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Taq DNA Polymerase (Buffer contains magnesium ions)

Taq DNA Polymerase (Buffer contains magnesium ions)

0.011 ~ 0.011 / Unit ( Negotiable )

|

Minimum Order

Place of Origin:

-

Price for Minimum Order:

Minimum Order Quantity:

20000 Unit

Packaging Detail:

in bottle

Delivery Time:

7-15 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

Taq DNA Polymerase (Buffer contains magnesium ions) Product number: T***2

Storage conditions: **0 ℃. Concentration: 5U/µl.

Product introduction

Taq DNA Polymerase is isolated and purified from Escherichia coli cloned with Thermu aquaticus DNA Polymerase gene after induction, and its molecular weight is *4 KD. Taq DNA Polymerase has 5′*3′ DNA polymerase activity and 5′*3′ exonuclease activity, but no 3′*5′ exonuclease activity. In the PCR reaction, the extension rate of Taq DNA Polymerase is **2 kb/min, and the product has A at the 3′ end, which can be directly used for T/A vector cloning.

Product composition

Taq DNA Polymerase **0U

*0xTaq Buffer+(with MgCl2) 1ml

Activity unit

1 unit (U) of Taq DNA Polymerase activity is defined as the amount of enzyme required to incorporate *0 nmol of deoxynucleotides into acid-insoluble substances using activated salmon sperm DNA as a template primer at *4C within *0 minutes.

Quality control

The purity detected by SDS-PAGE is greater than *9%, and no exogenous nuclease activity is detected; the PCR method detects no host residual DNA, and can effectively amplify single-copy genes in the human genome; there is no obvious change in activity after being stored at room temperature for one week.

Enzyme storage buffer

*0mMTris-HCl (pH8.0), 0.1 mM EDTA, 1mM DTT, **0 mM KC1, Stabilizers, *0% glycerol.

*0XTaq Buffer (containing Mg2):

**0 mM Tris-HCl (pH 8.4), **0 mM KC1, **0 mM (NH)z SO, *5 mM MgCl2, other ingredients.

★ *0X Taq Buffer is divided into two types: containing Mg°2+ and not containing Mg2+, which can be selected.

★ Buffer without Mg2+ is also equipped with *5 mM MgCl2.

★ If not specified, Buffer containing Mg2+ is usually provided.

Scope of application

Generally used for PCR amplification of DNA fragments, DNA labeling, primer extension, sequence determination, blunt end A addition, etc. The product can be directly used for T/A vector cloning.

Recommended PCR conditions: (Take *0 μl reaction system as an example)

Template <0.5 μg

Forward Primer (*0 μ M) 1 μl

Reverse Primer (*0 μ M) 1μ1

*0XBuffer* (with mgcl2) 5 μl

dNTP Mixture (2.5mM each) 4 μl

Taq DNA pol ymerase (5U/μ 1) 0.5~1 μ 1

dH*0 up to *0μ1

PCR reaction cycle settings:

1.*4°C:**5 min

2.*4C:*0 sec                  
3.****0°C:*0 sec 
4.*2*C:1 min/**2 kb
5.*2C:***0 mins
(2~5 : *0cycles)

Precautions

For your safety and health, please wear a lab coat and disposable gloves when operating.

This product is for experimental research only. Taq DNA Polymerase (Buffer contains magnesium ions)

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