A restriction enzyme binds to the same restriction site on both DNA strands then DNA ligase seals phosphodiester linkage

A primer binds to the gene of interest to facilitate the process of inserting the gene into the plasmid

A helicase unwinds the DNA to allow for the gene of interest to be inserted then DNA ligase seals phosphodiester linkages

A DNA polymerase uses the gene of interest as a template to insert the gene into the plasmid

The Taq polymerase is able to unwind the DNA double helix reducing the need of additional enzymes

The Taq polymerase binds to the DNA without a required primer facilitating the process of PCR.

The process of PCR requires prokaryotic polymerase as it is less complex.

The process of PCR requires extreme high temperatures that would denature other polymerases.

Small fragments are found near the well since it is negatively charged

Large fragments are found near the well while small fragments are found at the other end.

Small fragments are found near the well while small fragments are found at the other end.

Large fragments are found near the well since it is positively charged

This is a location where there is a secondary well in the gel

There are a large amount of fragments the same size

The DNA at that band absorbed more dye since it is more positively charged

This is an error in the gel electrophoresis caused by a clogged pore in the gel

10

16

64

32

Polymerase requires an open 3' end

Polymerase requires RNA for signaling

Polymerase requires an RNA template

Polymerase requires an open 5' end

To compare between the bacteria with and without the plasmid

To determine whether LB is required for the bacterial growth

To ensure the bacteria is viable after experimental set-up

To test whether temperature has an effect on growth