Transformation – Bio-Rad Ligation and Transformation Module User Manual

Possible ligation products.

Transformation

Once a gene or part of a gene has been amplified using PCR and ligated
into a plasmid, the next step in cloning is transformation, introducing the
plasmid into living bacterial cells so that it can be replicated. Heat shock
transformation and electroporation are the two methods of bacterial
transformation commonly used in the laboratory. Both methods require
competent cells, bacterial cells that can take up DNA. Not all cells are
naturally competent. For example some species, such as

Bacillus subtilis,

can be easily transformed, but for other species, such as

Escherichia coli,

only a small number of cells in a culture may be able to take up DNA.
Competent cells may be prepared in the laboratory or purchased
commercially.

PCR Fragment

PCR Fragment

PCR Fragment

PCR Fragment

PCR Fragment

PCR Fragment

20

No interruption of
lethal gene so
transformed
bacteria will die

Can be minimized
by controlling
molar ratio of
inserts

Product cannot
replicate

Desired product –
insert can be in
either orientation

Self-ligation

of vector

Multiple

inserts

Self-ligation

of inserts

Ligation

of vector

and insert