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DNA The Genetic Material 2006-2007 Chromosomes related to phenotype • T.H. Morgan – working with Drosophila – associated phenotype with specific chromosome • white-eyed male had specific X chromosome Genes are on chromosomes • Morgan’s conclusions – genes are on chromosomes – but is it the protein or the DNA ? The “Transforming Principle” • Frederick Griffith – Streptococcus pneumonia bacteria – Harmless bacteria (“rough”) + heat-killed disease bacteria (“smooth”) = fatal disease in mice – Something passed from dead bacteria to live bacteria to change their phenotype • “Transforming Principle” The “Transforming Principle” live pathogenic strain of bacteria A. mice die live non-pathogenic strain of bacteria B. mice live heat-killed pathogenic bacteria C. mice live mix heat-killed pathogenic & non-pathogenic bacteria D. mice die Transformation = change in phenotype something in heat-killed bacteria could still transmit disease-causing properties DNA is the “Transforming Principle” • Avery, McCarty & MacLeod – purified DNA & proteins from Streptococcus bacteria – injected protein into bacteria • no effect – injected DNA into bacteria • transformed harmless bacteria into virulent bacteria mice die Confirmation of DNA • Hershey & Chase – “blender” experiment – worked with bacteriophage • viruses that infect bacteria – grew phage viruses in 2 media, radioactively labeled with either • 35S in their proteins • 32P in their DNA – infected bacteria with labeled phages Protein coat labeled with 35S DNA labeled with 32P T2 bacteriophages are labeled with radioactive isotopes S vs. P Hershey & Chase bacteriophages infect bacterial cells bacterial cells are agitated to remove viral protein coats 35S radioactivity found in the medium 32P radioactivity found in the bacterial cells Chargaff • DNA composition: “Chargaff’s rules” – varies from species to species – all 4 bases not in equal quantity – bases present in characteristic ratio • humans: A = 30.9% T = 29.4% G = 19.9% C = 19.8% Structure of DNA • Watson & Crick – developed double helix model of DNA • other leading scientists working on question: – Rosalind Franklin – Maurice Wilkins – Linus Pauling Franklin Wilkins Pauling 1953 article in Nature Watson and Crick Watson Crick Double helix structure of DNA “It has not escaped our notice that the specific pairing we have postulated immediately suggests a possible copying mechanism for the genetic material.” Watson & Crick Directionality of DNA • You need to number the carbons! nucleotide PO4 N base – it matters! 5 CH2 O 4 1 ribose 3 OH 2 5 The DNA backbone PO4 • Putting the DNA backbone together base 5 CH2 O – refer to the 3 and 5 ends of the DNA • the last trailing carbon 4 1 C 3 O –O P O O 5 CH2 2 base O 4 1 2 3 OH 3 Anti-parallel strands • DNA backbone is bonded from phosphate to sugar between 3 & 5 carbons 5 3 3 5 – DNA molecule has “direction” – complementary strand runs in opposite direction Bonding in DNA hydrogen bonds 5 3 covalent phosphodiester bonds 3 5 Base pairing in DNA • Purines – adenine (A) – guanine (G) • Pyrimidines – thymine (T) – cytosine (C) • Pairing – A:T • 2 bonds – C:G • 3 bonds But how is DNA copied? • Replication of DNA – base pairing allows each side to serve as a template for a new strand Models of DNA Replication • Alternative models – become experimental predictions conservative P 1 2 semiconservative dispersive Semiconservative replication • Meselson & Stahl – label “parent” nucleotides in DNA strands with heavy nitrogen = 15N – label new nucleotides with lighter isotope = 14N parent 15N/15N 15N parent strands replication Predictions 14N/14N 1st round of replication 15N/15N conservative 2nd round of replication 15N/15N 1 15N/15N 2 15N parent strands semiconservative 15N/14N dispersive 14N/14N P 15N/14N conservative 14N/14N 15N/14N semiconservative 15N/14N dispersive