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Home > Equipment > Baths > Water Baths > Shaking Water Bath

Shaking Water Bath

Item #: ASH2OBATHS1

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Pfu DNA Polymerase
Pfu DNA polymerase is a heat stable DNA polymerase which has 5' 3' DNA polymerase and 3' 5' exonuclease (proofreading) activities. Pfu DNA polymerase retains the high fidelity, sensitivity and processivity with an error rate six-fold lower than Taq DNA polymerase, and significantly lower than the error rates of most other proofreading enzymes or DNA polymerase mixtures (1). This product is supplied with the unique Intact Genomics 10x PCR reaction buffer, containing MgCl2, which produces a final Mg2+ concentration of 1.5 mM, and 5X Magic Enhancer that enables efficient amplification of GC rich templates up to 84%. The physical purity of this enzyme is 98% as assessed by SDS-PAGE with CoomassieÂ® blue staining.

Quality Control
Quality control is performed following the production of each new lot of product to ensure that it meets the quality standards and specifications designated for the product. Each lot is repeatedly compared side-by-side with leading competitors to ensure our products outperform the competitor before product launching.

Product Source
E. coli strain expressing a Pfu DNA Polymerase gene from Pyrococcus furiosus.

Contents & Storage

Pfu DNA Polymerase
10x PCR Buffer with Mg²+
5x Magic Enhancer
10 mM dNTP (Cat. # 3312d, 3314d only)

Store all contents at -20 °C.

Storage Buffer
50 mM Tris-HCl, 50 mM KCl, 1 mM DTT, 0.1 mM EDTA, 50% Glycerol, pH 7.5 @ 25 °C.

10X PCR Buffer with Mg2+
100 mM Tris-HCl pH 9.0, 15 mM MgCl, 100 mM KCl, 80 mM (NH4)2SO4, 0.5% Igepal CA 630

Unit Definition
One unit is defined as the amount of enzyme that incorporates 10 nmoles of dNTP into acid-insoluble form in 30 minutes at 72 °C.

Protocol
1. Thaw 10x PCR Buffer, dNTP mix, primer solutions, 5x Magic Enhancer (if required) and mix thoroughly before use.
2. Prepare a reaction mix according to the following table: The reaction mix typically contains all the components needed for PCR except the template DNA.

PCR reaction set up:
Template DNA	xµl (0.01-0.5µMg)
10x PCR Buffer	10.0µl
dNTP (10 mM)	2.0µl
Forward Primer	xµl (0.1- 0.5µMM)
Reverse Primer	xµl (0.1- 0.5µMM)
5x Magic Enhancer (optional)	20µl
Pfu DNA Polymerase (5 U/Âµl)	0.5µl
H2O up to	100.0µl

3. Mix the reaction mixture thoroughly.
4. Add template DNA to the individual PCR tubes containing the reaction mixture.
5. Program the thermal cycler according to the manufacturerâs instructions. A typical PCR cycling program is outlined in the following table.

PCR cycling conditions:
Steps	Temp.	Time	Cycles
Initial denaturation	95 °C	3-5 min	1
Denaturation	94 °C	30-60 sec	25-35
Annealing	52-66 °C	30-60 sec
Extension	72-74 °C	1-2 min
Final extension	72-74 °C	10 min	1
Hold	4-12 °C	â

6. Place the PCR tubes in the thermal cycler and start the cycling program.

PNPCRREAG

Magnesium

Dye

No Dye

Enzymes

Intact Genomics

Pkg

Indiv

Type

Proofreading

SKU Number	Capacity/Volume	Style	Price	Quantity	Add to Cart
AAA44521	N/A	Universal Platform	268.0000 268.00 Each
AAA44522	N/A	Universal Platform	349.0000 349.00 Each
AAA44523	N/A	Universal Platform	471.0000 471.00 Each
AAA44524	N/A	Universal Platform	607.0000 607.00 Each
AAH44063U	17 L	Shaking	3692.0000 3692.00 Each
AAH44113U	25 L	Shaking	3850.0000 3850.00 Each
AAH44211K	37 L	Shaking	4063.0000 4063.00 Each
AAH44212K	37 L	Shaking	4063.0000 4063.00 Each
AAH44311K	55.52 L	Shaking	4634.0000 4634.00 Each
AAH44312K	55.52 L	Shaking	4634.0000 4634.00 Each