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2× GS Taq PCR mix (ST111)

2× GS Taq PCR mix (ST111)

It is a basic Taq DNA polymerase with wide applicability, high yield and extremely fast extension speed.

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Product Description

It is a basic Taq DNA polymerase with wide applicability, high yield and extremely fast extension speed.


Highlights


1) Simple operation: 2×Mix, only need to add primers, template and ddH2O for PCR amplification.

2) Extremely fast extension speed: 10~15 s/kb.



Introduction


    This product contains high-purity GS Taq DNA polymerase, dNTPs and an optimized buffer system with a concentration of 2×. PCR amplification can be performed only by adding primers, templates and ddH2O, and can effectively amplify DNA fragments within 3 kb. The system contains a blue electrophoresis indicator, which can be directly loaded for electrophoresis detection after amplification. Its migration speed is similar to that of a 500 bp double-stranded DNA fragment in a 1% TAE agarose gel.

    The PCR product amplified by this product has a protruding "A" base at the 3' end, which can be directly used for TA cloning after purification.




Composition


Contents

Amount

2×GS Taq PCR Mix

5×1.0 mL



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Introduction

High-Fidelity PCR

I-5™ 2×High-Fidelity Master Mix

SF001

5×1.0 mL

      The fidelity is 60 times that of wild-type Taq enzyme;             Extremely fast extension speed: 10~30 s/kb.

Nucleic Acid  

   Electrophoresis

Agarose

AG801

100 g

High purity and clear background

Topo Cloning

pTOPO001 Simple Cloning Kit

TC601

20 rxns

This product is suitable for TA cloning of DNA fragments within 5 kb; The connection reaction is completed within 5 min;

                       Not contain polyclonal restriction sites.




Q1Why is there no product or a small amount of product in the final result?

A1

    1)Template degradation or poor template purity. Use electrophoresis to check template quality and use high-quality templates.

    2)The template concentration is too low. Appropriately increase the template usage.

    3)The primers are not suitable. Optimize primer design.

    4)The annealing temperature is not suitable. Set the annealing temperature gradient and explore the appropriate annealing temperature.

    5)The number of cycles is too small. Appropriately increase 5~10 cycles.

    6)Insufficient extension time. For complex templates, the extension speed can be appropriately increased to 20~30 s/kb.

 

Q2Why do non-specific bands or diffuse bands appear in amplification

A2

    1)Poor primer specificity. Optimize primers to avoid nonspecific bands and amplification of primer dimers.

    2)The primer concentration is too high. Decrease primer concentration.

    3)Template excess or poor purity. Reduce the amount of templates and use high-quality templates.

    4)The annealing temperature is too low. Appropriately increase the annealing temperature or use the Touchdown PCR program.

    5)Too many cycles. Reduce the number of cycles to 25~30 cycles.



Manual: Click to download

[1] Zhu M, Wang Q, Mu H, et al. A fitness trade-off between growth and survival governed by Spo0A-mediated proteome allocation constraints in Bacillus subtilis. Science Advances. 2023,9(39):9733.

[2] Liu H, Zhang Y, Liu Y, et al. Virome analysis of an ectomycorrhizal fungus Suillus luteus revealing potential evolutionary implications. Frontiers In Cellular And Infection Microbiology. 2023,13:1229859.


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