Inverse polymerase chain reaction is a variant of the polymerase chain reaction that is used to amplifyDNA with only one known sequence. One limitation of conventional PCR is that it requires primers complementary to both termini of the target DNA, but this method allows PCR to be carried out even if only one sequence is available from which primers may be designed. Inverse PCR is especially useful for the determination of insertlocations. For example, various retroviruses and transposons randomly integrate into genomic DNA. To identify the sites where they have entered, the known, "internal" viral or transposonsequences can be used to design primers that will amplify a small portion of the flanking, "external" genomic DNA. The amplified product can then be sequenced and compared with DNA databases to locate the sequence which has been disrupted. The inverse PCR method involves a series of restriction digests and ligation, resulting in a looped fragment that can be primed for PCR from a single section of known sequence. Then, like other polymerase chainreaction processes, the DNA is amplified by the temperature-sensitive DNA polymerase:
A target region with an internal section of known sequence and unknown flanking regions is identified
Genomic DNA is digested into fragments of a few kilobases by a usually low-moderate frequency cutting restriction enzyme.
Under low DNA concentrations, self-ligation is induced to give a circular DNA product.
PCR is carried out as usual, with primers complementary to sections of the known internal sequence.*
Finally the sequence is compared with the sequence available in the data base. It is used in case of chromosome crawling.
Note: although the figure suggests that the circularized ligation product is digested prior to PCR, this is not the case. PCR does not require linear products and the use of another restriction enzyme to cut the known sequence could also cut within the unknown region, resulting in a failed PCR.