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Build-a-Gene X Edit. Two projects Traditional method – Using site-directed mutagenesis to edit a gene – Make red fluorescent protein brighter – Weeks.

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Presentation on theme: "Build-a-Gene X Edit. Two projects Traditional method – Using site-directed mutagenesis to edit a gene – Make red fluorescent protein brighter – Weeks."— Presentation transcript:

1 Build-a-Gene X Edit

2 Two projects Traditional method – Using site-directed mutagenesis to edit a gene – Make red fluorescent protein brighter – Weeks 1,2,4,5 New method – Using CRISPR to edit a gene (within the genome) – Edit the CAN1 gene of yeast so that yeast cells become resistant to a toxic chemical – Weeks 3,4,5

3 What is the relationship between DNA, chromosomes, genes, and the genome?

4 Using minipreps to extract DNA from cells – DNA is used for long-term storage of information in cells – Minipreps can be used to extract DNA from many cell types: Animal cells or tissue (patient samples) Plant cells or tissue Whole blood Yeast cells Bacterial cells

5 Why extract DNA from cells? Clinical applications – Tissue typing for organ transplant – Detection of pathogens – Human identity testing Downstream research applications (additional experiments) – Determine DNA sequence – Combine different DNAs together (make recombinant DNA) – Change or alter the DNA sequence

6 Genomic DNA (chromosome(s)) is located in the nucleus Plasmid DNA is located in the cytoplasm in bacterial and yeast cells Where is the DNA located in cells? Genomic DNA (chromosome)

7 What are plasmids? Genomic DNA (chromosome) Plasmids are small circles of DNA (they contain genes) Some plasmids can have hundreds of copies/cell They can be transferred between cells

8 Table 8.1 Genomes 3 (© Garland Science 2007) Cells have plasmids because they give the cells useful properties

9 Why are plasmids useful to us? They can be put into cells and taken out of cells easily We can insert a DNA of interest into a plasmid to make a recombinant DNA –This new DNA can be inserted back into the cells –The cells will copy the new DNA and make many copies of our DNA The DNA on plasmids can be easily manipulated in the lab

10 Okay, let’s stop and talk technique

11 Use good lab technique Wear gloves Do not leave bottles, etc. open Change pipet tips between each sample If your pipet tip touches anything besides your sample, change it Wash hands after using bacteria

12 P20P200 (1.0  l) P1000 0 1 0 0 2 0 0 2 0 (20  l)(200  l) P20P200 (20.0  l) P1000 2 0 0 2 0 0 1 0 0 (200  l)(1000  l) Minimum volume is…. Maximum volume is… Micropipettes

13 Back to minipreps….

14 Spin columns are the most common method for extracting DNA from cells Four steps: Lysis Binding Washing Elution

15 Step 1: Lysis Break down the cell membrane with detergent and NaOH Remove proteins by denaturing them (changing their shape) with salts Genomic DNA (chromosome)

16 Step 2: Binding DNA must be separated from the cell’s debris Uses selective binding of DNA to solid support (silica) In high salt, DNA binds silica In high salt, protein does not bind (flows through column) DNA Proteins

17 Step 3: Wash Most protein has washed through, but some might be left Wash column 1-2X to remove these impurities DNA Proteins

18 Step 4: Elute Elution buffer (low salt) releases the DNA from the membrane Now the DNA will flow through and be collected in the tube DNA

19 Gel electrophoresis

20 We can determine the quantity and quality of our nucleic acid using gel electrophoresis

21 Pouring a Gel The gel is made out of an agarose matrix Agarose is clear and colorless; we can see DNA by incorporating ethidium bromide or GelRed, which inserts into the DNA and fluoresces

22 Serial Dilutions In a serial dilution, the concentration decreases by the same amount in each successive step Serial dilutions are multiplicative –A 1:5 dilution followed by a 1:5 dilution =1:25 Why is it crucial to change pipet tips when performing dilutions? When performing serial dilutions, why is it crucial to mix thoroughly at each step?

23 Preparing your samples To get the clear and colorless DNA into the gel we mix it with loading dye

24 Running a Gel Cover the gel with buffer Hover over the well and pipet gently; do not push all the way down on pipet! Be sure to load a DNA ladder into one lane DNA ladder

25 Viewing your Gel DNA ladder Sample 1Sample 2 Sample 3 Remove carefully! Compare to the DNA ladder to determine DNA length

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