Team:Peking R/Project/Application/BS

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   <p class="notbookmaintitle" align=center>Fine-tuning Logic Gate Using Soft-coding of Genetic Program<a name="start" id="start"></a></p>
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   <p class="notbookmaintitle" align=center>The Bistable Switch Module <a name="start" id="start"></a></p>
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<p>&nbsp;</p>
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  <p class="mn"><a href="https://2011.igem.org/Team:Peking_R/Project/Application/AG">AND gate</a></p>
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  <p ><strong>Bistable switch</strong></p>
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  <table width="430" height="111" border="0" cellpadding="0" cellspacing="0">
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  <p><strong><a href="https://2011.igem.org/Team:Peking_R/Project/Application/VIO">Violacein synthetic pathway</a></strong><a href="https://2011.igem.org/Team:Peking_R/Project/Application/VIO"></a> </p>
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  <hr />
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      <th colspan="2" align="left" scope="col"><a href="https://2011.igem.org/Team:Peking_R/Project/Application" class="mainbody">Application</a></th>
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   <p class="MAINBODY">&nbsp;</p>
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  <p class="MAINBODY">To further demonstrate the power of genetic  softcoding, we applied our previously described methodology to a more complex,  nonlinear and milestone genetic device – the bistable switch. Usually, modulating such a device requires overwhelming amounts of workload using conventional screening approaches. When modulating with genetic softcoding methodology as depicted below, however, the behavior of bistable will be flexibly and quantitatively tuned and predicted. </p>
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<p align="center">   <img src="http://www.chem.pku.edu.cn/chenpeng/igem/images/clip_image002.png" alt="" width="554" height="221" /></p>
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      <td width="57">&nbsp;</td>
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<p align="center" class="MARKS">Figure 1 Detailed scheme of the bistable switch.<br />
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      <td width="373"><a href="https://2011.igem.org/Team:Peking_R/Project/Application/AG" class="project">AND gate</a></td>
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The straight arrows and the circles represent genes and their corresponding RBSs respectively. Curved arrows represent the transcription strength and the direction of the promoters. The PRM promoter is activated by its own  downstream gene product, CI, while repressed by CI434 whose expression is controlled by the PR promoter. The PR promoter is repressed by CI, thus forming a double-negative feedback necessary for the bistable switch property.</p>
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<p align="center" class="MARKS">&nbsp;</p>
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<p align="center" class="MAINBODY">The bistable switch, which was inherited from the iGEM 2007 Peking Team, mainly consistsofa positive feedback loop and a double-negative feedback loop. The expression of two mutually repressing repressors genes cI434</em> and <em>cI</em></a>are controlled by the promoters PR and PRM respectively.(Figure1)Promoter RM can be activated by CI and repressed by CI434. GFP and mRFP are placed downstream <em>cI434</em> and <em>cI</em> as reporters of two states, respectively. In the state when CI is dominant, it can activate its own gene&rsquo;s transcription and repress that of <em>cI434</em>, thus developing and stabilizinga stable high CI/low CI434  state, in which a red fluorescent protein (mRFP)gene co-transcriptedwith CI is expressed. Alternatively, when CI434 is dominant, a stable high CI434/low CI state will be established and GFP co-transcripted with CI434 is expressed to represent thethisstate. Each cell that bears the bistable switch is expected to express GFP or mRFP exclusively. The two states are believed to be stabilized over a long period while under certain circumstances one state may be turned over to the other.</p>
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      <td>&nbsp;</td>
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<p align="center" class="MAINBODY">&nbsp;</p>
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      <td><a href="https://2011.igem.org/Team:Peking_R/Project/Application/BS">Bistable switch</a></td>
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<p align="center" class="MAINBODY">When the bistable switch on pSB1C3 plasmid is transformed into DH5α strain, green colonies and red colonies could be observed. Interestingly, several mixed colonies could also be observed, which implied the random steady-state characteristic of the  bistable switch (Figure 2).A ratiometric of the green colonies to the red colonies(G/R ratio) was calculated on the LB agar plate. We  proposed that the G/R ratio is relevant to the translation strength of CI &ampCI434 genes, meaning that modulating the translation strength of one or more  could result in different ratios of G/R under current architecture of bistable  switch. </p><p align="center" class="MARKS">
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    <img src="http://www.chem.pku.edu.cn/chenpeng/igem/images/clip_image004.jpg" alt="" width="554" height="234" /> <br />
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  Figure 2 Images of colonies and individual cells bearing the genetic bistable switch.<br />
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      <td>&nbsp;</td>
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  (A) A red colony and a mixed colony captured by fluorescence  stereomicroscope</a>. (B) Individual cell images in the mixed colony captured by laser confocal microscope. Each rod represents a single cell, expressing GFP or mRFP exclusively</p>
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      <td><a href="https://2011.igem.org/Team:Peking_R/Project/Application/VIO">Violacein synthetic pathway</a></td>
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<p align="center" class="MARKS">&nbsp;</p>
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  <p align="left" class="MAINBODY"><span class="notbookmaintitle"> Model of the Bistable Switch</span><br />
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   </p>
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  <p align="left" class="MAINBODY">We first demonstrate through mathematical modelling that the genetic device we&rsquo;we constructed is indeed able to display properties characteristic of a bistable switch  within a particular parameter range. Since we are focusing on the translation level, the only variable will be the translation strength of the gene-of-interest(In our case, CI434, with reasons stated below). The original contruct did not display a bistable property because the promoter and the strength of the CI434 gene is too strong compared to that of CI, rendering the system monostable in the high CI434/low CI state. To endow the system with  bistability, the strength of CI434 production can be down-regulated by reducing translation strength. To quantitatively describe the system, we employed a set of ordinary differential equations(ODEs) to represent the transcription and translation control of the system(See Appendix)1. Taking into consideration the stochastic nature of the system2, we used a stochastic algorithm to produce the probability distribution of the system in every possible state(Figure 3). If the system is a monostable one(e.g., high  CI434/low CI), its states will be tightly distributed around a single peak value. As the translation strength of CI434 gradually decreases, the peak falls and another peak indicating the high CI/low CI434 state starts to grow, until  the first peak disappears and high CI/low CI434 becomes the predominant state,  bringing the system back to a monostable one. This can also be represented as the proportion of the &ldquo;green&rdquo;(high CI434/low CI) state versus translation  strength of the <em>cI434</em> gene(Figure 4). </p>
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    <img width="553" height="367" src="http://www.chem.pku.edu.cn/chenpeng/igem/images/clip_image006_0001.jpg" alt="说明: C:\Users\Leciel\Desktop\result.png" /> <br />
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<p>&nbsp;</p>
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  Figure 3 <br />
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<p>&nbsp;</p>
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  Changes in distribution of the number of CI434 molecules in response to changes in  translation strength(reflected by βSdcro, a parameter in the ODE model that describes translation rate of <em>cI434</em> gene. For more details, see Appendix). <br />
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<hr />
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  The surface plot was  generated using a stochastic algorithm that simulates the behaviour of 1000 cells. z-axis(height of the surface) correspond to the proportion of cells that express a certain number of CI434 molecules. It can be seen that when translation rate is low, the system&rsquo;s state is tightly distributed around a low-CI434 state, i.e., the system is monostabe. As translation strength grows higher, another distribution peak starts to appear, indicating a high-CI434 state.  The system thus enters the bistable region. When translation rate is too high(βSdcro above 0.6), the system returns to a monostable state again, with only the high-CI434 distribution peak.</p>
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<p>Screening for well performing devices  usually requires laborious, time-consuming refinement cycles, especially in the  case of information processing devices. Utilizing the platform introduced previously,  we aim at making tuning devices fast, affordable and more predictable. To demonstrate the versatility and validity of the platform, it was firstly  applied to modulating a genetic AND gate. We chose the AND gate as a proof of  concept primarily for two reasons:<br />
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  <p align="center" class="MARKS">&nbsp;</p>
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  (1) It presents biologically significant  functions in information processing, e.g., integration of environmental  information to generate appropriate responses in microorganisms.<br />
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   <p class="MARKS"><img width="554" height="391" src="http://www.chem.pku.edu.cn/chenpeng/igem/images/clip_image008_0000.jpg" alt="说明: C:\Users\Leciel\Desktop\model-mutation.png" /> <br />
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  (2) Engineering and screening a synthetic  AND gate module involves laborious characterization when using conventional  methods, which would best contrast with the advantages of our platform&rsquo;s  methodology.</p>
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    Figure 4 Proportion of cells in the high CI434/low CI(green) state derived from data in Figure 3 and experimental results.<br />
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<p>The AND gate we utilized was designed by Anderson  and his colleagues and consequently standardly redesigned by PKU_Beijing 09  team (BBa_K228258, Fig. 1A).</p>
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   The black data points were derived by counting the cells in the arbitrarily defined &ldquo;green&rdquo; state(cells with more than 300 CI434 molecules) under each translation rate. It can be clearly seen that as translation strength(Arbitrary △G values determined from ODE parameters and normalized to computationally determined values from the mutation library) increases, the system travels from a low CI434, monostable state to a transitional, bistable state and then to a high CI434, monostable state. The simulation data is normalized and fitted to experimental results of hardcoding(site-directed mutagenesis), shown in red data points(with error bar). The two sets of data showed fair fitness with each other, validating our previous assertion that translation strength regulates the device&rsquo;s behavior.</p>
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<p align="center" class="picturemark"><img src="http://www.chem.pku.edu.cn/chenpeng/igem/images/project Application final_clip_image002.jpg" alt="" width="553" height="188" /><br />
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  <p class="MARKS">&nbsp;</p>
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  <strong>Figure 1</strong><br />
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   <p class="MAINBODY">Experimentally modulating the device using conventional procedures (hardcoding) involves laborious work as derivation of parameters(e.g., translation strength) in the differential equations require complex experimental measurement and calculation, and large amounts of mutagenesis to produce sequences with desired translation strength may be needed. Our softcoding methodology saves huge amounts of time and effort by obviating the need for numerous rounds of measurement and selection.</p>
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  A. The standardly  redesigned AND gate of PKU_Beijing 09 team.<br />
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  <p class="MAINBODY">&nbsp;</p>
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  B. The topology and  mechanism of AND gate. Parts showing in box constitute the core processing module.</p>
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  <p class="MAINBODY"> Before manipulating the bistable module, a library mutating the RBS of <em>cI434</em> gene is constructed using site-directed mutagenesis method to verify the conformity of our model with experimental results. Each plasmid of the library is transformed into <em>E. coli</em> DH5α strain separately harboring the bistable switch logic device.(Figure </a>5) </p>
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<p class="mainbody">As shown in Fig. 1B, pBAD promoter serves as input 1. It is activated by arabinose, leading to the expression of SupD, an amber suppressor tRNA. The input 2 is pSal promoter activated by salicylate via  binding to NahR. It regulates the expression of a T7 polymerase coding sequence  with two amber codons reside in the position 8 and 14 (T7ptag), resulting in  premature translational termination. When both T7ptag and SupD tRNA genes are expressed, functional T7 polymerase would be synthesized and consequently active  output, T7 promoter. A green  fluorescent protein (GFP) generator regulated by T7 promoter serves as a reporter.</p>
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  <p align="center" class="picturemark"><img src="http://www.chem.pku.edu.cn/chenpeng/igem/images/clip_image010.jpg" alt="" width="554" height="604" /> <br />
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<p class="mainbody">It has been demonstrated that translation strength of T7ptag is a major determinant of AND gate quality. Mutagenesis of  RBS leads to various performance, thus we modeled the AND gate using transfer  function, as further illustrated by phase diagrams. The phase diagram displays  the system&rsquo;s output properties in response to all possible input combinations (Fig  2). In the case of AND gate, two inputs and one output are involved. Inputs are  the expression strength of pSal and pBAD induced by different concentration of the two inducers, salicylate and arabinose, respectively, and the output is the  fluorescence intensity of reporter GFP. To construct such a phase diagram, the  input promoter strengths are measured by GFP fluorescence in response to  varying inducer concentrations. We also normalized output fluorescence intensity  values to the maximum possible fluorescence determined by model parameters. Assuming that the output is measured at the system&rsquo;s steady state, we derived the output function using ordinary differential equations (ODEs):</p>
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    Figure 5  &nbsp;Construction of bistable switch library via site-directed mutagenesis.  Binding sites for forward and reverse primers are schematized.</p>
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<p align="center"><img src=" http://www.chem.pku.edu.cn/chenpeng/igem/images/project Application final_clip_image004.png" alt="" width="150" height="46" /></p>
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  <p align="center" class="picturemark">&nbsp;</p>
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<p class="mainbody">Where <em>F</em> is an arbitrary, unitless measure for output fluorescence and <em>F</em>max is the highest possible  level of output determined by parameters in ODEs describing the process of gene  expression and regulation. <em>I</em>1 and <em>I</em>2 are the inputs in units of fluorescence (au). <em>a</em> is a  parameter reciprocally proportional to the translation strength of the <em>T7ptag</em> coding region, and <em>b </em>merely results from a scaling factor  to unify units of measurement.<br />
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  <p class="MAINBODY">After growing on agar plates, G/R ratio is calculated for each of the sequences in the library, several images of which are captured by the fluorescence stereomicroscope. (Figure 6) The ability of translation strength to regulate the switch&rsquo;s behaviour is thus verified.</p>
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   (The detailed construction of each ODE  describing transcription and translation processes and integrating input values  into the output function can be found in Appendices.)</p>
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  <p class="MARKS"><br />
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<p class="mainbody">The phase diagrams were obtained by plotting  the output function as a color map over the 2-dimensional space with axes corresponding to the two inputs, <em>I</em>1  and <em>I</em>2. The variables&rsquo; space is extended to cover a sufficiently large range of inputs to represent a general AND gate module (Fig. 2(a)). In reality, the two inputs only vary within a limited range that is a sub-region of the <em>I</em>1-<em>I</em>2 space. For any particular AND gate module, variations in the translation strength of the <em>T7ptag</em> gene can be  reflected in changes in the range of the input <em>I</em>2, resulting in shifting of rectangular region in the  phase diagram that corresponds to the range of inputs. </p>
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    <img width="554" height="415" src="http://www.chem.pku.edu.cn/chenpeng/igem/images/clip_image012.png" alt="说明: C:\Users\Leciel\Desktop\Figure 6.png" /> <br />
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<p class="mainbody">The module in which translation strength of <em>T7ptag</em> gene is strong would be a poor AND gate because within its range of inputs, the &ldquo;ON&rdquo; state (high output) can be induced by addition of arabinose (<em>I</em>2)  alone even when <em>I</em>1 is low. This is probably due to leakage of the Psal promoter, i.e., the promoter has a  relatively high basal activation level.</p>
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   Figure 6 Experimental results of varying translation rate by altering the RBS sequence upstream of <em>cI434</em> gene.
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<p class="mainbody">The translational strength of T7ptag is dominantly regulated by RBS strength when the promoter strength is the same. Several AND gates with different RBSs, i.e., different T7ptag translation strengths in this condition, are characterized, of which experimental data fit the model prediction well.</p>
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  Images were acquired by applying excitation light with wavelengths of 470nm(for eGFP) and 580nm(for mRFP) to the agar plate respectively and merging two emission images  together. (A)Synthetic RBS with △G of about -3.029kJ/mol. Calculated proportion of &ldquo;green&rdquo; colonies is 0.95. (B)Synthetic RBS with△G of about -2.08kJ/mol. Calculated proportion of &ldquo;green&rdquo; state is 0.35. (C)Synthetic RBS with △G of  about 0.79kJ/mol. Calculated proportion of &ldquo;green&rdquo; state is 0.21. Apparently, translation strength indeed has a significant role in regulating the device&rsquo;s behavior.</p>
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  <p class="MARKS">&nbsp;</p>
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   <img src="http://www.chem.pku.edu.cn/chenpeng/igem/images/project Application final_clip_image009.gif" alt="" width="525" height="377" /><br />
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  <p class="MAINBODY">Avoiding laborious screening and assays, a down-regulating TPP ligand responsive hammerhead ribozyme TPP 2.5 is applied to the bistable switch modifying the translation rate of <em>cI434</em> gene to regulate the G/R ratio and a corresponding genetic device is constructed. (Figure 7) <br />
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  <strong>Figure 2</strong><br />
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  <img src="https://static.igem.org/mediawiki/2011/4/4a/PekingR_biostable_figure7.png" width="554" height="88" hspace="60" align="center" /></p>
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   (a)The output properties in response to all possible input combinations. AND gate performance  is influenced by translation strength of T7ptag. Color bar on the right  indicates the output strength corresponding to each color. Rectangular regions  represent the largest possible range of the two inputs in experimental conditions (right to left): AND gate with progressively lower translation rates  (more positive △G) of <em>T7ptag</em> gene (white, yellow, green and pink)<a name="_GoBack" id="_GoBack"></a>.<br />
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  <p>&nbsp;</p>
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   (b)Experimental result of the AND gate behaviour in response to changes in translation rate.  Output is plotted as a function of the two inducer concentrations, [arabinose]  and [salicylate]. Its values have been normalized to the maximal fluorescence  measured, facilitating comparison with the theoretical phase diagrams. (Left)An AND gate module with an RBS sequence which has a high translation rate(△G=-7.07kJ/mol). (Right)AND gate module with a weaker RBS(decreased translation rate, △G=-0.49kJ/mol). It can be seen that changing  translation rate result in different AND gate performance.</p>
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  <p align="center" class="MARKS">Figure 7 Construction of the bistable switch device carrying the RNA controller(TPP ribozyme, shown as the tuning switch named TPP2.5 in the  figure). The rest of the device is the same as that shown in Figure 5.</p>
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<p class="mainbody">In order to optimize the performance of AND  gate, the first step is to determine the optimal translation strength of the <em>T7ptag</em> gene using our RNA controller  toolkit. By placing a ligand-responsive RNA controller element upstream of the coding sequence, we obtained an AND gate modulator whose <em>T7ptag</em> gene translation rate varies in response to ligand  concentration (Fig. 3A). By optimizing the strength of translation, we are able  to make up for the leakage in transcription and a translation rate that endows the AND gate with satisfactory performance (Fig 3B). </p>
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  <p align="center" class="MARKS">&nbsp;</p>
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<p align="center"><img src="http://www.chem.pku.edu.cn/chenpeng/igem/images/project Application final_clip_image013.gif" alt="" width="577" height="531" />&nbsp;</p>
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  <p class="MAINBODY">Since the bistable  module&rsquo;s behaviour can only be quantified using agar plate culture, it is  difficult to apply a precise concentration gradient of TPP to the host <em>E.coli</em>. Therefore we set two experiment groups: one without addition of TPP and another with TPP sufficient for full induction of the genetic rheostate &rsquo;s funtions(self-cleavage of ribozyme). The experimental results are shown in Figure 8. It can be seen that the group with  excess TPP(down-regulated translation strength of <em>cI434</em> gene) displayed bistability. Therefore, the RNA controller(TPP ribozyme) is indeed capable of regulating the device&rsquo;s behavior.<br />
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<p align="center" class="picturemark"><strong>Figure 3 Optimization of AND  gate performance using RNA controller(TPP ribozyme).</strong><br />
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  <img width="584" height="490" src="http://www.chem.pku.edu.cn/chenpeng/igem/images/clip_image016.png" alt="说明: C:\Users\Leciel\Desktop\Figure 8.png" /></p>
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   (a) Output fluorescence of the AND gate device without addition of TPP ligand(corresponding  to a △G of -5.78kJ/mol). (b)Output fluorescence of the AND gate device with addition of maximal concentration of TPP ligand(1μM,corresponding to a △G of -3.38kJ/mol). Vertical and  horizontal axes indicate logarithm of the concentrations of arabinose and  salicylate respectively. Apparently, addition of TPP ligand(which attenuates  translation strength) improved the AND gate performance by decreasing the area of region for &ldquo;ON&rdquo; state. The two output color plots are mapped to their  corresponding positions in the full phase diagram in Figure 2, showing that  they display fair agreement with modeling results(white and yellow rectangular  respectively).</p>
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   <p align="center" class="MARKS">Figure  8 Fluorescence stereomicroscopic images of <em>E.coli</em> colonies with and without TPP treatment.</strong><br />
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<p class="mainbody">The translation rates are expressed in  terms of the parameter <em>a</em>, whose values can be determined using the <em>a</em> value corresponding to the original sequence without the RNA controller (<em>a</em> can be converted to a more direct indicator of translation strength - △G using a quantitative relationship derived in the Appendix). A dose(ligand  concentration) response curve used for finding the <em>a</em> value corresponding to a given TPP concentration is given in Figure 4.</p>
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   (A) <em>E.coli</em> colonies without TPP treatment(no decrease in translation rate) are all green(high CI434/low CI state), displaying monostability of the genetic device. (B)<em>E.coli</em> colonies with TPP treatment(no decrease in translation rate) are a mixture of green(high CI434/low CI state) and red(low CI434/high CI  state) colonies, displaying bistability of the genetic device. (C)Experimental results are mapped to the simulated &ldquo;green&rdquo; proportion–△G curve in Figure 4.</p>
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<p align="center" class="picturemark"><img src="http://www.chem.pku.edu.cn/chenpeng/igem/images/project Application final_clip_image015.jpg" alt="" width="315" height="219" /> <br />
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  <p align="center" class="MAINBODY">&nbsp;</p>
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   <strong>Figure 4 Correlation of parameter a with ligand (TPP) concentration.</strong> <br />
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  <p align="center" class="MAINBODY"><br />
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   It is shown that <em>a</em> increases(i.e., translation rate decreases) as TPP concentration increases, in agreement with the function  of TPP ribozyme(inhibiting translation via ligand-responsive cleavage). Notably, the dose response curve displayed saturation at TPP concentrations above 0.3μM.</p>
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    The final step then, is fixation of the RBS sequence upstream of <em>cI434</em> gene with the desired translation rate. Using the forward engineering curve(see the RBS Calculator section for more details), we are able to pick the right RBS sequence from the library and integrate it to the device to endow it with satisfactory bistability.</p>
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<p class="mainbody">The final step is to replace the RNA  controller together with the RBS sequence downstream of the controller with an  automatically designed RBS sequence that meets the translation strength configuration  determined by our RBS calculator, thus to &lsquo;fix&rsquo; the strength in genetic program,  producing desired performance.</p>
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  <p align="center" class="MAINBODY">&nbsp;</p>
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<p class="mainbody">As illustrated above, minor differences in  RBS strength may largely influence the performance of genetic program,  consistent with the fact that tuning genetic circuits requires laborious and refinement cycles, especially in the case of complex systems. However, when  applying our platform to the modulation of the AND gate, the whole process does  not require construction of mutation library while still allowing for high-throughput  screening for an optimal translation strength. Additionally, our platform  enables its user to quantitatively analyze the correlation between system  behavior and translation strength of core genetic component, thus to predictably  manipulate the performance of genetic devices. In brief, soft-coding of genetic  program makes synthetic biology fast, affordable and more  predictable.</p>
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  <p align="center" class="MAINBODY"><a href="https://static.igem.org/mediawiki/2011/9/9e/PekingR_Appendices_for_Bistable.pdf">Appendix</a></p>
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<p class="mainbody">(To validate the reliability of parameter<em> a</em> as the single variable used in the model, we plotted experimental  measurements of the AND gate output under each input combination against  varying <em>a </em>values (reflecting ligand concentration), and theoretical  curves were fitted to the experimental results to test the robustness of  parameters under different input combinations. For more detailed description of  this part, see section 3 in the Appendix.)</p>
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<p>Anderson, J. C. et al. (2007) Environmental signal integration by a modular AND gate. Nature Molecular Systems Biology 3; Article number 133; doi:10.1038/msb4100173</p>
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<p class="MAINBODY"> 1. Lou, C., Liu, X., Ni, M., et al. (2009). Synthesizing a novel genetic sequential logic circuit: a push-on push-off switch. Nature Molecular Systems Biology 6, 350.<br />
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2. Tian, T., and Burrage, K. (2006). Stochastic models for regulatory networks of the genetic toggle switch. PNAS 103, 8372-8377.<br />
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Latest revision as of 17:08, 28 October 2011

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The Bistable Switch Module


AND gate

Bistable switch

Violacein synthetic pathway


 

To further demonstrate the power of genetic softcoding, we applied our previously described methodology to a more complex, nonlinear and milestone genetic device – the bistable switch. Usually, modulating such a device requires overwhelming amounts of workload using conventional screening approaches. When modulating with genetic softcoding methodology as depicted below, however, the behavior of bistable will be flexibly and quantitatively tuned and predicted.

Figure 1 Detailed scheme of the bistable switch.
The straight arrows and the circles represent genes and their corresponding RBSs respectively. Curved arrows represent the transcription strength and the direction of the promoters. The PRM promoter is activated by its own downstream gene product, CI, while repressed by CI434 whose expression is controlled by the PR promoter. The PR promoter is repressed by CI, thus forming a double-negative feedback necessary for the bistable switch property.

 

The bistable switch, which was inherited from the iGEM 2007 Peking Team, mainly consistsofa positive feedback loop and a double-negative feedback loop. The expression of two mutually repressing repressors genes cI434 and cIare controlled by the promoters PR and PRM respectively.(Figure1)Promoter RM can be activated by CI and repressed by CI434. GFP and mRFP are placed downstream cI434 and cI as reporters of two states, respectively. In the state when CI is dominant, it can activate its own gene’s transcription and repress that of cI434, thus developing and stabilizinga stable high CI/low CI434 state, in which a red fluorescent protein (mRFP)gene co-transcriptedwith CI is expressed. Alternatively, when CI434 is dominant, a stable high CI434/low CI state will be established and GFP co-transcripted with CI434 is expressed to represent thethisstate. Each cell that bears the bistable switch is expected to express GFP or mRFP exclusively. The two states are believed to be stabilized over a long period while under certain circumstances one state may be turned over to the other.

 

When the bistable switch on pSB1C3 plasmid is transformed into DH5α strain, green colonies and red colonies could be observed. Interestingly, several mixed colonies could also be observed, which implied the random steady-state characteristic of the bistable switch (Figure 2).A ratiometric of the green colonies to the red colonies(G/R ratio) was calculated on the LB agar plate. We proposed that the G/R ratio is relevant to the translation strength of CI & CI434 genes, meaning that modulating the translation strength of one or more could result in different ratios of G/R under current architecture of bistable switch.


Figure 2 Images of colonies and individual cells bearing the genetic bistable switch.
(A) A red colony and a mixed colony captured by fluorescence stereomicroscope. (B) Individual cell images in the mixed colony captured by laser confocal microscope. Each rod represents a single cell, expressing GFP or mRFP exclusively

 

Model of the Bistable Switch

We first demonstrate through mathematical modelling that the genetic device we’we constructed is indeed able to display properties characteristic of a bistable switch within a particular parameter range. Since we are focusing on the translation level, the only variable will be the translation strength of the gene-of-interest(In our case, CI434, with reasons stated below). The original contruct did not display a bistable property because the promoter and the strength of the CI434 gene is too strong compared to that of CI, rendering the system monostable in the high CI434/low CI state. To endow the system with bistability, the strength of CI434 production can be down-regulated by reducing translation strength. To quantitatively describe the system, we employed a set of ordinary differential equations(ODEs) to represent the transcription and translation control of the system(See Appendix)1. Taking into consideration the stochastic nature of the system2, we used a stochastic algorithm to produce the probability distribution of the system in every possible state(Figure 3). If the system is a monostable one(e.g., high CI434/low CI), its states will be tightly distributed around a single peak value. As the translation strength of CI434 gradually decreases, the peak falls and another peak indicating the high CI/low CI434 state starts to grow, until the first peak disappears and high CI/low CI434 becomes the predominant state, bringing the system back to a monostable one. This can also be represented as the proportion of the “green”(high CI434/low CI) state versus translation strength of the cI434 gene(Figure 4).

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Figure 3
Changes in distribution of the number of CI434 molecules in response to changes in translation strength(reflected by βSdcro, a parameter in the ODE model that describes translation rate of cI434 gene. For more details, see Appendix).
The surface plot was generated using a stochastic algorithm that simulates the behaviour of 1000 cells. z-axis(height of the surface) correspond to the proportion of cells that express a certain number of CI434 molecules. It can be seen that when translation rate is low, the system’s state is tightly distributed around a low-CI434 state, i.e., the system is monostabe. As translation strength grows higher, another distribution peak starts to appear, indicating a high-CI434 state. The system thus enters the bistable region. When translation rate is too high(βSdcro above 0.6), the system returns to a monostable state again, with only the high-CI434 distribution peak.

 

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Figure 4 Proportion of cells in the high CI434/low CI(green) state derived from data in Figure 3 and experimental results.
The black data points were derived by counting the cells in the arbitrarily defined “green” state(cells with more than 300 CI434 molecules) under each translation rate. It can be clearly seen that as translation strength(Arbitrary △G values determined from ODE parameters and normalized to computationally determined values from the mutation library) increases, the system travels from a low CI434, monostable state to a transitional, bistable state and then to a high CI434, monostable state. The simulation data is normalized and fitted to experimental results of hardcoding(site-directed mutagenesis), shown in red data points(with error bar). The two sets of data showed fair fitness with each other, validating our previous assertion that translation strength regulates the device’s behavior.

 

Experimentally modulating the device using conventional procedures (hardcoding) involves laborious work as derivation of parameters(e.g., translation strength) in the differential equations require complex experimental measurement and calculation, and large amounts of mutagenesis to produce sequences with desired translation strength may be needed. Our softcoding methodology saves huge amounts of time and effort by obviating the need for numerous rounds of measurement and selection.

 

Before manipulating the bistable module, a library mutating the RBS of cI434 gene is constructed using site-directed mutagenesis method to verify the conformity of our model with experimental results. Each plasmid of the library is transformed into E. coli DH5α strain separately harboring the bistable switch logic device.(Figure 5)


Figure 5  Construction of bistable switch library via site-directed mutagenesis. Binding sites for forward and reverse primers are schematized.

 

After growing on agar plates, G/R ratio is calculated for each of the sequences in the library, several images of which are captured by the fluorescence stereomicroscope. (Figure 6) The ability of translation strength to regulate the switch’s behaviour is thus verified.


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Figure 6 Experimental results of varying translation rate by altering the RBS sequence upstream of cI434 gene. Images were acquired by applying excitation light with wavelengths of 470nm(for eGFP) and 580nm(for mRFP) to the agar plate respectively and merging two emission images together. (A)Synthetic RBS with △G of about -3.029kJ/mol. Calculated proportion of “green” colonies is 0.95. (B)Synthetic RBS with△G of about -2.08kJ/mol. Calculated proportion of “green” state is 0.35. (C)Synthetic RBS with △G of about 0.79kJ/mol. Calculated proportion of “green” state is 0.21. Apparently, translation strength indeed has a significant role in regulating the device’s behavior.

 

Avoiding laborious screening and assays, a down-regulating TPP ligand responsive hammerhead ribozyme TPP 2.5 is applied to the bistable switch modifying the translation rate of cI434 gene to regulate the G/R ratio and a corresponding genetic device is constructed. (Figure 7)

 

Figure 7 Construction of the bistable switch device carrying the RNA controller(TPP ribozyme, shown as the tuning switch named TPP2.5 in the figure). The rest of the device is the same as that shown in Figure 5.

 

Since the bistable module’s behaviour can only be quantified using agar plate culture, it is difficult to apply a precise concentration gradient of TPP to the host E.coli. Therefore we set two experiment groups: one without addition of TPP and another with TPP sufficient for full induction of the genetic rheostate ’s funtions(self-cleavage of ribozyme). The experimental results are shown in Figure 8. It can be seen that the group with excess TPP(down-regulated translation strength of cI434 gene) displayed bistability. Therefore, the RNA controller(TPP ribozyme) is indeed capable of regulating the device’s behavior.
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Figure 8 Fluorescence stereomicroscopic images of E.coli colonies with and without TPP treatment.
(A) E.coli colonies without TPP treatment(no decrease in translation rate) are all green(high CI434/low CI state), displaying monostability of the genetic device. (B)E.coli colonies with TPP treatment(no decrease in translation rate) are a mixture of green(high CI434/low CI state) and red(low CI434/high CI state) colonies, displaying bistability of the genetic device. (C)Experimental results are mapped to the simulated “green” proportion–△G curve in Figure 4.

 


The final step then, is fixation of the RBS sequence upstream of cI434 gene with the desired translation rate. Using the forward engineering curve(see the RBS Calculator section for more details), we are able to pick the right RBS sequence from the library and integrate it to the device to endow it with satisfactory bistability.

 

Appendix

 


Reference:

1. Lou, C., Liu, X., Ni, M., et al. (2009). Synthesizing a novel genetic sequential logic circuit: a push-on push-off switch. Nature Molecular Systems Biology 6, 350.
2. Tian, T., and Burrage, K. (2006). Stochastic models for regulatory networks of the genetic toggle switch. PNAS 103, 8372-8377.