Hot-Start Gene Taq
Taq DNA polymerase| Product Name | Code No. | Size | Price | Note |
|---|---|---|---|---|
Hot-Start Gene Taq |
313-07044 |
50 units |
||
Hot-Start Gene Taq |
319-07041 |
250 units |
||
Hot-Start Gene Taq |
315-07043 |
250 units x 4 |
Product Description
Hot-Start Gene Taq is a heat resistant-DNA polymerase for hot-start PCR. Before entering the PCR cycle, the enzyme is activated by heat treatment at 95°C for 5 min.
This product is chemically modified “Gene Taq FP”, which is a modified Taq DNA polymerase in which the contamination of DNA derived from the host bacteria is controlled as much as possible. As with Gene Taq, Hot-Start Gene Taq does not have 5'-3' exonuclease activity. Also, having a terminal transferase activity, the PCR product obtained can be used for TA cloning.
This product contains two kinds of reaction buffers which are conventional 10 x Gene Taq Universal Buffer and 10 x Brilliant Buffer. The 10 x Brilliant Buffer has the effect of increasing the specificity of PCR and can be used only for the amplification of short strand DNA.
Features
・High specificity and high DNA yield.・Having a Hot-Start function; the reaction solution can be prepared at room temperature.・Most suited for multiplex PCR・High purity, with the contamination of host-derived DNA reduced as much as possible.
Applications
- Hot-Start PCR
- multiplex PCR
| Molecular Weight | 68 kDa |
|---|---|
| Concentration | 2.5 units/µl |
| Storage Conditions | 20 mmol/l Tris-HCl(pH 8.0), 100 mmol/l KCl, 0.1 mmol/l EDTA, 0.5% Tween 20, 1 mmol/l DTT, 50% Glycerol |
| Unit Definition | One unit is defined as the enzyme activity incorporating 10 nmoles of deoxynucleotide into acid-insoluble precipitates at 74°C for 30 min using activated calf thymus DNA as a primer/template. |
| Purity | No change was observed in the agarose gel electrophoresis pattern of DNA after reacting 10 units of this enzyme and 1 µg of λ/Hind III digest at 74°C for 1 hr. |
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Product Components
| Component | Quantity | Storage | Description |
|---|---|---|---|
| Hot-Start Gene Taq | 50 units x 1 | -20°C | |
| dNTP Mixture (2.5 mmol/l each) | 160 µl x 1 | -20°C | |
| 10 x Gene Taq Universal Buffer (15 mmol/l Mg2+ ) | 1 ml x 1 | -20°C | |
| 10 x Brilliant Buffer (20 mmol/l Mg2+ ) | 0.2 ml x 1 | -20°C |
| Component | Quantity | Storage | Description |
|---|---|---|---|
| Hot-Start Gene Taq | 250 units x 1 | -20°C | |
| dNTP Mixture (2.5 mmol/l each) | 800 µl x 1 | -20°C | |
| 10 x Gene Taq Universal Buffer (15 mmol/l Mg2+) | 1 ml x 1 | -20°C | |
| 10 x Brilliant Buffer (20 mmol/l Mg2+) | 1 ml x 1 | -20°C |
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Usage
Example of use 1: Multiplex PCR
Multiplex PCR was performed using plasmid DNA as a template and nine pairs of primers. The two kinds of reaction buffers attached to the product were compared.
Lane M: OneSTEP Marker 11
Lane 1: Hot-Start Gene Taq Brilliant buffer
Lane 2: Hot-Start Gene Taq Universal buffer
Lane 3: N Corporation modified DNA polymerase
Template DNA |
2.5 µl |
Primer Mixture |
1 µl |
Reaction Buffer |
1X |
dNTP Mixture |
0.2 mM |
Polymerase |
0.3 U |
total |
50 µl |
| 95°C | 30 sec. | 10 cycles |
| 65°C | 1 min. | |
| 72°C | 1 min. | |
| 95°C | 30 sec. | 27 cycles |
| 60°C | 1 min. | |
| 72°C | 1 min. | |
| 72°C | 7 min. |
Example of use 2: Shuttle PCR
Shuttle PCR was performed using HeLa DNA (50 ng) as a template and the three kinds of primers described below, for which amplification was difficult.
| A-1 | F | 5'-AGTGGGCAGAGCCAGTCACT-3' |
| R | 5'-AGACTGGATGCCCAGCCTAA-3' |
|
| A-2 | F | 5'-CAGACTCTGGGGCTGCCCAT-3' |
| R | 5'-TCAAACACTGGCTTGGGGTA-3' |
|
| A-3 | F | 5'-CCTTGGAGCAATGAGCAATG-3' |
| R | 5'-CATCTTTCCAGGCTCCTTCC-3' |
Template DNA |
50 ng |
Primer (10 µM each) |
1 µl |
10 x Reaction Buffer |
5 µl |
dNTP Mixture |
0.2 mM |
Polymerase |
0.25 U |
Total |
50 µl |
| 95°C | 5 min. | |
| 95°C | 30 sec. | 30 cycles |
| 68°C | 1.5 min. | |
| 68°C | 3 min. | |
| 4°C |
Results
When the Brilliant Buffer was used for Hot-Start Gene Taq, a highly specific amplification was achieved even by using low specific primers, and the target amplified product was obtained with a high yield.
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Data Sheets
SDS(Safety Data Sheet)
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Related Information
Note
- This product is for research use only.
Related Products
| Product | Characteristics | 5' → 3' exonuclease activity | terminal transferase activity |
|---|---|---|---|
| Gene Taq | The amplification efficiency of DNA fragments not more than 1 kbp is especially high. | - |
+ |
| Gene Taq NT | Gene Taq NT has the same functions as natural Taq DNA polymerase. | + |
+ |
| Gene Taq FP | Gene Taq FP obtained by further purifying Gene Taq to a higher degree of purity and by controlling the contamination by the host-derived DNA as much as possible. It is suitable for RAPD PCR which is affected by contamination by the genomic DNA. |
- |
+ |
Contact us
- Distributor
- FUJIFILM Wako Pure Chemical Corporation
- Produced by
- NIPPON GENE CO., LTD.
- E-mail:Web Contact Form
