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1 CHAPTER 11 NUCLEIC ACID STRUCTURE AND DNA REPLICATION Prepared by Brenda Leady, University of Toledo

1 CHAPTER 11 NUCLEIC ACID STRUCTURE AND DNA REPLICATION Prepared by Brenda Leady, University of Toledo

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Page 1: 1 CHAPTER 11 NUCLEIC ACID STRUCTURE AND DNA REPLICATION Prepared by Brenda Leady, University of Toledo

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CHAPTER 11

NUCLEIC ACID

STRUCTURE AND

DNA REPLICATION

Prepared by

Brenda Leady, University of Toledo

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Genetic material must be able to:

Contain the information necessary to construct an entire organism

Pass from parent to offspring and from cell to cell during cell division

Be accurately copied Account for the known variation within and

between species

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Late 1800s scientists postulated a biochemical basis

Researchers became convinced chromosomes carry genetic information

1920s to 1940s expected the protein portion of chromosomes to be the genetic material

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Griffith’s bacterial transformations

Late 1920s Frederick Griffith was working with Streptococcus pneumoniae

S. pneumoniaeStrains that secrete capsules look smooth and

can cause fatal infections in miceStrains that do not secrete capsules look

rough and infections are not fatal in mice

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Rough strains (R) without capsule are not fatal No living bacteria found in

blood Smooth strains (S) with

capsule are fatal Capsule prevents immune

system from killing bacteria Living bacteria found in blood

If mice are injected with heat-killed type S, they survive

Mixing live R with heat-killed S kills the mouse Blood contains living S

bacteria Transformation

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Genetic material from the heat-killed type S bacteria had been transferred to the living type R bacteria

This trait gave them the capsule and was passed on to their offspring

Griffith did not know the biochemical basis of his transforming principle

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Avery, MacLeod, and McCarty used purification methods to reveal that DNA is the genetic material

1940s interested in bacterial transformation Only purified DNA from type S could transform type R Purified DNA might still contain traces of

contamination that may be the transforming principle Added DNase, RNase and proteases RNase and protease had no effect With DNase no transformation DNA is the genetic material

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Hershey and Chase

1952, studying T2 virus infecting Escherichia coliBacteriophage or phage

Phage coat made entirely of protein DNA found inside capsid

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Shearing force from a blender will separate the phage coat from the bacteria

35S will label proteins only 32P will label DNA only Experiment to find what is injected into bacteria-

DNA or protein? Results support DNA as the genetic material

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Levels of DNA structure

1. Nucleotides are the building blocks of DNA (and RNA).

2. A strand of DNA (or RNA) 3. Two strands form a

double helix. 4. In living cells, DNA is

associated with an array of different proteins to form chromosomes.

5. A genome is the complete complement of an organism’s genetic material.

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Nucleotides

3 componentsPhosphate groupPentose sugarNitrogenous base

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DNA 3 components

Phosphate groupPentose sugar

DeoxyriboseNitrogenous base

Purines Adenine (A),

guanine (G) Pyrimidines

Cytosine (C), thymine (T),

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RNA 3 components

Phosphate groupPentose sugar

RiboseNitrogenous base

Purines Adenine (A),

guanine (G) Pyrimidines

Cytosine (C), uracil (U)

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Conventional numbering system Sugar carbons 1’ to 5’ Base attached to 1’ Phosphate attached to 5’

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Strands

Nucleotides covalently bonded

Phosphodiester bond – phosphate group links 2 sugars

Phosphates and sugars from backbone

Bases project from backbone Directionality- 5’ to 3’ 5’ – TACG – 3’

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Solving DNA structure

1953, James Watson and Francis Crick, with Maurice Wilkins, proposed the structure of the DNA double helix

Watson and Crick used Linus Pauling’s method of working out protein structures using simple ball-and-stick models

Rosalind Franklin’s X-ray diffraction results provided crucial information

Erwin Chargoff analyzed base composition of DNA that also provided important information

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Watson and Crick put together these pieces of information

Found ball-and-stick model consistent with data

Watson and Crick awarded Nobel Prize in 1962

Rosalind Franklin had died and the Nobel is not awarded posthumously

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DNA isDouble strandedHelicalSugar-phosphate

backboneBases on the insideStabilized by

hydrogen bondingBase pairs with

specific pairing

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AT/GC or Chargoff’s rule A pairs with T G pairs with C

Keeps with consistent 10 base pairs per turn 2 DNA strands are

complementary 5’ – GCGGATTT – 3’ 3’ – CGCCTAAA – 5’

2 strands are antiparallel One strand 5’ to 3’ Other stand 3’ to 5’

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Space-filling model shows groovesMajor groove

Where proteins bindMinor groove

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Replication

3 different models for DNA replication proposed in late 1950sSemiconservativeConservativeDispersive

Newly made strands are daughter strands Original strands are parental strands

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In 1958, Matthew Meselson and Franklin Stahl devised experiment to differentiate among 3 proposed mechanisms

Nitrogen comes in a common light form (14N) and a rare heavy form (15N)

Grew E.coli in medium with only 15N Then switched to medium with only 14N Collected sample after each generation Original parental strands would be 15N while

newly made strands would be 14N Results consistent with semiconservative

mechanism

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During replication 2 parental strands separate and serve as template strands

New nucleotides must obey the AT/GC rule

End result 2 new double helices with same base sequence as original

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Origin of replication Site of start point for

replication Bidirectional

replication Replication proceeds

outward in opposite directions

Bacteria have a single origin

Eukaryotes require multiple origins

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Origin of replication provides an opening called a replication bubble that forms two replication forks

DNA replication occurs near the fork Synthesis begins with a primer Proceeds 5’ to 3’ Leading strand made in direction fork is

movingSynthesized as one long continuous molecule

Lagging strand made as Okazaki fragments that have to be connected later

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DNA helicase Binds to DNA and

travels 5’ to 3’ using ATP to separate strand and move fork forward

DNA topoisomerase Relives additional coiling

ahead of replication fork Single-strand binding

proteins Keep parental strands

open to act as templates

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DNA polymeraseCovalently links nucleotides

Deoxynuceloside triphosphates

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Deoxynuceloside triphosphatesFree nucleotides with 3 phosphate groupsBreaking covalent bond to release pyrophosphate (2 phosphate

groups) provides energy to connect adjacent nucleotides

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DNA polymerase has 2 enzymatic features to explain leading and lagging strands

1. DNA polymerase unable to begin DNA synthesis on a bare template strand

DNA primase must make a short RNA primer RNA primer will be removed and replaced with DNA

later

2. DNA polymerase can only work 5’ to 3’

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In the leading strandDNA primase makes one RNA primerDNA polymerase attaches nucleotides in a 5’ to 3’

direction as it slides forward In the lagging strand

DNA synthesized 5’ to 3’ but in a direction away from the fork

Okazaki fragments made as a short RNA primer made by DNA primase at the 5’ end and then DNA laid down by DNA polymerase

RNA primers will be removed by DNA polymerase and filled in with DNA

DNA ligase will join adjacent DNA fragments

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DNA replication is very accurate

3 reasons1. Hydrogen bonding between A and T or G

and C more stable than mismatches2. Active site of DNA polymerase unlikely to

form bonds if pairs mismatched3. DNA polymerase removes mismatched pairs

Proofreading results in DNA polymerase backing up and digesting linkages

Other DNA repair enzymes

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The family of DNA polymerases

3 important issues for DNA polymerase are speed, fidelity, and completeness

Nearly all living species have more than 1 type of DNA polymerase

Genomes of most species have several DNA polymerase genes due to gene duplication

Independent genetic changes produce enzymes with specialized functions suited to the organism

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E. coli has 5 DNA polymerasesDNA polymerase III with multiple subunits responsible

for majority of replicationDNA polymerase I has a single subunit whose job is to

rapidly remove RNA primers and fill in DNADNA polymerases II, IV and V are involved in DNA

repair and replicating damaged DNA DNA polymerases I and III stall at DNA damage DNA polymerases II, IV and V don’t stall but go slower and

make sure replication is complete

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Humans have 12 or more DNA polymerasesDesignated with Greek lettersDNA polymerase α has its own built in primase subunitDNA polymerase δ and ε extend DNA at a faster rateDNA polymerase γ replicates mitochondrial DNAWhen DNA polymerases α, δ or ε encounter

abnormalities they may be unable to replicateLesion-replicating polymerases may be able to

synthesize complementary strands to the damaged area

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Specialized form of DNA replication only in eukaryotes in the telomeres

Telomeres are a series of repeat sequences within DNA and special proteins

Telomere at 3’ does not have a complementary strand and is called a 3’ overhang

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DNA polymerase cannot copy the tip of the DNA strand with a 3’ endNo place for upstream primer to be made

If this replication problem were not solved, linear chromosomes would become progressively shorter

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Telomerase prevents chromosome shortening

Attaches many copies of repeated DNA sequences to the ends of the chromosomes

Provides upstream site for RNA primer

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Telomeres and aging

Body cells have a predetermined life span Skin sample grown in a dish will double a

finite number of times Infants, about 80 timesOlder person, 10 to 20 times

Senescent cells have lost the capacity to divide

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Progressive shortening of telomeres correlated with cellular senescence

Telomerase present in germ-line cells and in rapidly dividing somatic cells

Telomerase function reduces with age Inserting a highly active telomerase gene into

cells in the lab causes them to continue to divide

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Telomeres and cancer

When cells become cancerous they divide uncontrollably

In 90% of all types of human cancers, telomerase is found at high levels

Prevents telomere shortening and may play a role in continued growth of cancer cells

Mechanism unknown