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Natalie Biggs Mentor: Dr. Joseph Beckman
Copper Binding to Superoxide Dismutase Mutants in Amyotrophic Lateral Sclerosis (ALS) Natalie Biggs Mentor: Dr. Joseph Beckman
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ALS (Lou Gehrig’s Disease)
Fatal disease that causes death of motor neurons 30,000 Americans afflicted currently In 1993 mutations of Cu/Zn superoxide dismutase (SOD) were linked to the disease Dr. Beckman’s research focuses on understanding ALS in an attempt to find a cure Role of Cu/Zn SOD
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Superoxide Dismutase (SOD)
SOD protects the body from oxidative damage Superoxide (O2.-) is a radical that can harm the body SOD reduces (scavenges) superoxide into hydrogen peroxide, a less dangerous radical Michael Potter, UC San Diego
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Determining the Cause of ALS
Dr. Beckman’s hypothesis Zinc deficiency of SOD makes copper act toxically and causes oxidative stress Leads to motor neuron death
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The Controversy Continues
Another prevalent hypothesis Aggregation (clumping) of SOD creates toxicity in the motor neurons Cause of aggregation unknown Copper has no role in causing ALS
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Copper’s Role Challenged
Jiou Wang, et al. Fibrillar Inclusions and Motor Neuron Degeneration in Transgenic Mice Expressing Superoxide Dismutase 1 with a Disrupted Copper-Binding Site. Neurobiology of Disease Mutation of two copper-binding histidines H46R/H48Q mutant SOD Conclusions Aggregation of SOD is responsible for disease Copper has no effect in ALS development
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Project Hypothesis The H46R/H48Q mutant SOD still binds copper
Poor evidence in paper that mutated SOD cannot bind copper Test hypothesis Determine H46R/H48Q mutant SOD’s affinity for binding copper arginine glutamine
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Project Goals Recreate plasmid of H46R/H48Q SOD
Transform and express mutated SOD in Escherichia coli cells Purify mutated SOD Test H46R/H48Q SOD for affinity to bind copper
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Site-Directed Mutagenesis
Use methylated double stranded plasmid Replace with unmethylated H46R/H48Q SOD plasmid Plasmid Preparation Temperature Cycling Digestion Transformation
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Plasmid Purification Select a few E.coli colonies to grow up
Obtain bacterial pellet and add purification buffers Centrifuge again and apply supernatant to QIAGEN tip Precipitate DNA, wash, and resuspend in TE buffer
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Transformation and Expression
H46R/H48Q SOD plasmid is inserted into E.coli cells Colonies are selected to induce mutant SOD expression Large quantities of H46R/H48Q SOD produced
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Purification Lyse (break open) cells to release contents
Precipitate unwanted proteins using pH changes Anion exchange column
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PAR (4-pyridylazoresorcinol) Assay
PAR binds copper and zinc Measure absorbance at 500 nm Absorbance increases as PAR binds the metals Absorbance decreases if SOD can compete to bind copper and zinc Test H46R/H48Q SOD Determine affinity for copper
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Results and Conclusions
Created H46R/H48Q SOD plasmid DNA sequencing Screened a few colonies of E.coli None contained mutated SOD Started again at the transformation step Check purified SOD in mass spectrometer If correct mutant, begin testing with PAR assay
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Acknowledgments Howard Hughes Medical Institute
Linus Pauling Institute Dr. Joseph Beckman Dr. Kevin Ahern Keith Nylin Valerie Bomben
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