487182
Description
Mind Map by Lydia Buckmaster, updated more than 1 year ago
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Created by Lydia Buckmaster
almost 11 years ago
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Introduction to DNA 2
- Screening
- Immunological
Assay
- Cells lysed and
antigens bound
to a matrix
- Specific antibodies
for the recombinant
antigens are then
used to identify
transformed cells
- Primary
Antibodies
- These are added
first and bind to the
recombinant proteins
(antigens) from the
transformed cells
- These are added
first and bind to the
recombinant proteins
(antigens) from the
transformed cells
- Secondary
Antibodies
- Bind to the
already-bound
primary
antibodies
- Unbound
antibodies
are washed
away before
detection
- Unbound
antibodies
are washed
away before
detection
- Labelled
to allow
detection
- Fluorescently
labelled, or to induce
a colour change in
solution on binding
- Fluorescently
labelled, or to induce
a colour change in
solution on binding
- Bind to the
already-bound
primary
antibodies
- Primary
Antibodies
- Specific antibodies
for the recombinant
antigens are then
used to identify
transformed cells
- Cells lysed and
antigens bound
to a matrix
- Functional
Complementation
- To identify the
sequence of interest in
the library, cells unable
to produce the resulting
desired product or
function are cloned
- DNA fragments from
the library are taken
up into these cells,
transforming them
- The desired DNA
sequence allows the
cell to produce the
desired product, while
the others still can't
- Selecting for
the restored
function
- Selecting for
the restored
function
- The desired DNA
sequence allows the
cell to produce the
desired product, while
the others still can't
- DNA fragments from
the library are taken
up into these cells,
transforming them
- Example
- Mutant cells can be
used that do not grow
in a certain medium
- Recombinant DNA could
confer a survival trait,
meaning the only ones
left are recombinant
- This method can be
used in transgenic
mice to identify a
disease gene
- This method can be
used in transgenic
mice to identify a
disease gene
- Recombinant DNA could
confer a survival trait,
meaning the only ones
left are recombinant
- Mutant cells can be
used that do not grow
in a certain medium
- To identify the
sequence of interest in
the library, cells unable
to produce the resulting
desired product or
function are cloned
- Immunological
Assay
- Cloning
- PCR
- Useful when there
is not enough
material to start with
- Allows massive
amplification of specific
DNA sequences by
temperature cycling
- DNA is denatured in
hot temperatures
- Primers are
annealed to either
side of the region
to be amplified
- Temperature is cooled to
allow the DNA to renature,
and Taq polymerase carries
out DNA replication to
produce an identical stand
- Process is repeated 30-40
times to give millions of
copies of the sequence
- Process is repeated 30-40
times to give millions of
copies of the sequence
- Temperature is cooled to
allow the DNA to renature,
and Taq polymerase carries
out DNA replication to
produce an identical stand
- Primers are
annealed to either
side of the region
to be amplified
- After two cycles,
synthesis only occurs
between primers so
the new strands are
the unit lengths
- After three cycles, the
new copies are double
stranded and the
length of the amplicon
is the unit length
- The unit length
copies increase
in number with
every cycle
- By the end,
nearly all the
copies are
double stranded
DNA and unit
length products,
ready to be used
in cloning
- By the end,
nearly all the
copies are
double stranded
DNA and unit
length products,
ready to be used
in cloning
- The unit length
copies increase
in number with
every cycle
- After three cycles, the
new copies are double
stranded and the
length of the amplicon
is the unit length
- Useful when there
is not enough
material to start with
- PCR
- Single Nucleotide
Polymorphisms
- Single base
pair mutations
of normal DNA
- Fairly frequent and
important in inbred
populations like
domestic animals
because they are used
for selection purposes
- Correlated to quantitative
trait loci (QTLs) so these
can be produce a more
desirable phenotypic
response after a mutation
- Can be identified by
restriction fragment
length polymorphisms
(RFLPs)
- The base pair change
causes the new DNA
to become sensitive
to a certain restriction
endonuclease
- Causes different
length fragments - an
obvious indicator that
an SNP has occurred
and can be selected for
- e.g. a mutation in the
myostatin gene causes
muscle hypertrophy in Texel
sheep. Guanine changes to
Adenine, leading to
myostatin downregulation
and muscle hypertrophy
(very muscly sheep)
- e.g. a mutation in the
myostatin gene causes
muscle hypertrophy in Texel
sheep. Guanine changes to
Adenine, leading to
myostatin downregulation
and muscle hypertrophy
(very muscly sheep)
- Causes different
length fragments - an
obvious indicator that
an SNP has occurred
and can be selected for
- Method is also very
useful in DNA profiling -
blood on a suspect's
shirt can be analysed to
determine whose it is
- The base pair change
causes the new DNA
to become sensitive
to a certain restriction
endonuclease
- Single base
pair mutations
of normal DNA
- Gene Transfer
- Transfer into animal cells is
used to study gene function,
produce recombinant proteins
and to manipulate endogenous
gene expression
- Methods of delivery
- Transduction
- Virus particles infect
mammalian cells and
integrate themselves
into the genome
- Virus particles infect
mammalian cells and
integrate themselves
into the genome
- Bactofection
- Target DNA is carried
inside a bacterium, which
is taken up by the cell
- Digestion
releases
the DNA
- Digestion
releases
the DNA
- Target DNA is carried
inside a bacterium, which
is taken up by the cell
- Chemical transfection
- DNA and calcium
phosphate is taken
up by the cell via
endocytosis
- Usually
involved in
heat shock
- Usually
involved in
heat shock
- DNA and calcium
phosphate is taken
up by the cell via
endocytosis
- Physical transfection
- Microinjection,
electroporation
and ultrasound
- Electroporation increased
the permeability by an
electric field punching large
holes in the membrane. It is
very efficient and useful in
large plasmids
- Electroporation increased
the permeability by an
electric field punching large
holes in the membrane. It is
very efficient and useful in
large plasmids
- Microinjection,
electroporation
and ultrasound
- Transduction
- Transfer into animal cells is
used to study gene function,
produce recombinant proteins
and to manipulate endogenous
gene expression
- Gene Targeting
- Transgenic mice carrying
gene mutations are
useful for studying
human diseases such as
cystic fibrosis and cancer
- Form of in vivo
mutagenesis
- Where the
sequence of a target
gene is modified
within the cell
- Homologous
recombination
- Two types of vector
- Insertion vectors
- Simply
insert a
gene
- Simply
insert a
gene
- Replacement
vectors
- Replace
sections
of DNA
- Replace
sections
of DNA
- Insertion vectors
- Allows for the
generation of
animals with
human genes
- Two types of vector
- Site-specific
recombination
- Based on a recombinase
enzyme and a stretch of
DNA that is recognised
by the enzyme
- Cre-LoxP system
- Cre is an enzyme that
causes recombination, and
loxP is the site of action
- Swaps the target
sequences on
two DNA strands
- homologous
recombination
- Both are derived from
bacteriophage P1
- Cre recombinase is an
enzyme which catalyses
recombination between
two loxP sites
- Placing these loxP
sites appropriately
gives control over
recombination,
allowing transgenes
to be inserted
- Can be
modified to only
work in certain
types of cell
- Can be
modified to only
work in certain
types of cell
- Placing these loxP
sites appropriately
gives control over
recombination,
allowing transgenes
to be inserted
- Swaps the target
sequences on
two DNA strands
- homologous
recombination
- Cre is an enzyme that
causes recombination, and
loxP is the site of action
- Based on a recombinase
enzyme and a stretch of
DNA that is recognised
by the enzyme
- Where the
sequence of a target
gene is modified
within the cell
- Transgenic mice carrying
gene mutations are
useful for studying
human diseases such as
cystic fibrosis and cancer
- Transgenesis
- Transgenic mice can be
generated by retrieving
embryonic stem cells and
inserting a transgene by
transfection
- They are then
reinserted into the
embryo, which is
transferred into a
host mouse
- After birth, some
offspring will show
phenotypic signs of
the transgene
- These are selected and
bred again, eventually
leading to a homologous +/+
mouse for the transgene
- These are selected and
bred again, eventually
leading to a homologous +/+
mouse for the transgene
- Chimeras are
animals with
cells contributed
from two or more
embryos
- After birth, some
offspring will show
phenotypic signs of
the transgene
- They are then
reinserted into the
embryo, which is
transferred into a
host mouse
- Knockout animals
are used to study
gene function on
specific tissues
- Help to understand
disease and its
resistance and also
improve suitability for
xenotransplantation
- Help to understand
disease and its
resistance and also
improve suitability for
xenotransplantation
- Protein
Expression
Systems
- Cell free
- Wheat
embryos,
E.coli lysates
- Wheat
embryos,
E.coli lysates
- Bacterial
- Plasmids
and phages
- Plasmids
and phages
- Yeast
- Expression vectors
(plasmids and yeast artificial
chromosomes YACs)
- Expression vectors
(plasmids and yeast artificial
chromosomes YACs)
- Insect
cells
- Baculovirus
and plasmids
- Baculovirus
and plasmids
- Mammalian
- Viral expression
vectors (like adenovirus
and retrovirus), and
stable cell lines (like
CHO and HEK293)
- Viral expression
vectors (like adenovirus
and retrovirus), and
stable cell lines (like
CHO and HEK293)
- Cell free
- Transgenic mice can be
generated by retrieving
embryonic stem cells and
inserting a transgene by
transfection
- Fusion Proteins
- Created by the joining
of two or more genes
which originally coded
for separate proteins
- This is able to
carry out functions
of both the previous
separate proteins
- Useful in drug
design, creating a
pure product that
performs many
functions
- Useful in drug
design, creating a
pure product that
performs many
functions
- This is able to
carry out functions
of both the previous
separate proteins
- Created by the joining
of two or more genes
which originally coded
for separate proteins
- DNA Sequencing - Sanger Method
- Requires 4 separate
reactions - one for
each of the four
dideoxynucleotides
- Each reaction contains a
strand of DNA, a labelled
primer, DNA polymerase,
normal deoxynucleotides
and one of the
dideoxynucleotides
- e.g. ddATP is added to
the mix and DNA
polymerase starts
synthesising a new
strand, until ddATP is
randomly added to the
mix, which stops the
reaction due to ddATP not
having the 3'-OH group for
a phosphodiester bond
- This causes, at some point,
ddATP to be added to every
single point where there is
an adenine base at some
point in the replication cycle
- Creates lots of different
sized fragments, all
ending in ddATP
- Creates lots of different
sized fragments, all
ending in ddATP
- This causes, at some point,
ddATP to be added to every
single point where there is
an adenine base at some
point in the replication cycle
- e.g. ddATP is added to
the mix and DNA
polymerase starts
synthesising a new
strand, until ddATP is
randomly added to the
mix, which stops the
reaction due to ddATP not
having the 3'-OH group for
a phosphodiester bond
- All are radioactively or
fluorescently labelled
with a different colour
- Every possible
size fragment
has been
produced
- Every possible
size fragment
has been
produced
- Each reaction contains a
strand of DNA, a labelled
primer, DNA polymerase,
normal deoxynucleotides
and one of the
dideoxynucleotides
- Electrophoresis is
carried out separately
(but on the same gel) for
each dideoxynucleotide
reaction, separating the
fragments by size order
- The order of the sequence
can then be read by the
labelled nucleotides
separated by size order
- The order of the sequence
can then be read by the
labelled nucleotides
separated by size order
- Requires 4 separate
reactions - one for
each of the four
dideoxynucleotides
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