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<figcaption><b>Fig. 5 </b>. Characterization results of PesaS and PesaRp-RBS(B0034)-mKate in L19 and L31</figcaption> | <figcaption><b>Fig. 5 </b>. Characterization results of PesaS and PesaRp-RBS(B0034)-mKate in L19 and L31</figcaption> | ||
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Revision as of 15:45, 11 October 2023
PHB production Regulation: PesaS-B0034-gltA-PesaRwt-B0034-PHBcab-PYU16-B0034-SRRz
PesaS-B0034-gltA-PesaRwt-B0034-PHBcab-PYU16-B0034-SRRz
Usage and Biology
Many production processes using microorganisms face the dilemma of conflicting production products and key metabolic pathways. This means that simply introducing product-synthesising genes into engineered bacteria can greatly affect the growth of the microorganism, leading to a situation where production is too low. There are a number of current solutions to this problem. For example, metabolic engineering can regulate metabolic flow using methods such as gene knockdown, promoter replacement, etc. These static strategies are effective for productivity improvement, but are not responsive to changes in the cell or environment. Dynamic control is a favourable solution for the conditional knockdown of essential genes and balances the flow in the metabolic pathway.
The pathway of PHB synthetsis is conflict with TCA cycle. Both TCA cycle and PHB production pathways use acetyl-coA as raw material, so if only the PHB production gene circuit is simply added to the engineered bacteria, the growth of the bacteria will be greatly affected, and the final result is low PHB production. Quorum sensing system can automatically sense cell density to regulate downstream genetic on/off. It is independent of metabolic pathways and do not need exogenous inducers, which make it a perfect tool to solve this problem. PHB are a form of carbon storage by bacteria. PHB products take up most of the space inside the cell, but will not be released from the cell. The method of mechanical crushing or chemical solvent extraction used in traditional industry is not only expensive, but also brings great pressure to the environment, so we hope to design an auto-lysis system with specific expression time. This part is about PHB Production Regulation based on the Three-layer Dynamic Regulation Model. It dynamically regulate the PHB production by dividing the process into 3 phases: Growth Phase, Production Phase and Product-release Phase. In this way, the cell can firstly grow up and then put their all effort into PHB production. Finally, in the late stationary phase of cell growth, the enigneered bacteria can express lysis gene.
1. Three-layer Dynamic Regulation Model
2. The first and second layer--Growth and production control
Quorum Sensing is a way for cells to regulate downstream gene expression based on their own density. The concentration of the signaling molecule - AHL - secreted by the cell increases as the cell density increases. When the concentration of AHL reaches a certain level, it can bind to the corresponding binding protein and alter the expression of downstream genes.
In the first and second layer, this part using a QS-switch to regulate the flow of acetyl-coA. At the early stage of growth, using QS-switch turn on the TCA cycle and turn off the PHB production pathway, so that acetyl-coA flowed into the TCA cycle and the cells grew. When the cell grows to a certain extent, the TCA cycle is turned off, while the PHB production pathway is turned on, and the acetyl-coA flows to the PHB production pathway for PHB production.
4. The Third layer--Product-release control
In the third layer, this part uses a late stationary phase promoter and an lysis gene. The late stationary phase promoter is used to regulate the expressing time of the downstream gene. When the bacterial reach the stationary phase, the promoter will turn on and then the cell lysis.
Characterization
1. Design
- Step 1: Plasmid construct.
- Step 2: Verify the expression time difference between the first and second layers, and between the second and third layers。
- Step 3: Overall characterization
2. Protocols
Our experimental conditions for characterizing this part were as follows:
- E. coli MG1655
- 30oC, 48h, under vigorous shaking
- Plasmid Backbone: PACYC, pUC
- Equipment: Multi-Detection Microplate Reader (Synergy HT, Biotek, U.S.) and Molecular Devices SpectraMax i3x.
We used GFP (excitation at 485 nm and emission at 535 nm), mKate (excitation at 490 nm and emission at 645 nm), and BFP (excitation at 400 nm and emission at 450 nm) to characterize this part. As our focus was mainly on the expression time, we processed the obtained fluorescence data by means of the following equation: x'=(x-min)/(max-min). This treatment makes all data fall between 0 and 1, which is easier to use for comparisons between different fluorescence data (since our focus is on expression time).
- Fermentation analysis: 1% inoculated in 100mL fermentation medium at 37℃ at 250rpm. Three parallel experiments were conducted for each strain. Samples were taken every 3-4 hours in the first 20 hours, OD600 and glucose concentrations were measured every 6-10 hours after 20 hours, and PHB concentrations were measured after 11 hours. During this period, glucose is supplemented to approximately 20g/L in the fermentation broth based on glucose concentration data.
3. The Characterization of PesaS and PesaRwt/PesaRc/PesaRp
We characterized PesaS-RBS(B0034)-GFP together with PesaRwt-RBS(B0034)-mkate, PesaRc-RBS(B0034)-mkate and PesaRp-RBS(B0034)-mkate. The green curve in the figure shows the results for PesaS. PesaS expression peaks at around 4-6 h and then rapidly declines to 0 at around 8-10 h.
4. The Characterization of PesaRwt/PesaRc/PesaRp and PYU3/PYU7/PYU16/PYU92
Summary of Results
Our part provides an example for future iGEM team
Limitations
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21INCOMPATIBLE WITH RFC[21]Illegal BglII site found at 2740
Illegal BglII site found at 3565
Illegal BamHI site found at 1791
Illegal XhoI site found at 1511 - 23COMPATIBLE WITH RFC[23]
- 25INCOMPATIBLE WITH RFC[25]Illegal NgoMIV site found at 2046
Illegal NgoMIV site found at 2117
Illegal NgoMIV site found at 2717
Illegal NgoMIV site found at 3029
Illegal NgoMIV site found at 3308
Illegal NgoMIV site found at 3960
Illegal NgoMIV site found at 3982 - 1000INCOMPATIBLE WITH RFC[1000]Illegal BsaI site found at 5826
Illegal SapI.rc site found at 769