Polymerase chain reaction (PCR) is a technique that quickly makes millions to billions of copies of a DNA sample. It's based on the principle of enzymatic replication of nucleic acids. PCR is a basic method for DNA analysis and has revolutionized recombinant DNA technology. It's used to construct recombinant molecules by preparing a desired DNA fragment in large quantities. The PCR-amplified DNA is then cloned into a vector of choice. PCR works by using DNA polymerase's ability to synthesize a new DNA strand that's complementary to a template strand. The number of copies doubles after... Show more Polymerase chain reaction (PCR) is a technique that quickly makes millions to billions of copies of a DNA sample. It's based on the principle of enzymatic replication of nucleic acids. PCR is a basic method for DNA analysis and has revolutionized recombinant DNA technology. It's used to construct recombinant molecules by preparing a desired DNA fragment in large quantities. The PCR-amplified DNA is then cloned into a vector of choice. PCR works by using DNA polymerase's ability to synthesize a new DNA strand that's complementary to a template strand. The number of copies doubles after each cycle, and usually 25 to 30 cycles produce enough DNA. The PCR process is automated and can be completed in a few hours. A machine called a thermocycler alters the reaction's temperature every few minutes to allow DNA denaturing and synthesis. The steps of PCR are: Denaturation: Heat the reaction to separate the DNA strands. Annealing: Cool the reaction so the primers can bind to their complementary sequences on the single-stranded template DNA. To perform PCR, the template is mixed with primers, Taq polymerase, and nucleotides. The mixture is heated to 94°C to denature the DNA duplex. Show less
Polymerase chain reaction (PCR) is a technique that quickly makes millions to billions of copies of a DNA sample. It's based on the principle of enzymatic replication of nucleic acids.
PCR is a basic method for DNA analysis and has revolutionized recombinant DNA technology. It's used to construct recombinant molecules by preparing a desired DNA fragment in large quantities. The PCR-amplified DNA is then cloned into a vector of choice. PCR works by using DNA polymerase's ability to synthesize a new DNA strand that's complementary to a template strand. The number of copies doubles after each cycle, and usually 25 to 30 cycles produce enough DNA. The PCR process is automated and can be completed in a few hours. A machine called a thermocycler alters the reaction's temperature every few minutes to allow DNA denaturing and synthesis.
The steps of PCR are: Denaturation: Heat the reaction to separate the DNA strands. Annealing: Cool the reaction so the primers can bind to their complementary sequences on the single-stranded template DNA.
To perform PCR, the template is mixed with primers, Taq polymerase, and nucleotides. The mixture is heated to 94°C to denature the DNA duplex.
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