PCR Teaching kit
Cat# BB-MTK010S (5Reactions)
Cat# BB-MTK010 (10Reactions)
Objectives:
- To perform PCR amplification of specific target sequence from template
- To analyze the amplified product by Agarose gel
Principle: PCR (Polymerase Chain Reaction) is an in vitro method of enzymatic synthesis of specific DNA sequence, developed by Kary Mullis in 1983. It is a very simple technique for characterizing, analyzing & synthesizing any specific DNA or RNA from any source.
PCR consists of the following three basic steps:
Denaturation: During this step, two strands melt (open) to form single stranded DNA. This step is generally carried out at 92oC-96oC.
Annealing: In this step, primers anneal to each original strand of the template DNA for new strand synthesis. This step is carried out at 45oC to 60oC.
Extension: At this step the DNA polymerase synthesizes a new DNA strand complementary to the template DNA strand by adding dNTPs that are complementary to the template DNA in 5′ to 3′ direction, condensing the 5′-phosphate group of the dNTPs with the 3′-hydroxyl group at the end of the nascent (extending) DNA strand.
Materials provided: (for 10 reactions)
Materials | Quantity | Store at |
Taq DNA Polymerase | 10µl | -20oC |
10X Taq Buffer | 60 µl | -20oC |
Template DNA | 10µl | -20oC |
Forward Primer | 10µl | -20oC |
Reverse Primer | 10µl | -20oC |
Nuclease free water | 1 ml | -20oC |
1Kbp DNA ladder | 50 µl | -20oC |
dNTP mix | 10µl | -20oC |
6X DNA Loading Dye | 100µl | -20oC |
Agarose | 1gm | RT |
50X TAE | 15 ml | 4oC |
PCR Tubes | 10 Nos. | RT |
Ethidium bromide(EtBr) | 50 µl | RT |
Procedure:
Add the reagents to the PCR tubes in the following order:
Nuclease free water | 40µl |
Template DNA (100ng/ul) | 1 µl |
Forward Primer (10pmol/ul) | 1ul |
Reverse Primer (10pmol/ul) | 1 µl |
10X Taq Reaction Buffer | 5 µl |
dNTP Mix | 1 µl |
Tag DNA polymerase (1U/ul) | 1 µl |
Total Reaction Mix | 50 µl |
Mix the reagents properly, and place the tube in the PCR Machine
PCR Amplification: Carry out the amplification in a thermo cycler for 30 cycles using the following conditions:
Preparation of 1% Agarose gel:
- Prepare the gel casting tray by sealing the two ends with adhesive tape.
- Put the comb in the appropriate place of the gel casting tray.
- Prepare 1 X TAE by diluting appropriate amount of 50 X TAE Buffer (for carrying out one experiment approximately 200 ml buffer is needed).
- Weigh 0.5gm of Agarose and add 50ml of 1X TAE for preparing 1% Agarose
- Boil until the agarose dissolves completely, cool it to around 50⁰C, add 5µl EtBr to the agarose solution and mix
- Pour the Agarose solution slowly to avoid generation of any air bubble .Keep the gel undisturbed at room temperature till the agarose solidifies.
- Pour 1X TAE into the gel tank till the buffer level stands at 0.5 to 0.8 cm above the gel
- Gently lift the comb, ensuring the wells remain
Analysis on Agarose gel and Observation:
- Add 5ul of 6X DNA loading Dye in to the PCR tube and mix
- Carefully pipette 5µl of reaction mixture and load into the well of 1% Agarose
- Load 5µl of 1Kbp DNA ladder (ready to use) Run the sample at 100 volts till the blue dye front reaches 3/4th length of the gel.
Adapted from internet
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