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Chapter 19 • Eukaryotic Genomes Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Eukaryotes DNA-protein complex, chromatin – More complex structural levels than prokaryotes Figure 19.1 Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Both prokaryotes and eukaryotes – Must alter patterns of gene expression in response to changes in environment Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Chromatin structure based on successive levels of DNA packing • Eukaryotic DNA – Combined w/ protein • Eukaryotic chromosomes – Contain an enormous amount of DNA relative to their condensed length Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Nucleosomes, or “Beads on a String” • Basic packing unit • DNA wrapped around histone protein 2 nm DNA double helix Histones Histone tails Histone H1 Nucleosome (“string”) (“bead”) (a) Nucleosomes (10-nm fiber) Linker DNA Figure 19.2 a Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings 10 nm • Next level of packing – Forms 30-nm chromatin fiber 30 nm Nucleosome (b) 30-nm fiber Figure 19.2 b Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • The 30-nm fiber, in turn – Forms looped domains, making up a 300-nm fiber Protein scaffold Loops 300 nm (c) Looped domains (300-nm fiber) Figure 19.2 c Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Scaffold • Mitotic chromosome – Looped domains coil and fold forming the metaphase chromosome 700 nm 1,400 nm (d) Metaphase chromosome Figure 19.2 d Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Interphase cells – Most chromatin is highly extended (euchromatin) Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Gene expression can be regulated at any stage, but the key step is transcription • All organisms – regulate which genes are expressed at any given time • During development of a multicellular organism cell specialization in form and function (cell differentiation) Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Each cell of a multicellular eukaryote – Expresses only a fraction of its genes • In each type of differentiated cell – Unique subset of genes is expressed Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Signal NUCLEUS Chromatin • Many key stages of Chromatin modification: DNA unpacking involving histone acetylation and DNA demethlation DNA Gene available gene expression for transcription Gene Transcription RNA (regulation) Exon Primary transcript Intron RNA processing Tail In eukaryotic cells Cap mRNA in nucleus Transport to cytoplasm CYTOPLASM mRNA in cytoplasm Degradation of mRNA Translation Polypetide Cleavage Chemical modification Transport to cellular destination Active protein Degradation of protein Degraded protein Figure 19.3 Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Genes within highly packed heterochromatin usually not expressed Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Histone acetylation – Loosens chromatin structure enhances transcription Unacetylated histones Figure 19.4 b Acetylated histones (b) Acetylation of histone tails promotes loose chromatin structure that permits transcription Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Addition of methyl groups to DNA bases – Associated w/ reduced transcription Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Multiple control elements – Noncoding DNA that regulate transcription Enhancer (distal control elements) Proximal control elements Poly-A signal sequence Exon Intron Exon Intron Termination region Exon DNA Downstream Upstream Promoter Chromatin changes Transcription Exon Primary RNA 5 transcript (pre-mRNA) Intron Intron RNA RNA processing mRNA G P P Cleared 3 end of primary transport P 5 Cap Figure 19.5 Exon Coding segment Translation Protein processing and degradation Intron RNA processing: Cap and tail added; introns excised and exons spliced together Transcription mRNA degradation Exon Poly-A signal 5 UTR (untranslated region) Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Start codon Stop codon Poly-A 3 UTR tail (untranslated region) Alternate RNA Processing • Different mRNA molecules produced from same primary transcript, depending on which RNA segments are treated as exons and which as introns Chromatin changes Transcription RNA processing mRNA degradation Translation Protein processing and degradation Exons DNA Primary RNA transcript RNA splicing Figure 19.8 mRNA Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings or mRNA Degradation • Life span of mRNA molecules in the cytoplasm – Important in protein synthesis Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • RNA interference (RNAi) by single-stranded microRNAs (miRNAs) – degradation of mRNA or block its translation 1 The microRNA (miRNA) precursor folds back on itself, held together by hydrogen bonds. 22 An enzyme called Dicer moves along the doublestranded RNA, cutting it into shorter segments. 3 One strand of each short doublestranded RNA is degraded; the other strand (miRNA) then associates with a complex of proteins. 4 The bound miRNA can base-pair with any target mRNA that contains the complementary sequence. 55 The miRNA-protein complex prevents gene expression either by degrading the target mRNA or by blocking its translation. Chromatin changes Transcription RNA processing mRNA degradation Translation Protein processing and degradation Protein complex Dicer Degradation of mRNA OR miRNA Target mRNA Figure 19.9 Hydrogen bond Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Blockage of translation • Proteasomes – Giant protein complexes that degrade molecules 3 Enzymatic components of the 1 Multiple ubiquitin molChromatin changes ecules are attached to a protein by enzymes in the cytosol. 2 The ubiquitin-tagged protein is recognized by a proteasome, which unfolds the protein and sequesters it within a central cavity. proteasome cut the protein into small peptides, which can be further degraded by other enzymes in the cytosol. Transcription RNA processing mRNA degradation Proteasome and ubiquitin to be recycled Ubiquitin Translation Proteasome Protein processing and degradation Protein to be degraded Ubiquinated protein Protein entering a proteasome Figure 19.10 Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Protein fragments (peptides) • Cancer results from genetic changes that affect cell cycle control • The gene regulation systems that go wrong during cancer are same systems found in embryonic development Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Oncogenes – Cancer-causing genes • Proto-oncogenes – Normal genes that code for proteins that stimulate normal cell growth and division Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • DNA changeproto-oncogene excessively active oncogeneexcessive cell division cancer Proto-oncogene DNA Translocation or transposition: gene moved to new locus, under new controls Gene amplification: multiple copies of the gene Oncogene New promoter Normal growth-stimulating protein in excess Point mutation within a control element Normal growth-stimulating protein in excess Figure 19.11 Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Normal growth-stimulating protein in excess Point mutation within the gene Oncogene Hyperactive or degradationresistant protein • Tumor-suppressor genes – Code f/ proteins that inhibit abnormal cell division Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • p53 gene encodes a tumor-suppressor protein – (cell cycle–inhibiting proteins) – ‘Guardian angel’ of the genome (b) Cell cycle–inhibiting pathway. In this pathway, 1 DNA damage is an intracellular signal that is passed via 2 protein kinases and leads to activation of 3 p53. Activated p53 promotes transcription of the gene for a protein that inhibits the cell cycle. The resulting suppression of cell division ensures that the damaged DNA is not replicated. Mutations causing deficiencies in any pathway component can contribute to the development of cancer. 2 Protein kinases UV light 3 1 DNA damage in genome Active form of p53 DNA Protein that inhibits the cell cycle Figure 19.12b Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings MUTATION Defective or missing transcription factor, such as p53, cannot activate transcription • Mutations that knock out the p53 gene excessive cell growth and cancer (c) Effects of mutations. Increased cell division, possibly leading to cancer, can result if the cell cycle is overstimulated, as in (a), or not inhibited when it normally would be, as in (b). EFFECTS OF MUTATIONS Protein overexpressed Cell cycle overstimulated Figure 19.12c Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Protein absent Increased cell division Cell cycle not inhibited • Normal cells are converted to cancer cells – By the accumulation of multiple mutations affecting proto-oncogenes and tumorsuppressor genes Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • A multistep model for the development of colorectal cancer Colon Loss of tumorsuppressor Colon wall gene APC (or other) 1 Activation of ras oncogene 2 Loss of tumorsuppressor gene DCC 3 Normal colon epithelial cells Small benign growth (polyp) Figure 19.13 Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Larger benign growth (adenoma) Loss of tumor-suppressor gene p53 4 5 Additional mutations Malignant tumor (carcinoma) • Certain viruses – Promote cancer by integration of viral DNA into a cell’s genome Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Inheritance of a mutant oncogene increased risk of developing cancer Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Noncoding DNA sequences • Bulk of eukaryotic genomes – In the past called “junk DNA” • Evidence is accumulating – noncoding DNA plays important roles in the cell Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Genomes of eukaryotes (v. prokaryotic) – Larger – Longer genes – Much greater amount of noncoding DNA Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Most of the 98.5% that does not code for proteins rRNAs, or tRNAs Exons (regions of genes coding for protein, rRNA, tRNA) (1.5%) Repetitive DNA that includes transposable elements and related sequences (44%) Alu elements (10%) Figure 19.14 Simple sequence DNA (3%) Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Repetitive DNA unrelated to transposable elements (about 15%) Introns and regulatory sequences (24%) Unique noncoding DNA (15%) Large-segment duplications (5-6%) Transposable Elements and Related Sequences • Wandering DNA segments – Barbara McClintock’s breeding experiments with Indian corn Figure 19.15 Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Movement of Transposons and Retrotransposons • Transposons: move by means of a DNA intermediate • Retrotransposons: move by means of an RNA intermediate Transposon DNA of genome Transposon is copied New copy of transposon Insertion Mobile transposon (a) Transposon movement (“copy-and-paste” mechanism) Retrotransposon New copy of retrotransposon DNA of genome RNA Reverse transcriptase Figure 19.16a, b (b) Retrotransposon movement Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Insertion • Multiple copies of transposable elements – scattered throughout genome • In humans and other primates – are called Alu elements Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Other Repetitive DNA • Simple sequence DNA – Copies of tandemly repeated short sequences – Common in centromeres and telomeres (structural roles in chromosome) Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Genes and Multigene Families • Most eukaryotic genes – present in one copy per haploid set of chromosomes • The rest of the genome – Occurs in multigene families, collections of identical or very similar genes Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • e.g. related families of genes that encode globins -Globin Heme Hemoglobin -Globin -Globin gene family -Globin gene family Chromosome 16 Chromosome 11 Figure 19.17b The human -globin and -globin gene families Embryo 1 2 1 2 Fetus and adult Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings G A Embryo Fetus Adult • Duplications, rearrangements, and mutations of DNA contribute to genome evolution • The basis of change at the genomic level is mutation which underlies much of genome evolution Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Duplication of Chromosome Sets • Accidents in cell division – extra copies of all or part of a genome, which may then diverge if one set accumulates sequence changes Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Unequal crossing over – one chromosome with a deletion and another with a duplication Transposable element Gene Nonsister chromatids Crossover Incorrect pairing of two homologues during meiosis and Figure 19.18 Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Genes for various globin proteins – Evolved from one common ancestral globin gene, which duplicated and diverged Ancestral globin gene Duplication of ancestral gene Mutation in both copies Transposition to different chromosomes Further duplications and mutations Figure 19.19 2 2 1 1 -Globin gene family on chromosome 16 Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings G A -Globin gene family on chromosome 11 • Similarity in the amino acid sequences of the various globin proteins – Supports this model of gene duplication and mutation Table 19.1 Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • The copies of some duplicated genes – Have diverged so much during evolutionary time that the functions of their proteins are now substantially different Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Rearrangements of Parts of Genes: Exon Duplication and Exon Shuffling Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings • Exon shuffling – Mixing and matching of different exons either within a gene or between two nonallelic genes EGF EGF EGF Epidermal growth factor gene with multiple EGF exons (green) EGF Exon shuffling F F F Exon duplication F Fibronectin gene with multiple “finger” exons (orange) F EGF K K Plasminogen gene with a “kfingle” exon (blue) Figure 19.20 Portions of ancestral genes Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings Exon shuffling TPA gene as it exists today K How Transposable Elements Contribute to Genome Evolution • Movement of transposable elements – Can generates new sequence combinations that are beneficial to the organism • Some mechanisms – Alter functions of genes or their patterns of expression and regulation Copyright © 2005 Pearson Education, Inc. publishing as Benjamin Cummings
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