StablePlus™ 2X RT-LAMP Master Mix
Croyez StablePlus™ 2X RT-LAMP Master Mix is an optimized master mix for reverse-transcription loop-mediated isothermal amplification (RT-LAMP) reactions. This product is a dual enzyme system, providing a rapid and sensitive detection in one pot. The amplified products can be detected by agarose gel electrophoresis.
The StablePlus™ version contains nucleic acid stabilizing agent to protect the amplified products.
The StablePlus™ version contains nucleic acid stabilizing agent to protect the amplified products.
The following procedure is a general guideline for RT-LAMP reaction. To maintain an RNase-free environment, always wear disposable gloves, and use laboratory consumables and water of nuclease-free grade during the whole experiment course.
RT-LAMP reaction set-up:
1.10X LAMP primer mix
2. An overview of the reaction set-up is listed in the table below. Place all required reagents on ice. Distribute appropriate volumes into each tube before adding template.
* See Usage Notes for additional guidelines on primer/template preparation.
3. Add target RNA template to the detection tube. Gently mix the reaction thoroughly to achieve uniform distribution and avoid making bubbles.
4. Incubate at 65°C for 30-60 min.
5. After LAMP reaction complete, the enzyme can be inactivated by heating at 80°C for 10 min.
Shipping Conditions:
Blue ice
RT-LAMP reaction set-up:
1.10X LAMP primer mix
Component | 10X concentration | Final concentration |
FIP | 16 μM | 1.6 μM |
BIP | 16 μM | 1.6 μM |
F3 | 2 μM | 0.2 μM |
B3 | 2 μM | 0.2 μM |
LOOP F | 8 μM | 0.8 μM |
LOOP B | 8 μM | 0.8 μM |
2. An overview of the reaction set-up is listed in the table below. Place all required reagents on ice. Distribute appropriate volumes into each tube before adding template.
Component | Amount | Final concentration |
StablePlus™ 2X RT-LAMP Master Mix | 12.5 μL | 1X |
10X LAMP primer mix | 2.5 μL | 1X |
RNA template | 1-2 μL | variable |
Nuclease-Free H2O | X μL | - |
Total reaction volume | 25 μL | - |
3. Add target RNA template to the detection tube. Gently mix the reaction thoroughly to achieve uniform distribution and avoid making bubbles.
4. Incubate at 65°C for 30-60 min.
5. After LAMP reaction complete, the enzyme can be inactivated by heating at 80°C for 10 min.
Shipping Conditions:
Blue ice