Model
Contents
1. Overview
To recreate the story of ”Snow White”, we have designed a cell-cell communication system with improved or characterized parts and collected data from comprehensive experiments. Furthermore, we constructed the mathematical model to simulate the behavior of the whole system and to confirm the feasibility of our story. This simulation successfully contributed to give the suggestions to wet lab experiments. In addition, in order to help us utilize our Toxin-Antitoxin (TA) system, we developed a new software in Java for adjusting the number of ACA sequences, which MazF dimer recognizes and cleaves in mRNAs.
2. Story simulation
2-1. Mathematical model
In order to simulate our gene circuits, we developed an ordinary differential equation model.
2-2. Results
We obtained and confirmed the desirable behavior of the whole system by modifying and improving parts. As described below, our simulation showed an appropriate transition of concentration of RFP and GFP for the story.
In the blue area of Fig.5-2-2, the concentration of fluorescence proteins starts to increase. The concentration of RFP of Snow White coliexceeds the concentration of GFP of the Queen coli.
It is as if Snow White got fairer more and more.
In the pink area of Fig.5-2-2, C12 is being synthesized and increased thanks to the appearance of C4. As a result, the MazF inside Snow White coli and the Queen coli, suppressing the increment of fluorescent proteins.
It is as if the Queen, influenced by the Mirror's answer, transforming into a Witch in order to give Snow White a poisoned apple.
In the green area of Fig.5-2-2, C12 increases and the MazF inside Snow White coli induced by it increases even more. So the concentration GFP exceeds that of RFP.
It looks as if Snow White bit the apple, sinking into unconsciousness promptly.
In the yellow area of Fig.5-2-2, the AmiE synthesized by the introduced the Prince coli decomposes C12 so the MazF inside Snow White coli diminishes and C4 increases.
It looks as if the Prince lifted Snow White and she opened her eyes.
3. Fitting
3-1. Population growth
First, we tried to model the growth curve of the system. When the number of E. coli approaches a certain value, the growth will stop. We defined this value in the culture as Pmax. Then the population growth equation for our system is described as follows:
$$ \frac{dP}{dt} = g\left(1 - \frac{P}{P_{max}}\right)P$$
where g is the population growth rate.
This equation can be analytically solved as:
$$ P = \frac{P_{0} P_{max} e^{gt}}{P_{max} - P_{0} + P_{0} e^{gt}}$$
where P 0 is the population at t = 0. We used this equation to fit the experimental data.
Using the experimental data from the Toxin assay for this fitting, we estimated the following parameters:
g = 0.0123
and
Pmax =3.3
respectively.
These parameters can be used for Snow White coli, the Queen coli and the Prince coli in the same way.
3-2. Toxin-Antitoxin system
3-3. Promoters
3-4. More realistic model with mRNA
4. Analysis
4-1. The Prince coli should be put in during the process
We run simulations in order to determine whether we would get a better behavior let we introduce the Prince coli at the beginning or halfway of the story.
As a result, if we introduce the Prince coli from the beginning, the number of Prince coli increases too much (Fig.5-4-1-1) so the AmiE the Prince coli produces augments and the decomposition of C12 also occurs overly. So C12 is almost inexistent in the medium (Fig.5-4-1-2).
On the other hand, if we introduce the Prince coli at t = 600, the number of Prince coli does not increment much (Fig.5-4-1-3), so C12 can exist until t = 700 and then decreases thanks to the augment of AmiE (Fig.5-4-1-4).
In conclusion, if we introduce the Prince coli at t = 700, the circuit will behave accordingly.
4-2. Prhl should be changed
In order to confirm the feasibility of the story with our gene circuit by the combination of the existing promoters, we performed some simulations based on the results of our assays.
The diagram above shows that the intensity of the two promoters should be in the red region of the figure.The combination of promoters which we were originally going to use is shown in the graph by the green point. To move this point into the red region, we had to improve Prhl to raise its expression level.
4-3. Requirements
4-4. Production rate of C4HSL and 3OC12HSL by RhlI and LasI
4-5. Translation rate of protein
4-6. Decomposition rate of C12 by AmiE
4-7. Degradation rate of AmiE
4-8. Degradation rate of RFP and GFP
5. Software
5-1. Abstract
We developed a new software named ACADwarfs. This software helps to control the sensitivity of the protein to MazF by regulating the number of ACA sequences in the mRNA sequence. ACADwarfs can increase or decrease the number of ACA sequences on mRNA without changing the amino acid sequences that the mRNA specifies or frameshifts resulted from insertion of bases without considering.
Then we improve the practicality of the characteristic of the mazEF system. For example you can let protein A express constantly by eliminating ACA sequences of the sequence, while letting protein B stop being expressed, at the desirable timing, by expression of MazF.
This software also evades the use of rare codons, so you don’t have to worry about them.
5-2. Key achievements
・Provided the tool regulating the number of ACA sequences
・Released under open-source license so everyone can use it
・Able to correspond to any base arrangements
・Rare codons are evaded
・Extend the application field of mazEF system
5-3. Work flow
5-4. Demonstration
We created a demo to present the features of this software. Using this, we regulated the number of ACA sequences and control the sensitivity of the protein to MazF.
Gene | Pre number of ACA sequences | Post number of ACA sequences |
RFP | 10 | 30 |
GFP | 23 | 39 |
MazF | 2 | 1 |
MazE | 2 | 1 |
We increased the numbers of ACA sequences of RFP and GFP decreased the numbers of ACA sequences of MazF and MazE .
We can see that the concentration of expressed MazF reacts more keenly after adjusting the ACA sequences than before doing so.