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DNA Form & Function.

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Presentation on theme: "DNA Form & Function."— Presentation transcript:

1 DNA Form & Function

2 DNA: Structure & Replication
Understanding DNA replication – and the resulting transmission of genetic information from cell to cell, and generation to generation – lays the groundwork for understanding the principles of heredity Understanding DNA structure and replication is a prerequisite for understanding/using the principal tools of molecular biology R RR R0 00 R R0

3 DNA: Structure & Replication
Three features of DNA makes it an ideal genetic material Faithful replication Information content Capable of change

4 DNA: Nucleotides Overall structure

5 DNA: Nucleotides Bases

6 DNA: Nucleotides Bases
The combination of a base and a pentose sugar is a nucleoside

7 Nucleotide + Nucleotide + Nucleotide + ……
DNA: Polymerisation Nucleotide + Nucleotide + Nucleotide + ……

8 DNA: Replication Complementary base pairing and the double helix
Replication is semi-conservative

9 DNA: Synthesis Essentials
DNTPs: dATP, dGTP, dTTP, and dCTP Template DNA (a pre-existing single strand) DNA polymerase 1. DNTPs

10 2. Template DNA (a pre-existing single strand)
DNA: Synthesis Essentials 2. Template DNA (a pre-existing single strand) ATCGGTCAACGTTAAAGTTAGCGG

11 DNA: Synthesis Essentials
3. DNA Polymerases There are multiple forms of DNA polymerase Different forms have different activities Replicases have direct roles in replication Others have secondary roles in replication and/or repair synthesis. DNA replication – polymerization of deoxyribonucleotides Polymerases catalyze the formation of a phosphodiester bond between the 3'-OH of the deoxyribose on the last nucleotide and the 5' phosphate of the dNTP precursor Process is repeated forming a synthesized DNA chain

12 3. DNA Polymerases (continued)
DNA: Synthesis Essentials 3. DNA Polymerases (continued) Polymerase binds to the DNA template strand and moves along as the synthesisied polynucleotide chain grows At each template base, the dNTP precursor is identified that can base pair with it The frequency of error is low, but errors can occur. Polymerases can have exonuclease activity (removal of nucleotides from the 3' end of the chain) This is a proof-reading mechanism An unpaired nucleotide from the 3'OH end of the growing chain triggers exonuclease activity The unpaired nucleotide is cleaved from the end of the growing chain by the polymerase.

13 DNA: Synthesis Essentials
Replication is 5’ to 3’

14 DNA: Synthesis Essentials
Replication is 5’ to 3’

15 DNA: Synthesis Essentials
Replication is 5’ to 3’

16 DNA: Synthesis Essentials
Replication is 5’ to 3’

17 DNA: Synthesis Essentials
Replication is 5’ to 3’

18 DNA: Synthesis Essentials
Replication is 5’ to 3’

19 DNA Replication: 1-Origins
Replication begins at a fixed point, called the origin, and proceeds bi-directionally. In a higher plant chromosome there are thousands of origins. Consider The size of the genome The rate of DNA replication The length of the S phase  

20 DNA Replication: 1-Origins

21 DNA Replication: 1-Origins

22 DNA Replication: 1-Origins

23 DNA Replication: 1-Origins

24 Replication: 2-Unwinding, 3-Stabilisation
Unwinding: The DNA helix needs to be opened up. This is accomplished by helicase enzymes, which break the hydrogen bonds holding the two strands of the helix together. Gyrase facilitates helicase action by relieving tension in coiled DNA Stabilization: The unwound DNA is stabilized by a protein (single strand binding protein (SSB)), which speeds up DNA replication.

25 Replication: 4 - Priming
Primases form a short RNA primer DNA polymerases use the primer to synthesise a new chain Polymerases cannot start synthesis on their own RNA primers subsequently removed by exonuclease activity of a polymerase and replaced with DNA

26 Replication: 5 – Leading & Lagging Strands
DNA polymerases synthesize new chains only from 5' to 3‘ DNA molecule is antiparallel and DNA synthesis is semi-conservative. DNA synthesis is continuous on 5’-3’ strand - leading strand Synthesis discontinuous on 3’-5’ strand - lagging strand Multiple priming sites on the lagging strand DNA therefore formed in fragments on lagging strand - Okazaki fragments

27 Replication: 5 – Leading & Lagging Strands

28 Replication: 5 – Leading & Lagging Strands

29 Replication: 5 – Leading & Lagging Strands

30 Replication: 5 – Leading & Lagging Strands

31 Replication: 5 – Leading & Lagging Strands

32 Replication: 5 – Leading & Lagging Strands

33 Replication: 5 – Leading & Lagging Strands

34 Replication: 6 Termination
DNA Pol I exonuclease removes RNA Primers in lagging strand DNA Polymerase adds complementary nucleotides to fill the gaps DNA Ligase adds phosphate in the remaining gaps of the phosphate - sugar backbone Can’t backfill RNA primer site at telomere of lagging strand Telomere shortening during replication Role of Telomerase

35 The telomerase solution

36 Replication: 7 Proof-Reading
Mis-matched bases can be added in error during polymerisation Specific polymerases with 3’-5’ exonuclease activity identify and remove any detected mis-matches on the synthesized strand Proofreading starts at the 3' end of the synthesised strand and proceeds 3’ -> 5’ Two exact copies of original, each with one original and one new strand

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