Recombinant DNA and Biotechnology presentation

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Title: Recombinant DNA and Biotechnology

1
Recombinant DNA and Biotechnology
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16 Recombinant DNA and Biotechnology

16.1 How Are Large DNA Molecules Analyzed?
16.2 What Is Recombinant DNA?
16.3 How Are New Genes Inserted into Cells?
16.4 What Are the Sources of DNA Used in Cloning?
16.5 What Other Tools Are Used to Manipulate DNA?
16.6 What Is Biotechnology?

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16.1 How Are Large DNA Molecules Analyzed?

Naturally occurring enzymes that cleave and
repair DNA are used in the laboratory to
manipulate and recombine DNA.

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16.1 How Are Large DNA Molecules Analyzed?

Restriction enzymes (restriction endonucleases)
cut double-stranded DNA into smaller pieces.
Bacteria use these as defense against DNA from
bacteriophage.
DNA is cut between the 3' hydroxyl group of one
nucleotide and the 5' phosphate group of the
nextrestriction digestion.

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Figure 16.1 Bacteria Fight Invading Viruses with
Restriction Enzymes
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16.1 How Are Large DNA Molecules Analyzed?

There are many restriction enzymes that cut DNA
at specific base sequencesthe recognition
sequence, or restriction site.

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16.1 How Are Large DNA Molecules Analyzed?

Restriction enzymes do not cut bacterias own DNA
because the recognition sequences are modified.
Methylases add methyl groups after replication
makes sequence unrecognizable by restriction
enzyme.

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16.1 How Are Large DNA Molecules Analyzed?

Bacterial restriction enzymes can be isolated
from cells.
DNA from any organism will be cut wherever the
recognition site occurs.
EcoRI (from E. coli) cuts DNA at this sequence

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16.1 How Are Large DNA Molecules Analyzed?

The sequence is palindromicit reads the same in
both directions from the 5' end.
EcoRI occurs about once every four genes in
prokaryotes. DNA can be chopped into small pieces
containing a few genes.

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16.1 How Are Large DNA Molecules Analyzed?

The EcoRI sequence does not occur anywhere in the
genome of the phage T7. Thus it can survive in
its host, E. coli.

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16.1 How Are Large DNA Molecules Analyzed?

After DNA is cut, fragments of different sizes
can be separated by gel electrophoresis.
Mixture of fragments is place on a well in a
porous gel. An electric field is applied across
the gel. Negatively charged DNA fragments move
towards positive end.
Smaller fragments move faster than larger ones.

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Figure 16.2 Separating Fragments of DNA by Gel
Electrophoresis (Part 1)
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Figure 16.2 Separating Fragments of DNA by Gel
Electrophoresis (Part 2)
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Figure 16.2 Separating Fragments of DNA by Gel
Electrophoresis (Part 3)
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16.1 How Are Large DNA Molecules Analyzed?

Electrophoresis provides information on
Size of fragments. Fragments of known size
provide comparison.
Presence of specific sequences. These can be
determined using probes.
DNA is denatured while in the gel, then
transferred to a nylon filter to make a blot.

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Figure 16.3 Analyzing DNA Fragments by Southern
Blotting
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16.1 How Are Large DNA Molecules Analyzed?

DNA fingerprinting uses restriction analysis and
electrophoresis to identify individuals.
Works best with genes that are polymorphichave
multiple alleles.

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16.1 How Are Large DNA Molecules Analyzed?

Two types of polymorphisms
Single nucleotide polymorphisms (SNPs) inherited
variation involving a single base
Short tandem repeats (STRs) moderately
repetitive sequences side by side

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16.1 How Are Large DNA Molecules Analyzed?

STRs are recognizable if they lie between two
restriction sites.
Several different STRs can be used to determine
the unique pattern for an individual.

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Figure 16.4 DNA Fingerprinting with Short Tandem
Repeats
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16.1 How Are Large DNA Molecules Analyzed?

DNA fingerprinting requires at least 1 µg of DNA
(amount in about 100,000 human cells).
This is not always available, so amplification by
PCR is used.

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16.1 How Are Large DNA Molecules Analyzed?

DNA fingerprinting is used in forensics.
It is more often used to prove innocence than
guilt.
Only a small portion of the genome is examined
there is the possibility that two people could
have the same sequence.

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16.1 How Are Large DNA Molecules Analyzed?

DNA fingerprinting has been used to analyze
historical events.
The skeletal remains of Russian Tsar Nicholas II
and his family were identified from DNA in bone
fragments.
DNA also showed relationships with living
descendents of the Tsar.

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Figure 16.5 DNA Fingerprinting the Russian Royal
Family
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16.1 How Are Large DNA Molecules Analyzed?

DNA technology can be used to identify species.
A proposal to identify all known species and look
for unknowns has been put forth by the Consortium
for the Barcode of Life (CBOL)
Use a short sequence from a gene (cytochrome
oxidase) as a barcode for each species.

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Figure 16.6 A DNA Barcode
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16.1 How Are Large DNA Molecules Analyzed?

The barcode project could contribute to
Evolution research
Species diversity issues
Identification of new species
Identification of undesirable microbes or
bioterrorism agents

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16.2 What Is Recombinant DNA?

DNA fragments can be rejoined by DNA ligase.
Any two DNA sequences can be spliced.
First done in 1973 with two E. coli plasmids
Recombinant DNA was born

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Figure 16.7 Making Recombinant DNA (Part 1)
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Figure 16.7 Making Recombinant DNA (Part 2)
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16.2 What Is Recombinant DNA?

Some restriction enzymes cut both DNA strands
exactly opposite each other.
Others (such as EcoRI) make a staggered cut.
Results in single-stranded tails at the ends of
fragments.
Tails are called sticky endscan bind by base
pairing to other sticky ends.

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Figure 16.8 Cutting and Splicing DNA
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16.2 What Is Recombinant DNA?

Sticky ends of fragments that were cut by the
same restriction enzyme are all the samethus
fragments from different species can be joined.
When temperature is lowered, the fragments
annealjoin by hydrogen bonding. Must be
permanently spliced by DNA ligase.

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16.3 How Are New Genes Inserted into Cells?

Recombinant DNA technology can be used to clone,
or make exact copies of genes.
The gene can be used to make a proteinbut it
must first be inserted, or transfected, into host
cells.
The altered host cell is called transgenic.

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16.3 How Are New Genes Inserted into Cells?

To determine which of the host cells contain the
new sequence, the recombinant DNA is often tagged
with reporter genes.
Reporter genes have easily observed phenotypes or
genetic markers.

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16.3 How Are New Genes Inserted into Cells?

The first host cells used were bacteria,
especially E. coli.
Yeasts (Saccharomyces) are commonly used as
eukaryotic hosts.
Plant cells are also usedthey have totipotency,
the ability of any differentiated cell to develop
into a new plant.

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16.3 How Are New Genes Inserted into Cells?

The new DNA must also replicate as the host cell
divides. It must become a segment with an origin
of replicationa replicon or replication unit.

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16.3 How Are New Genes Inserted into Cells?

New DNA can become part of a replicon in two
ways
Inserted near an origin of replication in host
chromosome.
It can be part of a carrier sequence or vector
that already has an origin of replication.

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16.3 How Are New Genes Inserted into Cells?

A vector should have four characteristics
Ability to replicate independently of the host
cell
A recognition sequence for a restriction enzyme
A reporter gene
Small size in comparison with hosts chromosomes

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16.3 How Are New Genes Inserted into Cells?

Plasmids have all these characteristics.
Plasmids are small, many have only one
restriction site.
Genes for antibiotic resistance can be used as
reporter genes.
And they have an origin of replication and can
replicate independently.

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Figure 16.9 Vectors for Carrying DNA into Cells
(A)
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16.3 How Are New Genes Inserted into Cells?

Plasmids can be used for genes of 10,000 bp or
less. Most eukaryote genes are larger than this.
Viruses can be used as vectorse.g.,
bacteriophage. The genes that cause host cell to
lyse can be cut out and replaced with other DNA.

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16.3 How Are New Genes Inserted into Cells?

Bacterial plasmids dont work for yeasts because
the origins of replication use different
sequences.
A yeast artificial chromosome (YAC) has been
created contains yeast origin of replication,
plus yeast centromere and telomere sequences.
Also contains artificial restriction sites and
reporter genes

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Figure 16.9 Vectors for Carrying DNA into Cells
(B)
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16.3 How Are New Genes Inserted into Cells?

A plasmid from the soil bacterium Agrobacterium
tumefaciens is used as a vector for plant cells.
Plasmid Ti (tumor inducing) causes crown gall.
Plasmid has a region called T DNA, which inserts
copies of itself into chromosomes of infected
plants.

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16.3 How Are New Genes Inserted into Cells?

T DNA has several restriction sites, where new
DNA can be inserted.
With altered T DNA, plasmid no longer causes
tumors, but can still insert itself into host
chromosomes.

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Figure 16.9 Vectors for Carrying DNA into Cells
(C)
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16.3 How Are New Genes Inserted into Cells?

Usually only a small proportion of host cells
take up the vector, and they may not have the
appropriate sequence.
Host cells with the desired sequence must be
identifiable.

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16.3 How Are New Genes Inserted into Cells?

One method
E. coli is host pBR322 plasmid is the vector.
Plasmid has genes for resistance to ampicillin
and tetracycline.
Plasmid has only one restriction site for enzyme
BamHI, within the gene for tetracycline
resistance.

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16.3 How Are New Genes Inserted into Cells?

If new DNA is inserted at that restriction site,
it inactivates the gene for tetracycline
resistance.
Plasmid then has gene for ampicillin resistance,
but not for tetracycline. This can be used to
select for host cells with new DNA.

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Figure 16.10 Marking Recombinant DNA by
Inactivating a Gene
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16.3 How Are New Genes Inserted into Cells?

Other reporter genes
Artificial vectors with restriction sites within
the lac operon. If new DNA is inserted there,
vector no longer carries its original function
into the host cell.
Green fluorescent protein, which normally occurs
in the jellyfish Aequopora victoriana.

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16.4 What Are the Sources of DNA Used in Cloning?

DNA fragments used for cloning come from three
sources
Gene libraries
Reverse transcription from mRNA
Artificial synthesis or mutation of DNA

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16.4 What Are the Sources of DNA Used in Cloning?

Human chromosomes contain an average of 80
million bp each.
The DNA is cut into fragments by restriction
enzymes, the fragments are stored as a gene
library.
Each fragment is inserted into a vector, which
goes into a host cell.

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Figure 16.11 Constructing a Gene Library
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16.4 What Are the Sources of DNA Used in Cloning?

If phage ? is used as a vector, about 50,000
volumes are required to store the library.
One petri plate can hold 80,000 phage colonies,
or plaques.
DNA in the plaques is screened using specific
probes.

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16.4 What Are the Sources of DNA Used in Cloning?

Smaller DNA libraries can be made from
complementary DNA (cDNA).
mRNA is extracted from a tissue and the poly A
tails allowed to hybridize with oligo dTa string
of thymine bases.
Oligo dT serves as a primer for reverse
transcriptase to synthesize a complementary DNA
strand.

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Figure 16.12 Synthesizing Complementary DNA
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16.4 What Are the Sources of DNA Used in Cloning?

cDNA libraries are made from particular tissues
at particular times and represent a snapshot of
the mRNA present at that time.
Used to compare gene expression in different
tissues at different stages of development.
cDNA is also used to clone eukaryotic genes.

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16.4 What Are the Sources of DNA Used in Cloning?

DNA can be synthesized if the amino acid sequence
of a protein is known.
This process is now automated, and labs can make
custom DNA sequences overnight.
Flanking sequences for transcription initiation,
termination, and regulation and start and stop
codons are also added.

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16.4 What Are the Sources of DNA Used in Cloning?

Synthetic DNA can be used to create specific
mutations in order to study the consequences of
the mutation.
Called mutagenesis techniques.
These techniques have revealed many
cause-and-effect relationships, e.g., determining
signal sequences.

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16.5 What Other Tools Are Used to Manipulate DNA?

Three additional ways of manipulating DNA
Knockout experiments
Gene silencing
DNA chips

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16.5 What Other Tools Are Used to Manipulate DNA?

A knockout experiment involves homologous
replication to replace a gene with an inactive
gene, and determine results in a living organism.
The normal allele of a gene is inserted into a
plasmid restriction enzymes are used to insert a
reporter gene in the middle of the normal gene.

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16.5 What Other Tools Are Used to Manipulate DNA?

The gene is thus inactivated.
The plasmid is then transfected into a stem cell
of a mouse embryo.
Stem cell undifferentiated cell that divides and
differentiates to form different tissues.

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16.5 What Other Tools Are Used to Manipulate DNA?

Much of the normal gene is still present, so
homologous recognition takes place between the
normal allele and the inactive allele on the
plasmid.
Recombination can occur, and inactive allele is
swapped for the normal allele.
The transfected stem cell is then inserted into
an early mouse embryo.

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Figure 16.13 Making a Knockout Mouse (Part 1)
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Figure 16.13 Making a Knockout Mouse (Part 2)
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16.5 What Other Tools Are Used to Manipulate DNA?

Translation of mRNA can be blocked by
complementary micro RNAsantisense RNA.
Antisense RNA can be synthesized, and added to
cells to prevent translationthe effects of the
missing protein can then be determined.

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16.5 What Other Tools Are Used to Manipulate DNA?

Interference RNA (RNAi) is a rare natural
mechanism that blocks translation.
Short, double stranded RNA is unwound and binds
to complementary mRNA by a protein complex, which
also catalyzes the breakdown of the mRNA.
Small interfering RNA (siRNA) can be synthesized
in the laboratory.

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Figure 16.14 Using Antisense RNA and RNAi to
Block Translation of mRNA
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16.5 What Other Tools Are Used to Manipulate DNA?

Antisense RNA and RNAi are also used to study
cause-and-effect relationships.
Example Antisense RNA is used to block
translation of proteins essential for growth of
cancer cellsthe cells revert to normal phenotype.

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16.5 What Other Tools Are Used to Manipulate DNA?

DNA chip technology provides a large array of
sequences for hybridization experiments.
A series of DNA sequences are attached to a glass
slide in a precise order.
The slide has microscopic wells which each
contain thousands of copies of sequences up to 20
nucleotides long.

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Figure 16.15 DNA on a Chip
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16.5 What Other Tools Are Used to Manipulate DNA?

To analyze mRNA, it is incubated with reverse
transcriptase to make cDNA.
The cDNA is amplified using PCR.
Technique is called RT-PCR.
Amplified cDNA is tagged with a fluorescent dye
and used as a probe of the DNA on the chip.

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16.5 What Other Tools Are Used to Manipulate DNA?

DNA chip technology has been developed to
identify gene expression patterns in women with a
propensity for breast cancer tumors to recura
gene expression signature.

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16.6 What Is Biotechnology?

Biotechnology is the use of living cells to
produce materials useful to people.
Examples use of yeasts to brew beer and wine,
use of bacteria to produce cheese, yogurt, etc.
Use of microbes to produce antibiotics such as
penicillin, alcohol, and other products.

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16.6 What Is Biotechnology?

Gene cloning is now used to produce proteins in
large amounts.
Almost any gene can be inserted into bacteria or
yeasts, and the resulting cells induced to make
large quantities of the product.
Requires specialized vectors.

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16.6 What Is Biotechnology?

Expression vectors are synthesized that include
sequences needed for expression of the transgene
in the host cell.

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Figure 16.16 An Expression Vector Allows a
Transgene to Be Expressed in a Host Cell
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16.6 What Is Biotechnology?

Expression vectors can be modified by
Inducible promoters enhancers can also be added
so that protein synthesis takes place at high
rates.
Tissue-specific promoters
Signal sequencese.g., a signal to secrete the
product to the extracellular medium.

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Table 16.1
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16.6 What Is Biotechnology?

Example of a medical application
After wounds heal, blood clots are dissolved by
plasmin. Plasmin is stored as an inactive form
called plasminogen.
Conversion of plasminogen is activated by tissue
plasminogen activator (TPA).
TPA can be used to treat strokes and heart
attacks, but large quantities are neededcan be
made using recombinant DNA technology.

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Figure 16.17 Tissue Plasminogen Activator From
Protein to Gene to Drug (Part 1)
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Figure 16.17 Tissue Plasminogen Activator From
Protein to Gene to Drug (Part 2)
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16.6 What Is Biotechnology?

Pharming production of medically useful proteins
in milk.
Transgenes for a protein are inserted into the
egg of a domestic animal, next to the promoter
for lactoglobulina protein in milk. The
transgenic animal then produces large quantities
of the protein in its milk.

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Figure 16.18 Pharming
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16.6 What Is Biotechnology?

Through cultivation and selective breeding,
humans have been altering the traits of plants
and animals for thousands of years.
Recombinant DNA technology has several
advantages
Specific genes can be targeted.
Any gene can be introduced into any other
organism.
New organisms are generated quickly.

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Table 16.2
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16.6 What Is Biotechnology?

Crop plants have been modified to produce their
own insecticides
The bacterium Bacillus thuringiensis produces a
protein that kills insect larvae.
Dried preparation of B. thuringiensis are sold as
a safe alternative to synthetic insecticides. The
toxin is easily biodegradable.

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16.6 What Is Biotechnology?

Genes for the toxin have been isolated, cloned,
and modified, and inserted into plant cells using
the Ti plasmid vector.
Transgenic corn, cotton, soybeans, tomatoes, and
other crops are being grown. Pesticide use is
reduced.

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16.6 What Is Biotechnology?

Some transgenic crops are resistant to
herbicides.
Glyphosate (Roundup) is widely used to kill
weeds.
Expression vectors have been used to make plants
that synthesize so much of the target enzyme of
glyphosate that they are unaffected by the
herbicide.

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16.6 What Is Biotechnology?

The gene has been inserted into corn, soybeans,
and cotton.
About half of U.S. crops of these plants contain
this gene.

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16.6 What Is Biotechnology?

Crops with improved nutritional characteristics
Rice does not have ß-carotene, but does have a
precursor molecule.
Genes for enzymes that synthesize ß-carotene from
the precursor are taken from daffodils and
inserted into rice by the Ti plasmid.

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16.6 What Is Biotechnology?

The transgenic rice is yellow, and can supply
ß-carotene to improve the diets of many people.
ß-carotene is converted to vitamin A in the body.

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Figure 16.19 Transgenic Rice Is Rich in ß-Carotene
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16.6 What Is Biotechnology?

Recombinant DNA is also used to adapt a crop
plant to an environment.
Example plants that are salt-tolerant
Genes from a protein that moves sodium ions into
the central vacuole were isolated from
Arabidopsis and inserted into tomato plants.

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Figure 16.20 Salt-Tolerant Tomato Plants
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16.6 What Is Biotechnology?

Concerns over biotechnology
Genetic manipulation is an unnatural interference
in nature.
Genetically altered foods are unsafe to eat.
Genetically altered crop plants are dangerous to
the environment.

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16.6 What Is Biotechnology?

Advocates of biotechnology point out that all
crop plants have been manipulated by humans.
Advocates say that since only single genes for
plant function are inserted into crop plants,
they are still safe for human consumption.
Genes that affect human nutrition may raise more
concerns.

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16.6 What Is Biotechnology?

Concern over environmental effects centers on
escape of transgenes into wild populations
For example, if the gene for herbicide resistance
made its way into the weed plants.
Beneficial insects can also be killed from eating
plants with B. thuringiensis genes.

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