Direct PCR

TIANcombi DNA Lyse & Det PCR Kit

Fast purification of DNA from various materials for PCR detection

Catalog number / packaging

Cat. no

ID

No. of preps

4992528

KG203-03 20 µl×200 rxn

4992527

KG203-02 20 µl×50 rxn
  • Storage

    Store at -20℃ .
  • Description

    The TIANcombi DNA Lyse & Det PCR Kit adopts a unique packaging design that includes all the reagents for rapid genomic DNA preparation and PCR amplification. It is applicable for the one-step genome DNA purification from various samples (plant tissues, seeds, animal tissues, blood, yeast and bacteria) and the subsequent PCR amplification and detection. Protein, RNA and other secondary metabolites removal, organic solvent extraction as well as the ethanol precipitation steps are not needed in the whole purification process, making the operation simple and fast. The product quality is stable and reliable.

    The 2× Det PCR MasterMix provided by this kit is a highly compatible PCR reagent that can efficiently and specifically amplify DNA without the need for removing impurities such as proteins. This reagent contains Taq DNA polymerase, dNTPs, MgCl2, buffer, as well as the enhancer, optimizer and stabilizer for PCR reaction. Application of the reagent makes PCR reaction fast, simple, sensitive, specific and stable. Therefore, this kit is especially suitable for high-throughput screening.

  • Applications

    ■ Gene detection: Ideal choice for large-scale gene detection.

  • Features

    ■ Simple and fast: DNA from different tissues can be extracted in 5 min without the need for liquid nitrogen grinding.

    ■ Wide applications: Applicable for plant leaves, seeds, animal tissues, blood samples (fresh blood, anticoagulation, blood clots, dried blood spots, etc.), yeast and bacteria.

    ■ Strong compatibility: The PCR reagent is suitable for amplification of DNA extracted from various sample sources.

  • Important Notes

    ■ For samples containing high level of phenols, such as cotton leaves, the sample input amount should strictly be less than 0.4 mg, otherwise the PCR reaction will be affected.

  • DNA was extracted from 5 mg of the leaves and seeds of corn, wheat, rice, soybean and cotton, respectively. The DNA was amplified by PCR using specific primers. 6 μl DNA from the total 20 μl eluents was loaded per lane.

    1: Positive control genome; 2: leave samples; 3: seed samples; 4: NTC; 5: D2000 primers

  • M: TIANGEN Marker D2000; 1: Positive control;

    2-7: The number of dried blood spots on the filter paper is 1-6 respectively; 8: Negative control.

    The 3 mm puncher was used to take the dried blood spots from the filter paper as the material for the extraction test.

    6 μl DNA from the total 20 μl eluents was loaded per lane.

  • M: TIANGEN Marker D2000; 1: Positive control (genomic DNA was used as template); 2-7: The amount of blood added are 10 μl, 20 μl, 30 μl, 40 μl, 50 μl and 60 μl, respectively; 8-13: The amount of blood added are 10 μl, 20 μl, 30 μl, 40 μl, 50 μl and 60 μl, respectively; 14: NTC.

    6 μl DNA from the total 20 μl eluents was loaded onto the agarose gel.