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Download Past iGEM Projects: Case Studies
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Past iGEM Projects: Case Studies 2006 Projects: Neat Gadgets • University of Arizona: Bacterial water color • BU: Bacterial nightlight • Brown: Bacterial freeze tag, tri-stable toggle switch • University of Calgary: Dance with swarms • Chiba University, Japan: Swimmy bacteria, aromatic bacteria • Davidson: Solving the pancake problem • Duke: Underwater power plant, cancer stickybot, human encryption, protein cleavage switch, xverter predator/prey • Missouri Western State University: Solving the pancake problem • MIT: Smelly bacteria (best system) • Penn State: Bacteria relay race (passing QS molecules off as batons) • Purdue: Live color printing • Tokyo Alliance: Bacteria that can play tic-tac-toe • UCSF: Remote control steering of bacteria through chemotaxis 2006 Projects: Research Tools • Bangalore: synching cell cycles, memory effects of UV exposure • Berkeley: riboregulator pairs, bacterial conjugation • University of Cambridge: Self-organized pattern formation • Freiburg University: DNA-origami • ETH: Bacterial adder • Harvard: DNA nanostructures, surface display, circadian oscillators • Imperial College: oscillator (great documentation) • University of Michigan: algal bloom, Op Sinks, • McGill: Split YFP / Repressilator • Rice: quorumtaxis • University of Oklahoma: Distributed sensor networks • IPN_UNAM, Mexico: cellular automata (simulations) • University of Texas: Edge detector 2006 Projects: Real World • University of Edinburgh: arsenic detector, (best real world, 3rd best device) • Slovenia: Sepsis prevention (grand prize winner, 2nd best system) • Latin America: UV-iron interaction biosensor • Mississippi State University: H2 reporter • Prairie View: Trimetallic sensors • Princeton: Mouse embryonic stem cell differentiation using artificial signaling pathways (2nd runner up) • University of Toronto: Cell-see-us thermometer Edinburgh: Arsenic Biosensor • Goal: Develop a bacterial biosensor that responds to a range of arsenic concentrations and produces a change in pH that can be calibrated in relation with the arsenic concentration. • Lots of previous research into arsenic biosensors – – – – Gene promoters that respond to presence of arsenic Different outputs available pH is easy, practical, and cheap to measure Signal conversion: ABC where C is easy to detect • System: Arsenate/arsenite detector reporter (pH change) Basic Parts arsR gene codes for repressor that bind to arsenic promoter in absence of arsenate/arsenite Arsenate/arsenite ArsR sensitive promoter arsR gene Link to LacZ, metabolism of lactose creates acidified medium decreased pH Pars arsR lacZ Sensitivity!! Arsenic sensor system diagram 8.5 Lactose Lac regulator Activator gene pH: 7.0 6.0 Activator molecule A1 4.5 A1 binding site Urease gene Promoter |A| Urease enzyme |R| (NH2)2CO + H2O = CO2 + 2NH3 Repressor molecule R1 R1 binding site Ammonia Arsenic (5ppb) Ars regulator 1 Repressor gene R1 LacZ enzyme Arsenic (20ppb) Ars regulator 2 LacZ gene Lactic Acid System Design Results: Increased As sensitivity range: time against pH 7.5 0 ppb 5 ppb 7 15 ppb 30 ppb 6.5 45 ppb pH 60 ppb 6 5.5 • Can detect WHO guideline levels of arsenate • Average overnight difference of 0.81 pH units • Response time of 5 hrs 5 4.5 0 200 400 600 800 1000 1200 Time (in min) 1400 1600 1800 2000 Take Home Message (part 1): • Sensors are relatively straight-forward in design (ABC) • I/O signal sensitivity is key • Tight regulation of detector components • Most of the components were available (engineering vs. research) • Real world applications Slovenia: Sepsis Prevention Goal: Mimic natural tolerance to bacterial infections by building a feedback loop in TLR signaling pathway, which would decrease the overwhelming response to the persistent or repeated stimulus with Pathogen Associated Molecular Patterns (PAMPs). • Engineering mammalian cells • Medical application Altering Signaling Pathway PAMPs TLR MyD88 IRAK4 NFκB cytokines • MyD88: central protein of TLR signaling pathway that transfers signal from TLR receptor to downstream proteins (IRAK4) resulting in the NFκB activation • Method: – Use dominant negative MyD88 to tune down signaling pathway to NF-κB – Addition of degradation tags to dnMyD88 with PEST sequence temporary inhibition to NF-κB CellDesigner: http://www.systems-biology.org/cd/ Measurements / Results • • • Flow cytometry: antibody to phosphorylated ERK kinase to detect TLR activation Luciferase and ELISA assays: level of NF-kB Microscopy 26 new BioBricks for Mammalian Cells Registration number Part's Name BBa_J52008 rluc BBa_J52024 NFκB+dnMyD88-linker-rLuc-linkPEST191 BBa_J52010 NFκB BBa_J52026 dnMyD88-linker-GFP BBa_J52011 dnMyD88-linker-rLuc BBa_J52027 NFκB+dnMyD88-linker-GFP BBa_J52012 rluc-linker-PEST191 BBa_J52028 GFP-PEST191 BBa_J52013 dnMyD88-linker-rluc-linkpest191 BBa_J52029 NFκB+GFP-PEST191 BBa_J52014 NFκB+dnMyD88-linker-rLuc BBa_J52034 CMV BBa_J52016 eukaryotic terminator BBa_J52035 dnMyD88 BBa_J52017 eukaryotic terminator vector BBa_J52036 NFκB+dnMyD88 BBa_J52018 NFκB+rLuc BBa_J52038 CMV-rLuc BBa_J52019 dnTRAF6 BBa_J52039 CMV+rLuc-linker-PEST191 BBa_J52021 dnTRAF6-linker-GFP BBa_J52040 CMV+GFP-PEST191 BBa_J52022 NFκB+dnTRAF6-linker-GFP BBa_J52642 GFP BBa_J52023 NFκB+rLuc-linker-PEST191 BBa_J52648 CMV+GFP Take Home Message (part 2): • Lessons from their team: – Use reliable oligo vendors – Double check biobrick parts for incorrectly registered parts • Lot of work to find out optimal parameters for cell activation (inducer conc., etc.) • Mammalian cells are more challenging to work with • Requires more sophisticated readouts • Make new biobricks! • Reward is great