logging in or signing up Gel Electorphoresis Lecture 2006 lalo34 Download Post to : URL : Related Presentations : Share Add to Flag Embed Email Send to Blogs and Networks Add to Channel Uploaded from authorPOINT lite Insert YouTube videos in PowerPont slides with aS Desktop Copy embed code: (To copy code, click on the text box) Embed: URL: Thumbnail: WordPress Embed Customize Embed The presentation is successfully added In Your Favorites. Views: 36 Category: Science & Tech.. License: All Rights Reserved Like it (0) Dislike it (0) Added: December 23, 2011 This Presentation is Public Favorites: 0 Presentation Description No description available. Comments Posting comment... Premium member Presentation Transcript PowerPoint Presentation: Discover the Microbes Within How many species have Wolbachia?Agarose Gel Electrophoresis: Agarose Gel Electrophoresis Gel electrophoresis is a widely used technique for the analysis of nucleic acids and proteins . Agarose gel electrophoresis is routinely used for the preparation and analysis of DNA. Gel electrophoresis is a procedure that separates molecules on the basis of their rate of movement through a gel under the influence of an electrical field. We will be using agarose gel electrophoresis to determine the presence and size of PCR products. PCR products indicate the presence of Wolbachia.PowerPoint Presentation: http://gslc.genetics.utah.edu/units/biotech/gel/ Virtual Gel Electrophoresis Additional Information on Gel Electrophoresis:PowerPoint Presentation: • DNA is negatively charged. + - Power DNA • When placed in an electrical field, DNA will migrate toward the positive pole (anode). H O 2 • An agarose gel is used to slow the movement of DNA and separate by size. Scanning Electron Micrograph of Agarose Gel (1×1 µm) • Polymerized agarose is porous, allowing for the movement of DNAPowerPoint Presentation: + - Power DNA How fast will the DNA migrate? strength of the electrical field , buffer, density of agarose gel… Size of the DNA! *Small DNA move faster than large DNA …gel electrophoresis separates DNA according to size small large Within an agarose gel, linear DNA migrate inversely proportional to the log10 of their molecular weight.PowerPoint Presentation: Agarose Agarose is a linear polymer extracted from seaweed. D-galactose 3,6-anhydro L-galactose Sweetened agarose gels have been eaten in the Far East since the 17th century. Agarose was first used in biology when Robert Koch* used it as a culture medium for Tuberculosis bacteria in 1882 *Lina Hesse , technician and illustrator for a colleague of Koch was the first to suggest agar for use in culturing bacteriaPowerPoint Presentation: Making an Agarose GelPowerPoint Presentation: An agarose gel is prepared by combining agarose powder and a buffer solution. Agarose Buffer Flask for boiling PowerPoint Presentation: Casting tray Gel combs Power supply Gel tank Cover Electrical leads Electrophoresis EquipmentPowerPoint Presentation: Gel casting tray & combsPowerPoint Presentation: Seal the edges of the casting tray and put in the combs. Place the casting tray on a level surface. None of the gel combs should be touching the surface of the casting tray. Preparing the Casting TrayPowerPoint Presentation: Agarose Buffer Solution Combine the agarose powder and buffer solution. Use a flask that is several times larger than the volume of buffer.PowerPoint Presentation: Agarose is insoluble at room temperature (left). The agarose solution is boiled until clear (right). Gently swirl the solution periodically when heating to allow all the grains of agarose to dissolve. ***Be careful when boiling - the agarose solution may become superheated and may boil violently if it has been heated too long in a microwave oven. Melting the AgarosePowerPoint Presentation: Allow the agarose solution to cool slightly (~60ºC) and then carefully pour the melted agarose solution into the casting tray. Avoid air bubbles. Pouring the gelPowerPoint Presentation: Each of the gel combs should be submerged in the melted agarose solution.PowerPoint Presentation: When cooled, the agarose polymerizes, forming a flexible gel. It should appear lighter in color when completely cooled (30-45 minutes). Carefully remove the combs and tape.PowerPoint Presentation: Place the gel in the electrophoresis chamber.PowerPoint Presentation: buffer Add enough electrophoresis buffer to cover the gel to a depth of at least 1 mm. Make sure each well is filled with buffer. Cathode (negative) Anode (positive) wells DNA PowerPoint Presentation: 6X Loading Buffer: Bromophenol Blue (for color) Glycerol (for weight) Sample Preparation Mix the samples of DNA with the 6X sample loading buffer (w/ tracking dye). This allows the samples to be seen when loading onto the gel, and increases the density of the samples, causing them to sink into the gel wells.PowerPoint Presentation: Loading the Gel Carefully place the pipette tip over a well and gently expel the sample. The sample should sink into the well. Be careful not to puncture the gel with the pipette tip.PowerPoint Presentation: Place the cover on the electrophoresis chamber, connecting the electrical leads. Connect the electrical leads to the power supply. Be sure the leads are attached correctly - DNA migrates toward the anode (red). When the power is turned on, bubbles should form on the electrodes in the electrophoresis chamber. Running the GelPowerPoint Presentation: wells Bromophenol Blue Cathode (-) Anode (+) Gel After the current is applied, make sure the Gel is running in the correct direction. Bromophenol blue will run in the same direction as the DNA. DNA (-) PowerPoint Presentation: 100 200 300 1,650 1,000 500 850 650 400 12,000 bp 5,000 2,000 DNA Ladder Standard Inclusion of a DNA ladder (DNAs of know sizes) on the gel makes it easy to determine the sizes of unknown DNAs. - + DNA migration bromophenol blue Note: bromophenol blue migrates at approximately the same rate as a 300 bp DNA moleculePowerPoint Presentation: As an alternative to purchasing costly DNA ladders, one can be created using meal worm ( Tenebrio molitor ) DNA and a restriction enzyme. http://people.uis.edu/rmosh1/DNAexerciseVIIa02.pdfPowerPoint Presentation: Staining the Gel ***CAUTION! Ethidium bromide is a powerful mutagen and is moderately toxic. Gloves should be worn at all times . • Ethidium bromide binds to DNA and fluoresces under UV light, allowing the visualization of DNA on a Gel. • Ethidium bromide can be added to the gel and/or running buffer before the gel is run or the gel can be stained after it has run.PowerPoint Presentation: Safer alternatives to Ethidium Bromide Methylene Blue BioRAD - Bio-Safe DNA Stain Ward’s - QUIKView DNA Stain Carolina BLU Stain …others advantages Inexpensive Less toxic No UV light required No hazardous waste disposal disadvantages Less sensitive More DNA needed on gel Longer staining/destaining timePowerPoint Presentation: Staining the Gel • Place the gel in the staining tray containing warm diluted stain. • Allow the gel to stain for 25-30 minutes. • To remove excess stain, allow the gel to destain in water. • Replace water several times for efficient destain.PowerPoint Presentation: Ethidium Bromide requires an ultraviolet light source to visualizePowerPoint Presentation: Visualizing the DNA (ethidium bromide) 100 200 300 1,650 1,000 500 850 650 400 5,000 bp 2,000 DNA ladder DNA ladder PCR Product 1 2 3 4 5 6 7 8 wells + - - + - + + - Samples # 1, 4, 6 & 7 were positive for Wolbachia DNA Primer dimers PowerPoint Presentation: Visualizing the DNA (QuikVIEW stain) 250 1,500 1,000 500 750 2,000 bp DNA ladder PCR Product wells + - - - - + + - - + - + March 12, 2006 Samples # 1, 6, 7, 10 & 12 were positive for Wolbachia DNA You do not have the permission to view this presentation. In order to view it, please contact the author of the presentation.
Gel Electorphoresis Lecture 2006 lalo34 Download Post to : URL : Related Presentations : Share Add to Flag Embed Email Send to Blogs and Networks Add to Channel Uploaded from authorPOINT lite Insert YouTube videos in PowerPont slides with aS Desktop Copy embed code: (To copy code, click on the text box) Embed: URL: Thumbnail: WordPress Embed Customize Embed The presentation is successfully added In Your Favorites. Views: 36 Category: Science & Tech.. License: All Rights Reserved Like it (0) Dislike it (0) Added: December 23, 2011 This Presentation is Public Favorites: 0 Presentation Description No description available. Comments Posting comment... Premium member Presentation Transcript PowerPoint Presentation: Discover the Microbes Within How many species have Wolbachia?Agarose Gel Electrophoresis: Agarose Gel Electrophoresis Gel electrophoresis is a widely used technique for the analysis of nucleic acids and proteins . Agarose gel electrophoresis is routinely used for the preparation and analysis of DNA. Gel electrophoresis is a procedure that separates molecules on the basis of their rate of movement through a gel under the influence of an electrical field. We will be using agarose gel electrophoresis to determine the presence and size of PCR products. PCR products indicate the presence of Wolbachia.PowerPoint Presentation: http://gslc.genetics.utah.edu/units/biotech/gel/ Virtual Gel Electrophoresis Additional Information on Gel Electrophoresis:PowerPoint Presentation: • DNA is negatively charged. + - Power DNA • When placed in an electrical field, DNA will migrate toward the positive pole (anode). H O 2 • An agarose gel is used to slow the movement of DNA and separate by size. Scanning Electron Micrograph of Agarose Gel (1×1 µm) • Polymerized agarose is porous, allowing for the movement of DNAPowerPoint Presentation: + - Power DNA How fast will the DNA migrate? strength of the electrical field , buffer, density of agarose gel… Size of the DNA! *Small DNA move faster than large DNA …gel electrophoresis separates DNA according to size small large Within an agarose gel, linear DNA migrate inversely proportional to the log10 of their molecular weight.PowerPoint Presentation: Agarose Agarose is a linear polymer extracted from seaweed. D-galactose 3,6-anhydro L-galactose Sweetened agarose gels have been eaten in the Far East since the 17th century. Agarose was first used in biology when Robert Koch* used it as a culture medium for Tuberculosis bacteria in 1882 *Lina Hesse , technician and illustrator for a colleague of Koch was the first to suggest agar for use in culturing bacteriaPowerPoint Presentation: Making an Agarose GelPowerPoint Presentation: An agarose gel is prepared by combining agarose powder and a buffer solution. Agarose Buffer Flask for boiling PowerPoint Presentation: Casting tray Gel combs Power supply Gel tank Cover Electrical leads Electrophoresis EquipmentPowerPoint Presentation: Gel casting tray & combsPowerPoint Presentation: Seal the edges of the casting tray and put in the combs. Place the casting tray on a level surface. None of the gel combs should be touching the surface of the casting tray. Preparing the Casting TrayPowerPoint Presentation: Agarose Buffer Solution Combine the agarose powder and buffer solution. Use a flask that is several times larger than the volume of buffer.PowerPoint Presentation: Agarose is insoluble at room temperature (left). The agarose solution is boiled until clear (right). Gently swirl the solution periodically when heating to allow all the grains of agarose to dissolve. ***Be careful when boiling - the agarose solution may become superheated and may boil violently if it has been heated too long in a microwave oven. Melting the AgarosePowerPoint Presentation: Allow the agarose solution to cool slightly (~60ºC) and then carefully pour the melted agarose solution into the casting tray. Avoid air bubbles. Pouring the gelPowerPoint Presentation: Each of the gel combs should be submerged in the melted agarose solution.PowerPoint Presentation: When cooled, the agarose polymerizes, forming a flexible gel. It should appear lighter in color when completely cooled (30-45 minutes). Carefully remove the combs and tape.PowerPoint Presentation: Place the gel in the electrophoresis chamber.PowerPoint Presentation: buffer Add enough electrophoresis buffer to cover the gel to a depth of at least 1 mm. Make sure each well is filled with buffer. Cathode (negative) Anode (positive) wells DNA PowerPoint Presentation: 6X Loading Buffer: Bromophenol Blue (for color) Glycerol (for weight) Sample Preparation Mix the samples of DNA with the 6X sample loading buffer (w/ tracking dye). This allows the samples to be seen when loading onto the gel, and increases the density of the samples, causing them to sink into the gel wells.PowerPoint Presentation: Loading the Gel Carefully place the pipette tip over a well and gently expel the sample. The sample should sink into the well. Be careful not to puncture the gel with the pipette tip.PowerPoint Presentation: Place the cover on the electrophoresis chamber, connecting the electrical leads. Connect the electrical leads to the power supply. Be sure the leads are attached correctly - DNA migrates toward the anode (red). When the power is turned on, bubbles should form on the electrodes in the electrophoresis chamber. Running the GelPowerPoint Presentation: wells Bromophenol Blue Cathode (-) Anode (+) Gel After the current is applied, make sure the Gel is running in the correct direction. Bromophenol blue will run in the same direction as the DNA. DNA (-) PowerPoint Presentation: 100 200 300 1,650 1,000 500 850 650 400 12,000 bp 5,000 2,000 DNA Ladder Standard Inclusion of a DNA ladder (DNAs of know sizes) on the gel makes it easy to determine the sizes of unknown DNAs. - + DNA migration bromophenol blue Note: bromophenol blue migrates at approximately the same rate as a 300 bp DNA moleculePowerPoint Presentation: As an alternative to purchasing costly DNA ladders, one can be created using meal worm ( Tenebrio molitor ) DNA and a restriction enzyme. http://people.uis.edu/rmosh1/DNAexerciseVIIa02.pdfPowerPoint Presentation: Staining the Gel ***CAUTION! Ethidium bromide is a powerful mutagen and is moderately toxic. Gloves should be worn at all times . • Ethidium bromide binds to DNA and fluoresces under UV light, allowing the visualization of DNA on a Gel. • Ethidium bromide can be added to the gel and/or running buffer before the gel is run or the gel can be stained after it has run.PowerPoint Presentation: Safer alternatives to Ethidium Bromide Methylene Blue BioRAD - Bio-Safe DNA Stain Ward’s - QUIKView DNA Stain Carolina BLU Stain …others advantages Inexpensive Less toxic No UV light required No hazardous waste disposal disadvantages Less sensitive More DNA needed on gel Longer staining/destaining timePowerPoint Presentation: Staining the Gel • Place the gel in the staining tray containing warm diluted stain. • Allow the gel to stain for 25-30 minutes. • To remove excess stain, allow the gel to destain in water. • Replace water several times for efficient destain.PowerPoint Presentation: Ethidium Bromide requires an ultraviolet light source to visualizePowerPoint Presentation: Visualizing the DNA (ethidium bromide) 100 200 300 1,650 1,000 500 850 650 400 5,000 bp 2,000 DNA ladder DNA ladder PCR Product 1 2 3 4 5 6 7 8 wells + - - + - + + - Samples # 1, 4, 6 & 7 were positive for Wolbachia DNA Primer dimers PowerPoint Presentation: Visualizing the DNA (QuikVIEW stain) 250 1,500 1,000 500 750 2,000 bp DNA ladder PCR Product wells + - - - - + + - - + - + March 12, 2006 Samples # 1, 6, 7, 10 & 12 were positive for Wolbachia DNA