Primer extension

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Primer Extension Assay

Primer extension is a fundamental technique in molecular biology and genetics used for DNA synthesis. It involves the elongation of a primer molecule by a DNA polymerase enzyme, which adds nucleotides to the 3' end of the primer, allowing for the synthesis of a new DNA strand complementary to the template strand. This method is crucial in various applications, including DNA sequencing, PCR (Polymerase Chain Reaction), and site-directed mutagenesis.

Overview[edit | edit source]

The process of primer extension begins with the annealing of a short, single-stranded DNA primer to a complementary region on the template DNA. This primer provides the free 3' hydroxyl group that is necessary for the DNA polymerase to initiate the synthesis of the new DNA strand. Once the primer is annealed, the DNA polymerase enzyme adds nucleotides to the primer in a 5' to 3' direction, complementary to the template strand, until the synthesis is terminated or the end of the template is reached.

Applications[edit | edit source]

Primer extension has a wide range of applications in genetic and molecular biology research:

  • DNA Sequencing: Primer extension is a critical step in the Sanger sequencing method, where it is used to generate a set of DNA fragments of varying lengths that are then separated by gel electrophoresis to determine the DNA sequence.
  • Polymerase Chain Reaction (PCR): PCR utilizes primer extension in every cycle to amplify a specific DNA region, making it possible to generate millions of copies of a DNA segment from a small initial amount.
  • Site-Directed Mutagenesis: This technique uses primer extension to introduce specific mutations into a DNA sequence, allowing researchers to study the effects of these mutations on protein function.
  • Gene Cloning: Primer extension can be used to add restriction enzyme sites to the ends of a DNA fragment, facilitating its insertion into a cloning vector.

Procedure[edit | edit source]

The primer extension procedure involves several key steps: 1. Primer Design: A primer complementary to the target DNA region is designed and synthesized. 2. Annealing: The primer is annealed to the template DNA by heating and then slowly cooling the mixture. 3. Extension: A DNA polymerase enzyme is added along with a mixture of the four deoxynucleotide triphosphates (dNTPs). The enzyme extends the primer by adding nucleotides complementary to the template. 4. Termination: The reaction is stopped by inactivating the enzyme, either through heat denaturation or by adding a specific inhibitor.

Challenges and Considerations[edit | edit source]

  • Primer Design: The specificity and efficiency of primer extension are highly dependent on the primer design. Primers must have a high specificity to the target sequence and an appropriate melting temperature (Tm).
  • DNA Polymerase Selection: Different DNA polymerases have varying fidelity, processivity, and resistance to inhibitors, which can affect the outcome of the primer extension.
  • Optimization: Conditions such as temperature, ion concentration, and the ratio of enzyme to substrate often require optimization for efficient primer extension.

Conclusion[edit | edit source]

Primer extension is a versatile and powerful technique in the field of molecular biology, enabling researchers to synthesize DNA, sequence genomes, amplify specific DNA regions, and introduce mutations for study. Its applications have been pivotal in advancing our understanding of genetics and in the development of biotechnological tools and therapies.

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Contributors: Prab R. Tumpati, MD