Teaching Evolution through Inquiry with Bio
Welcome! Teaching Evolution through Inquiry with Bio-Rad & Vernier Workshop Timeline • Introduction • Comparative Proteomics I : Protein Profiler – Introduction to Kit – Load and electrophorese protein samples – Compare protein profiles – Stain polyacrylamide gels – Construct cladograms – BLAST to construct cladograms • Biofuel Enzyme Kit: Activity 6 – Introduction to Kit – Extract Cellobiase from Mushrooms – Run enzyme reaction – Obtain quantitative data with spectrophotometry – Compare Mushroom activities • Look at Protein Profiler gels • Other evolution labs brief – PV92 How does this fit with AP Biology? Big Idea 1 Protein Profiler Biofuel Enzyme PV92 PCR pGLO Transformation DNA Fingerprinting DNA Protein Trait Ways to analyze evolutionary relatedness Comparative Proteomics Kit I: Protein Profiler Module Technology Engineering Math Science Inquiry Comparative Proteomics I: Protein Profiler Kit Advantages • Analyze protein profiles from a variety of fish • Study protein structure/function • Use polyacrylamide electrophoresis to separate proteins by size • Construct cladograms using data from students’ gel analysis • Compare biochemical and phylogenetic relationships. Hands-on evolution wet lab • Sufficient materials for 8 student workstations • Can be completed in three 45 minute lab sessions Workflow Set Up Protein Electrophoresis units Mini-Protean TGX Gels Using a Micropipette Plunger Two stops 1st – defines volume 2nd – ejects volume Tip Ejector Run Protein Electrophoresis Lane 1-2 Lane 3 Lane 4-8 Lane 9 Empty 5ul Protein ladder 5ul Fish samples 5ul Actin & Myosin Standards 300V 18 minutes Samples Actin • 5% of total protein • 20% of vertebrate muscle mass • 375 amino acids = 42 kD Myosin •Tetramer •two heavy subunits (220 kD) •two light subunits (15-25 kD) •Uses ATP for muscle contraction Muscle Contains Proteins of Many Sizes Protein kD Function Titin 3000 Center myosin in sarcomere Dystrophin 400 Anchoring to plasma membrane Filamin 270 Cross-link filaments 210 Slide filaments Myosin heavy chain Spectrin 265 Attach filaments to plasma membrane Nebulin 107 Regulate actin assembly -actinin 100 Bundle filaments Gelosin 90 Fragment filaments Fimbrin 68 Bundle filaments Actin 42 Form filaments Tropomysin 35 Strengthen filaments Myosin light chain 15-25 Slide filaments 30, 19, 17 Mediate contraction Troponin (T.I.C.) Thymosin 5 Sequester actin monomers Levels of Protein Organization 1o 2o 3o 4o What’s in the Sample Buffer? & Why? • Tris buffer to provide appropriate pH • Glycerol to make samples sink into wells • Bromophenol Blue dye to visualize samples • SDS (sodium dodecyl sulfate) detergent to dissolve proteins and give them a negative charge Sample Prep heat Protein Gel (polyacrylamide) Separates Proteins based ONLY on their size TGS Buffer • Tris-HCL • Glycine (shielding for stacking) • SDS Why Use Polyacrylamide Gels to Separate Proteins? • Smaller pore size than agarose – Polyacrylamide gel 20-200nm pores – 3% agarose 40-80 nm pores – 1% agarose 200-1200 nm pores • Proteins are much smaller than DNA – Average amino acid = 110 daltons – Average nucleotide pair = 649 daltons – 1 kilobase of DNA = 650 kD – 1 kilobase of DNA encodes 333 amino acids = 36 kD Can Proteins be Separated on Agarose Gels? 250 150 100 75 50 37 250 Myosin Heavy Chain Actin Tropomyosin 25 Myosin Heavy Chain 150 100 75 50 Actin Tropomyosin 37 20 Myosin Light Chains 15 25 Myosin Light Chains 20 10 Polyacrylamide 3% Agarose Retrieve Gels Cut off wells and foot of gel Gel Staining Water – 5 minutes Stain – 1 hour Gel Imaging GelDoc EZ White Digital Bioimaging system Polyacrylamide Gel Analysis 250 150 100 75 50 37 Myosin Heavy Chain (210 kD) Actin (42 kD) Tropomyosin (35 kD) 25 20 Myosin Light Chain 1 (21 kD) Myosin Light Chain 2 (19 kD) Myosin Light Chain 3 (16 kD) 15 10 Using Protein Bands between 30 and 10 kb for analysis Molecular Mass Estimation 50 45 40 37 (12 mm) 25 (17 mm) 20 (22 mm) 15 (27.5 mm) 10 (36 mm) Size (kD) 35 30 25 20 15 10 5 0 0 10 20 Distance migrated (mm) 30 40 Molecular Mass Analysis With Semi-log Graph Paper Size (kD) 100 10 0 10 20 30 Distance migrated (mm) 40 Each Fish Has a Distinct Set of Proteins Shark Salmon Trout Catfish Sturgeon Total # proteins 8 10 13 10 12 Distance proteins migrated (mm) 25, 26.5, 29, 36, 36.5, 39, 44, 52 26, 27.5, 29, 32, 34.5, 36.5, 37.5, 40.5, 42, 45 26, 27.5, 29, 29.5, 32, 34.5, 36.5, 37.5, 40.5, 42, 45, 46.5, 51.5 26, 27.5, 29, 32, 36.5, 38, 38.5, 41, 46, 47.5 26, 27.5, 30, 30.5, 33, 35.5, 37, 39, 39.5, 42, 44, 47 26 31.5 26.5 31.0 27.5 30.0 28.5 29.1 29 28.6 30 27.6 30.5 27.1 32 25.6 33 24.7 34.5 23.2 35.5 22.2 36 21.7 X 36.5 21.2 X 37 20.7 37.5 20.2 38 19.7 X 38.5 19.3 X Sturgeon X Catfish Shark 32.5 Trout Size (kD) 25 Salmon Distance (mm) Some of Those Proteins Are Shared Between Fish X X X X X X X X X X X X X X X X X X X X X X X X X X X X X Character Matrix Is Generated and Cladogram Constructed Shark Salmon Trout Catfish Sturgeon Shark 8 2 2 2 2 Salmon 2 10 10 5 3 Trout 2 10 13 5 4 Catfish 2 5 5 10 2 Sturgeon 2 3 4 2 12 Shark Sturgeon Catfish Trout Salmon Phylogenetic Tree Evolutionary tree showing the relationships of eukaryotes. (Figure adapted from the tree of life web page from the University of Arizona (www.tolweb.org).) Pairs of Fish May Have More in Common Than to the Others Shark Salmon Trout Catfish Sturgeon Carp Shark 8 2 2 2 2 2 Salmon 2 10 10 5 3 5 Trout 2 10 13 5 4 5 Catfish 2 5 5 10 2 8 Sturge on 2 3 4 2 12 2 Carp 2 5 5 8 2 11 Shark Sturgeon Catfish Carp Trout Salmon BLAST Searches with Protein Profiler (Appendix B) Uses Myosin Heavy Chain from Rainbow trout •Pre-run blast searches in manual •Protocol to run your own searches Chart Differences: 0 8 8 9 9 7 11 11 13 11 Clustal-W Analysis (Sequence) Biofuel Enzyme Kit Activity 6 – a functional proteomics approach to evolution in fungi Engineering Technology Math Science Inquiry Biofuel Enzyme Kit Advantages • Aligns with AP Biology Learning Objectives LO 1.14, LO 1.17, LO 1.18, LO 1.19, LO 2.1, LO 2.2, LO 2.3, LO 2.4, LO 2.10, LO 4.14, LO 4.15, LO 4.18) • Can be run qualitatively or quantitatively • Construct and use a standard curve (mathematics and technology) • Determine the effects on the reaction rate by changing: – pH – temperature – enzyme/substrate concentration • Mushroom extract activity for student run inquiry • Extension for Michaelis-Menten analysis What are enzymes? Molecules, usually proteins, that speed up the rate of a reaction by decreasing the activation energy required without themselves being altered or used up Enzyme Class Example Oxidoreductase Firefly Luciferase – oxidizes luciferin to produce oxyluciferin and light Transferase Hexokinase – transfers a phosphate group to glucose to make glucose-6-phosphate Hydrolase Cellobiase – breaks down cellobiose Lyase Histidine decarboxylase – generates histimine from histidine Isomerase Glucose-6-Phosphate isomerase – converts G-6-P to fructose-6phosphate Ligase DNA Ligase – covalently bonds two pieces of DNA (transfer of electrons) (group-transfer reactions) (hydrolysis reactions) (double bond reactions) (transfers to create a new isomers) (forms covalent bonds) Substrate (S) How do enzymes work? Energy considerations Enzyme Product (P) S* E N E R G Y S*enz Eact Eact S P REACTION COORDINATE How do enzymes work? Substrate free in solution Substrate binds to a specific cleft or groove in the enzyme Physical considerations Activation energy barrier is overcome and reaction occurs Product is released and enzyme is free to catalyze another reaction What are biofuels? Fuels that are produced from a biological source • Oil – biofuel, but very long production cycle (millions of years) Short cycle Biofuels • Biodiesel • Ethanol from starches/sugars • Cellulosic ethanol •Butanol Cellulosic ethanol production A B C D Cellulose breakdown 1. Heat, acid, ammonia or other treatment 2. Enzyme mixture added Glucose Endocellulases Exocellulases Cellobiase Cellobiose breakdowna closer look 4 1 4 6 5 3 + Cellobiose + H2O 2 1 2 Glucose Protocol Highlights: Using a colorimetric substrate to track reaction rate • Cellobiose and glucose are colorless when dissolved • Use of the artificial substrate p-nitrophenyl glucopyranoside allows the reaction to be tracked by monitoring the appearance of yellow color cellobiose p-nitrophenyl glucopyranoside Cellobiase breakdown of pnitrophenyl glucopyranoside + p-nitrophenyl glucopyranoside + H2O glucose + p-nitrophenol Basic conditions Clear Yellow Biofuels Activity 1 Overview How can this enzymatic reaction be easily quantified? Basic solution (STOP SOLUTION): - will develop color of any p-nitrophenol present - will stop the reaction • Qualitative - Each reaction time point can be directly compared to a standard of known concentration of p-nitrophenol • Quantitative- The amount of yellow color in the reaction solution can be quantified by measuring the absorbance at 410 nm using a spectrophotometer or microplate reader. Biofuel Enzyme Kit Procedure Overview Collaborative approach: • Each student group does activity 1 • Student groups do one activity each from 2-5 • Groups share data • All groups do activity 6 and share data Activities: 1. Reaction Rate & Std curve 2. Effect of Temperature 3. Effect of pH 4. Effect of Enzyme Concentration 5. Effect of Substrate Concentration 6. Bio-prospecting for Celliobiase S1 0 0 S2 12.5 0.2 S3 25 0.4 S4 50 0.8 S5 100 1.6 410 nm Standard Curve 1.8 Absorbance at 410 nm 1. Std curve / Std Reaction Rate 2. Effect of Temperature 3. Effect of pH 4. Effect of Enzyme Concentration 5. Effect of Substrate Concentration 6. Bio-prospecting for Celliobiase Absorbance Standard Amount of p-nitrophenol (nmol) 1.6 1.4 1.2 1.0 0.8 0.6 0.4 0.2 0.0 0 20 40 60 80 100 Amount of p -nitrophenol (nmol) 120 Standard Curve 1.8 Absorbance at 410 nm 1. Std curve / Std Reaction Rate 2. Effect of Temperature 3. Effect of pH 4. Effect of Enzyme Concentration 5. Effect of Substrate Concentration 6. Bio-prospecting for Celliobiase 1.6 1.4 1.2 1.0 0.8 0.6 0.4 0.2 0.0 0 20 40 60 80 100 Amount of p -nitrophenol (nmol) 120 Reaction Rate with Enzyme Amount of p -nitrophenol (nmol) 1. Std curve / Std Reaction Rate 2. Effect of Temperature 3. Effect of pH 4. Effect of Enzyme Concentration 5. Effect of Substrate Concentration 6. Bio-prospecting for Celliobiase 100 80 60 40 20 0 0 2 4 6 8 10 Time (min) Initial reaction rate = Amount of p-nitrophenol produced (nmol) Time (min) Initial reaction rate = 50 nmol - 0 nmol 4 min - 0 min = 12.5 nmol/min Activity 2 : Effect of Temp on Reaction Rate rate p-nitrophenol produced (nmol/min) 1. Std curve / Std Reaction Rate 2. Effect of Temperature 3. Effect of pH 4. Effect of Enzyme Concentration 5. Effect of Substrate Concentration 6. Bio-prospecting for Celliobiase 100 90 80 70 60 50 40 30 20 10 0 Expon. 0 10 20 Temperature (C) 30 40 Initial reaction rate = Time (min) •This is the amount of p-nitrophenol produced in 2 minutes Effect of pH on Initial Reaction Rate 20 Rate of p -nitrophenol produced (nmol/min) 1. Std curve / Std Reaction Rate 2. Effect of Temperature 3. Effect of pH 4. Effect of Enzyme Concentration 5. Effect of Substrate Concentration 6. Bio-prospecting for Celliobiase Amount of p-nitrophenol produced (nmol) 18 16 14 12 10 8 6 4 2 0 4 5 6 7 pH 8 9 Amount of pnitrophenol formed (nmol) 1. Std curve / Std Reaction Rate 2. Effect of Temperature 3. Effect of pH 4. Effect of Enzyme Concentration 5. Effect of Substrate Concentration 6. Bio-prospecting for Celliobiase High enzyme concentration Low enzyme concentration Time (minutes) 1. The initial reaction rate is faster when there is a higher enzyme concentration 2. Given enough time, the same amount of product will be formed for both the high and low enzyme concentration reactions Amount of pnitrophenol formed (nmol) 1. Std curve / Std Reaction Rate 2. Effect of Temperature 3. Effect of pH 4. Effect of Enzyme Concentration 5. Effect of Substrate Concentration 6. Bio-prospecting for Celliobiase 1.5 mM substrate [High] 0.25 mM substrate [Low] Time (minutes) 1. Effect of substrate concentration on the initial rate 2. Final amount of product formed with varying substrate concentrations 1. Std curve / Std Reaction Rate 2. Effect of Temperature 3. Effect of pH 4. Effect of Enzyme Concentration 5. Effect of Substrate Concentration 6. Bio-prospecting for Celliobiase Where can we find things that break down cellulose? 1. Std curve / Std Reaction Rate 2. Effect of Temperature 3. Effect of pH 4. Effect of Enzyme Concentration 5. Effect of Substrate Concentration 6. Bio-prospecting for Celliobiase Mushrooms – Ecological niche for food •Mycorrhizal –associated with plant roots •Porcini •Chanterelle •Saprotrophic – decomposers •Shiitake •Morel •Button •Parasitic – attacks plants •Honey Mushroom •Endophytes – grows in plant cells Activity 6 Protocol 1. Pick a mushroom 2. Add 0.25g of mushroom to microcentrifuge tube 3. crush with blunted pipette tip 4. Add 500 µl extraction buffer and continue crushing 5. Spin down extract in microcentrifuge to separate mushroom particle from liquid fraction Activity 6 Protocol 6. 7. 8. Activity 6 Protocol SmartSpec™ Plus Photodiode Array UV-VIS Spectrometer Measures Absorbance , %T Specifications Range: 200-800 nm Optical Resolution: ± 2 nm Light Source: Xenon Flash Lamp Power: 120 VAC, 60 Hz Standalone Research Grade Instrument 170-2525EDU SpectroVis® Plus CCD Array VIS-NIR Spectrometer/Fluorometer Measures Multiple Parameters Specifications SVIS-PL Absorbance , %T Fluorescence (excitation at 405 or 500 nm) Emissions Spectra (fiber optic cable required) Range: 380950 nm Optical Resolution: ± 2.5 nm Reporting Interval: 1 nm Light Source: LED boosted tungsten bulb Power: USB port LabQuest or Logger Pro Software required S1 0 0 S2 12.5 0.2 S3 25 0.4 S4 50 0.8 S5 100 1.6 410 nm Standard Curve 1.8 Absorbance at 410 nm 1. Std curve / Std Reaction Rate 2. Effect of Temperature 3. Effect of pH 4. Effect of Enzyme Concentration 5. Effect of Substrate Concentration 6. Bio-prospecting for Celliobiase Absorbance Standard Amount of p-nitrophenol (nmol) 1.6 1.4 1.2 1.0 0.8 0.6 0.4 0.2 0.0 0 20 40 60 80 100 120 Amount of p -nitrophenol (nmol) Y = mx + b, solve for X M = slope b = y-intercept (can use 0 for ease) 1. Std curve / Std Reaction Rate 2. Effect of Temperature 3. Effect of pH 4. Effect of Enzyme Concentration 5. Effect of Substrate Concentration 6. Bio-prospecting for Celliobiase Derive p-nitrophenol concentrations from Abs data X = (y-b)/m Absorbance Time #1 – 1 min #2 – 2 min #3 – 4 min #4 – 6 min #5 – 8 min #6 - Blank 410 nm Amount of p-nitrophenol (nmol) 125 Add your Data! (general trend line is fine) P-nitrophenol (nmol) 100 75 50 25 1 2 3 4 Time (minutes) 5 6 7 8 P-nitrophenol (nmol) 1. Std curve / Std Reaction Rate 2. Effect of Temperature 3. Effect of pH 4. Effect of Enzyme Concentration 5. Effect of Substrate Concentration 6. Bio-prospecting for Celliobiase Time (minutes) Rate correlates to ecological niche which is based upon its evolution Chromosome 16: PV92 PCR Informatics Kit Advantages • Aligns with new AP Biology Big Ideas 1 & 3 • Inquiry: Extract genomic DNA and amplify student samples • Introduce the polymerase chain reaction (PCR) • Apply PCR to population genetics / evolution – Hardy-Weinberg analysis • Directly measure human diversity at the molecular level • Compare results to online Alu data; DNA Learning Center • Sufficient materials for 8 student workstations • Complete activity in three 45 minute sessions Additional Resources • Investigating Biology through Inquiry by Vernier • Dropbox curriculum folders – Powerpoints, electronic copies of manuals, tips/tricks, links to animations/videos, etc – eMail your CTS • 20 Questions to Master Inquiry Bio-Rad CTS Contacts & Vernier Biology Specialists Bio-Rad Curriculum and Training Specialists: Sherri Andrews, Ph.D. – Eastern U.S. [email protected] Damon Tighe – Western U.S. [email protected] Leigh Brown, M.A. – Central U.S. [email protected] Vernier: John Melville [email protected] Michael Collins [email protected]
© Copyright 2024