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Ch 12 DNA Technology and Genomics DNA Technology • Methods for studying and manipulating genetic material • Cloning • Genetically Modified • Gene Therapy • DNA Profiling • Genomics Recombinant DNA • Combining nucleotide sequences from 2 sources to form a single DNA • Bacteria often used – Plasmid Creating Recombinant DNA • Restriction Enzymes – Restirction site • Sticky Ends • Ligase 5 Cloning the Gene • Bacteria containing the gene are cloned – Typically, antibiotic resistance genes are also inserted – Bacteria are grown on antibiotic medium • All bacteria without the resistance (and target) gene die • Only those with gene reproduce • Stored in genomic library – Plasmids used to “store” genetic information Uses • Gene Cloning – Produces multiple copies of gene-carrying DNA • Genetic Engineering – Direct manipulation of genes cDNA • Express Eukaryotic genes in Prokaryotic cells – What about introns? – Prokaryotes don’t have machinery to splice • mRNA – Already spliced • Work from mRNA to create cDNA Fig. 12-4 Cell nucleus DNA of eukaryotic gene Exon Intron Exon Intron Exon 1 Transcription RNA transcript 2 RNA splicing mRNA 3 Isolation of mRNA Test tube Reverse transcriptase cDNA strand being synthesized and addition of reverse transcriptase; synthesis of DNA strand 4 Breakdown of RNA 5 Synthesis of second DNA strand cDNA of gene (no introns) Uses • Diagnosis and treatment of disease • Vaccines • Therapeutic hormones Probes • Genomic Library – How to find the right gene? • Nucleic Acid Probe – Locate specific gene or nucleotide sequence Probes • Synthesize short sequence of singe stranded DNA of complimentary sequence • Label radioactive tag • Mix with genomic library – Bacteria with gene of interest will glow Fig. 12-5 Radioactive DNA probe Mix with singlestranded DNA from genomic library Single-stranded DNA Base pairing indicates the gene of interest Genetically Modified • Organisms who have acquired genes by artificial means – If from another species= transgenic organism Agrobacterium tumefaciens Plant cell DNA containing gene for desired trait 1 Ti plasmid Insertion of gene into plasmid Recombinant Ti plasmid 3 2 Introduction into plant cells Regeneration of plant DNA carrying new gene Restriction site Plant with new trait Gene Therapy • Altering an afflicted persons genes for therapeutic purposes – Treatment of genetically based disorders – Technology still in infancy Fig. 12-10 Cloned gene (normal allele) 1 Insert normal gene into virus Viral nucleic acid Retrovirus 2 Infect bone marrow cell with virus 3 Viral DNA inserts into chromosome Bone marrow cell from patient Bone marrow 4 Inject cells into patient DNA Profiling • Forensics – Scientific analysis of evidence • DNA Profiling – Analysis of DNA fragments – Determine if they originate form a particular individual – PCR – Gel Electrophoresis PCR • 3 step cycle – Heat separates strands – Cooling allows primers to form H bonds with end of target sequence – DNA Polymerase adds nucleotides • Creates double stranded DNA – Repeat PCR • Significant breakthrough in genetics • Original polymerase was from E. coli – Heating traditionally denatured polymerase – New polymerase added after each heating cycle – Giant pain in the butt PCR • Discovery of T. aquaticus – Lives in hotsprings – Not denatured under high temps • Could now be done at higher temps – Better success rates PCR Cycle 1 yields 2 molecules Genomic DNA 3 1 3 5 3 Target sequence 5 5 5 3 Cycle 2 yields 4 molecules 5 5 2 Cool to allow 3 Heat to primers to form separate DNA strands hydrogen bonds with ends of target sequences 5 3 5 3 Primer 3 5 DNA polymerase adds nucleotides to the 3 end of each primer 5 3 New DNA Cycle 3 yields 8 molecules Gel Electrophoresis • Use of gel to separate DNA strands by size (molecular weight) or charge • DNA must first be “digested” – Strands must be cut into different sizes • Use Restriction Enzymes – Cut DNA in specific places • Looks for specific nucletoide sequences Gel Electrophoresis Mixture of DNA molecules of different sizes – – Longer molecules Power source Gel + Shorter molecules + Figure 12.10 Completed gel Gel Electrophoresis • STR – Short sequences of DNA repeated many times in a row – STR analysis compared lengths of STR sequences at specific sites on the genome • Create a genetic profile of individuals – STR’s differ among individuals Gel Electrophoresis • RFLP – Restriction fragment length polymorphisms – Difference between two samples of homologous DNA arising from differing locations of restriction sites Crime scene Suspect w Cut C G C G G C G C z A T C G G C G C C G C G G C G C x C G Cut C G G C y Cut y G C DNA from chromosomes – After digestion by restriction enzymes the fragments are run through a gel 1 – 2 Longer fragments z x w Shorter fragments Figure 12.11B + y y • DNA profiling Crime scene 1 DNA isolated 2 DNA of selected markers amplified 3 Amplified DNA compared Suspect 1 Suspect 2 • Used in forensic investigations STR site 1 STR site 2 Crime scene DNA Number of short tandem Number of short tandem repeats match repeats do not match Suspect’s DNA Genomics • Studying the entire genome and their interactions Human Genome Project • identify all the approximately 20,000-25,000 genes in human DNA, • determine the sequences of the 3 billion chemical base pairs that make up human DNA, • store this information in databases, • improve tools for data analysis, • transfer related technologies to the private sector, and • address the ethical, legal, and social issues (ELSI) that may arise from the project. Fig. 12-18 Exons (regions of genes coding for protein or giving rise to rRNA or tRNA) (1.5%) Repetitive DNA that includes transposable elements and related sequences (44%) Introns and regulatory sequences (24%) Unique noncoding DNA (15%) Repetitive DNA unrelated to transposable elements (15%) HGP • 3.2 billion nucleotide pairs – ~21000 genes – How are we so complex? • RNA splicing • Non-coding • Repetitive DNA – Telomeres • Transposable elements Shotgun Method 1. Chop up genome 1. Squeeze it through a small, pressurized syringe 2. Clone fragments 1. Insert them into a vector 3. Sequence 4. Search for overlapping segments 5. Reassemble the overlaps Chromosome Chop up with restriction enzyme DNA fragments Sequence fragments Align fragments Reassemble full sequence • Recombo DNA – http://www.youtube.com/watch?v=-sI5vycD2g&feature=related • PCR – http://www.youtube.com/watch?v=2KoLnIwoZ KU&feature=related – PCR and Gel • http://www.youtube.com/watch?v=_uoPkavtXgs Videos • Ch Overview – http://www.youtube.com/watch?v=Nc3jArZXHj s