The first step in the Polymerase Chain Reaction (PCR) process is Denaturation, where the double-stranded DNA template is heated to separate the strands.

DNA denaturation typically occurs in PCR at a temperature range of 90-95°C, allowing the DNA strands to separate for amplification.

The purpose of the annealing step in PCR is to allow primers to bind to the DNA template, facilitating the initiation of DNA replication.

DNA polymerase is crucial for the extension step in PCR as it synthesizes new DNA strands by adding nucleotides to the growing DNA chain.

The typical annealing temperature in PCR is 50-60°C, making the correct answer choice 50-60°C.

The initial denaturation step in PCR is longer in duration compared to subsequent denaturation steps to ensure complete separation of DNA strands for the start of the amplification process.

The main purpose of PCR is to amplify specific DNA sequences, not to cut DNA, join DNA fragments, or visualize DNA on a gel.