1. D. Replication at the Molecular Level

2. 1. Replication in E. coli a. A specific sequence of bases is recognized as the binding site for the replication complex – this is called the Replication Origin, and the DNA replicated from this site is called a replicon.

3. D. Replication at the Molecular Level 1. Replication in E. coli a. A specific sequence of bases is recognized as the binding site for the replication complex – this is called the Replication Origin, and the DNA replicated from this site is called a replicon. - Bacteria have only a single replication origin, and the entire circular chromosome is replicated from this point.

4. 1. Replication in E. coli a. Replication Origin has 9-mers and 13- mers – homologous sequences… b. Three enzymes (DNaA,B, C), collectively called “helicases” bind to the origin and break the hydrogen bonds holding the helices together. “Single-strand binding proteins” stabilize the DNA.

5. 1. Replication in E. coli a. Replication Origin has 9-mers and 13- mers – homologous sequences… b. Three enzymes (DNaA,B, C), collectively called “helicases” bind to the origin and break the hydrogen bonds holding the helices together. “Single-strand binding proteins” stabilize the DNA. c. The enzyme gyrase works downstream, cutting single or double strands to relieved the torque on the molecule. (topoisomerases affect shape).

6. 1. Replication in E. coli d. DNA Polymerases: There are 5 enzymes that can lengthen a DNA strand by adding new bases. The first was isolated in 1957 by A. Kornberg (1959 Nobel) – DNA Polymerase I.

7. 1. Replication in E. coli d. DNA Polymerases: There are 5 enzymes that can lengthen a DNA strand by adding new bases. The first was isolated in 1957 by A. Kornberg (1959 Nobel) – DNA Polymerase I.

8. 1. Replication in E. coli d. DNA Polymerases: There are 5 enzymes that can lengthen a DNA strand by adding new bases. The first was isolated in 1957 by A. Kornberg (1959 Nobel) – DNA Polymerase I. DNA Poly III is the primary replication enzyme, but I-V have repair functions

9. 1. Replication in E. coli d. DNA Polymerases: And note that NONE can initiate chain synthesis!!!!

10. 1. Replication in E. coli d. DNA Polymerases: There are 5 enzymes that can lengthen a DNA strand by adding new bases. The first was isolated in 1957 by A. Kornberg (1959 Nobel) – DNA Polymerase I. DNA Poly III is the primary replication enzyme, but I-V have repair functions DNA Poly’s are very complex enzymes with multiple polypeptides and functional groups. And actually, two DNA Poly III enzymes work in parallel as a DIMER

11. 1. Replication in E. coli d. DNA Polymerases: The DNA Polymerases, the helicases and Gyrase, the Stabilization Proteins, and other enzymes we’ll mention form a HUGE functional replication unit = Replisome

12. D. DNA Replication at the Molecular Level 1. Replication in E. coli 2. The Process – Replication at the fork: a. Initiation: i. Helicases bind and separate helices, stabilizing protein stabilize the single strands, gyrase relives torque ii. Primase, an RNA Polymerase, begins synthesis of an RNA strand in the 5’  3’ direction on both strands: 3’ 5’3’

13. 2. The Process – Replication at the fork: a. Initiation: b. Polymerization: NOW, with a free-3’-OH to add bases to, DNA Polymerase III displaces the Primase and adds DNA bases to extend the new helix in both directions (@50,000 bases/min!):

14. 2. The Process – Replication at the fork: a. Initiation: b. Polymerization: the B-subunit of DNA Poly III “is a “sliding clamp” that holds the enzymes on the helices:

15. videos Video 1 – pick up at 2:30 Video 2

16. 2. The Process a. Initiation: b. Polymerization: As the replisome moves down the helix, replication is continuous on the “leading strand”, 5’  3’, and discontinuous on the “lagging strand” (though the new strand is still synthesized 5’  3’).

17. 2. The Process a. Initiation: b. Polymerization: As the replisome moves down the helix, replication is continuous on the “leading strand”, 5’  3’, and discontinuous on the “lagging strand” (though the new strand is still synthesized 5’  3’). The short sections of discontinuously synthesized DNA are called “Okazaki Fragments”.

18. 2. The Process a. Initiation: b. Polymerization: As the replisome moves down the helix, replication is continuous on the “leading strand”, 5’  3’, and discontinuous on the “lagging strand” (though the new strand is still synthesized 5’  3’). The short sections of discontinuously synthesized DNA are called “Okazaki Fragments”. This is what is happening at one fork; how about the other?

19. 2. The Process a. Initiation: b. Polymerization: c. Repair: The RNA must be removed… 5’3’ 5’

20. 2. The Process a. Initiation: b. Polymerization: c. Repair: DNA Poly I, with 5’  3’ exonuclease capability, cuts out the RNA primer… 5’3’ 5’3’5’

21. 2. The Process a. Initiation: b. Polymerization: c. Repair: DNA Poly I, with 5’  3’ exonuclease capability, cuts out the RNA primer…DNA Poly I and II, “fill the gap” with DNA bases, using the free-3’-OH group on the last DNA base to add bases to.... the epsilon subunit is critical in repair… 5’3’ 5’3’5’

22. 2. The Process a. Initiation: b. Polymerization: c. Repair: DNA Poly I, with 5’  3’ exonuclease capability, cuts out the RNA primer…DNA Poly I and II, “fill the gap” with DNA bases, using the free-3’-OH group on the last DNA base to add bases to… then Ligase make the last phosphodiester bond, linking the fragments of DNA together. 5’3’ 5’

23. 2. The Process a. Initiation: b. Polymerization: c. Repair: d. Termination: With a circular chromosome (bacteria), it is easy to complete the process.

24. D. Replication at the Molecular Level 1. Replication in E. coli 2. The Process - Replication at the fork 3. Modifications in Eukaryotes

25. D. Replication at the Molecular Level 1. Replication in E. coli 2. The Process - Replication at the fork 3. Modifications in Eukaryotes a. Multiple Origins - with 10 3 – 10 6 times as many bases, multiple origins to speed the replication process by simultaneous replicon replication.

26. D. Replication at the Molecular Level 1. Replication in E. coli 2. The Process - Replication at the fork 3. Modifications in Eukaryotes a. Multiple Origins - with 10 3 – 10 6 times as many bases, multiple origins to speed the replication process by simultaneous replicon replication. - mammalian cells have 25,000 replicons; in eukaryotes these are Autonomously Replicating Sequences (ARS).

27. D. Replication at the Molecular Level 1. Replication in E. coli 2. The Process - Replication at the fork 3. Modifications in Eukaryotes a. Multiple Origins - with 10 3 – 10 6 times as many bases, multiple origins to speed the replication process by simultaneous replicon replication. - mammalian cells have 25,000 replicons; in eukaryotes these are Autonomously Replicating Sequences (ARS). - How are they found by the replisome? - proteins bind to these specific sequences/regions during the G1 phase – these proteins form an “Origin Recognition Complex” (ORC).

28. D. Replication at the Molecular Level 1. Replication in E. coli 2. The Process - Replication at the fork 3. Modifications in Eukaryotes a. Multiple Origins - with 10 3 – 10 6 times as many bases, multiple origins to speed the replication process by simultaneous replicon replication. - mammalian cells have 25,000 replicons; in eukaryotes these are Autonomously Replicating Sequences (ARS). - How are they found by the replisome? - proteins bind to these specific sequences/regions during the G1 phase – these proteins form an “Origin Recognition Complex” (ORC). - at the onset of the S phase, protein kinase enzymes bind and form a ‘pre-replication complex’ that binds the DNA Polymerase and helicases and initiates replication. The activated kinases, bound with the replisome, inhibit the formation of more pre-RC, so replication of a region occurs only once.

29. D. Replication at the Molecular Level 1. Replication in E. coli 2. The Process - Replication at the fork 3. Modifications in Eukaryotes a. Multiple Origins b. Histone Complexes: - The ‘core’ DNA bound to histones in a nucleosome must be unwound to be replicated. After this occurs, new histones are made to bind the new double-helices.

30. D. Replication at the Molecular Level 1. Replication in E. coli 2. The Process - Replication at the fork 3. Modifications in Eukaryotes a. Multiple Origins b. Histone Complexes: c. Polymerase Production - base replication rates are 25x slower in eukaryotes - but they have multiple origins and 50,000 x as many Polymerase III enzymes…so the process occurs faster at a cellular level.

31. 3. Modifications in Eukaryotes a. Multiple Origins b. Histone Complexes: c. Polymerase Production d. Telomere Replication - Problem: shortening chromosomes RNA primer

32. 3. Modifications in Eukaryotes a. Multiple Origins b. Histone Complexes: c. Polymerase Production d. Telomere Replication - Problem: shortening chromosomes - This is bad, because intact telomeres protect the chromosomes from degradation and end-end fusion (translocations).

33. d. Telomere Replication - Problem: shortening chromosomes - This is bad, because intact telomeres protect the chromosomes from degradation and end-end fusion (translocations). - Telomerase is a ribonucleoprotein, with an enzymatic RNA molecule coupled to a protein.

34. d. Telomere Replication - Problem: shortening chromosomes - This is bad, because intact telomeres protect the chromosomes from degradation and end-end fusion (translocations). - Telomerase is a ribonucleoprotein, with an enzymatic RNA molecule coupled to a protein. The RNA has several repeats of CCCCAA, which act as a template for the formation of GGGGTT DNA in the process of reverse transcription (reading RNA and making DNA).

35. d. Telomere Replication - Problem: shortening chromosomes - This is bad, because intact telomeres protect the chromosomes from degradation and end-end fusion (translocations). - Telomerase is a ribonucleoprotein, with an enzymatic RNA molecule coupled to a protein. The RNA has several repeats of AACCCC, which act as a template for the formation of TTGGGG DNA in the process of reverse transcription (reading RNA and making DNA). The process continues, forming a long and non-coding platform for primase to begin discontinuous synthesis.

36. d. Telomere Replication - Problem: shortening chromosomes - Curiously, most mature cells lack telomerase. The shortening of chromosomes may be a signal, or an inhibitor, that prevents further cell division. GOOD because mutations accumulate in a lineage with each division BAD because it reduces rate of tissue repair = AGING

37. - The shortening of telomeres correlates with aging... and organisms may live longer if their telomeres are longer and their cells are capable of more cell divisions. Genetically engineered to over-express telomere binding protein

38. Relationship between mean telomere length (± SEM, measured by T/S ratio using qPCR) and age at measurement in 99 zebra finches. Heidinger B J et al. PNAS 2012;109:1743-1748 ©2012 by National Academy of Sciences Length declines with age

39. Relationship between natural log-transformed relative telomere length (T/S ratio from qPCR) at 25 d and lifespan in zebra finches (n = 99). Heidinger B J et al. PNAS 2012;109:1743-1748 ©2012 by National Academy of Sciences Individuals with longer telomeres live longer

40. Relationship between mean (± SEM) telomere length (T/S ratio from qPCR) and age at measurement (first sample, shown as year = 0, was collected at 25 d) in zebra finches in three lifespan categories. Heidinger B J et al. PNAS 2012;109:1743-1748 ©2012 by National Academy of Sciences Green = mean lifespan of 1.6 yrs Red = mean lifespan of 3.6 yrs Black = mean lifespan of 6.3 yrs And, short life correlates with shorter telomeres

41. HOW might telomere length influence division of cells?

42. Telomere shortening activates p53 and drives formation of epithelial cancers through gene amplification and deletion. Artandi S E, and DePinho R A Carcinogenesis 2009;31:9- 18 © The Author 2009. Published by Oxford University Press. All rights reserved. For Permissions, please email: journals.permissions@oxfordjournals.org Telomere shortening drive p53 activation

43. Trade-off between CANCER (high division) and AGING/TISSUE DAMAGE (no division) Telomeres: - p53 is a tumor suppressor. - Tyner (et al. 2002): - mice who were deficient in p53 were susceptible to cancer (no repair). - They also isolated a strain that had overproduction of p53. These mutants had a reduce susceptibility to cancer, but they aged more rapidly than normal mice.