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Testing Procedure

PCR

PCR (Polymerase Chain Reaction) is a revolutionary method developed by Kary Mullis in the 1980s. PCR is based on using the ability of DNA polymerase to  synthesize new strand of DNA complementary to the offered template strand.  Because DNA polymerase can add a nucleotide only onto a preexisting 3'-OH group,  it needs a primer to which it  can add the first nucleotide. This requirement makes it possible to delineate a  specific region of template sequence that the researcher wants to amplify. At  the end of the PCR reaction, the specific sequence will be accumulated in  billions of copies(amplicons).


How It Works

The PCR reaction requires the following components:

DNA template - the sample DNA that contains the target sequence. At the beginning of the reaction, high temperature is applied to the original double-stranded DNA molecule to separate the strands from each other.

DNA polymerase - a type of enzyme that synthesizes new strands of DNA complementary to the target sequence. The first and most commonly used of these enzymes is Taq DNA polymerase (from Thermis aquaticus), whereas Pfu DNA polymerase (from Pyrococcus furiosus) is used widely because of its higher fidelity when copying DNA. Although these enzymes are subtly different, they both have two capabilities that make them suitable for PCR: 1) they can generate new strands of DNA using a DNA template and primers, and 2) they are heat resistant.

Primers - short pieces of single-stranded DNA that are complementary to the target sequence. The polymerase begins synthesizing new DNA from the end of the primer.

Nucleotides (dNTPs or deoxynucleotide triphosphates) - single units of the bases A, T, G, and C, which are essentially "building blocks" for new DNA strands. 

RT-PCR (Reverse Transcription PCR) is PCR  preceded with conversion of sample RNA into cDNA with enzyme reverse transcriptase.

Applications of PCR:
cloning, genetic engineering, sequencing

Imitations of PCR and RT-PCR:
The PCR reaction starts to generate copies of the target sequence exponentially. Only during the exponential phase of the PCR reaction is it possible to extrapolate back to determine the starting quantity of the target sequence contained in the sample. Because of inhibitors of the polymerase reaction found in the sample, reagent limitation, accumulation of pyrophosphate molecules, and self-annealing of the accumulating product, the PCR reaction eventually ceases to amplify target sequence at an exponential rate and a "plateau effect" occurs, making the end point quantification of PCR products unreliable. This is the attribute of PCR that makes
Real-Time Quantitative RT-PCR so necessary.

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  • Home
  • Research
    • CCR5 Delta32
    • APOBEC3G
    • HLA-B27 and HLA-B57
    • DRB1*13 and DQB1*6
    • MTHFR C677T and A1298C
    • Breakthrough Research
    • WHAT WE'RE WORKING ON
  • Instructions
    • Instructions
    • About Test
    • Testing Procedure
    • Procedure
  • Accuracy
    • CANADA'S LARGEST PRIVATE LABORATORY
    • Accuracy
    • What is PCR?
    • Why PCR Testing?
    • DNA Structure and PCR
    • Basic Process of PCR
    • PCR Testing Machines
    • Use of PCR
  • Privacy Policy
    • Privacy Policy
    • FAQ
  • Buy Now
  • Contact Us