A molecular biology technique used to amplify and replicate a specific segment of DNA, allowing for the detection and analysis of genetic material.
A diagnostic test based on the Polymerase Chain Reaction method, widely used to identify and analyze genetic material, particularly for detecting the presence of viruses, bacteria, or other pathogens.
Biological molecules, such as DNA or RNA, that carry genetic information and serve as the target for amplification in a PCR test.
The specific region of DNA or RNA that the PCR test is designed to amplify and analyze, providing information about the presence or absence of a particular genetic material.
Short DNA sequences that serve as starting points for DNA synthesis during the PCR process, defining the boundaries of the target sequence.
Laboratory equipment that controls temperature variations during the PCR process, facilitating the denaturation, annealing, and extension steps required for DNA amplification.
The first step in the PCR cycle, involving the separation of DNA strands by heating, allowing the target sequence to be exposed and available for amplification.
The second step in the PCR cycle, where the temperature is lowered to allow the primers to bind to complementary sequences on the target DNA, initiating the amplification process.
The third step in the PCR cycle, involving DNA synthesis at an optimal temperature, where a DNA polymerase enzyme adds nucleotides to the primers, creating copies of the target sequence.
Enzyme responsible for synthesizing new DNA strands during the PCR process, using the original DNA strand as a template.