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Title: Genetics Lecture Notes ACE1013
Description: 1st year biology course, Introduction to Genetics ACE1013, covers: - Mitosis & meiosis - Mendel & laws - PCR - DNA Replication - Recombinant DNA - Gene Expression
Description: 1st year biology course, Introduction to Genetics ACE1013, covers: - Mitosis & meiosis - Mendel & laws - PCR - DNA Replication - Recombinant DNA - Gene Expression
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Introduction to Genetics
ACE1013
5
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15
Genetics is the science of heredity:
How organisms pass on biological information
Study of biologically inherited traits
Study of genes
Fields of genetics
Transmission genetics (inheritance patterns)
Cytogenetics (chromosomes)
Molecular genetics (DNA Technology)
Population genetics (variation & evolution)
Genomics and information sciences (gene sequencing)
Selective breeding
For biggest, most useful production
o E
...
10
...
of chromosomes
Diploid: (2n) both sets
Haploid (n) half diploid – one set
Mitosis maintains chromosome no
...
Introduction to Genetics
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Mitosis
Part of the cell cycle
Identical daughter cells produced
Used in asexual reproduction of egg division
Genome: cells total DNA (3m long)
Cell Cycle
Interphase mitotic phase
Cell physically divides
90% of the cell cycle
Cell grows & copies DNA
Includes G1, S & G2
After DNA duplication the chromosomes condense before cell division
Each chromatid forms 2 sister chromatids with identical DNA
Mitosis
Prophase
Chromosomes
become visible
Spindle forms
Contromeres
move away
Prometaphase
Nuclear
envelope breaks
down
Microtubules
stick to
chromosomes
Metaphase
Anaphase
Telophase
Chromosomes
line up on the
equator
Chromosomes
separate
Identical sets of
chromosomes at
poles
Migrate to poles
Cell becomes egg
shaped
Chromosomes
uncoil
16
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15
Meiosis
Sexual reproduction involves:
o Meiosis
o Gamete production
o Fertilization
o It produces variation through different new combinations of alleles
The Role of Meiosis
Life cycle
o Stages in the reproductive history of an organism
o Meiosis alternates with fertilization
Meiosis reduces the chromosome number from diploid (2n) to haploid (n)
This promotes genetic diversity among gametes
Gametes (n) combine by fertilization to produce a zygote (2n)
2n --> meiosis --> n --> fertilization --> 2n
2 nuclear
enevlopes
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Phenotype: the visible characteristics EG seed wrinkle or coat colour
Genotype: the genetic make-up & alleles present
Homozygous: the same EG SS or ss alleles
Heterozygous: different EG Ss alleles
Homologous Pair
Sister Chromatids
Meiosis I
The homologous chromosomes line up together, homologue to homologue, these
homologues then separate
Prophase I
90% of meiotic division
Homologues pair together
Crossing over occurs at chiasmata
The segments swap and exchange genetic information
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Metaphase I
Chromosomes on the metaphase plate are still in homologous pairs
Kinetochore microtubules attach to one chromosome from each pair
Anaphase I
Homologous pairs are separated
The spindle pulls each chromosome to
opposite poles of the cell
The sister chromatids remain attached
Telophase I
Cytokinesis occurs and two daughter cells are produced
There is no further replication of DNA before the 2nd meiotic division
Meiosis II
Metaphase II
The chromosomes on the metaphase plate line up on the equator
The spindle fibres attach to one chromatid from each of the
sisters
Anaphase II
The centromeres finally separate and the sister chromatids
move to opposite sides of the cell
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Telophase II
21
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15
Separate nuclei form
Cytokinesis occurs
This results in four haploid daughter cells
Transmission Genetics
Segregation
The two alleles for each trait separate during gamete formation (meiosis), then unite at
random, one forms each parent at fertilisation
The Test Cross
Used to distinguish genotype
o Unknown individual is bred with a homozygous recessive
Y y
Y YY Yy
y Yy yy
Dihybrid Cross
How will the alleles be assorted when the double heterozygous F1 plants produce gametes?
o SY & sy only
o SY, Sy, sY & sy?
Mendel saw 4 phenotypes in F2
o Recombinant types appeared
o 9:3:3:1 ratio
Independent Assortment
During gamete formation, different pairs of alleles segregate independently or each other
Not as universal as the law of segregation
o Some genes are linked (on the same chromosome)
o But chromosomes do assort independently during meiosis
Mendel’s law indicated that pairs of genes on homozygous chromosomes segregated during
gamete formation
o True for many
o Some didn’t fit and produced ratios of 3:1 & 9:3:3:1
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15
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Dominance
Incomplete Dominance (i
...
partial or semi dominance)
The heterozygous phenotype is somewhere in between the two homozygous phenotypes
o EG Belgian blue cattle – they have an extreme muscularity gene
Codominance
The phenotype is a mixture of both homozygous phenotypes
o Both alleles are expressed
o EG ABO blood type
o Shorthorn coat colour
Red or white homozygotes
Heterozygotes are roan colour
Many alleles are codominant at the molecular level
Pleiotropy
There are multiple effects of a single gene
o EG albino tiger has a white coat and is cross eyed due to one gene
Lethal Alleles
EG Overo allele in horses
o Homozygous foals die within a few days
o They have a white coat and no nerve cells
EG the Manx allele in cats
o Heterozygotes die in utero
o They lack a tail
o 2:1 ratio
Multiple Alleles
Coat colour in rabbits
o One gene has 4 alleles
Multiple Genes
Most traits are controlled by two or more genes and influenced by the environment
o Called multifunctional or polygenic
Some gene interactions further modify phenotype ratios
o EG Epistasis: one gene at one locus influences another gene at a different locus
o Common in control of fur/petal colour
o EG Labrador
B/b for melanin in skin
E/e for melanin in hairs
Gene interactions and new combinations can generate hybrid vigour
o Offspring perform better than both pure bred parents
o The influence of multiple genes can produce continuous (quantitate) variation
Environmental variables influence the transmission of a gene: called the phenotype
o Seen in polygenic & single gene traits
o EG Siamese cat coat colour
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Sex Linked Alleles
Chromosome theory of Inheritance
Chromosome movement during meiosis parallels the behaviour of genes
Chromosome Compliment
Each somatic cell contains a set number of chromosomes
o EG 46 chromosomes in humans
o 22 sets of autosomes
o 1 set of sex chromosomes: XY in men or XX in women
Sex Chromosomes
The SRY gene on the Y chromosome ensure that testes and sexual organs develop
The segregation of sex chromosomes into gametes ensures equal numbers of males and
females are produced
The single X chromosome in males must come from the mother
X Chromosome Genes
Males only carry one copy of the X chromosome gene
The pattern of inheritance of these genes differs from that of autosomal genes
Traits determined by these genes are X or sex linked
o EG white & red eyes in fruit flies
Recessive X linked traits are seen more frequently in males than females since only one of the
recessive gene is needed
o This results in different phenotypic ratios
Reciprocal crosses give different results – breaks Mendel’s rules
Linked Genes
Two genes close together on the same chromosome may be independent of each other
o Their alleles aren’t sorted independently
o Dihybrid F2 ratios are atypical
o When chromosomes are far apart on the chromosome, crossing over may break the
line
Sex Limiting Traits
Traits that are only expressed by one sex
The genes are carried by both sexes
o e
...
milk yield
o egg production
o cryptorchidism – unable to grow
o cock feathering
Sex-Inherited Traits
Expressed in both sexes, one sex more often
o EG Sheep horns
o Hip dysplasia in dogs
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Changes in Chromosome Number
Disrupts the development
o influence of changes is more substantial than alterations in individual genes
Aneuploidy
o One or more extra / missing chromosomes
o Caused by nondisjunction
o e
...
Trisomy 21 where there is an extra 21 chromosome causing down syndrome
Polyploidy
o Three or more complete sets of chromosomes
o Normal condition in many plants
o Lethal condition in humans and many animals
Mutations in Chromosomes
Deletions
Duplications
Inversions
Translocations
28
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15
Introduction to Molecular Genetics
Proteins
Are central to the phenotype of the organism
They act as:
o Enzymes
o Structural proteins
o Receptors
o Messengers
Hormones
Cytokines
Most genes encode a single protein
DNA Form & Function
Genes consist of deoxyribonucleic acid
DNA is two strands of nucleotides
DNA nucleotide:
o Phosphate
o Sugar- deoxyribose
o Base
Adenine
Guanine
Cytosine
Thymine
o Four different nucleotides in DNA (G, A, T & C)
o They differ only in their base
o The carbons in the sugar are named 1’, 2’, 3’, 4’ and 5’
o The base is linked to the 1’ carbon
o The phosphate is linked to the 5’ carbon
Introduction to Genetics
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The nucleotides in DNA are linked by phosphate bonds
(phosphodiester) between the sugars
The 3’ carbon of one sugar is linked to the 5’ carbon of the next
nucleotide
Ends of the DNA strand are called the 5’ and 3’ ends
5’ end: the 5’ carbon of the terminal nucleotide is free
3’ end: the 3’ carbon of the terminal nucleotide is free
A to T: 2 hydrogen bonds
G to C: 3 hydrogen bonds
Structure is called antiparallel because each helical strand travels in
opposite directions
DNA Structure
Right handed double helix: two polynucleotide chains are coiled in a spiral
Sequence of nucleotides are linked by phosphodiester bonds, joining adjacent deoxyribose
groups
The two strands are held together by hydrogen bonding between bases on opposing strands
Purine Is always paired to Pyrimidine
Functions of Genetic Material
Genotypic function: information storage and replication
o Genetic material must store genetic information and accurately transmit that
information from parents or offspring, generation after generation
Phenotypic function: gene expression
o Genetic material must undergo changes so that organisms can adapt to modifications
in the environment
o Without these changed, evolution wouldn’t occur
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Diversity of Life
DNA in all species shows:
o Molecular consistency (similar structure)
o Variation (unique base sequences)
EG:
o Bacteria: 106 nucleotides; one circular
chromosome
o Yeast/fungi:107-108;
linear
chromosomes
o Plants: 108-1011; linear chromosomes
o Mammals: (humans): 3
...
11
...
The strand of DNA has to be unwound
2
...
Each old strand acts as a template that determines the order of nucleotides to
form the new strand
4
...
i
...
each daughter stand contains
one new and one old backbone
Replication Bubble
These bubbles are produced
where the DNA helix has
unwound to allow for synthesis
of proteins
...
o Each small stretch is called an Okazaki fragment
o DNA polymerase III then synthesises the addition of nucleotides until it reaches the
previous primer
o DNA polymerase I then removes the old
primer and replaces it with DNA
nucleotides
o Between each Okazaki strand there is a
small space, the enzyme DNA ligase
catalyses the formation of the
phosphodiester bond
RNA
This is a nucleotide polymer
Nucleotides of adenine, guanine, cytosine and uracil
Has a sugar of ribose
DNA Mutations
Mutations can occur in DNA
o EG during replication process
o Or due to environmental damage, e
...
radioactive substances
DNA proofreading can correct errors as soon as DNA polymerase makes them
Mismatch repair: scans DNA immediately after it has been replicated and corrects any base
pairing mismatches
Excision repair: removes abnormal bases that have formed because of chemical damage and
replaces them with functional bases
06
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15
From Genes to Proteins
Proteins: Functional Gene Products
Genes direct protein production, they dictate every reaction in cells and produce measurable
characteristics
o EG enzymes control chemical reactions
o Genetic polymorphism for the enzyme can lead to differences in enzyme activity EG
Rubisco
Understanding these pathways to protein production enable:
o Precision crop breeding
o Rapid diagnosis of plant or animal health problems
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Location of Gene Protein
Karyon: the cell nucleus
Eukaryotes have a nucleus/nuclear envelope and membrane bound organelles
Prokaryotes don’t have a nucleus and have no membrane bound organelles
Genes
Phenotype
DNA
Transcription
RNA
Translation
Protein
Proteins are synthesised from genes via two processes:
1
...
Translation (protein synthesis)
Using RNA as a template to synthesise protein
Structure of DNA & RNA
DNA is double stranded, it’s very stable and so doesn’t degrade
RNA is single stranded
There is no thymine in RNA, uracil replaces it
RNA nucleotides have an additional O atom
Transcription
3 essential components
o Protein coding gene
Important structural features that inform the building of RNA
Promoter region: specific DNA sequence where transcription begins
Coding sequence: specific DNA sequence, coding information for the protein
Terminator: a specific DNA sequence that determines the end of the RNA
transcript (in prokaryotes)
o RNA polymerase
An enzyme to catalyse the building of RNA from DNA
Also acts as a primase that initiates DNA replication (aka transcriptase)
It has 5 different polypeptides, two alpha, two beta and a sigma copy, this is
called the Halo enzyme, it initially binds onto the DNA promoter region, the
DNA helix is then unwound and transcription can begin
o NTPs (nucleoside Triphosphates)
The building blocks of the new RNA
A nucleoside is the base attached to the ribose
Uridine, cytidine, adenosine, guanosine are the 4 different nucleosides
3 stages:
o Initiation
Occurs at the promoter region
RNA polymerase binds to the promoter and begins to unwind the DNA
As the DNA and RNA transcript exits the RNA polymerase, the RNA is removed
from the DNA template and the DNA rewinds together
o Elongation
o Termination
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When the RNA polymerase reaches the termination site, the RNA transcript
is released from the template
RNA polymerase dissociates from the DNA and can perform other rounds of
transcription
mRNA carries the gene sequence for translation of the protein production
Other RNAs also produced by transcription, involved in protein production
The type of RNS produced depends on the DNA sequence used to transcribe it
o Different DNA sequences encode different types of RNA
10
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15
RNA Processing
Eukaryotic Promoters
There are 3 phases of transcription:
o Initiation: occurs at the promoter region, the RNA polymerase binds to the promoter
and begins to unwind the DNA
TATA box: a DNA sequence within the promoter region of DNA, rich
in AT base pairs
o
o
Transcription factors: proteins the bind to the DNA and influence
transcription
One transcription factor recognises the TATA box and binds and the
additional TFs recognise the bound TF and bind
RNA polymerase recognises the transcription factors which enable it
to bind to the DNA in the correct place and direction
RNA polymerase: with a sigma subunit
The additional transcription factors bind to the DNA using RNA
polymerase, the transcription initiation complex
The RNA polymerase then unwinds the double helix and RNA
synthesis begins at the start codon on the template strand
Elongation
Termination
When RNA polymerase reaches the termination site, the RNA transcript is
released from the template
Polyadenylation signal sequence: this is a DNA sequence within the
termination site region of the DNA, this codes for the polyadenylation signal
in the mRNA, usually AAUAAA
Enzyme: this recognises the polyadenylation signal and releases the mRNA
from RNA polymerase
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RNA Processing
Characteristic
Site of transcription & Translation
Gene structure
Modification of mRNA after
transcription before translation
Prokaryotes
Cytoplasm
Complementary to
protein structure
None
Eukaryotes
Transcription – nucleus; Translation
- cytoplasm
Noncoding sequences “introns”
A) Additions to mRNA ends
B) Intron removal
A) additions to mRNA ends
I
...
3’ tail
this is added immediately after the mRNA transcript has been released from
RNA polymerase
Called a ‘Poly A Tail’ which is 100-300 adenine nucleotides long
Enables the mRNA to be exported from the nucleus to the cytoplasm
Helps to promote mRNA stability and prevent degradation
B) intron removal (splicing)
Eukaryotic gene sequences contain non-coding sections that don’t code for a protein
These are transcribed into mRNA sequences which produces introns
Small nuclear Ribonucleoproteins (snRNPs): these are proteins that perform the
splicing
RNA polymerase transcribes both the introns and exons, this material is called the
pre-mRNA
For the mRNA to leave the nucleus for translation to occur in the cytoplasm the
introns need to be removed
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Splicing means to form connections
Things needed for RNA splicing:
Pre-mRNA
snRNPs
o At the boundaries between introns & exons there are consensus
sequences which are short stretches of DNA that appear in many
different genes, this is complementary to the consensus sequence on
the 5’ boundary and so it binds by base pairing
o
o
o
o
Other snRNPs also attach at
additional point along the premRNA
These then join together to form
a spliceosome which will loop out the intron
The Spliceosome cuts the pre-mRNA at the intron-exon boundary
RNA Splicing
I
...
The free 3’OH group at the end of the cut exon reacts with
the 5’ phosphate of the other exon
III
...
The excised intron is degraded in the nucleus & recycled
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Translation
Translation
Codons
These are a series of three nucleotides in mRNA
that codes for an amino acid
Codons direct the placement of specific amino
acids into a protein
There are 64 codons, 3 functions as stop signals
marking where ribosomes end translation, there are
20 amino acids and 1 start codon
Translation Stages
Initiation
1
...
Prokaryotes: a recognition
sequence (AGGAGG)
b
...
Methione
charge
tRNA-containing
complementary sequence to start codon
(anticodon, UAC) binds to the start codon (AUG)
The first amino acid in the polypeptide
chain is methionine
The combination of mRNA, ribosome
small subunit and tRNA forms the
initiation complex
3
...
A: anticodon
b
...
E: exit
Methionine charged tRNA occupies the site
The A site is aligned with the next mRNA codon (CCG)
Elongation
1
...
Peptide bond formation:
Proline is linked to methionine by
peptidyl transferase activity of the
ribosome large subunit
Peptidyl transferase has catalytic
activity for 2 reactions:
a
...
Forms a bond between that
amino acid and the new amino
acid attached to its tRNA in the
A site
3
...
The process then repeats
The free site A attracts complementary charged anticodon (AUA) for the
codon in the A site
The bond between the amino acids and tRNA in the P site breaks
These amino acids bond to the new amino acid
on the tRNA in the A site
The ribosome then moves along the mRNA to
the next codon, the old tRNA is release and the
new tRNA is in the P site
Termination
1
...
The release factor disconnects the polypeptide from the
tRNA in the P site
3
...
Stay within the cell: complete translation and be released to an organelle, or remain
in the cytosol
Proteins contain signal sequence that direct them to the nucleus,
mitochondria, plastids or peroxisomes, if there is a lack of signal sequence
they will remain in the cytosol
2
...
Most proteins are not identical to the polypeptide chains
2
...
This is essential to the final function of the protein
Proteolysis: cutting the polypeptide allowing the fragments to fold into
different shapes
EG cutting the signal sequence from the growing polypeptide chain in
the ER
Some proteins made from polypeptides are cut into their final
products by proteases
Proteases are essential to some viruses (EG HIV) and larger viral
polypeptides can’t fold without being cut
Some drugs for AIDS work by inhibiting HIV protease, which prevents
the formation of proteins needed for viral reproduction
Glycosylation: the addition of sugars to the polypeptide, important for
targeting and recognition
The addition of sugars forms glycoproteins
It is catalysed by enzymes in the ER and Golgi apparatus
This is essential for directing proteins to lysosomes and important in
the conformation of proteins and their recognition at the cell surface
Phosphorylation: the addition of phosphate groups to alter the shape of the
protein
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Catalysed by protein kinases
Charged phosphate groups change the conformation of a protein
which often exposes the active site of an enzyme or binding site to
another protein
Important for cell signalling
Transport to Cellular Destination
1
...
Or the translation is stopped and it is moved to the ER to finish synthesis
17
...
15
Regulation of Gene Expression
Regulation of Gene Expression
Temporal variation in gene expression and protein synthesis EG butterflies
Organisms go through development stages produced by different sets of proteins, controlled
by regulated gene expression
Regulating gene expression also allows organisms to respond to changes in their environment
o EG plant in a drought
Plants must simultaneously produce multiple proteins whose genes are
scattered throughout the genome (different chromosomes)
The synthesis of these proteins is called ‘stress response’
To coordinate expression, each stress gene has a specific regulatory sequence
near its promoter called the stress response element (SRE)
1
...
The TF binds to the SRE of each gene, which stimulates the
transcription of each gene that has the same SRE sequence,
3
...
E
...
Glucose =, the preferred energy source is the easiest
sugar to metabolise or lactose that is composed of βglucose which is more complex to metabolise
3
...
Functional genes: genes for enzymes involved in
lactose metabolism
Activator Protein: positive regulation
Introduction to Genetics
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o
o
o
o
o
The binding of the activator protein stimulates transcription
to allow for the RNA polymerase to bind to the promoter
region
o When glucose levels are low, positive regulation can increase
the efficiency of lac operon transcription (not turned on
when glucose levels are high)
Two environments affect the rate of lac operon:
o Low glucose (when lactose is also present)
1
...
RNA polymerase then binds more efficiently to the
promoter
3
...
cAMP is low, CRP is inactive and does not bind to the
promoter, RNA polymerase is unable to bind
efficiently
2
...
Bind to the enhancer and regulatory protein sites
2
...
11
...
They cleave double
stranded DNA at a position either within or outside the recognition site
This recognition site can be of 4, 6 or 8 nucleotides long
Restriction enzymes can release:
- Cohesive/sticky ends
- Blunt ends
There are more than 3600 restriction enzymes
o
Modifying enzymes
Methyltransferases
This catalyses the transfer of a methyl (CH3) group to DNA bases (N6Methyladenine, N4-Methylcytosine, C5-Methylcytosine)
Used to block restriction sites
Approximately 1% of DNA bases undergo DNA methylation
Nucleases (DNases, RNases)
Enzymes that cleave randomly nucleic acids
Deoxyribonucleases, DNases: nucleases that cleave single stranded or
double stranded DNA
o Endonucleases: cut inside the sequence
o Exonucleases: cut from the extremities
Ribonucleases, RNases: nucleases that cut the RNA
DNA ligases
These catalyse the formation of a phosphodiester bond between the
5’ phosphate of one DNA fragment & the 3’ hydroxyl of another
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There are two types:
o ATP-dependent DNA ligases
o NAD-dependent DNA ligases
T4 DNA ligase is used in cloning to ligate DNA fragments
Polymerases
These copy a DNA strand into another DNA strand
There are 2 domains and 3 functions:
o C-ter
...
Small fragment has: 5’ to 3’ exonuclease activity
There are 3 main types of DNA polymerases in bacteria:
o DNA pol I: main enzyme for DNA replication in bacteria, the
DNA polymerases use in PCR belong to this group
o DNA pol II: involved in DNA repair
o DNA pol III: involved in DNA replication
Processivity: number of nucleotides added to the new strand per
second
Fidelity: the rate of errors (wrong nucleotides added)
RNA Polymerases
o
o
These transcribe single stranded DNA into RNA
In prokaryotes: the same RNA polymerase produces
messenger RNA and non-coding RNA (rRNA, tRNA, sRNA)
o In eukaryotes:
RNA polymerase I: large ribosomal RNAs
RNA polymerase II: messenger RNA
RNA polymerase III: transfer RNA and small RNA
Mitochondrial & chloroplast RNA polymerases
Reverse transcriptase
RBA dependent DNA polymerase
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Transcribe single-stranded RNA into single-stranded complementary
DNA (cDNA)
Used mainly by retroviruses (EG HIV, AMV)
In the lab Reverse Transcriptase are used to produce in vitro cDNA
from RNA
Molecular tools
o Vectors
They are small DNA molecules having regulatory and coding sequences
Foreign DNA can be inserted into them
They are used as carriers of foreign DNA host cells
Origin of replication: replication of the vector, together with the foreign DNA
fragment inserted into it
Genetic markers: selection of cells which have taken up the plasmid DNA
Multiple cloning site: a site where DNA is inserted
Transfer DNA (some vectors): transfer a gene into a target genome, vector
DNA can be used as a DNA vaccine
o Plasmids
Double stranded circular bacterial DNA used for molecular cloning to amplify
or express insert DNA into bacterial hosts
Phagemids or phasmids
DNA cloning vectors derived from phage DNA and containing an
origin of replication
...
They are used to carry large insert DNA up to 300kb
and are used to create and store genomic libraries
...
11
...
6 and 2
...
The charged molecules are first retained on a resin having the opposite charge
to them
2
...
The retained molecules are then eluted using a salt solution
Size-Exclusion chromatography
o Separates molecules based on their size
o The small molecules are retained in the resin particles
o Large molecules pass through between the resin particles
DNA & RNA Detection
Fluorescent intercalating agents:
o Ethidium bromide: orange fluorescence under UV light
o SYBRGreen: green fluorescence under UV light
Dyes: Hoechst & silver
Radioactive labelling: 32P(ATP)
Fluorescent labelling: Cy3, Cy5, 6-FAM, Rox, TAMRA, etc
...
Each spot contains a probe for a gene
The chips are hybridised with DNA or RNA samples for detection and quantification of
particular sequences
Macro chips:
o Contain hundreds of macroscopic spots (Probes) on glass or membrane supports
Microchips:
o Contain thousands of microscopic spots (probes) on glass
supports
DNA Sequencing
Sanger & Coulson method (termination method, 1977):
o This method used dideoxynucleotides (ddATP, ddTTP,
ddGTP and ddCTP) for early termination of DNA
polymerisation
Sequencing reaction:
1
...
A primer is required
3
...
Labelled ddNTPs (ddATP, ddTTP, ddGTP
and ddCTP) (big dye terminator) are
required
5
...
11
...
The double stranded DNA is denatured
in 95°C
2
...
The primers are extended by the
attachment of free nucleotides
4
...
Initial denaturation
2
...
Annealing temperature and time are depended
of the type of primer
4
...
12
...
The DNA is digested with the appropriate
restriction enzymes
2
...
Different DNA fragments can be successively
ligated to produce rDNA
4
...
Complementary DNA (cDNA) libraries
Collections of bacterial clones containing cDNA representing expressed genes
in a given tissue at specific conditions and corresponding to a specific
physiological situation
Only expressed genes are represented
2
...
RNA extraction and mRNA purification
2
...
Ligation of the adaptors and their digestion
4
...
Packing of he rDNA (cDNA in the vector) into the phage capsule
6
...
gDNA extraction & purification
2
...
Ligation of DNA fragments into the digested vector
4
...
Plating the phage library into host bacteria
Screening libraries
Probes
Labelled RNA or DNA fragments with a known sequence used to detect a complementary
sequence in a DNA or RNA population
Homologous probes: from the same organism
Heterologous probes: from a different organism, used to detect similar sequences in the
studied organism
The isolated clone is then sequenced and the sequence is analysed
Genomics: Genome Analysis
Sequencing of the transcriptome (total expressed genes in a tissue) or the entire genome
Transcriptome analysis:
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o
Expressed sequence tags (ESTs): random sequencing of thousands of clones from a
cDNA library prepared from a given tissue at specific conditions
Genome analysis:
o Sequencing DNA libraries containing fragments representing the entire genome of a
given organism
o The obtained sequences are made available to the scientific community via databases
Genome Sequences
Coding sequences
Regulatory sequences
Mapping genomes
o Assigning/locating a specific gene to a particular region of a chromosome and
determine the location and relative distances between genes on the chromosome
Physical map:
o The physical, DNA-base-pair distances from one gene to another
Genetic linkage map:
o Order of genes on a chromosome and the relative distances between these genes
o Tracing the inheritance of multiple gene traits
Associating Gene with Function/Phenotype
Associating change in gene expression with function
o Single gene approach
Northern blotting
Quantitative reverse transcription-polymerase chain reaction (QRT-OCR)
o Global approach
Checking the expression of thousands of genes at the same time
Microarray technology
RNA sequencing
Gene silencing with function
o Knock down technologies
Antisense RNA
Used to reduce the expression of a gene to check the impact on the
physiology
Antisense RNA are RNA sequences complementary to the target RNA,
they hybridise to it and block its translation
They are produced by transforming the target organism with a cDNA
that is transcribed into antisense RNA
RNA interference using small RNA
Small RNA are natural or synthetic double stranded RNA molecules of
20-15 nucleotides complementary to the target RNA
They hybridise to the target RNA and block its translation, they lead
to its degradation by specific RNases
Antisense RNA and siRNA allow to identify gene function
Introduction to Genetics
o
Knock-out Technology
Knock-out are collections of insertional mutants produced by rDNA
technology
A vector is used to transfer randomly or specifically a tDNA to a location in
the genome to alter a gene at that locus
Each mutant has an alteration in a single gene
By tracing the tDNA it is possible to find which gene was affected
By identifying the change in the phenotype it is possible to link gene with
function
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Transgenesis
ACE1013
The transfer of a gene from
one species to another species
o Direct transfer
o Semi-direct transfer
o Mediated transfer
Recombinant DNA Technology II
Introduction to Genetics
Methods used for DNA transfer
o Transformation/Transfection:
This method uses competent cells induced chemically (Lithium Acetate) to
take in the DNA
The DNA is added to competent cells and left to
enter the cells on ice
Usually a heat shock (42°C) is required to complete
the DNA transfer
o Electroporation
This method uses an electric pulse to drive DNA into
cells
DNA is added to cells and placed in a cuvette having electrodes on two sides
An electric pulse is applied to the electrodes using a pulse power supply
o Microinjection
This method involves the injection of naked DNA into cells
using a pipette that has a microscopic tip
It is mainly used for transforming animal cells (eggs)
Done under a microscope
o Bombardment
This method uses a gene gun to transfer DNA coated on gold particles into
host tissues
The gene gun uses compressed helium, which is pulse to project the gold
particles into the cells
Methods using Mediated DNA Transfer
o Liposome mediated transfer
The DNA is packaged into liposomes which fuse to the
plasma membrane releasing the DNA inside the cell
o Bacterial and Viral Mediated Transfer
DNA is introduced in bacterial or viral strains which
infect the target cells and transfer DNA into their genome
Agrobacterium tumefaciens: is a bacterial strain capable of transferring DNA
to many plant species
Vaccine virus: transfers DNA to different animal and human cell types
o Selective breeding
This method is used to transfer DNA from one species to a close species via
successive crosses using a number of intermediates
Applications of rDNA Technology
ACE1013
Production of recombinant proteins:
o The production of proteins using an expression
system transformed with rDNA containing the
coding sequence for the protein of interest
o Expression systems:
Host cells together with compatible
expression vectors allowing high
expression of recombinant proteins in
these cells
Introduction to Genetics
ACE1013
o
Hosts:
Bacteria: Escherichia coli
Rapid growth
Inducible system
Yeast: Saccharomyces ceriviseae
Eukaryotic protein folding system
Good for producing functional recombinant eukaryotic proteins
Protein Production systems
o The recombinant protein can represent up to 50% of proteins produced by the cell
Protein secretion: no extraction:
o A single peptide (SP) is usually required for protein secretion outside the cells
o The nucleotide sequence encoding the SP is added to the sequence encoding the
recombinant protein in the rDNA
Example of therapeutic Recombinant Proteins
o Insulin: hormone controlling glucose uptake by cells EG diabetes
o Growth factor: used by young people with slow growth
o Coagulation factors: used by haemophiliac patients
o Recombinant vaccines
Molecular Pharming
The production of pharmaceuticals in plants and
animals
o High production systems
o Low production costs
o Possibility for integrating pharmaceuticals
in food
o Lower risk
Pharming in plants:
o Many plant systems are easy to transform
o Highly productive systems
o Low maintenance and low cost
o No possibility of disease transfer to humans
o It is possible to produce pharmaceuticals in seeds: the possibility of storage at room
temperature for many years
Proteins would remain stable for many years
Introduction to Genetics
ACE1013
Easy to store
Pharming in Animals:
Genetically Modified Organisms
Organisms who’s genome was
modified via the insertion of rDNA to
improve their phenotype
GM Plants:
o GM crops represent about 30% (increasing) of the world’s total crop production
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Title: Genetics Lecture Notes ACE1013
Description: 1st year biology course, Introduction to Genetics ACE1013, covers: - Mitosis & meiosis - Mendel & laws - PCR - DNA Replication - Recombinant DNA - Gene Expression
Description: 1st year biology course, Introduction to Genetics ACE1013, covers: - Mitosis & meiosis - Mendel & laws - PCR - DNA Replication - Recombinant DNA - Gene Expression