Chapter 9 DNA Mutations and Genetic Engineering • MHR 3039.3 The Chimera: From Legend to Lab
The chimera is described in Greek mythology as a
fire-breathing monster with the head and shoulders
of a lion, the body of a goat, and a serpent for a tail
(see Figure 9.20). Today, geneticists often use the
term “chimera” to describe genetically engineered
organisms that contain genes from unrelated species.
The name may prove very fitting. The mythical
chimera combined the strengths of many different
animals to produce one creature that was
exceptionally powerful. But this chimera was also
frightening — it breathed fire and could be ferocious.
In the same way, modern genetic chimeras bring
together elements of different genomes in ways that
can produce important social benefits. These new
chimeras and the genetic technologies that create
them also pose some disturbing risks; consequently,
many people consider them to be dangerous.
Figure 9.20The chimera is a mythical beast that combines
parts of a lion, goat, serpent, and dragon.
As you saw in the last section, the first chimeric
organism was created in 1973 when Stanley Cohen
and Herbert Boyer successfully developed a bacterial
plasmid that could express an amphibian gene.
The work initiated by Cohen and Boyer remains
the foundation of much of the genetic engineering
done today.
Recombinant DNA Technology
All mammals produce a growth hormone called
somatotropin. When cows are treated with high
levels of this hormone they grow bigger, develop
larger udders, and produce more milk than they
normally would. In 1990, the gene coding for this
hormone in cattle (bovine somatotropin, or BST)
was successfully cloned and inserted into a
bacterial vector using recombinant DNA technology.
Produced on a commercial scale, the resulting
hormone became the first transgenic, or genetically
engineered, product approved for agricultural
use in North America.
To insert a mammalian gene into a prokaryotic
cell, two basic requirements must be met. First,
researchers must isolate the target mammalian gene
from the genome as a whole. Second, the researchers
must find a way to ensure that the prokaryotic cell
can express the mammalian gene correctly.Creating and Isolating the Target Gene
In the previous section, you learned how
restriction endonucleases can be used to break
DNA into fragments, and how these fragments can
then be inserted into bacterial plasmids for cloning.
Recombinant DNA technology relies on a similar
technique that employs an additional step to
isolate plasmids containing the target gene.
To begin, the eukaryotic chromosome and
selected bacterial plasmids to be used as a cloning
vector are treated with a restriction endonuclease.
When the eukaryotic DNA fragments are combined
with the broken plasmids, some of the plasmids
recombine with eukaryotic DNA. The plasmids
are then returned to the host bacteria by simply
culturing both in solution so that some of the
bacteria will take up the plasmids. However, many
of the plasmids will not contain recombinant DNA;
of those that do, only a small portion will contain
the target mammalian gene. Therefore, the nextEXPECTATIONS
Demonstrate an understanding of genetic manipulation, and of its industrial
and agricultural applications.
Outline contributions of genetic engineers, molecular biologists, and
biochemists that have led to the further development of the field of genetics.
Discuss social and ethical issues associated with genetic engineering.