Replication, Transcription, and Translation PDF

Summary

These lecture notes cover replication, transcription, and translation in molecular biology. The document includes course outlines, learning objectives, and a basic overview of the processes. The notes also discuss the central dogma of molecular biology.

Full Transcript

REPLICATION, TRANSCRIPTION, AND TRANSLATION Strands
LECTURER: Ms. Rianne Aubrey P. Lopez, RMT ○ DNA: Double stranded
○ RNA: Single stranded
COURSE OUTLINE
A. DNA AS A TEMPLATE
I. Central Dogma of Molecular Biology
A. DNA as a Template
For a molecule to serve as a genetic material, it must exhibit
B. Central Dogma
II. DNA Replication the following crucial characteristics:
A. Models
B. Enzymes Capable of replication
C. Replication Process ○ No matter what, DNA must replicate because
D. Eukaryotic Replication some of it will die out and it needs to create
III. DNA Transcription more. It also needs to adapt and change for
A. Transcription Process an individual to survive.
B. Post-Termination and RNA Processing
Storage of information
IV. Kinds of RNA
A. Major Kinds of RNA ○ There are many types of storage:
B. Minor Kinds of rna ○ Example: Melanin. Sometimes melanin
V. DNA Translation activates, sometimes it doesn’t. Sometimes
A. The Genetic Code you have melanin that will be shown,
B. Translation Process sometimes it doesn’t.
C. Post Translation ○ It stores that information until it is going to be
VI. Genetic Mutations used. Repository in a sense.
A. Molecular Types
Expression of information
B. Effects when Translated into Proteins
○ Phenotypic characteristics or observable
characteristics.
LEARNING OBJECTIVES Variation by mutation
Understand the significance of Central Dogma
Determine roles of different enzymes in DNA Replication This serves 2 purposes:
Discuss the stages of DNA Replication
Discuss steps in DNA Transcription Source of information for protein synthesis
Differentiate Introns from Exons ○ Which is transcription.
Explain the process of RNA processing, modification, and splicing Provides information inherited by daughter cells
Enumerate and understand the different types of RNA
Discuss the process of translation
Note: Until 1944 it wasn't clear what is the component in our
Correlate relationship of code defects to corresponding mutations
body, that is our genetic material, until different experimentations
occurred. Lots of these experiments came from the
I. CENTRAL DOGMA OF MOLECULAR BIOLOGY experimentation of a specific bacteria.

DNA B. CENTRAL DOGMA

Also known as Deoxyribonucleic Acid, is the raw Describes the flow of genetic information in all of life.
material of inheritance. This is a template as to what Dogma = truth
makes you, you. Without it, we would be nothing. And
with too much DNA, we would be something extra.
These are bound mostly by 5’ to 3’ phosphodiester
bonds.
Composition:
○ Phosphoric Acid
○ Sugar: 2-deoxy-D-ribose
○ Nitrogenous bases
Purines (Adenine and Guanine)
Pyrimidines (Thymine and Cytosine)

DNA vs RNA

Name itself
Sugar
○ DNA: 2-deoxy-D-ribose
○ RNA: D-ribose
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Process of Central Dogma Semi-Conservative model

1. Everything starts with DNA. DNA is located inside the This was discovered by Matthew Meselson and
nucleus. For DNA to become an amino acid, it has to Franklin Stahl in 1958 through experimentation with E.
undergo different processes. coli (Escherichia coli) DNA
2. The DNA replicates itself to have multiple copies. Each daughter strand is only half of a new DNA (has
3. The DNA undergoes transcription. Through this, it can both old and new DNA)
become multiple types of DNA. Most importantly, your One original strand is used as a template.
mRNA. But it can also turn into your rRNA and tRNA. This is where our DNA lies because our DNA is not
4. As this becomes mRNA, it will undergo a process of always the same. It will change, it will continue on,
RNA processing. that’s how we adapt in the world. It has new and old.
5. After which it will leave your nucleus, proceed to your ○ Old: because we need our memories and we
cytoplasm and undergo translation into proteins and need our information from the past.
amino acids. ○ New: because we need to adapt to the
environment that we have today.
How many chromosomes do we have in our body?
SEMI-CONSERVATIVE MODEL DISPERSIVE MODEL
46 Chromosomes
23 Pairs Consistent strand of “new” Each strand is a mix of “new”
and “old” and “old”
II. DNA REPLICATION One strand is old
A strand is new-old-new-old
One strand is new
The synthesis of a new molecule of DNA by copying
existing DNA.
B. ENZYMES INVOLVED
○ Needed in order to ensure that each new cell
receives the correct number of
Helicase
chromosomes.
This is how DNA copies itself into more than one
Catalyzes the unwinding of double helix ahead of DNA
strand because we can't just have one strand of DNA.
polymerase
We have multiples and these multiples have copies of
It is the first enzyme involved because it will unwind
each other to make sure we continue to live.
the double helix.
DNA starts as double, but they are replicated
A. MODELS
separately because the two strands will have different
ways of replicating, depending on which direction they
will be.

Single Stranded Binding proteins or Helix Destabilizing
proteins

Also sometimes acronymed SSB
Bind specifically to single stranded DNA to prevent
reannealing.
This one hates realignment. Hates pairs. This prevents
any recombination because if DNA recombines before
it is replicated, it will not replicate at all.

Primase
Conservative Semi-conservative Dispersive
Model Model Model
From the key word “Prime”, it catalyzes the synthesis
The parental The parental of the short segment RNA primers (roughly 6-12
The parental
strands stay strands are nucleotides long) to the template strands.
strands do not
together or dispersed into two It starts the process.
reassociate
reassociate new double helices
DNA Gyrase or Topoisomerase
Each strand of both
Each replicated Each replicated
daughter molecules
DNA molecule is DNA molecule Relieves coiling tension ahead of the replication fork
contains a mixture
“conserved” as the consists of an ”old” and prevents supercoiling.
of the old and new
original and “new” strand As DNA tries to unwind, sometimes it will tighten, and
synthesized DNA.
the top portion of the DNA will be coiled, and will be
Table 1. Models of DNA Replication tangled.
This enzyme makes sure nothing tangles. Because if it
The human DNA follows the semi-conservative model. tangles, replication stops prematurely, and you will
have the wrong DNA.

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DNA Polymerase III Involves four components (seen through electron
microscope):
Very major enzyme. It is the most important out of the ○ DNA helicase: separates double helix.
three DNA polymerases. ○ Primase: initiates synthesis of an RNA
It binds nucleotides to form new strands. molecule.
Extends the strand in the 5’ to 3’ direction. ○ DNA polymerase: initiates nascent, daughter
strand synthesis.
DNA Polymerase I (Exonuclease) ○ SSBs: binds to single stranded DNA to make
sure they do not realign and to prevent any
Removes RNA primer and replaces it with DNA/inserts base pairing to happen.
the correct bases. The replication fork is bidirectional:
○ One strand goes from the 5’ to 3’ (leading
Ligase strand)
○ The other goes from the 3’ to 5’ (lagging
Joins DNA fragments (Okazaki fragments) into strand)
continuous daughter strands and seals other nicks in
the phosphate backbone.

C. REPLICATION PROCESS

1. Unwinding of DNA Strands

Origins of Replication (Ori): a special site where
replication begins.
Single-strand binding proteins: will stick to each
strand of DNA to make sure they will not come back
together, and they will stay single through the process.
From there, these are separated with the use of your
helicase.
○ Helicase: makes sure that the strands
separate. Imagine a zipper; when you pull it
down, it separates into two separate strands
of the zipper. With the formation of the replication fork, leading and lagging
Then, your helicase proteins will bind to your DNA strands were mentioned:
sequences, known as origins, which allow for
processive unwinding of DNA Leading strand (Forward strand)
The two strands here are now going to be your ○ DNA is synthesized continuously
templates. These are your templates as to how this Lagging strand (Retrograde strand)
will be replicated and the new strand will be elongated ○ DNA is synthesized into small fragments or
by the hydrogen bonding throughout the process. Okazaki fragments (discontinuously).
○ It is called lagging strand because it lags
behind the leading strand.

Okazaki fragments

Small fragments produced from the lagging strand.
Produced discontinuously from a 5’ to 3’ direction
Discovered in 1960 by Reiji and Tsuneko Okazaki
whilst studying DNA replication through
experimentation with E. coli
Crucial in discovering what is the importance of DNA
for humans.

3. DNA Polymerase Complex
Polymerases:
2. Formation of Replication Fork
The first purified enzyme shown to catalase DNA
The Ori is where replication begins. Meanwhile, the replication was designated as DNA Polymerase (pol l)
replication fork is where it is currently happening, DNA Polymerase II (pol Il) and Polymerase III (pol IIl)
meaning it will continuously move. were later discovered.
Replication fork: the bidirectional thing that represents Pol III has the most function compared to the pol I and
where the replication is happening currently. pol II.
Pol Ill is the main polymerizing enzyme during bacterial
replication.
Several different DNA polymerase molecules engage in
DNA replication.

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Why are these important? III. DNA TRANSCRIPTION

Chain Elongation Copying of one strand of DNA into RNA by a process
○ accounts for the rate at which polymerization like replication.
occurs. The synthesis of RNA under the direction of DNA,
Processivity particularly mRNA.
○ an expression of the number of nucleotides
added to the nascent chain before the Why do we need RNA? Why can’t we just copy DNA
polymerase disengages from the template. completely?
Proofreading function
○ identifies copying errors and corrects them, DNA only stores information.
and an important function of DNA that is not It has to be transcribed into RNA to make amino acids
in RNA. and proteins because DNA can’t make amino acids on
its own. But, DNA can make sure we make the correct
4. Initiation and Elongation of DNA Synthesis RNA, so that the correct RNA can make the correct
protein.
Initiation requires a short length of RNA (roughly DNA does make proteins but it just needs to be RNA
10-200 nucleotides long) first.
The replication complex begins to remove RNA
primers. SIMILARITIES DIFFERENCES
These gaps from the Okazaki fragments are now filled TO DNA SYNTHESIS TO DNA SYNTHESIS
with the appropriate base-paired deoxynucleotide.
The newly synthesized fragments of DNA are then Steps of initiation, Use of Ribonucleotides
sealed through the action of DNA ligase. elongation, termination. Primer is not involved
Large, multicomponent Uracil replaces Thymine as
5. Formation of Replication Bubble initiation complexes: base pair of Adenine
○ DNA: Uses DNA Only some portions of the
As replication occurs, both strands are simultaneously polymerase complex genome are copied once
replicated ○ RNA: Uses RNA
This replication process generates Replication Bubbles polymerase complex
Any nicks are resealed by DNA ligase. Adherence to Watson-Crick
base pairing rules
6. Reconstitution of new chromatin structure ○ Adenine to Thymine
(RNA: replace Thymine
Newly replicated DNA is rapidly assembled into to Uracil)
nucleosomes, the pre-existing and newly assembled ○ Guanine to Cytosine
histone octamers are randomly distributed to each arm
of the replication fork. A. TRANSCRIPTION PROCESS
These are facilitated through the actions of Histones.
RNA Polymerase

Main enzyme involved in RNA transcription.
Links ribonucleotides together in a sequence
complementary to the DNA template strand.
Catalyzes RNA synthesis.

D. EUKARYOTIC REPLICATION

Eukaryotic Replication

Eukaryotic DNA replication is more complex than the
replication process of a prokaryote (E. coli), but it is
similar.
Eukaryotes have large genome size, they have much
more chromosomes than prokaryotes. In addition, the
eukaryotic DNA is associated with histones and
non-histone chromosomal proteins. Hence, eukaryotic
DNA is replicated not as bare DNA but as chromatin.
1. Initiation

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 RNA polymerase and supporting accessory protein will
bind to around 6-10 base pairs sequence of
nucleotides on the DNA to be copied.
The initial step in bacterial gene transcription is
referred to as template binding.
This region is known as the Promoter Regions or
Initiation Sites.
Once RNA polymerase has recognized and bound to
the promoter, DNA is locally converted from its double
stranded form to an open structure, exposing the
template strand.
○ It will become single-stranded, but not RHO-DEPENDENT
INTRINSIC TERMINATION
completely. Only a small area will be opened, TERMINATION
as opposed to replication where it completely Dependent on Dependent on the termination
splits. self-complementary GC-rich factor, rho (r) and a
sequences (inverted repeats) termination sequence that is
within the transcript, which transcribed into a hairpin
form a stable GC-rich hairpin structure in the transcript.
structure, immediately
followed by a string of uracil
residues.

Why is this important?

This will vary its sequence and its ability to initiate transcription.
From there, it will begin in the promoter region in a 5’ to 3’
direction.

B. POST-TERMINATION and RNA PROCESSING

The primary transcript, known as pre-mRNA,
2. Elongation undergoes extensive processing in the nucleus before
being exported into the cytoplasm.
As RNA polymerase moves down the strand and adds Contained within pre-mRNA, are sequences found in
ribonucleotide complementary to the base sequence the DNA and mRNA known as EXONS and found in the
of the DNA template strand (elongating the strand as DNA and not in the mRNA known as INTRONS.
RNA transcript).
The Sense strand of the template has a sequence
identical to that of the RNA complex.
The 5’ end of the synthesized RNA protrudes from the
transcription complex

3. Termination

Occurs once RNA polymerase reaches a specific
termination sequence in the DNA.
Sequences called terminators signal that the RNA
transcript is complete. Once they are transcribed, they
cause the transcript to be released from the RNA
polymerase.

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 Addition of a methylated guanine nucleotide A. MAJOR KINDS OF RNA
CAPPING (7-methylguanosine OR m7G cap) to 5’ end of
RNA molecule.
Process where introns are removed from the
primary transcript and exons are bound
together.
SPLICING Splicing occurs within spliceosomes.
Once completed, the mRNA travels from
nucleus to cytoplasm. Coupled with mRNA rRNA tRNA
transcription.
messenger RNA ribosomal RNA transfer RNA
Enzyme poly A polymerase adds 100-200
residues of adenylic acid to the end of 3’ end Contains and Forms the Transfer activated
of the RNA transcript. carries the genetic ribosomes. amino acids to the
TAILING code to the ribosomes to be
Aid in export of mature mRNA.
Render stability. cytoplasm for Largest used in assembling
Serve as a recognition signal. controlling the type components of the protein
of protein formed. RNA (80-90%) molecule.

B. MINOR KINDS OF RNA

snRNA / siRNA miRNA pre-mRNA
Small Nuclear RNA Precursor
Micro RNA
/ Splicing RNA messenger RNA
Directs the splicing Single-stranded Has not yet
of pre-mRNA to RNA molecules of undergone RNA
form mRNA. 21-23 nucleotides processing.
that regulate gene
Helps in removing transcription and Its main difference
introns. translation. from mature mRNA
is that pre-mRNA
Very small; support has not undergone
IV. KINDS OF RNA the process. RNA processing.

RNA TYPES ABUNDANCE STABILITY V. DNA TRANSLATION
PROTEIN CODING
5
>10 different Unstable to
mRNA 2% - 5%
species very stable
NON-PROTEIN CODING
Large ncRNA
28s, 18s, 5.8s, 5s
rRNA (found in 80% - 90% Very stable
eukaryotes)
Unstable to
IncRNA = 1000s 1% - 2%
very stable
Small ncRNA RNA-directed synthesis of a polypeptide which involves:
60 different
tRNA 15% Very stable mRNA
species
Ribosomal RNA (rRNA)
30 different Transfer RNA (tRNA)
snRNA < or = 1% Very stable
species Genetic Coding (Codons)
mi/SiRNA 100s-1000 < or = 1% Stable
Importance of DNA Translation

mRNA is not yet a protein so we cannot use it, it has no
purpose to us, and it is just holding the message so we
need to translate that message into the protein that we
need in our body.

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 A. THE GENETIC CODE B. TRANSLATION PROCESS

Properties of the Genetic Code (explained further in lecture 2):

Degenerate: multiple codons decode the same amino
acid.
Unambiguous: a single codon can only code for a
single amino acid.
Non-overlapping: no codons overlap in the reading.
Without punctuation: the code is read continuously
without punctuation.
Universal: Applies to multiple (most) species

1. Initiation

Starts with the interaction of mRNA, tRNA carrying the
first amino acid of the polypeptide, and two subunits of
a ribosome.
A small ribosomal subunit binds to a molecule of
mRNA.
This signals the beginning of polypeptide chain
Genetic Coding Dictionary sequencing.
Four important parts of your translation: mRNA, tRNA,
First suggested by Francis Crick rRNA, genetic Codons
It has a pattern of degeneracy: Anticodon: are the 3 RNA bases that match the 3
○ Example: UUA, UUG, CUU, CUC, CUA, CUG can bases of the mRNA molecule
only code for Leu (Leucine) It starts in the interaction of your mRNA and tRNA,
Francis Crick discovered the Wobble Hypothesis carrying the first amino acids
○ Suggest that the initial two nucleotides of the First it will search for your START codon (AUG), from
triple holds more significance than the 3rd in there it will start translation.
attracting the correct tRNA:
Example: UUG : the first two letters, U
and U are more important than the
third letter G.
In genetic mutations, silent mutation
usually affects the third codon.

Codons

ALWAYS triplets of RNA bases.
Determine which amino acid will be produced.
There are 64 possible codons
START codon (initiator) : AUG (Methionine)
STOP codon : UAA, UAG, UGA 2. Elongation

Once it catches the start codon, it will get the
elongation factors.
A large ribosomal subunit is where reading happens.
As it moves along the line, it connects and as it moves
away, ones that are not inside the ribosomal unit will
be kicked out and those are now the new proteins.
That’s how amino acids are formed.

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Upon recruitment of an elongation factor and the large POSITIVE EFFECTS NEGATIVE EFFECTS
ribosomal subunit, polypeptide chain synthesis progresses:
Source of new alleles Cell death
Codon recognition: anticodon of an incoming Genetic variation Genetic diseases (ex.
aminoacyl tRNA base pairs with the complementary Selective advantage that cancer)
mRNA codon. one specie gains over
Peptide bond formation another
Translocation
A. MOLECULAR TYPES

Substitution Mutation

Occurs when a base at a certain position is replaced by
another. From this, the substituted base will be paired
with its appropriate base-paired partner.
Transition
○ Pyrimidine to Pyrimidine or Purine to Purine
Transversion
○ Pyrimidine to Purine and vice versa
3. Termination

Occurs when a STOP codon in mRNA is encountered. Deletion Mutation
○ The stop codons are UAA, UAG, and UGA. It
only needs to catch one stop codon to stop Occurs when one or more nucleotide pairs in a DNA
and not all 3. molecule are lost or removed
Upon recognition of the Stop codon, a release factor is
given and interacts with the ribosome and polypeptide Insertion Mutations
chain. It attaches to the Stop codon and basically tells
the line that they’re done.
Addition of one or more nucleotide pairs to the DNA
○ It will be clipped away and a new line of
strand
proteins is produced.
From this, the large ribosomal subunits and release
factor are removed and recycled to use with other Inversion Mutations
mRNAs.
○ Elongation, From the start codon A complex 180-degree rotation of a segment of the
(AUG/Methionine), large ribosomal units DNA without a loss or gain in nucleotide number
recognize everything, moves along the line,
and forms peptide bonds then once it finds a B. EFFECT WHEN TRANSLATED TO PROTEINS
stop codon, it connects and then clips it out
and recycles again. Silent Mutations (Synonymous)

C. POST TRANSLATION No detectable change because of the degeneracy of
the code.
Most polypeptides undergo modification before they Mostly a change in the 3rd nucleotide of a codon.
consider their final forms and functions.
These forms (primary, secondary, tertiary, and
quaternary) could be chemical change, folding, or
formation of multi-subunit structures.
Once folded, some are physiologically active as single
subunits while others are then bound to other subunits
to form Quaternary structures (e.g., Hemoglobin).

VI. GENETIC MUTATIONS

Mutations are heritable changes in the nucleotide
sequence of DNA.
Common misconception: mutations are bad.
Mutations can be caused by many things:
○ Genetically: cause is natural, the body just
makes mutations.
○ Environmentally: an example is radiation
poisoning. In Chernobyl, most animals and
plants in the area were exposed to high
amounts of radiation to the point that they
have mutations.

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Missense Mutations (Non-Synonymous) Frameshift Mutation

Occurs when a different amino acid is incorporated A frameshift is a shift in reading frame by insertion or
into site of the protein molecule deletion of a nucleotide (may be one of the two or both)
Acceptable Deletion and insertion of a single nucleotide alters the
○ Resulting protein molecule may not be reading frame.
distinguishable. ○ Reading frames are done in codon triplets.
○ AAA → AAU
Partially Acceptable
○ Will result in a protein molecule with partial
but abnormal function.
○ GAA → GUA
○ The first nucleotide is considered to be the
most important. However, due to the Wobble
Hypothesis, both the first and second
nucleotides are important.
Unacceptable
○ Not capable of normal function.
○ Usually, Genetic mutation of this kind will
cause severe damage to the body.
○ CAU → UAU

Nonsense Mutation

Convert a triple coding for an amino acid into a
terminator.
Premature termination of translation. Suppressor Mutation
○ Effects: protein line will be either too short it
could not be secondary, tertiary, quaternary When the body mutates itself, the body reacts
structures. naturally. The body creates a suppressor mutation to
○ Example: In trying to make hemoglobin then suppress a mutation.
you have a premature Stop, you will have a This can counteract some of the effects of missense,
very non functional hemoglobin structure nonsense, and frameshift mutation.
completely. Very dangerous mutation. ○ Not all suppressor mutations are successful.
Suppressor tRNA molecules, usually formed as a result
of alteration in the anticodon regions, are capable of
suppressing mutations
○ Sometimes they exist but they can’t stop the
mutation.
○ Sometimes mutations are too strong for our
body.

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Buckingham, L. (2019). Molecular diagnostics:
Fundamentals, Methods, and Clinical Applications.
Gersen, S., & Keagle, M. B. (2010). The principles of
clinical cytogenetics. Humana Press.
Klug, W. S., Cummings, M. R., Spencer, C. A., Palladino,
M.A., & Killian, D. (2019). Concepts of Genetics, Global
Edition.
Patalinhug, R (2021). DNA Replication, Transcription
and Translation.
Rosenberg, L. E., & Rosenberg, D. D. (2012). Human
genes and genomes: Science, Health, Society.
Academic Press.
Weil, P. A. (2017). Protein Synthesis & the Genetic
Code. Basic medical Key. Retrieved August 23, 2024,
from
https://basicmedicalkey.com/protein-synthesis-the-ge
netic-code/

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