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Genetically Engineered H 2 Detector Mississippi State University.

Published byEugene Stanley Modified over 8 years ago

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Presentation on theme: "Genetically Engineered H 2 Detector Mississippi State University."— Presentation transcript:

1 Genetically Engineered H 2 Detector Mississippi State University

2 Present Areas of Interest  Departmental Goal – Produce oil for biodiesel  Dr. To wanted to find out if we could engineer bacteria to produce biodiesel efficiently  We decided to start small

3 Team Goals  Learn procedure for genetically engineered machines  Combine knowledge from several departments ABE, BCH, ChE, ECE  Develop network with MIT and other iGEM partners to allow for future collaboration

4 Our Team

5 Our Team - Professors  Agricultural and Biological Engineering Dr. Filip To  Biochemistry Dr. Din-Pow Ma  Electrical and Computer Engineering Dr. Bob Reese  Chemical Engineering Dr. Todd French

6 Our Team - Students  Agricultural and Biological Engineering Graduate  Brendan Flynn, Robert Morris Undergraduate  Teri Vaughn, Lauren Beatty, Scott Tran, Joe Chen, Sam Pote, Paul Kimbrough  Biochemistry Graduate  Victor Ho

7 Desired Machine Function  We wanted to design a machine to detect the presence of H 2  The machine would function when “turned on” by an inducer  The machine would produce quantifiable fluorescence dependent on H 2 concentration

8 Uses  Quantifiable detection of H 2  This function could possibly be incorporated into bacteria used in the production of H 2 in the future

9 Design - Parts Our Composite Part - J43001 J45503 Q04121 E0430 H 2 Promoter LacI QPI YFP Reporter

10 Design – Part Descriptions J45503Cold shock promoter and H 2 promoter Q04121LacI QPI (Quad Part Inverter), composite E0430YFP output device, composite J45503 Q04121 E0430

11 Design – Subparts – Q04121 SubpartDescription B0034Strong RBS C0012LacI coding region B0015Double terminator R0011Strong promoter, Repressed by LacI, Induced by IPTG B0034 C0012 B0015 R0011 = Q04121

12 Design – Subparts – E0430 SubpartDescription B0034Strong RBS E0030YFP coding B0015Double terminator B0034 E0030 B0015 = E0430

13 Design - Components hybB H 2 Promoter LacI repress or gene LacI promo ter YFP reporter Ribosome Binding Site Terminator

14 XX YFP J43000 In Action Lac promoter naturally shows an active but low transcription level

15 IPTG XX YFP J43000 In Action IPTG is a synthetic inducer

16 IPTG XX YFP J43000 In Action IPTG induces a high level of transcription at the Lac Promoter

17 XX IPTG YFP J43000 In Action A large amount of YFP is transcribed and translated

18 H2H2 XX IPTG YFP J43000 In Action Hydrogen is introduced to the machine

19 H2H2 X IPTG YFP J43000 In Action Hydrogen turns on the hybB promoter

20 lacI H2H2 IPTG YFP J43000 In Action The lacI gene is transcribed

21 lacI IPTG Competitive Inhibition H2H2 YFP J43000 In Action LacI repressor inhibits the lac promoter

22 lacI IPTG Competitive Inhibition H2H2 YFP J43000 In Action Lac promoter transcription is reduced, leading to lower YFP transcription

23 lacI IPTG Competitive Inhibition H2H2 YFP H2H2 H2H2 J43000 In Action Hydrogen concentration is increased

24 lacI IPTG Competitive Inhibition H2H2 YFP H2H2 H2H2 J43000 In Action Lac promoter is further repressed, leading to lower YFP production

25 lacI IPTG Competitive Inhibition H2H2 YFP H2H2 H2H2 H2H2 H2H2 J43000 In Action Machine is exposed to a high H 2 concentration

26 lacI IPTG Competitive Inhibition H2H2 YFP H2H2 H2H2 H2H2 H2H2 J43000 In Action Lac promoter is strongly repressed, YFP production is reduced to minimum

27 Testing Our Machine Requirements Introduction of inducer (IPTG)  Provides a broader range in fluorescence levels Varied H 2 concentrations Fluorescence quantification

28 Testing Our Machine  Gasing Cells were grown in septum topped vacuum ready tubes A vacuum pump is used to extract air from the tube Each tube is filled with a specific H 2 concentration

29 Testing Our Machine  Photos The samples were exposed to light wavelengths close to YFP absorption wavelength Pictures were taken using a digital camera with fixed settings Pictures were taken before, immediately after, and 5 hours after gassing

30 Our Machine Visible fluorescence compared to unmodified E. coli

31 Testing Our Machine  Analysis MatLAB pixel analysis  Averaged pixel value for a selected area 5 data sets were taken for each sample Fluorescence change was calculated for pre-gassing samples and samples 5 hours after gassing Changes were zeroed to wild type E.Coli fluorescence changes

32 Results

33 Results – Functional Machine  Minimal YFP production without addition of IPTG  Strong YFP production with addition of IPTG  Proportional reduction in fluorescence with addition of H 2

34 Further Work Required Fluorescence in 100% H 2 was actually higher than fluorescence in 75% H 2  Why? Positive results were obtained after incubating for 5 hours  Detection is NOT immediate More precise testing using wavelengths specific to YFP absorption and emission

35 Acknowledgements  Advisors Dr. Filip To, Dr. Din-Pow Ma, Dr. Todd French  MSU Bagley College of Engineering  MSU College of Agriculture and Life Sciences  iGEM Ambassador James Brown  iGEM Staff

36 Future Ideas Controlled Lipid Synthesis  Produce efficient energy source from inefficient organic energy sources Water Splitting  Efficient, portable H 2 production Tar Digestion  Yield cleaner energy sources Insulin and/or Blood Sugar regulator  Diabetes Control

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