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Anfinsen Experiment: Denature ribonuclease (RNase) Remove denaturant Assay for RNase activity -- does the protein regain its 3-D structure and its enzymatic activity?. Proteins: Sequence --> Structure --> Function. Molecular chaperones - Anfinsen cages for folding proteins. - PowerPoint PPT Presentation
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Proteins: Sequence --> Structure --> Function
Anfinsen Experiment: Denature ribonuclease (RNase)Remove denaturantAssay for RNase activity -- does the protein regain its 3-D structure and its enzymatic activity?
GroEL-GroES-(ADP)7 complexXu et al., 1997, Nature 388: 741
Molecular chaperones - Anfinsen cages for folding proteins
Inverse Protein Folding ProblemInverse Protein Folding Problem
• Given a structure (or a functionality), identify an amino acid sequence whose fold will be that structure (exhibit that functionality).
• Can we make designer proteins with desired functions?
Central dogma I -- Replication
• DNA -> RNA -> protein• But for retroviruses, DNA can also be
made by reverse transcription of RNA.• To understand the lifecycle of a
retrovirus, we need to know more about how DNA is replicated and transcribed, and how RNA is translated into protein.
Vocabulary• Replication -- copying DNA before
cell division• Transcription -- making an RNA
copy (messenger RNA or mRNA) of DNA
• Translation -- making a protein from the mRNA
DNA ---------> DNADNA ---------> RNA ----------> ProteinRNA ---------> DNA
transcription translation
reversetranscription
replication
Polymerase enzymes
DNA ---------> DNA
DNA ---------> RNA
RNA ---------> DNA
transcription
reversetranscription
replication (DNA polymerase plus other proteins)
(HIV reverse transcriptase)
(RNA polymerase plus other proteins)
HIV reverse transcriptase (RT) is a RNA-dependent DNA polymerase with many similarities to host cell DNA polymerase, therefore we will discuss RT in this lecture.
Genes are the functional units of heredity
• The genetic information carried in DNA must be duplicated before a cell can produce two genetically identical daughter cells.
• The genetic information carried in DNA is in the form of genes: a gene is a segment of DNA containing the instructions for making a protein or set of closely-related proteins.
• Cells contain elaborate machines to accurately copy or replicate their DNA and to repair it when it is damaged (e.g., by chemicals or environmental radiation).
The structure of DNA explains how genetic information is copied
• Each strand of the DNA double helix is complementary to its partner strand, so each can act as a template for synthesis of a new complementary strand (“semi-conservative” replication).
• Base-pairing allows a simple way for cells to pass on their genes to descendents.
What you need to remember about DNA structure to understand replication
Clicker question
DNA can be used to:
A) Code for proteinsB) Make origami picturesC) Build smaller, faster computersD) All of the above
Clicker question
DNA can be used to:
A) Code for proteinsB) Make origami picturesC) Build smaller, faster computersD) All of the above
B & C will be discussed in the next lecture
DNA replication
• Begins at an A-T rich replication origin.
• Initiator proteins bind and separate the two DNA strands.
• A protein machine containingDNA polymerase is assembled.
• DNA polymerase synthesizesnew DNA using one old strand as a template.
• Replication forks move bidirectionally from origins of replication.
Clicker questionWhy are origins of replication AT-rich?
A) DNA polymerase binds AT basepairs with high affinity.
B) AT-rich regions are easier to copy.C) The free energy required to separate AT-rich
regions is lower than for GC-rich regions.D) Origins always start with the first letter of the
alphabet, hence they must start at an “A”.E) DNA is almost entirely AT-rich, so there’s a
higher probability that replication will begin at an AT-rich than a GC-rich region.
DNA always synthesized in 5’ to 3’ direction
• A new deoxyribonucleotide is always added to the 3’ OH end of the new strand.• One new DNA strand at the replication fork is made on a template that runs 3’ to 5’; the other strand is made on a template that runs 5’ to 3’.
How can the top strand be made in the direction of
the replication fork?
Clicker question
DNA must be synthesized in the 5’ to 3’ direction. How is it possible to make two new strands, both going in the direction of the replication fork?
A) The top strand is synthesized backwards.B) The top strand makes a parallel double helix with the
DNA strand from the parental helix. C) The top strand is synthesized in short 5’ - 3’ pieces, then
stitched together.D) Individual nucleotides basepair with the top strand in the
parental DNA helix, then covalently bond with each other to form a new strand.
One DNA strand is synthesized continuously; the other in synthesized discontinuously and then stitched
together
Leading strand: DNA strand that is synthesized continuously in the direction of replication fork.Lagging strand: DNA strand that is synthesized discontinuously (Okazaki fragments), then stitched together.
5’
5’ 3’3’
DNA polymerase video
DNA polymerase is part of a protein machine that replicates DNA --
Sliding clamp is another component
DNA replication (DNA interactive video)
DNA polymerase corrects its mistakes to avoid mutations
• DNA polymerase error rate: 1 mistake per 107 nucleotides.– Proofreading activity of DNA
polymerase: if it adds an incorrect nucleotide, it cleaves the phophodiester bond (acts as a 3’ - 5’ exonuclease as well as a polymerase), then tries again.
• DNA replication error rate including mismatch repair: 1 mistake per 109 nucleotides.
DNA polymerase structure shows separate sites for DNA synthesis and for
editing
“E” is the catalytic site for the error-correcting
exonuclease activity.
“P” is the catalytic site for the polymerization
activity.
DNA Mismatch Repair System serves as a backup to prevent copying
mistakes• Fidelity of DNA replication increases 100-fold when add in
mismatch repair system: 1 mistake in 107 nucleotides for DNA polymerase alone compared with 1 mistake in 109 nucleotides.
What is the problem with mutations?
• Genetic changes are what drive evolution -- they allow organisms to adapt to changing conditions and colonize new habitats.
• BUT … from the perspective of a single organism (e.g., you or me), a permanent genetic change (mutation) can have profoundly negative consequences:– Sickle cell anemia, an inherited disease, is caused by a change
in one nucleotide leading to a single amino acid change in hemoglobin.
– Cancers are caused by a gradual accumulation of random mutations in DNA of somatic* cells.
• From the perspective of a virus, mutations are great because they allow emergence of rare variants that have increased fitness and/or can evade the host immune system more effectively.
*Somatic cells are all the cells in an organism other than germ cells (the reproductive cells).
HIV reverse transcriptase is a low-fidelityDNA polymerase with no proof-reading activity
All polymerases have a common architectural framework consisting of three canonical subdomains termed the fingers, palm, and thumb subdomains.
HIV RT is a DNA polymerase that can use DNA or RNA as a template.
*p66 subunit of HIV RT
Kohlstaedt et al., 1992, Science 256, 1783-1790
Klenow fragment of DNA pol
*Note on nomenclature: proteins are often named pX, where X is the molecular weight in kilodaltons.
Reverse transcription is critical for the lifecycle of a retrovirus
Structural studies of HIV reverse transcriptase
• RT is a heterodimer containing two subunits: p66 and p51(p51 is derived from p66 by proteolytic cleavage).Note on nomenclature: proteins are often named pX, where X is the molecular weight in kilodaltons.• Polymerase domains p66
and p51 each contain fingers, palm and thumb subdomains.
• Cleft between subdomains in p61 polymerase domain binds template-primer.• Cleft is closed in p51 subunit.• p51 contains only a polymerase domain.
• p66• includes a C-terminal RNase H domain, which degrades the RNA strand of an RNA/DNA hybrid.
Tantillo et al., 1994, J. Mol. Biol. 243: 369-387
HIV reverse transcriptase -- Two enzymes in one
After building a DNA strand from the RNA template using polymerase activity, the RNase activity destroys the RNA strand, then a second DNA strand is constructed from the first by the polymerase.
http://www.rcsb.org/pdb/static.do?p=education_discussion/molecule_of_the_month/pdb33_2.html
HIV reverse transcriptase has no proof-reading activity
• In vitro assays suggest error rates of ~1/1700 nucleotides (compare with 1/10,000,000 for DNA polymerase).
• Base substitution, addition, deletion errors.• Some template positions are mutational hotspots
with error rates of 1/70 nucleotides.• The exceptional diversity of the HIV-1 genome
results from error-prone reverse transcription.• Most of the mutant viruses are inferior or not viable,
but some are better than the parental virus at escaping from the immune system or from anti-viral drugs. Natural selection at work!
Roberts et al., 1988, Science 242: 1171-1173.
What should you target to make an anti-viral drug?
A) An activity that is critical for viral functionB) An activity that is virally-encodedC) An activity that is not similar to host
activitiesD) All of the above
Clicker question
What should you target to make an anti-viral drug?
A) An activity that is critical for viral functionB) An activity that is virally-encodedC) An activity that is not similar to host
activitiesD) All of the above
Logical candidate for an anti-retroviral drug: Reverse transcriptase
Clicker question
Reverse transcriptase inhibitorsRT inhibitors prevent synthesis of double stranded viral DNA, thus
prevent HIV from multiplying
• Nucleoside analog RT inhibitors (NARTIs or NRTIs)– Competitive substrate inhibitors
Lacks 3’ OH so causes chain terminationExample: AZT, the first anti-HIV drug
– Conversion to nucleotide by phosphorylation in body can cause toxicity
• Nucleotide analog RT inhibitors (NtARTIs or NtRTIs)– Competitive substrate inhibitors
Lacks 3’ OH so causes chain termination– Doesn’t need to be converted by body, so
less toxic• Non-nucleoside RT inhibitors (NNRTIs)
– Non-competitive substrate inhibitors– Not incorporated into viral DNA– Inhibit polymerase through conformational changes in active
site
Crystal structure of HIV RT bound to Nevirapine, a NNRTI that binds near, but not in, the polymerase
active site
http://www.rcsb.org/pdb/static.do?p=education_discussion/molecule_of_the_month/pdb33_2.html
PDB code 1jlb
The PDB contains >100 RT/inhibitor complexes.
FDA-approved reverse transcriptase inhibitors
http://www.hivandhepatitis.com/hiv_and_aids/hiv_treat.html
What should you target to make an anti-viral drug?
• An activity that is critical for viral function• An activity that is virally-encoded• An activity that is not similar to host activities
but RT is a polymerase similar to host polymerases…
– Fortunately NRTIs and NtRTIs bind RT more tightly (higher affinity) than they bind DNA polymerase.– Also if they did get incorporated by DNA polymerase, NRTIs would be removed from host cell DNA during DNA repair.– HOWEVER -- mitochondrial DNA is replicated by polymerase gamma, which binds NRTIs, so mitochondrial DNA can be damaged, resulting in cell death due to low energy production.
• Different NRTIs affect mitochondria of different types of cells, so have different side effects.
Side effects of some reverse transcriptase inhibitors include:
• Headaches, high blood pressure, nausea, vomiting, fatigue (can disappear with time)• Less frequent, but more serious side effects include anemia (shortage of red blood cells), myopathy (muscle pain and weakness), neutropenia (low number of neutrophils)
Note: RT inhibitors are usually used in combination with other types of anti-retroviral drugs (protease or fusion inhibitors).