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Announcements Lab notebooks due Monday by 5 No Ch. 9 Part 2 homework

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Presentation on theme: "Announcements Lab notebooks due Monday by 5 No Ch. 9 Part 2 homework"— Presentation transcript:

1 Announcements Lab notebooks due Monday by 5 No Ch. 9 Part 2 homework
We will have lab next week. It just isn’t a typical lab-discussing individual projects

2 Ch. 9 Part 2: Biotechnology and Recombinant DNA

3 Toolkit: DNA Sequencing-Why It Is Important
Human Genome Project produced great advances Rapid growth in field of genomics Sequencing of numerous organisms Spawned new field of bioinformatics to analyze data Allows determination of amino acid sequences Comparisons of different proteins, various organisms Evolutionary relatedness of organisms Technology so efficient that new Human Microbiome Project aims to determine biological diversity of normal microbiota

4 Toolkit: DNA Sequencing How It Works
Dideoxy chain termination most common method Automated and fast In vitro DNA synthesis Template DNA DNA polymerase Primer Deoxynucleotides dNTPs Dideoxynucleotides ddNTPs Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Primer 5′ 3′ T G G C C G T T G C C G T A C C G G C C C T T A A A T T G A A T 3′ 5′ Primer is added to single-stranded DNA. DNA polymerase Nucleotide 5′ 3′ G A C T G G C C G T T T G C C G T A C C G G C C C T T A A A T T G A A T 3′ 5′ Primer anneals to complementary sequence, serving as the nucleic acid fragment to which DNA polymerase can add nucleotides. 5′ 3′ T G G C C G G G A A T T T A A C T T A T T G C C G T A C C G G C C C T T A A A T T G A A T 3′ 5′ Final product

5 Toolkit: DNA Sequencing How It Works
Dideoxy chain termination most common method (continued…) Dideoxynucleotides (ddNTPs) Serve as chain terminators Lack 3′OH Synthesis stops Yields mixture of DNA of different lengths Denature DNA Separate ssDNA via electrophoresis Read fluorescent label on ddNTPs to obtain sequence Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. PO4 OH Incorporation of a deoxynucleotide (dNTP) elongates the chain. A subsequent nucleotide can be added to the 3′OH. 5′ 3′ OH 3′ 5′ PO4 H Incorporation of a dideoxynucleotide (ddNTP); the ddNTP lacks a 3′OH. 5′ 3′ OH 3′ 5′ H PO4 Chain elongation is terminated. No additional nucleotides can be added due to the lack of a 3′OH. OH 5′ X 3′ 5′

6 Toolkit: DNA Sequencing
Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. 1 Key ingredients in the reaction: • Primer and template (shown annealed) A T A G C T A C C T A G • DNA polymerase • Deoxynucleotides (dATP, dTTP, dGTP, dCTP) • Fluorescently labeled dideoxynucleotides (ddATP, ddTTP, ddGTP, ddCTP; a very small amount of each) Gel electrophoresis Laser reads color Determines sequence 2 Chain elongation is terminated randomly when DNA polymerase incorporates a dideoxynucleotide (indicated by a colored box and an asterisk). Products of the reaction: 3 The fragments are denatured, and the single strands then separated by gel electrophoresis. The color of the fluorescent marker indicates the terminating dideoxynucleotide. Results: T A T C G A T G G A T C* A T A G C T A C C T A G T A T C G A T G G A T* A T A G C T A C C T A G T A T C G A T G G A* A T A G C T A C C T A G T A T C G A T G G* A T A G C T A C C T A G T A T C G A T G* A T A G C T A C C T A G T A T C G A T* A T A G C T A C C T A G Decreasing fragment size T A T C G A* A T A G C T A C C T A G T A T C G* A T A G C T A C C T A G T A T C* A T A G C T A C C T A G T A T* A T A G C T A C C T A G T A* A T A G C T A C C T A G T* A T A G C T A C C T A G

7 Toolkit: Polymerase Chain Reaction (PCR)
Allows amplification to millions of copies of DNA Matter of hours Products can be visualized via gel electrophoresis Allows detection of specific sequences Can detect organisms without culturing E.g., pathogens Requires template DNA, polymerase, primers, deoxynucleotides (dATP, dGTP, dCTP, dTTP) Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. DNA from Patient A DNA from Patient B PCR amplifies specific sequence of interest. No DNA amplified Gel electrophoresis of PCR amplified samples Patient A Patient B Conclusion: Patient A is positive (infected); Patient B is negative.

8 Toolkit: Polymerase Chain Reaction (PCR)
Three-step amplification cycle DNA denatured by heating (~95°C) Temperature lowered (~50°C) to allow primers to anneal Temperature raised (~70°C) to allow DNA synthesis DNA doubled in each cycle, so exponential increase Heat-stable Taq polymerase from Thermus aquaticus critical Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. 5′ Region of DNA to be amplified 3′ 3′ 5′ 1 Heating to 95°C denatures DNA. 5′ 3′ Primer Primer 3′ 5′ 2 Cooling to 50°C allows the added primers to anneal to the single- stranded templates. 5′ 3′ 3′ 5′ 5′ 3′ 3′ 5′ 3 DNA synthesis occurs when the temperature is raised to 72°C. 5′ 3′ 3′ 5′ 5′ 3′ 3′ 5′ 5′ 3′ 3′ 5′ 5′ 3′ 3′ 5′ The products of one 3-step cycle of PCR

9 Toolkit: Polymerase Chain Reaction (PCR)
Primers define length of PCR product Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. 1 Target DNA Mid-length strands are synthesized from the full-length templates. The sites to which the primers annealed determine the 5′ ends of these strands. 5′ Template 3′ 3′ 5′ Mid-length fragment Primer Outcome of cycle 1 (as well as subsequent cycles) Primer Mid-length fragment 5′ 3′ 3′ 5′ Template 2 Short fragment 5′ 3′ When the mid-length strands made in the reaction above are used as templates, short strands are generated. The 3′ ends of the fragments are complementary to the 5′ ends of the primers. 3′ 5′ Cycle 1 mid-length fragment (template) Outcome of cycle 2 (as well as subsequent cycles) Cycle 1 mid-length fragment (template) 5′ 3′ 3′ 5′ Short fragment 3 Short fragment When short strands made in the reaction above are used as templates, like-sized strands are generated. This is the double- stranded target molecule that will be amplified exponentially. 5′ 3′ 3′ 5′ Cycle 2 short fragment (template) Outcome of cycle 3 (as well as subsequent cycles) Cycle 2 short fragment (template) 5′ 3′ Produced when full-length molecule is used as a template 3′ 5′ Produced when mid-length molecule is used as a template Short fragment Produced when target fragment is used as a template

10 Toolkit: Polymerase Chain Reaction (PCR)
Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Exponential amplification of DNA Increasing numbers of product of correctly defined length ~30 cycles typical Time 0 End of cycle 1 End of cycle 2 End of cycle 3 End of cycle 4 End of cycle 5 (2) (8) (22)

11 Gel Electrophoresis of PCR Product

12 Toolkit: Probe Technologies-Why Important
DNA probes locate specific nucleotide sequence Probe is single-stranded piece of DNA Will hybridize to complementary sequence Labeled with marker Numerous different probe technologies Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Probe Label 3′ T G G C C G T T G C C G T A C C G G C C C T T A A A T T G A A T 3′ 5′ Probe is added to single-stranded DNA that has been attached to a solid surface. 5′ 3′ T G G C C G T T G C C G T A C C G G C C C T T A A A T T G A A T 3′ 5′ Probe anneals to complementary sequence. Because of the label it carries, its location can easily be determined.

13 Toolkit: Probe Technologies
Colony Blotting Allows detection of colonies that have specific sequence of DNA Commonly used to identify which clones in a collection contain sequence of interest Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Nylon membrane Probe bound to DNA 1 Colonies on an agar plate. 2 Colonies are transferred in place (“blotted”) to a nylon membrane. 3 The membrane is soaked in an alkaline solution to lyse the cells and denature their DNA. 4 Probe is added that binds to DNA of interest. 5 By locating the positions to which probe has bound, colonies that have the DNA of interest can be located.

14 Toolkit: Probe Technologies
Fluorescence in situ Hybridization (FISH) Probe hybridizes to nucleotide sequences in intact cells fixed to microscope slide Cells visualized via fluorescence microscope Probe often binds to rRNA sequences since numerous Rapid identification in specimen without culturing Related organisms or specific species

15 Toolkit: Probe Technologies
DNA Microarrays Studies of gene expression Also used to detect DNA sequences mRNA is isolated, converted to labeled cDNA, hybridized to array Array has numerous short probes specific to each gene of interest Allows comparisons of conditions

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