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The use of the polymerase chain reaction is an effective way of identifying

and amplifying the gene of interest. Amplifying the gene will produce large
amounts of copies of the DNA sequence of interest that can be subjects to
research and experimental purposes. A successful PCR amplification should
yield an agarose gel with fluorescent DNA under the UV light. PCR is done by
3 steps; Denaturation, Annealing and Extension

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