My question is about polymerase chain reaction. From what I've learned the forward and reverse primers are important for directing the heat tolerant polymerase to amplify a genetic sequence, and then the gene can analyzed on a gel with a negative control not containing the polymerase or with the polymerase to see if you amplified the gene, and if you did it should be the expected size.
So from what I know, to amplify the gene that you want you need to find it on a plasmid, select primers near the gene (but I'm not sure which one should be forward and which one reverse), with the PCR mixture setup with nucleotides, the plasmid, heat tolerant polymerase, and polymerase buffer, the primers, and deionized water.
I've read about polymerase chain reaction in my textbooks, but the authors don't give much time to talk about the PCR primers, so I was wondering what the protocol is for selecting primers.
If I wanted to amplify a catalase gene, for example, with PCR, how should I do it? How should I select the primers, and the plasmid?
Thanks!