The target sequence in PCR refers to the specific segment of DNA that is being amplified during the process. This is the DNA that the primers will bind to and replicate.

Primers are short sequences of nucleotides that provide starting points for DNA synthesis during PCR. They bind to the target DNA and allow DNA polymerase to extend the new DNA strands, making them essential for amplification.

During PCR, deoxynucleoside triphosphates (dNTPs) are added as they are the building blocks for DNA synthesis. They provide the necessary nucleotides to create new DNA strands, unlike RNA nucleotides or monophosphates.

The thermal cycler is essential in PCR as it precisely controls the temperature cycles required for denaturation, annealing, and extension, enabling the amplification of DNA sequences.

Taq polymerase synthesizes a complementary DNA strand at 72 degrees Celsius, which is the optimal temperature for its activity during the elongation phase of PCR. Other temperatures are not suitable for this process.

At 95°C, the heat causes the hydrogen bonds between DNA bases to break, leading to denaturation. This process separates the two strands of DNA, disrupting its stability and function.

Primers typically attach to DNA strands at a temperature range of 50-65 degrees Celsius, which allows for optimal binding without denaturation, making this the correct choice.