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Download Genetic Data I. Basics of genetic information A. Nuclear genetic
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Genetic Data I. Basics of genetic information A. Nuclear genetic information is contained on chromosomes. Chromosomes composed of DNA: Purines: Adenine and Guanine Pyrimidines: Thymine and Cytosine B. The Central Dogma DNA RNA Proteins Transcription Translation II. Other forms of genetic material in cells Mitochondria – circular DNA, haploid, non‐recombining Chloroplasts – circular DNA, haploid, non‐recombining Table 1: Comparison of the genomes in plant cells Genome size (kbp) Inheritance Ploidy Utility Chloroplast 135‐160 Maternal or parental Haploid High Mitochondrion 200‐2500 Maternal or parental Haploid Low* 1.1 x 106 – 1.1 x Biparental Diploid+ High 11 10 + Could be polyploidy * Mitochondrial markers are widely used in animals, but the mitochondrial genome in plants exhibits rearrangements, gene duplications and gene losses, making it difficult to use III. Coding vs. non‐coding regions A. Coding: Exon = coding part of a gene; transcribed and translated B. Non‐coding: Intron = non‐coding part of a gene; transcribed but not translated Intergenic spacers = regions between genes C. We target non‐coding regions for studies of population structure and gene flow. IV. Exercise on selecting an appropriate genetic marker – see associated handouts A. Studies of mating systems B. Studies of hybridization C. Studies of adaptation and selection V. Classes of genetic data A. What makes for an ideal molecular marker? Nucleus The best markers are highly variable, inexpensive and easy to use. Co‐dominant markers contain more information. B. Classes of genetic markers 1. Protein Allozymes – co‐dominant, but often low polymorphism and may not be neutral 2. DNA a. Fragments vs. sequences b. RFLP – restriction fragment length polymorphism; coded as presence/absence of a band c. Polymerase chain reaction – a molecular Xerox machine d. RAPD/ISSR/AFLP – dominant markers; coded as presence/absence of a band; primers are not species‐specific. e. Microsatellites – co‐dominant markers representing variation in the number of repeats (e.g., CACACACA); alleles are identified in homozygous and heterozygous individuals; the most commonly used markers currently; must be isolated and developed for species. f. SNP’s – single nucleotide polymorphisms; considered to be highly polymorphic but can be difficult to develop g. Sequences – nucleotide sequence for a gene region; high information content; co‐dominant. 3. RNA – not yet used extensively, but next‐generation methods are making RNA studies easier to do VI. Measures of genetic diversity – what do we want to know? A. Relative levels of diversity examples: Genetically depauperate Inbreeding Clonality B. Genetic structure examples: Genetic drift Bottlenecks Cryptic taxa Gene flow C. Candidate loci example: Local adaptation VII. Examples from the literature – see associated handouts A. Neostapfia colusana – microsatellites B. Astragalus ampullarioides – AFLP’s
