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Transcript
Chapter 20
Biotechnology
PowerPoint® Lecture Presentations for
Biology
Eighth Edition
Neil Campbell and Jane Reece
Lectures by Chris Romero, updated by Erin Barley with contributions from Joan Sharp
Copyright © 2008 Pearson Education, Inc., publishing as Pearson Benjamin Cummings
Overview: The DNA Toolbox
• Sequencing of the human genome was
completed by 2007
• DNA sequencing has depended on advances
in technology, starting with making
recombinant DNA
• In recombinant DNA, nucleotide sequences
from two different sources, often two species,
are combined in vitro into the same DNA
molecule
Copyright © 2008 Pearson Education Inc., publishing as Pearson Benjamin Cummings
DNA Cloning and Its Applications: A Preview
• Most methods for cloning pieces of DNA in the
laboratory share general features, such as the
use of bacteria and their plasmids
• Plasmids are small circular DNA molecules
that replicate separately from the bacterial
chromosome
• Cloned genes are useful for making copies of a
particular gene and producing a protein product
Copyright © 2008 Pearson Education Inc., publishing as Pearson Benjamin Cummings
• Gene cloning involves using bacteria to make
multiple copies of a gene
• Foreign DNA is inserted into a plasmid, and the
recombinant plasmid is inserted into a bacterial
cell
• Reproduction in the bacterial cell results in
cloning of the plasmid including the foreign
DNA
• This results in the production of multiple copies
of a single gene
Copyright © 2008 Pearson Education Inc., publishing as Pearson Benjamin Cummings
Fig. 20-2
Cell containing gene
of interest
Bacterium
1 Gene inserted into
plasmid
Bacterial
Plasmid
chromosome
Recombinant
DNA (plasmid)
Gene of
interest
DNA of
chromosome
2 Plasmid put into
bacterial cell
Recombinant
bacterium
3 Host cell grown in culture
to form a clone of cells
containing the “cloned”
gene of interest
Gene of
Interest
Protein expressed
by gene of interest
Copies of gene
Basic
Protein harvested
4 Basic research and
various applications
research
on gene
Gene for pest
resistance inserted
into plants
Gene used to alter
bacteria for cleaning
up toxic waste
Protein dissolves
blood clots in heart
attack therapy
Basic
research
on protein
Human growth hormone treats stunted
growth
Using Restriction Enzymes to Make Recombinant
DNA
• Bacterial restriction enzymes cut DNA
molecules at specific DNA sequences called
restriction sites
• A restriction enzyme usually makes many cuts,
yielding restriction fragments
• The most useful restriction enzymes cut DNA in
a staggered way, producing fragments with
“sticky ends” that bond with complementary
sticky ends of other fragments
Animation: Restriction Enzymes
Copyright © 2008 Pearson Education Inc., publishing as Pearson Benjamin Cummings
• DNA ligase is an enzyme that seals the bonds
between restriction fragments
Copyright © 2008 Pearson Education Inc., publishing as Pearson Benjamin Cummings
Fig. 20-3-3
Restriction site
DNA
1
5
3
3
5
Restriction enzyme
cuts sugar-phosphate
backbones.
Sticky end
2
DNA fragment added
from another molecule
cut by same enzyme.
Base pairing occurs.
One possible combination
3
DNA ligase
seals strands.
Recombinant DNA molecule
• A probe can be synthesized that is
complementary to the gene of interest
• For example, if the desired gene is
5 … G G C T AA C TT A G C … 3
– Then we would synthesize this probe
3 C C G A TT G A A T C G 5
Copyright © 2008 Pearson Education Inc., publishing as Pearson Benjamin Cummings
• The DNA probe can be used to screen a large
number of clones simultaneously for the gene
of interest
• Once identified, the clone carrying the gene of
interest can be cultured
Copyright © 2008 Pearson Education Inc., publishing as Pearson Benjamin Cummings
Fig. 20-7
TECHNIQUE
Radioactively
labeled probe
molecules
Multiwell plates
holding library
clones
Probe
DNA
Gene of
interest
Single-stranded
DNA from cell
Film
•
Nylon membrane
Nylon
Location of
membrane
DNA with the
complementary
sequence
Expressing Cloned Eukaryotic Genes
• After a gene has been cloned, its protein
product can be produced in larger amounts for
research
• Cloned genes can be expressed as protein in
either bacterial or eukaryotic cells
Copyright © 2008 Pearson Education Inc., publishing as Pearson Benjamin Cummings
Amplifying DNA in Vitro: The Polymerase Chain
Reaction (PCR)
• The polymerase chain reaction, PCR, can
produce many copies of a specific target
segment of DNA
• A three-step cycle—heating, cooling, and
replication—brings about a chain reaction that
produces an exponentially growing population
of identical DNA molecules
Copyright © 2008 Pearson Education Inc., publishing as Pearson Benjamin Cummings
Fig. 20-8
5
TECHNIQUE
3
Target
sequence
3
Genomic DNA
1 Denaturation
5
5
3
3
5
2 Annealing
Cycle 1
yields
2
molecules
Primers
3 Extension
New
nucleotides
Cycle 2
yields
4
molecules
Cycle 3
yields 8
molecules;
2 molecules
(in white
boxes)
match target
sequence
Gel Electrophoresis and Southern Blotting
• One indirect method of rapidly analyzing and
comparing genomes is gel electrophoresis
• This technique uses a gel as a molecular sieve
to separate nucleic acids or proteins by size
• A current is applied that causes charged
molecules to move through the gel
• Molecules are sorted into “bands” by their size
Video: Biotechnology Lab
Copyright © 2008 Pearson Education Inc., publishing as Pearson Benjamin Cummings
Fig. 20-9
TECHNIQUE
Mixture of
DNA molecules of
different
sizes
Power
source
– Cathode
Anode +
Gel
1
Power
source
–
+
Longer
molecules
2
RESULTS
Shorter
molecules
• In restriction fragment analysis, DNA fragments
produced by restriction enzyme digestion of a
DNA molecule are sorted by gel
electrophoresis
• Restriction fragment analysis is useful for
comparing two different DNA molecules, such
as two alleles for a gene
• The procedure is also used to prepare pure
samples of individual fragments
Copyright © 2008 Pearson Education Inc., publishing as Pearson Benjamin Cummings
Fig. 20-10
Normal -globin allele
175 bp
DdeI
Sickle-cell
allele
Large fragment
201 bp
DdeI
Normal
allele
DdeI
DdeI
Large
fragment
Sickle-cell mutant -globin allele
376 bp
DdeI
201 bp
175 bp
Large fragment
376 bp
DdeI
DdeI
(a) DdeI restriction sites in normal and
sickle-cell alleles of -globin gene
(b) Electrophoresis of restriction fragments
from normal and sickle-cell alleles
• Reverse transcriptase-polymerase chain
reaction (RT-PCR) is quicker and more
sensitive
• Reverse transcriptase is added to mRNA to
make cDNA, which serves as a template for
PCR amplification of the gene of interest
• The products are run on a gel and the mRNA
of interest identified
Copyright © 2008 Pearson Education Inc., publishing as Pearson Benjamin Cummings
Fig. 20-13
TECHNIQUE
1 cDNA synthesis
mRNAs
cDNAs
2 PCR amplification
Primers
-globin
gene
3 Gel electrophoresis
RESULTS
Embryonic stages
1 2 3 4 5
6
• In situ hybridization uses fluorescent dyes
attached to probes to identify the location of
specific mRNAs in place in the intact organism
Copyright © 2008 Pearson Education Inc., publishing as Pearson Benjamin Cummings
Fig. 20-14
50 µm
Fig. 20-18
TECHNIQUE
Mammary
cell donor
Egg cell
donor
2
1
Egg cell
from ovary
3 Cells fused
Cultured
mammary cells 3
4 Grown in
Nucleus
removed
Nucleus from
mammary cell
culture
Early embryo
5 Implanted
in uterus
of a third
sheep
Surrogate
mother
6 Embryonic
development
RESULTS
Lamb (“Dolly”)
genetically identical to
mammary cell donor
Stem Cells of Animals
• A stem cell is a relatively unspecialized cell
that can reproduce itself indefinitely and
differentiate into specialized cells of one or
more types
• Stem cells isolated from early embryos at the
blastocyst stage are called embryonic stem
cells; these are able to differentiate into all cell
types
• The adult body also has stem cells, which
replace nonreproducing specialized cells
Copyright © 2008 Pearson Education Inc., publishing as Pearson Benjamin Cummings
Fig. 20-20
Embryonic stem cells
Adult stem cells
Early human embryo
at blastocyst stage
(mammalian equivalent of blastula)
From bone marrow
in this example
Cells generating
all embryonic
cell types
Cells generating
some cell types
Cultured
stem cells
Different
culture
conditions
Different
types of
differentiated
cells
Liver cells
Nerve cells
Blood cells
Fig. 20-24
(a) This photo shows Earl
Washington just before
his release in 2001,
after 17 years in prison.
Source of
sample
STR
marker 1
STR
marker 2
STR
marker 3
Semen on victim
17, 19
13, 16
12, 12
Earl Washington
16, 18
14, 15
11, 12
Kenneth Tinsley
17, 19
13, 16
12, 12
(b) These and other STR data exonerated Washington and
led Tinsley to plead guilty to the murder.
Environmental Cleanup
• Genetic engineering can be used to modify the
metabolism of microorganisms
• Some modified microorganisms can be used to
extract minerals from the environment or
degrade potentially toxic waste materials
• Biofuels make use of crops such as corn,
soybeans, and cassava to replace fossil fuels
Copyright © 2008 Pearson Education Inc., publishing as Pearson Benjamin Cummings
• Most public concern about possible hazards
centers on genetically modified (GM)
organisms used as food
• Some are concerned about the creation of
“super weeds” from the transfer of genes from
GM crops to their wild relatives
Copyright © 2008 Pearson Education Inc., publishing as Pearson Benjamin Cummings
Fig. 20-UN3
Vector
DNA fragments from genomic DNA
or cDNA or copy of DNA obtained
by PCR
Cut by same restriction enzyme,
mixed, and ligated
Recombinant DNA plasmids
Fig. 20-UN4
5
3
TCCATGAATTCTAAAGCGCTTATGAATTCACGGC
AGGTACTTAAGATTTCGCGAATACTTAAGTGCCG
Aardvark DNA
A
Plasmid
3
5
Fig. 20-UN7