductions and clonality in Spanish populations of Fusarium circinatum. Phytopathology, 103(8), 851-861.
- Alaniz, S., Armengol, J., León, M., García-Jiménez, J., & Abad-Campos, P. (2009). Analysis of genetic and virulence diversity of Cylindrocarpon liriodendri and C. macrodidymum associated with black foot disease of grapevine. Mycological research, 113(1), 16-23.
- Mohammadi, H., Alaniz, S., Banihashemi, Z., & Armengol, J. (2009). Characterization of Cylindrocarpon liriodendri associated with black foot disease of grapevine in Iran. Journal of Phytopathology, 157(10), 642-645.
- Rafael, R., Márquez, M. C., Papke, R. T., & Ventosa, A. (2012). Multilocus sequence analysis of the family Halomonadaceae. International journal of systematic and evolutionary microbiology, 62(3), 520-538.
- Ruiz, R., Barroso-Deljesus, A., Lara, L., & Rubio, L. A. (2015). The use of multiple restriction enzymes in terminal restriction fragment length polymorphism analysis and identification of performance-related caecal bacterial groups in growing broiler chickens. The Journal of Agricultural Science, 153(08), 1491-1505.
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- García-Carneros, A. B., García-Ruiz, R., & Molinero-Ruiz, L. (2014). Genetic and Molecular Approach to Verticillium dahliae Infecting Sunflower. Helia, 37(61), 205-214.
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- Soto, E. C., Molina-Alcaide, E., Khelil, H., & Yáñez-Ruiz, D. R. (2013). Ruminal microbiota developing in different in vitro simulation systems inoculated with goats’ rumen liquor. Animal Feed Science and Technology, 185(1), 9-18.
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- González‐Domínguez, E., León, M., Armengol, J., & Berbegal, M. (2015). A Nested Polymerase Chain Reaction Protocol for in planta Detection of Fusicladium eriobotryae, Causal Agent of Loquat Scab. Journal of Phytopathology, 163(5), 415-418.
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- Salem, I. B., Correia, K. C., Boughalleb, N., Michereff, S. J., León, M., Abad-Campos, P., … & Armengol, J. (2013). Monosporascus eutypoides, a cause of root rot and vine decline in Tunisia, and evidence that M. cannonballus and M. eutypoides are distinct species. Plant disease, 97(6), 737-743.
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Safety Statements
This product is developed, designed and sold exclusively for Research purposes and in vitro use only (RUO). The product was not tested for use in diagnostics or for drug development, nor is it suitable for administration to humans or animals. For more info, please check its Material Safety Data Sheet available in this website.
Customers Review
FAQs
Q1: What is the advantage of using TruePure™ dNTPs?
They provide ultrapure, nuclease-free nucleotides that improve reproducibility and amplification accuracy.
Q2: What fragment length can this enzyme amplify?
Typically up to 5 kb for standard templates.
Q3: Is it suitable for high-throughput PCR?
Yes. The formulation ensures batch-to-batch consistency for large-scale workflows.
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