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Comparison of Genetic Material and Replication for Eukaryotes and Prokaryotes BacteriaArchaeaEukaryotes Genomehaploid; circular diploid; linear HistonesAbsentPresent;

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Presentation on theme: "Comparison of Genetic Material and Replication for Eukaryotes and Prokaryotes BacteriaArchaeaEukaryotes Genomehaploid; circular diploid; linear HistonesAbsentPresent;"— Presentation transcript:

1 Comparison of Genetic Material and Replication for Eukaryotes and Prokaryotes BacteriaArchaeaEukaryotes Genomehaploid; circular diploid; linear HistonesAbsentPresent; nucleosome Rate Faster Slower Point of originSingleMultiple TelomeresAbsent Present # DNA Polymerase ~5 ~15

2 Comparison of Transcription for Eukaryotes and Prokaryotes BacteriaArchaeaEukaryotes # RNA Polymerase 11 – similar to eukaryotic 3 # genes on transcript polycistronic monocistronic Post- transcription modification NoneIntronsIntrons, cap and tail Transcription factors No Sigma Factor Yes Promoter UniqueSimilar

3 Enzymes are common feature of biochemical pathways Constitutive enzymes (60-80%) Inducible enzymes  Default position off Repressible enzymes  Default position on Regulation of Gene Expression

4 Operon model of gene expression  Regulatory gene, operator, promoter and series of structural genes  divided into three regions: Regulatory gene – codes for regulatory protein Control region - operator and promoter Structural genes - genes being transcribed

5 Operon structure Promoter – Binding site for RNA polymerase Operator – binding site for the repressor protein Structural Genes – DNA sequence for proteins of interest Operator Gene 1Gene 3Gene 2 Promoter Regulatory gene Regulatory gene – DNA sequence for repressor protein Control region

6  Operon controlled by regulatory region Protein acts as “on/off” switch  Can act as repressor or inducer  Operon model based on studies of induction of the enzymes of lactose catabolism on E. coli

7 Inducible enzyme Default position is off Enzymes not made until needed

8 Catabolite Repression  glucose represses enzymes for lactose degradation  Low glucose levels corresponds to high cAMP  cAMP binds to catabolite activating protein (CAP) alarmone  CAP binds to promoter and induces RNA polymerase to bind

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11 2-step diauxic growth caused by catabolite repression E.coli grows on either substrate

12 Repressible enzyme Default position is on Enzymes made until no longer needed

13 Operons rare in eukaryotes  Function differently Eukaryotes utilize transcription factors or alternate splicing of exons Expression may be regulated at translation level Unsure of regulation of expression in archaea  May be more similar to eukaryotes than bacteria

14 Many microbes adapt to changing environments by altering level of gene expression  Global Regulatory Systems Signal transduction  Transmits information from external environment to inside cell  Allows cell to respond to environmental changes

15  Two-component regulatory systems Sensors recognize change in environment  Kinase protein in membrane Response regulators activate or repress gene expression  DNA binding protein

16  Quorum sensing Based on density of cell population Activation of genes beneficial only when produced by multiple cells  Vibrio fisheri  Biofilm formation

17 Natural selection  Antigenic variation Alteration in characteristics of certain surface proteins Ex. Neisseria gonorrhoeae varies pilin gene at expression locus

18 Regulation may occur at the translation level  Riboswitches  Antisense RNA

19 Bacterial Genetics and Genetic Transfers

20 Eukaryotes - sexual reproduction  Gametes have various genetic combinations Prokaryotes - asexual reproduction  All offspring are clones of parent cell  No genetic variation Genetic Diversity

21 Diversity in Bacteria Bacterial mechanisms for genetic diversity  Mutation  Gene transfer

22 Change in genotype  Wild type vs. mutant May or may not cause phenotypic changes  silent, beneficial, or harmful Passed vertically to all offspring  Selective pressure can lead to evolution through natural selection Mutations

23 Point Mutation (base substitution)  Missense Types of Mutations Change in one base Results in change of amino acid

24  Nonsense Results in a stop codon

25 Frame-shift mutation Insertion or deletion of one or more bases

26 Mutagen  Agent that induces mutations  Physical or chemical agents Spontaneous mutations  Occur in the absence of a mutagen  May be due to error or transposons

27 Transposable Elements (Transposons)  May disrupt proper gene function  Contain insertion sequences (transposase)  Complex (composite) transposons carry other genes

28 Nucleotide excision repair Endonuclease, DNA ligase & DNA Polymerase Light repair Direct repair Photoactivation of enzymes (photolyase)

29 Induced Mutations Mutations are essential for understanding genetics  Intentionally produced ( induced) to demonstrate function of particular gene or set of genes Mutations can be induced via  Chemical mutagens  Transposition  Radiation

30 Ames Test Mutational reversion assay Tests mutagenicity of compounds Utilizes a histidine auxotroph

31 Mutations followed by selection may produce microbes with desirable traits  Positive (direct) selection detects mutant cells because they grow or appear different Ex. Penicillin resistant mutants growing on penicillin containing agar – non mutants will not grow Eliminates wild type

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33  Negative (indirect) selection detects mutant cells because they do not grow Replica plating to isolate mutants requiring a specific growth factor – auxotroph Selects for wild type

34 Replica Plating Figure 8.21


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