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home > Rhodamine-12-dUTP, min. 95 %, 1 mM solution, 25 µl, plastic > Rhodamine-12-dUTP, min. 95 %, 1 mM solution, 25 µl, plastic
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Rhodamine-12-dUTP, min. 95 %, 1 mM solution, 25 µl, plasticRhodamine 12 dUTP, min. 95 %, 1 mM solution, Molar mass (M) 990,7 g mol, Density (D) 1 g cm, Boiling point (bp) 100 C, Storage temp. 20 C, Empirical formula C39H41N6O19P3 DNAse , RNAse and Protease free Free of PCR inhibitors like modified bases and tetra pyrophosphate Adjusted to pH 7,5 for optimzed enzyme compatibility Highly efficient enzymatic fabrication Can be optimally combined with Carl ROTH ROTIPol DNA polymerases Suitable for All Carl ROTH
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Rhodamine-12-dUTP, min. 95 %, 1 mM solution, Molar mass (M) 990,7 g/mol, Density (D) 1 g/cm³, Boiling point (bp) 100 °C, Storage temp. -20 °C, Empirical formula C39H41N6O19P3

  • DNAse-, RNAse- and Protease-free
  • Free of PCR inhibitors like modified bases and tetra-pyrophosphate
  • Adjusted to pH 7,5 for optimzed enzyme compatibility
  • Highly efficient enzymatic fabrication
  • Can be optimally combined with Carl ROTH ROTI®Pol DNA polymerases
Suitable for

All Carl ROTH nucleotides are manufactured from highest-quality reagents and are most thoroughly tested for quality. This testing procedure not only includes standard-PCR but also “long range PCR”, repeated quantitative light-cycling reactions, and tests for physical stability.

Rhodamine-12-dUTP is able to replace dTTP in growing DNA-strands and is used for efficient non-radioactive DNA-labelling. Detection of labelled nucleic acids can easily be done by direct analysis of fluorescent signals (e. g. by fluorescence microscopy). Rhodamine-12-dUTP can also be used for double staining techniques in combination with fluorescein-12-dUTP or biotin-11-dUTP and corresponding antibodies or streptavidin-complexes, respectively.Excitation: 505 nmEmission: 530 nm (red)

Application examples

Non-radioactive labelling of DNA by enzymatic reactions, e.g. PCR, reverse transcription, nick-end-translation, end-labelling or random-primed DNA-labelling. Incorporation can be done with all established DNA-polymerases (e.g. Taq-polymerase, T4 DNA-polymerase, Klenow fragment).Tested for the lack of endo-, exodeoxyribonuclease, ribonuclease and phosphatase.

Rhodamine Green, mixture of 5/6 isomeresε505 (pH 7) = 8,5 E x mmol-1 x cm-1; pH: 7,5 ±0,2

Rhodamine-12-dUTP, min. 95 %, 1 mM solution, 25 µl, plastic

Item no : 19598386741
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