1 / 52

FCH 532 Lecture 4

FCH 532 Lecture 4. Chapter 5: DNA. The Watson and Crick double helix model for DNA. Forces in DNA Double Helix. DNA Double helix is stabilized by two types of forces: H-bonds between complementary bases on opposite strands: 2 H-bonds in A-T pair 3 H-bonds in G-C pair

irisa
Télécharger la présentation

FCH 532 Lecture 4

An Image/Link below is provided (as is) to download presentation Download Policy: Content on the Website is provided to you AS IS for your information and personal use and may not be sold / licensed / shared on other websites without getting consent from its author. Content is provided to you AS IS for your information and personal use only. Download presentation by click this link. While downloading, if for some reason you are not able to download a presentation, the publisher may have deleted the file from their server. During download, if you can't get a presentation, the file might be deleted by the publisher.

E N D

Presentation Transcript


  1. FCH 532 Lecture 4 Chapter 5: DNA

  2. The Watson and Crick double helix model for DNA

  3. Forces in DNA Double Helix • DNA Double helix is stabilized by two types of forces: • H-bonds between complementary bases on opposite strands: • 2 H-bonds in A-T pair • 3 H-bonds in G-C pair • Van der Waals forces and hydrophobic interactions between “stacked bases” • Aromatic bases have p-electrons that interact via attractive Van der Waals forces.

  4. Structure of DNA determines heredity • Watson-Crick bp structure will allow any sequence on one polynucleotide strand as long as the opposite strand has complementary sequence. • Each polynucleotide strand can act as the template for its complementary strand. • In order to replicate, the parental strands must separate so that a complementary daughter strand can be synthesized on each parent strand. • Results in duplex (double-stranded) DNA consisting of one polynucleotide parental strand from the parental molecule and another from the newly synthesized daughter strand. • This is called semi-conservative replication. • Shown by the Meselson-Stahl experiment in 1958. • Increased density of DNA by labeling with 15N and monitored the overall DNA density as a function of growth using equilibrium density gradient centrifugation.

  5. Page 89

  6. Denaturation and renaturation • Duplex DNA can be heated above a certain temperature to separate the complementary strands into a random coil conformation. • Denaturation is followed by a change in the physical properties of DNA.

  7. Figure 5-14 Schematic representation of the strand separation in duplex DNA resulting from its heat denaturation. Page 90

  8. Denaturation is cooperative • DNA can be monitored by UV absorbance. • When DNA denatures, UV abs is due to aromatic bases and increases compared to the double stranded DNA • Results from disruptions of electronic interactions among nearby bases. • This is called the hyperchromic effect.

  9. Figure 5-15 UV absorbance spectra of native and heat-denatured E. coli DNA. Page 90

  10. Denaturation is cooperative • The hyperchromic effect takes place over a narrow temperature range. • Indicates that collapse of one part of the DNA duplex will destabilize the rest of the structure (cooperative process). • Melting curves are used to demonstrate the stability of the DNA double helix and determine the melting temperature (Tm) which is the midpoint of a melting curve. • Tm is dependent on the • solvent • concentrations and types of ions • pH • Mole fraction of GC base pairs

  11. Figure 5-16 Example of a DNA melting curve. Page 90

  12. Denaturation is cooperative • The hyperchromic effect takes place over a narrow temperature range. • Indicates that collapse of one part of the DNA duplex will destabilize the rest of the structure (cooperative process). • Melting curves are used to demonstrate the stability of the DNA double helix and determine the melting temperature (Tm) which is the midpoint of a melting curve. • Tm is dependent on the • solvent • concentrations and types of ions • pH • Mole fraction of GC base pairs

  13. Figure 5-17 Variation of the melting temperatures, Tm, of various DNAs with their G + C content. Page 91

  14. Denatured DNA can be renatured • If a solution of DNA is rapidly cooled below the Tm, the resulting DNA is only partially base paired. • However, if the temperature is maintained at 25 ºC belowe the Tm, the base paired regions will rearrange until DNA completely renatures. • These are called annealing conditions and are important for hybridization of complementary strands of DNA or RNA-DNA hybrid double helices.

  15. Figure 5-18 Partially renatured DNA. Page 91

  16. Size of DNA molecules • DNA molecules are very large. • Mass can be determined by • ultracentrifugation • length measurements by electron microscopy • Autoradiography-technique in which the position of a radioactive substance in a sample is recorded by exposure to film. • Contour lengths - end to end lengths of stretched out native molecules of DNA. • Genome - complement of genetic information • kb - kilobase pair = 1000 bp

  17. Figure 5-19 Electron micrograph of a T2 bacteriophage and its DNA. Page 91

  18. Figure 5-20 Autoradiograph of Drosophila melanogaster DNA. Page 92

  19. Table 5-2 Sizes of Some DNA Molecules. Page 92

  20. Size of DNA molecules • DNA is highly susceptible to mechanical damage outside of the cell. • Shearing forces generated by ordinary lab techniques can result in shearing of the DNA into small pieces.

  21. Figure 5-21 The central dogma of molecular biology. Page 93

  22. Figure 5-22 Gene expression. Page 93

  23. Transcription • Catalyzed by RNA polymerase. • Couples NTPs (ATP, CTP, GTP, UTP) to make RNA • (RNA)n residues + NTP  (RNA)n+1 residues + P2O74- • 5’  3’ nucleotides are added to the free 3’-OH group • Nucleotides must meet Watson-Crick base pairing requirements with the template strand

  24. Figure 5-23 Action of RNA polymerases. Page 93

  25. Transcription • Transcribes only one template DNA strand at a time. • RNA polymerase will move along the duplex DNA it is transcribing and creates a transcription bubble • This forms a short DNA-RNA hybrid with newly synthesized RNA. • DNA template strand is read 3’  5’

  26. Figure 5-24 Function of the transcription bubble. Page 94

  27. Transcription • DNA template contains control sites consisting of specific base sequences that specify where the RNA polymerse initiates transcription and the rate of transcription. • activators and repressors control the sites in prokaryotes. • Transcription factors bind to these sites in eukaryotes. • messenger RNA (mRNA) - RNAs that encode proteins • Rates at which cells synthesize a protein are determined by the rate at which mRNA synthesis is initiated. • Promoter-in prokaryotes-a sequence that precedes the transcriptional initiation site.

  28. Transcription • Prokaryotes can control transcriptional initiation in complex manners. • Example E. coli lac operon. • Has 3 consecutive genes (Z, Y, and A) that are necessary to metabolize lactose. • In the absence of lactose, the lac repressor protein binds a control site in the lac operon called an operator. • This prevents the RNA polymerase from initiating transcription. • If lactose is present, some of the lactose is converted to allolactose which binds to the lac repressor causing it to fall of the operator sequence. • This allows RNA polymerase to initiate transcription of the genes.

  29. Figure 5-25 Control of transcription of the lac operon. Page 95

  30. Eukaryotic RNA undergoes post-transcriptional modification • In order for mRNAs in eukaryotes to become functional, they must undergo modifications. • 7-methylguanosine-containing “cap” is added to the 5’ end. •  250 nucleotide polyadenylic acid [poly(A)] tail is added to the 3’ end. • Undergo gene splicing in which RNA segments called introns are excised from the RNA and the remaining exons are rejoined to form the mature mRNA.

  31. Figure 5-26 Post-transcriptional processing of eukaryotic mRNAs. Page 95

  32. mRNA • In prokaryotes, transcription and translation both take place in the cytosol. • Prokaryotic mRNAs have a short lifetime (avg. 1-3 min). They are degraded by nucleases. • Rapid turnover in prokaryotes allows the prokaryote to respond quickly to the environment. • In eukaryotic cells, RNAs are transcribed and post-translationally modified in the nucleus, then sent to cytosol. • Eukaryotic mRNAs have lifetimes of several days.

  33. Translation: Protein synthesis • Polypeptides are synthesized from mRNA by ribosomes. • Ribosomes are 2/3 rRNA (ribosomal RNA) and 1/3 protein. • Prokaryote ribosomes approx. 2500 kD, eukaryotes 4300 kD • Transfer RNAs (tRNAs) deliver amino acids to the ribosome. • mRNA sequences can be broken down to codons-consecutive 3-nucleotide segments that specify a particular amino acid. • Once the mRNA binds to the ribosome, they specifically bind to the tRNA that is covalently linked to an amino acid.

  34. Figure 5-27 Transfer RNA (tRNA) drawn in its “cloverleaf” form. tRNA has 76 nucleotides Has an anticodon-complementary sequence to the mRNA sequence Amino acid is linked to the 3’ end of the tRNA to form aminoacyl-tRNA. tRNAs are “charged” with amino acids by specific enzymes (aminoacyl-tRNA synthetases or aaRSs) Page 95

  35. Figure 5-28 Schematic diagram of translation. Page 96

  36. Figure 5-29 The ribosomal reaction forming a peptide bond. Page 96

  37. Genetic code • Correspondence between the sequence of bases in a codon and the amino acid residue it specifies. • Nearly universal. • 4 possible bases (U[T], C, A, and G) can occupy three positions of codon, therefore 43 = 64 possible codons. • 61 codons specify amino acids, and three UAA, UAG, and UGA are stop codons (cause ribosome to end polypeptide synthesis and release the transcript). • All but two amino acids (Met, Trp) are specified by more than one codon. • Three (Leu, Ser, Arg) are specified by six codons. • Synonyms-multiple codons can code the same amino acid. • tRNA may recognize up to 3 synonymous codons because the 5’ base of a codon and 3’ base of the anticodon can interact in ways other than via Watson-Crick base pairs. • Translation is initiated at the AUG codon (Met) but this tRNA differs from the tRNA for internal amino acid the Met codon.

  38. Page 97

  39. Figure 5-30 Nucleotide reading frames. Page 98

  40. DNA replication • DNA is replicated similar to RNA with some differences: • 1. Deoxynucleotide triphosphates (dNTPs) are used instead of NTPs • 2. Enzyme is the DNA polymerase • Other differences: • RNA polymerase can link together two nucleotides on DNA template, but DNA polymerase can only extend (in the 5’ to 3’) direction an existing polynucleotide that is base paired to the template strand. • DNA polymerase needs an oligonucleotide primer to initiate synthesis. • Primers are RNA.

  41. Figure 5-31 Action of DNA polymerases. Page 99

  42. DNA strands replicated in different ways • DNA strands are simultaneously replicated. • Takes place at replication fork - junction where the two parental DNA are pried apart and where the two daughter strands are synthesized. • Leading strand is continuously copied from the 3’ to 5’ parental template in the 5’ to 3’ direction • Lagging strand is discontinuously replicated in pieces from the 5’ to 3’ parental strands.

  43. Figure 5-32a Replication of duplex DNA in E. coli. Page 100

  44. Figure 5-32b Replication of duplex DNA in E. coli. Page 100

  45. DNA strands replicated in different ways • DNA strands are simultaneously replicated. • Takes place at replication fork - junction where the two parental DNA are pried apart and where the two daughter strands are synthesized. • Leading strand is continuously copied from the 3’ to 5’ parental template in the 5’ to 3’ direction • Lagging strand is discontinuously replicated in pieces from the 5’ to 3’ parental strands. • E. coli has 2 DNA polymerases necessary for survival. DNA polymerase III (Pol III) synthesizes the leading strand and most of the lagging strand. • DNA polymerase I (Pol I) removes RNA primers and replaces them with DNA. This enzymes also has a 5’ to 3’ exonuclease activity.

  46. Figure 5-33 The 5¢® 3¢ exonuclease function of DNA polymerase I. Page 100

  47. Figure 5-34 Replacement of RNA primers by DNA in lagging strand synthesis. Page 101

  48. Lagging strand synthesis • Synthesis of the leading strand of DNA is completed by the replacement of the RNA primer by DNA. • Lagging strand is completed after nicks between multiple disconinuously synthesized segments are sealed by DNA ligase. • Catalyzes the links of 3’-OH to 5’-phosphate groups.

  49. Figure 5-35 Function of DNA ligase. Page 101

  50. Errors in DNA sequence can be corrected • RNA polymerase has an error rate of 1 in 104 base pairs in E. coli. • Pol I and Pol III have 3’  5’ exonuclease activities. • This activity degrades the newly synthesized 3’ end of a daughter strand one nucleotide at a time to edit out mistakes that are sometimes incorporated. • Other enzymes are present that detect and correct errors in DNA damage that occurs from UV radiation and mutagens (chemical substances that damage DNA) and hydrolysis.

More Related