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2XTaq PCR Mix including dye

2XTaq PCR Mix including dye

6 ~ 6 / Milliliter ( Negotiable )

|

Minimum Order

Place of Origin:

-

Price for Minimum Order:

Minimum Order Quantity:

100 Milliliter

Packaging Detail:

box

Delivery Time:

7~20 days if in stock

Supplying Ability:

500 Box per Month

Payment Type:

T/T

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1st Año

Persona de contacto Ying

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Description

Product name :2×Taq PCR Mix (including dye)

Cat. No. T***1

Product number: T***1

Storage conditions: **0℃

Product description

The concentration of Taq PCR Mix (containing dye) is 2×. It is easy and quick to use and can reduce contamination during PCR operation. When using, just take an appropriate amount of 2×Taq PCR Mix (containing dye), add template and primer, and add ddH2O to make up the volume, so that the concentration of the reaction system is 1×, and then you can carry out PCR reaction. The Taq in this Mix is ​​the mutant Taq-AS (Advanced Strong) DNA Polymerase obtained by screening. It can efficiently amplify DNA fragments ≤5Kb and has good inhibitor tolerance. Its amplification speed is about 3 times that of ordinary Taq DNA polymerase. Therefore, it can greatly reduce the time required for the PCR extension process, so as to shorten the entire PCR reaction. Different from the fast Taq polymerase based on the fusion protein principle, the use of Taq-AS is closer to WT-Taq, and it is not easy to have electrophoretic band diffusion, dragging or fragment size changes. This PCR Mix contains two dyes. The PCR product can be directly spotted for electrophoresis without adding Loading Buffer, and two indicator bands, purple and yellow, will appear during the electrophoresis. The dye does not affect the PCR amplification efficiency, but for experiments that require optical analysis of the PCR product such as absorbance and fluorescence, it is recommended to purify the PCR product before analysis. The PCR product has an A base at the 3\' end and can be directly used for T/A cloning after purification.

Quality Control

Endonuclease Residual Detection

The enzyme solution was incubated with supercoiled plasmid DNA at *7℃ for 4h, and no change in the plasmid was detected by DNA electrophoresis.

Exonuclease Residual Detection

The enzyme solution was incubated with double-stranded DNA substrate at *7℃ for *6h, and no change in the double-stranded DNA substrate was detected by DNA electrophoresis.

Stability Test

No obvious activity change after storage at room temperature for one week.

Functional detection

Using Arabidopsis genomic DNA and human genomic DNA as templates, a 5kb fragment was amplified, and the target band was visible after *0 cycles of agarose gel electrophoresis.
  2XTaq PCR Mix including dye

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