Polymerase Chain Reaction (PCR)
Polymerase Chain Reaction (PCR)
Polymerase Chain Reaction (PCR)
Polymerase chain reaction (PCR) is a technique that allows the generation of large
amounts of a single DNA sequence from a mixture of sequences; the fragment
generated can be designed to contain specific starting and ending positions based on
the needs of the experiment.
The two strands of the DNA template are separated by heating (usually to 94°C).
The temperature is then decreased to allow the primers to bind to the template
DNA. Once the primers have bound, the polymerase is allowed to synthesize new
DNA strands (the polymerase most commonly used has a temperature optimum of
72°C.)
Good primers contain approximately 50% G+C and 50% A+T. This reduces problems
in inducing template strand separation caused by the high affinity of G for C, and
reduces non-specific priming common with high AT content.
The primer should be long enough to have a reasonable melting temperature (i.e. a
melting temperature of 55-70°C). Melting temperature depends on a number of
variables. In most cases, an approximation [∑(4°C for each G or C) + (2°C for each A
or T)] will yield a value close enough to design the PCR experiment.
PCR also allows the generation of mutations at the ends of the fragment, because
the primer does not need to be an exact match to the template DNA (it needs to be a
sufficiently good match to allow primer binding, but it does not need to be a perfect
match). In most cases, the introduction of mismatches at the 5´ end of the primer
has little effect. However, mismatches at the 3´ end of the primer may prevent
synthesis of the new strand.
The mutations inserted by PCR are frequently used to generate restriction sites to
simplify cloning of the PCR fragment. Although PCR can also be used to generate
mutations within coding sequences, this is somewhat more complex, because the
PCR primers only affect the sequence at the ends of the PCR fragments. However,
modified forms of PCR are quite useful for site-directed mutagenesis experiments.
In order to amplify a sequence, we need a source of the actual coding sequence, and
we need to know the sequence of the ends to allow the design of primers. If the PCR
is intended to generate a coding sequence, genomic DNA from prokaryotes can be
used as a template. For higher eukaryotes, however, cDNA must be used as a
template to allow contiguous coding sequences to be amplified.
PCR requires the use of a DNA polymerase to make the copies of the DNA sequence
used as a template. As noted in the figure above, the PCR method involves heating
the sample to ~94°C to separate the chains of the double-stranded DNA. In
addition, while the oligonucleotide binding and polymerization reactions can occur
at a range of temperatures, oligonucleotide binding is much more specific (i.e. it is
more likely that the oligonucleotide will bind the correct sequence) at higher
temperatures. To prevent problems with low temperature incubations and problems
due to denaturation of the polymerase, most PCR experiments employ thermostable
DNA polymerases. The DNA polymerase most commonly used for PCR is derived
from the bacterium Thermus aquaticus. T. aquaticus prefers to live at a
temperature of about 70°C, and therefore its proteins (including its DNA
polymerases) are stable at elevated temperatures.
The Taq polymerase has a primer extension rate of 60-100 bases/second under
optimum conditions; thus it may be advantageous to use short (1-10 second)
extension times, particularly for short products (i.e. below 500 bp) to decrease
formation of non-specific products. However, for longer fragments (greater than
1000 bases), optimum primer extension rates are rarely achieved, and longer
extension times should be used.
Although the Taq polymerase is a popular enzyme due to its ability to catalyze
primer extension under a wide variety of conditions, it has some drawbacks. Its
worst drawback is its relative lack of fidelity; it has a significant error rate (1 in 103
to 1 in 10 5 depending on the sequence), and lacks proofreading functions. As a
result, many experiments employ thermostable DNA polymerases that have lower
probabilities of misincorporation. The use of other polymerases may require minor
modifications to the PCR procedure described below.
The temperature profile shown below is a typical one that works for many different
primers and templates:
Run the PCR program as shown above (with appropriate modifications if necessary
for the specific polymerase, primers, and template being used in the experiment).