Team:Ehime-Japan/Project

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<p>Light sensor genes</p></font size><p>
<p>Light sensor genes</p></font size><p>
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We utilized the light sensor mechanism in our project. In this page, we explain the mechanism of the original green, red, and green+red light sensor.</p>
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<p><font size="3"><font color=green>
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<p><font size="3"><font color=green>・Green light sensor :pJT118, pPLPCB(S)
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・Green light sensor :pJT118, pPLPCB(S) [1]
 <p>Ho1 and PcyA synthesize 3z-phycocyanobirin (PCB) depending on ferredoxin (Fd).
 <p>Ho1 and PcyA synthesize 3z-phycocyanobirin (PCB) depending on ferredoxin (Fd).
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When PCB binds to Ccas, It catches light and affects the function of CcaS depending on the wavelength of the light. When the light is green,  autophosphorylation of CcaS and phosphate transfer to CcaR increase. When CcaR is phosphorylated, it promotes the transcription from the PcpcG2 promoter. On the other hand, when the receive light is red, it CcaS responds reversely, to cause depression of the PcpcG2 promoter.
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When PCB binds to Ccas, it catches light and affects the function of CcaS depending on the wavelength of the light. When the light is green,  autophosphorylation of CcaS and phosphate transfer to CcaR increase. When CcaR is phosphorylated, it promotes the transcription from the P<sub>cpcG2</sub> promoter. On the other hand, when the received light is red, CcaS responds reversely, to cause depression of the P<sub>cpcG2</sub> promoter.
  In the original system, pPLPCB(S) provide Ho1 and PcyA, and pJT118 provides Ccas and CcaR in addition to the reporter lacZ gene under the control of PcpcG2.We replaced the LacZ gene in pJT118 with the gene coding for a fluorescent protein.</p>
  In the original system, pPLPCB(S) provide Ho1 and PcyA, and pJT118 provides Ccas and CcaR in addition to the reporter lacZ gene under the control of PcpcG2.We replaced the LacZ gene in pJT118 with the gene coding for a fluorescent protein.</p>
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<br><img src="https://static.igem.org/mediawiki/2012/4/4b/Pcb%E5%8E%9F%E7%90%86.png" width=300px>
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<p><font size="3"><font color=red>・Red light sensor :pCph8, pJT106b, pPLPCB(S)<p>
<p><font size="3"><font color=red>・Red light sensor :pCph8, pJT106b, pPLPCB(S)<p>
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Cph8 (a Cph1-EnvZ chimaeras) is expressed from P(LTetO-1) promoter in the phosphorylated ground state.
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Cph8 (a Cph1-EnvZ chimaeras) is expressed from P<sub>LTetO-1</sub> promoter in the phosphorylated ground state.
The Cph1 part of Cph8 is synthesized as the apo from, and holo Cph1 is formed when apo Cph1 ligates PCB.
The Cph1 part of Cph8 is synthesized as the apo from, and holo Cph1 is formed when apo Cph1 ligates PCB.
Holo Cph1 can absorb light. When far red light (705 nm) is absorbed, the rate of phosphotransfer from the EnvZ
Holo Cph1 can absorb light. When far red light (705 nm) is absorbed, the rate of phosphotransfer from the EnvZ
domain of Cph8 to OmpR and the affinity of the phosphorylated OmpR (OmpR-P) to the OmpC promoter is increased.
domain of Cph8 to OmpR and the affinity of the phosphorylated OmpR (OmpR-P) to the OmpC promoter is increased.
This raises transcription of the cI gene downstream an OmpC promoter. The cI repressor represses transcription of
This raises transcription of the cI gene downstream an OmpC promoter. The cI repressor represses transcription of
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a lacZ ORF under the control of the promoter. On the contrary, when red light (650 nm) is absorbed, the rate
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a lacZ ORF under the control of the P<sub>&lamda;</sub> promoter. On the contrary, when red light (650 nm) is absorbed, the rate
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of phosphotransfer of the EnvZ part of Cph8 is decreased and less cI is expressed. As a result, the amount of transcription from promoter is increased.<br><a href="http://www.ncbi.nlm.nih.gov/pmc/articles/PMC3053042/">Multichromatic control of gene expression in Escherichia coli
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of phosphotransfer of the EnvZ part of Cph8 is decreased and less cI is expressed. As a result, the amount of transcription from P<sub>&lamda;</sub> promoter is increased.
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<br><a href="http://www.ncbi.nlm.nih.gov/pmc/articles/PMC3053042/">  
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[1] Tabor, J. J. et al. (2011) Multichromatic control of gene expression in Escherichia coli. J. Mol. Biol., 405, 315-324.
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<br><font color=black>
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[2] Levskaya, A. et al. (2005) Engineering Escherichia coli to see light. Nature, 438, 441-442.
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<br>
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[3] Gambetta, G. A. and Lagarias, J. C. (2001) Genetic engineering of phytochrome biosynthesis in bacteria.
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Proc. Natl. Acad. Sci. USA, 98, 10566-10571
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<br>
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[4] Mattison, K. and Kenney, L.J. (2002) Phosphorylation Alters the Interaction of the Response Regulator OmpR with Its Sensor Kinase EnvZ. J. Biol. Chem., 277
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In most bacteria, ssrA-tagged proteins are degraded by protease. In E.coli, the ssrA t tag has 11-amino acid sequence that is recognized mainly by the ClpXP protease. The tag has been minimized into the three amino acid LVA tag, and this minimum tag is utilized widely in synthetic biology and in iGEM for temporal expression and degradation of stable protein, such as GFP and repressors.
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In most bacteria, ssrA-tagged proteins are degraded by protease. In E. coli, the ssrA tag has 11-amino acid sequence that is recognized mainly by the ClpXP protease. The tag has been minimized into the three amino acid LVA tag, and this minimum tag is utilized widely in synthetic biology and in iGEM for temporal expression and degradation of stable protein, such as GFP and repressors.
Mycoplasamas, however, do not have the ClpXP protease. The ssrA tag sequences are quite different from those of the other bacteria. It was found that the tag is degraded mainly by the Lon protease in Mesoplasma florum, a Mycoplasma species [1].So, we call the tag “Lon-tag”.
Mycoplasamas, however, do not have the ClpXP protease. The ssrA tag sequences are quite different from those of the other bacteria. It was found that the tag is degraded mainly by the Lon protease in Mesoplasma florum, a Mycoplasma species [1].So, we call the tag “Lon-tag”.
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The Lon-tagged proteins of M. florum are efficiently recognized and degraded by the M. florum Lon protease. M. florum Lon does not degrade proteins bearing the E.coli-ssrA tag, and E.coli Lon does not efficiently degrade proteins bearing the M.  florum ssrA tag .  
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The Lon-tagged proteins of M. florum are efficiently recognized and degraded by the M. florum Lon protease. M. florum Lon does not degrade proteins bearing the E. coli-ssrA tag, and E. coli Lon does not efficiently degrade proteins bearing the M.  florum ssrA tag .  
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In principle, Lon-tagged proteins in E.coli cells should be degraded more rapidly upon induction of the M.florum Lon protease.
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In principle, Lon-tagged proteins in E. coli cells should be degraded more rapidly upon induction of the M.florum Lon protease.
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<p>
In order to make a circulatable communication system, we used the green and red light sensor
In order to make a circulatable communication system, we used the green and red light sensor
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plasmids: pJT122, pJT106b, and pPLPCB(S). The E.coli having those plasmids expresses lacZ
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plasmids: pJT122, pJT106b, and pPLPCB(S). The E.coli having these plasmids expresses lacZ
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when the E.coli absorbs the green or red light. First, we constructed the plasmids below.
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when the E. coli absorbs the green or red light. First, we constructed the plasmids below.
<br><br>
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<br>Fig. 1 PcocG2-GFP-mf-ssrA(pJT122)
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<br>Fig. 1 PcpcG2-GFP-mf-ssrA(pJT122)
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<img src="https://static.igem.org/mediawiki/2012/d/d4/%E5%9B%B3PJT122.png" width=500px>
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<img src="https://static.igem.org/mediawiki/2012/d/d4/%E5%9B%B3PJT122.png" width=500px><br>
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Fig. 2 Pλ-mf.Lon-LVA<br>
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Fig. 2 Pλ-mf.Lon-LVA(pJT106b)<br>
<img src="
<img src="
https://static.igem.org/mediawiki/2012/6/6d/%E5%9B%B3PJT106b.png" width=500px>
https://static.igem.org/mediawiki/2012/6/6d/%E5%9B%B3PJT106b.png" width=500px>
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<br></font size><p>
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<p><font size="3">
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<p>
We replaced the lacZ of pJT122 with GFP+ssrA tag (mf. lon) and the lacZ of pJT106b with  
We replaced the lacZ of pJT122 with GFP+ssrA tag (mf. lon) and the lacZ of pJT106b with  
mf.Lon+LVA. As a result, GFP+ssrA tag is synthesized when the E.coli is exposed green light
mf.Lon+LVA. As a result, GFP+ssrA tag is synthesized when the E.coli is exposed green light
and mf.Lon+LVA is expressed by red light. This mechanism is shown next. </p>
and mf.Lon+LVA is expressed by red light. This mechanism is shown next. </p>
<p><font color=green>
<p><font color=green>
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<p align="center">
 
<p>
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1. Expose one of the E.coli (pJT122, pJT106b, and pPLPCB(S)) in two test tubes to green light.
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1. Expose one of the two test tubes with E. coli (pJT122, pJT106b, and pPLPCB(S)) to green light.
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The E.coli exposed to green light expresses GFP+ssrA tag.
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The E. coli exposed to green light expresses GFP+ssrA tag.
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2. GFP emits by UV (364 nm) and the light is transferred to the other test tube through an
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2. GFP emits its green light byactivation with UV (364 nm) and the light is transferred to the other test tube through an
optical fiber.  
optical fiber.  
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</p><br>
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The other E.coli receives the green light and expresses GFP too.
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The other E. coli receives the green light and expresses GFP too.
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<p><font color=red>
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3. Expose the E.coli to red light.
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3. Expose the E. coli to red light.
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4. mf.Lon+LVA tag is degraded by ClpX from E.coli
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4. mf.Lon+LVA tag is degraded by ClpX preexisting in E. coli
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Finally, we can make an E-mail system by getting this system small!!
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Finally, we could construct an E-mail system by making this system smaller !!
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Furthermore, the circulatable system will go well by the two degradation system because those are independent each other. The details are on "Degradation system".
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Furthermore, the circulatable system could work well owing to the two degradation systems which
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are independent each other. The details are on "Degradation system".
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<br>
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<br>
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</p>
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<br>
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<p>
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Because it was difficult to regulate the quantitative control, we did not
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carry out the experiment to check if mf-ssrA tag is recognized by mf-Lon more speedily than
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the Lon and LVA tag from E. coli. 
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</p>
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<br>
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<br>
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<br>
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<font size="5">
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<br>E.co-mail AssayⅠ
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<br></font size="5"></p><br><br><p>
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We made 6 E. coli samples harvoring a combination of 3 plasmids including pPLPCB(S) in common for
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studying "The effect of mf-Lon","The effect of LVA tag ", JW4092 (Lon-deficient)
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The combinations of the plasmids are as follows.
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</p>
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<br>
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1. The effect of mf-Lon <br>
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<p> pJT122 (GFP+mf-ssrA tag), pPLPCB(S)and either.
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</p><br><br>
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(1) pJT106b with the mf-Lon gene replacing the lacZ gene. <br><br>
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(2) pJT106b without lacZ. <br><br>
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2. The effect of mf-ssrA <br><br>
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<p>pJT106b (mf-Lon) and pPLPCB(S), and either.</p> <br>
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<br>(3) pJT122 with the GFP+mf-ssrA tag gene replacing lacZ gene. <br><br>
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(4) pJT122 with the GFP gene (no mf-ssrA tag) replacing the lacZ gene. <br><br>
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3. The effect of LVA tag <br><br>
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<p>pJT122 (GFP+mf-ssrA tag), pPLPCB(S), and either.</p><br><br>
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(5) pJT106b with the mf-Lon+LVA tag gene replacing the lacZ gene or. <br><br>
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(6) pJT106b with the mf-Lon gene (no LVA tag) replacing the lacZ gene.
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<br><br>
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<font size="5">
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<br>E.co-mail ResultⅠ
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<br></font size="5"></p>
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<br><br>
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1. The effect of mf-Lon
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<br> <br>
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(1)
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<img src="https://static.igem.org/mediawiki/2012/3/31/%E2%91%A0%E2%91%A2%E2%91%A5.png" width=500px><br>
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(2)
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<img src="https://static.igem.org/mediawiki/2012/f/f3/%E2%91%A1kanaxa.png" width=500px><br>
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2. The effect of mf-ssrA <br><br>
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(3)<img src="https://static.igem.org/mediawiki/2012/3/31/%E2%91%A0%E2%91%A2%E2%91%A5.png" width=500px><br>
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(4)<img src="https://static.igem.org/mediawiki/2012/9/92/%E2%91%A3dayouna.png" width=500px><br>
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3. The effect of LVA tag<br><br>
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(5)<img src="https://static.igem.org/mediawiki/2012/3/30/%E2%91%A4ahaha.png
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" width=500px><br>
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(6)<img src="https://static.igem.org/mediawiki/2012/3/31/%E2%91%A0%E2%91%A2%E2%91%A5.png" width=500px><br>
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<font size="5">
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<br>E.co-mail DiscussionⅠ
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<br><br></font size="5"></p><br><br>
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<p>We could not tell based on Figures I and II whether the pair of mf-Lon and mf-ssrA tag worked. However, Figure III by itself could be interpreted as a result of degradation by mf-Lon: mf-Lon with the LVA tag should be less stable that without LVA, and the GFP with the mf-ssrA tag should be more slowly degraded by the LVA-tagged mf-Lon. It is possible that the expression of mf-Lon was lower in the cases of (1), (3), and (4).  </p><br>
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<font size="5">
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<br>E.co-mail AssayⅡ
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<br></font size="5"></p><br><br>
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<p>Next, we constructed the simple device to confirm whether GFP is expressed by the green light of GFP through an optical fiber. </p><br><br>
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<img src="
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https://static.igem.org/mediawiki/2012/d/d4/%E3%81%B4%E3%81%8B%E3%81%A1%E3%82%85%E3%81%86.JPG" width=300px><br>
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<br>
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<p>With an optical fiber, one test tube containing GFP protein emitting by UV (364 nm) was connected to the other containing the E.coli and shaded. </p><br>
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<p>Because it was difficult to regulate the quantitative control, we did not carry out the experiment to check if mf-ssrA tag is recognized by mf-Lon more speedy than those from E.coli. </p><br><br><br>
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<font size="5">
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<br>E.co-mail ResultⅡ
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<br></font size="5"></p><br>
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<table border="3">
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<tr>
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<th></th>
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<th>Light intensity
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2</th>
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</tr>
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<tr>
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<td>Dark</td>
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<td>40.201</td>
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</tr>
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<tr>
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<td>Green light</td>
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<td>46.427</td>
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</tr>
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</table><br>
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<img src="https://static.igem.org/mediawiki/2012/8/84/Light_intensity.png" width=300px><br>
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<font size="5"><br>
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<br>E.co-mail Discussion Ⅱ
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<br></font size="5"></p>
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<p>Above picture shows that E.,coli lit GFP light develops more than that inhibited proteosynthesis and set a darkroom.</p><br>
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<font size="5">
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<br><p>E.co-mail Refecence
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<br></font size="5"></p>
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<p>Evolution of the ssrA degradation tag in Mycoplasma:
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Specificity switch to a different protease.</p><br>
   
   
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<br>Let's make toppling dominoes with E.coli
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<br>Let's make toppling dominoes with E.coli !
<p>This project is based on an idea that, if E.coli transformants that emit green light when they catch green light are placed along a line on an agar plate, and if the end is activated with UV or blue light so that it emit green light, it would look like domino toppling with the green light moving along the line toward the other end. We planned to construct this light transfer system by using the red and green light sensor systems, the light receptor PCB catches light and activate transcription of a specific promoter upstream the lacZ reporter gene. So, we replaced the lacZ gene with the sequences coding for GFP and RFP.</p>
<p>This project is based on an idea that, if E.coli transformants that emit green light when they catch green light are placed along a line on an agar plate, and if the end is activated with UV or blue light so that it emit green light, it would look like domino toppling with the green light moving along the line toward the other end. We planned to construct this light transfer system by using the red and green light sensor systems, the light receptor PCB catches light and activate transcription of a specific promoter upstream the lacZ reporter gene. So, we replaced the lacZ gene with the sequences coding for GFP and RFP.</p>
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 <p>We are trving to draw a movie of a firework that goes upward and bursts scattering light-emitting pieces.
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 <p>We are trying to draw a movie of a firework that goes upward and bursts scattering light-emitting pieces.
The basic green light sensor needs two plasmids.pPLPCB provides a light-sensing molecule that binds to CcaS molecule. pJT118 harbors the genes for CcaS and CcaR and the reporter lacZ gene under the control of the PcpcG2 promoter. CcaS activates PcpcG2,when the light-sensing molecule catches green light, by activating phosphorylation of CcaR. We will substitute the lacZ gene with the GFP gene. Therefore, our green sensor should produce GFP in reaponse to green light.</p>
The basic green light sensor needs two plasmids.pPLPCB provides a light-sensing molecule that binds to CcaS molecule. pJT118 harbors the genes for CcaS and CcaR and the reporter lacZ gene under the control of the PcpcG2 promoter. CcaS activates PcpcG2,when the light-sensing molecule catches green light, by activating phosphorylation of CcaR. We will substitute the lacZ gene with the GFP gene. Therefore, our green sensor should produce GFP in reaponse to green light.</p>
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  <p>We will draw, with E coli harboring pPLPCB and the GFP-substituted pJT118,a picture of a trajectory of a rising firework on an ager plate, and will “fire”with a pilot light at the bottom. Under the blue LED light(or weak UV light),the bottom part of the picture should begin to emit green light that should activate the neighboring bacteria.
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  <p>We will draw, with E. coli harboring pPLPCB and the GFP-substituted pJT118,a picture of a trajectory of a rising firework on an ager plate, and will “fire”with a pilot light at the bottom. Under the blue LED light(or weak UV light),the bottom part of the picture should begin to emit green light that should activate the neighboring bacteria.
Because the GFP has a degradation tag, the emission will stop soon. It is exposed that, as a result, the green light will move upward along the trajectory until it reaches the top.</p>
Because the GFP has a degradation tag, the emission will stop soon. It is exposed that, as a result, the green light will move upward along the trajectory until it reaches the top.</p>
  <p>At the top, we put E.coli with pPLPCB and an RFP-substituted pJT118.This will sense the green light coming from the neighboring bacteria and emit red light.</p>   
  <p>At the top, we put E.coli with pPLPCB and an RFP-substituted pJT118.This will sense the green light coming from the neighboring bacteria and emit red light.</p>   
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1.We amplified a sequence in pJT118 spanning almost all of the plasmid except the region of the lacZ ORF, by PCR with KOD Fx Neo. (using the primers GCGGCCGCTCGAGTCTAATTTTTTTG and ATCTATCATAGATAAAGTTAGTAATTAAAC). The 5780bp fragment was obtained and gel-purified. </p>
1.We amplified a sequence in pJT118 spanning almost all of the plasmid except the region of the lacZ ORF, by PCR with KOD Fx Neo. (using the primers GCGGCCGCTCGAGTCTAATTTTTTTG and ATCTATCATAGATAAAGTTAGTAATTAAAC). The 5780bp fragment was obtained and gel-purified. </p>
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<p>2.We amplified the sequence of the GFP ORF from BioBrick(BBa-E0040) using the primers CTTTATCTATGATAGATATGCGTAAAGGAGAAGAACTT and GACCTGAGCGGCCGCTTTGTATAGTTCATCCATGCCAT.The 750bp fragment was gel-purified.</p>
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<p>2.We amplified the sequence of the GFP ORF from BioBrick (BBa-E0040) using the primers CTTTATCTATGATAGATATGCGTAAAGGAGAAGAACTT and GACCTGAGCGGCCGCTTTGTATAGTTCATCCATGCCAT.The 750bp fragment was gel-purified.</p>
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<p>3.We put the fragment from 1and2 together by the InFusion svstem (Clontech). The miniprep plasmid sample from acolony was checked by agarose gel electrophoresis (Figure1,the middlelabeled as118+GFP). The other plasmids were constructed in almost the same way, and checked on agarose gels (Figures 1and 2).</p>
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<p>3.We put the fragment from 1 and 2 together by the InFusion svstem (Clontech). The miniprep plasmid sample from acolony was checked by agarose gel electrophoresis (Figure1,the middlelabeled as118+GFP). The other plasmids were constructed in almost the same way, and checked on agarose gels (Figures 1and 2).</p>
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<br>figur1 <td><img src="https://static.igem.org/mediawiki/2012/a/a6/P1000457.JPG" width=120px></td> figur2<td><img src="https://static.igem.org/mediawiki/2012/5/5e/9.7_EP.JPG" width=120px></td> figur3<td><img src="https://static.igem.org/mediawiki/2012/a/a5/Picture_Ehime_Japan1026PJT118-GFP-.png" width=300px></td><br>figur4<td><img src="https://static.igem.org/mediawiki/2012/7/7c/Ehime-JapanPJT118-RFP%29.png" width=300px></td> <br>figur5<td><img src="https://static.igem.org/mediawiki/2012/7/72/%E5%9B%B3PJT106b%28RFP%29.png" width=300px></td>
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<br>figure1 <td><img src="https://static.igem.org/mediawiki/2012/a/a6/P1000457.JPG" width=120px></td> figur2<td><img src="https://static.igem.org/mediawiki/2012/5/5e/9.7_EP.JPG" width=120px></td> figure3<td><img src="https://static.igem.org/mediawiki/2012/a/a5/Picture_Ehime_Japan1026PJT118-GFP-.png" width=300px></td><br>figure4<td><img src="https://static.igem.org/mediawiki/2012/7/7c/Ehime-JapanPJT118-RFP%29.png" width=300px></td> <br>figure5<td><img src="https://static.igem.org/mediawiki/2012/7/72/%E5%9B%B3PJT106b%28RFP%29.png" width=300px></td>
</p>
</p>
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<p>fig1:center is 118+GFP right is 118+RFP fig2 thirdline is 106b+RFP fig3 plasmid of 118+GFP fig4 plasmid of 118+RFP
+
<p>figur1  figur2  figur3
-
fig5 plasmid of 106b+RFP</font size><p>
+
figur4 
 +
figur5 
 +
fig. 1: An agarose gel separating the plasmids. center, 118+GFP; right, 118+RFP.  fig. 2: An agarose gel separating plasmids. 106b+RFP is on the third lane. fig, 3: Schematic representation of plasmid 118+GFP.  fig. 4: An illustration of 118+RFP. fig. 5: An illustration of 106b+RFP
 +
 
 +
</font size><p>
Line 305: Line 461:
<br>
<br>
-
<p><font size="6">
+
<p><font size="5">
 +
 
 +
Assay
-
Results
 
-
</font size><p>
 
-
<p><font size="5">
 
-
E.co-Domino
 
</font size><p>
</font size><p>
<p><font size="3">
<p><font size="3">
-
・The function of light sensor  
+
The function of light sensor  
 +
<br>
<br>
<br>
 +
・In liquid medium
<p>   
<p>   
-
In order to confirm if the light sensor system normally works, the control experiment (shown on
+
In order to confirm if the light sensor system normally works, a control experiment (shown on
-
Table1) were carried out.
+
Table1) was carried out.
</p>  
</p>  
</font size="3"><p>
</font size="3"><p>
Line 344: Line 500:
<td>RFP was expressed</td>
<td>RFP was expressed</td>
</tr>
</tr>
 +
</table>
 +
<br>
 +
<br>
 +
<img src="https://static.igem.org/mediawiki/2012/a/a8/P1000432.JPG" width=200px>
 +
<img src="https://static.igem.org/mediawiki/2012/3/39/P1000433.JPG" width=200px>
 +
<img src="https://static.igem.org/mediawiki/2012/5/5d/P1000431.JPG" width=200px>
-
</table>
+
<br>
 +
<br>
<br>
<br>
<p><font size="3">
<p><font size="3">
-
We transformed the plasmids into JT2 (ΔEnvZ strain) and picked up an individual colony to put into
+
We transformed JT2 (ΔEnvZ strain) with the plasmids and picked up an individual colony to put into liquid medium. Incubation with shaking at 37℃ was continued for 42 hours. We expected that the E. coli under white light will express GFP or RFP, and on the other hand, the E. coli under Dark will not express them. Unfortunately, we were not able to see that the E. coli having pJT118 (GFP and RFP) worked.  
-
liquid medium. Shaking incubate on 37℃ was continued for 42 hours. We expected that the E.coli under white light will express GFP or RFP, and on the other hand, the E.coli under Dark will not express them. Unfortunately, we were not able to watch that the E.coli having pJT118 (GFP and RFP) worked.
+
-
</p>
+
<br>
<br>
<p>
<p>
-
We wanted to try to find the best condition for GFP or RFP expression (green sensor), but time was running out, so we decided to use the red light sensor only for our project.
+
We wanted to try to find the best condition for GFP or RFP expression (green sensor), but time was running out, so we decided to use the red light sensor only for our project.  
 +
 
</p></font size="3"><p>
</p></font size="3"><p>
<br>
<br>
<p><font size="3">
<p><font size="3">
-
<br>Purpose: search condition that expression RFP
+
・On plate
-
We used JT2 transformde plasmids(106b+RFP,cph8,pPLPCB) shaking incubate on37℃ 16 hours exposing white light. And it centrifuge, sprinkle M9 plate and incubate 24hours  by three conditions (room temperature ).
+
<br>
-
<br>1, red light
+
<br>To investigate the condition for expression of RFP, We incubated JT2 transformed with three plasmids (106b+RFP, cph8, and pPLPCB) with shaking at 37℃ for 16 hours, exposing white light to them. After centrifugation, the bacteria were plated on M9 agar and were incubated for 24 hours under three different conditions (at room temperature).  
-
<br>2, white light
+
 
-
<br>3, dark
+
<br>1. Red light
-
<br>Result→ all condition expressed RFP 目的 RFPが発現する条件を調べる。プラスミドを入れたJT2を使用。37度で白色光を当てながら浸透培養をしました。それを遠心機にかけ、大腸菌を集めてM9のプレートに撒きました。3つの条件で24時間培養しました。(温度はすべて室温)
+
<br>2. White light
-
1、赤い光を当てて
+
<br>3. Dark
-
2、白色光をあてて
+
<br>Result → RFP was expressed under the all condition. 
-
3、暗闇
+
-
結果 すべて発現した 
+
</p><font size>
</p><font size>
-
<p><br>Purpose: measure time until activate red light sensor by RFP light.
+
<br>
-
<br>We use JT2 transformed the plasmids(106b+RFP,cph8,pPLPCB). Shaking incubate on 37℃was constituted for 12 hours. Centrifuge, remove buffer(LB), added 100μℓbuffer(MQ). Put micro plate as a picture. And we observed E.coli. We try this experiment two condition.<br>1,exposing UV <br>2,Dark<br><font size=4>Result</font><br>expressed RFP for 9 hours
+
・Make E.co-Domino
 +
<br>
 +
<p><br>Purpose: To measure time required for activation of the red light sensor by RFP light.
 +
<br>We useed JT2 transformed with the plasmids(106b+RFP,cph8, and pPLPCB). It was first incubated with shaking incubate on 37℃ was constituted for 12 hours in LB medium. After centrifugation, the medium was replaced with  100&mu;L of buffer(MQ). The samples were put into the wells of a microtiter plate. They were observed under a UV light. We tried this experiment under two different conditions.<br>1.Exposing UV <br>2.Dark<br><font size=4>Result</font><br>RFP was expressed in 9 hours.
</p>
</p>
-
<br><p><br><td>0hour<img src="https://static.igem.org/mediawiki/2012/8/84/P1000531.JPG" width=120px></td>→9hour<img src="https://static.igem.org/mediawiki/2012/b/b5/P1000559.JPG" width=120px></td><br>up line:All holl E.coli not expressed RFP<br>botom line left holl E.coli expressed RFP,others not:</p>目的 RFPの光によって何時間でレッドライトセンサーが働くかを調べる。
+
<br><p><br><td>0hour<img src="https://static.igem.org/mediawiki/2012/8/84/P1000531.JPG" width=200px></td>→9hour<img src="https://static.igem.org/mediawiki/2012/d/d7/P1000557.JPG" width=200px>
-
7度で白色光を当てながら浸透培養を12時間しました。それを遠心機にかけ、培地を取り除き、MQを100マイクロリットルくわえました。それをマイクロプレートに下記の図のように入れて2つの条件で観察しました。1,UVを当てて2、暗闇で 上の列には発現していない大腸菌を入れました。下の列の一番左には発現したものを、残りの二つは発現していないものを入れました.
+
</td><br>
 +
<br></p>
 +
 
 +
<br>
 +
Result and Discussion
 +
<br>
 +
<br>
 +
・Compare the time for expressing RFP from the different cells ( cell (1)-(3) ).
 +
<br>
 +
<br>
 +
The cells are named (1)-(3) on above the picture.
 +
<br>
 +
<p>
 +
(1) The E.coli on the top of E.coli expressing RFP (RFP-E.coli)
 +
<br>
 +
(2)The E.coli on the right of (1)
 +
<br>
 +
(3) The E.coli on the right of RFP-E.coli
 +
<br>
 +
<br>
 +
 
 +
RFP was expressed on the center of the cell.
 +
</p>
 +
<br>
 +
 
 +
<table border="3">
 +
<caption>Table2. The assay of E.co-Domino</caption>
 +
<tr>
 +
<th>(1)</th>
 +
<th>(2)</th>
 +
<th>(3)</th>
 +
</tr>
 +
<tr>
 +
<td>7 hours</td>
 +
<td>9 hours</td>
 +
<td>10 hours</td>
 +
</tr>
 +
</table>
 +
 
 +
<br>
 +
<br>
 +
<p>
 +
In comparison with the cell (2), the amount of RFP in the cell (3) was more. Also, the cell (1) and cell (2) expressed RFP.
 +
From the result above, we found that the red sensor genes are induced by UV (364 nm) and UV+RFP. Furthermore, the condition of RFP+UV is more effective for red sensor genes than UV only.
 +
</p>
 +
<br>
 +
<br>
 +
<p>
 +
Therefore, E.co-Domino will be realized by the red light sensor system.
 +
</p>
 +
<br>
 +
<br>
<br>
<br>
<br>
<br>
Line 389: Line 603:
<p><font size="3"><font color=red>・Heat Shock Sensor</font size> </font color>
<p><font size="3"><font color=red>・Heat Shock Sensor</font size> </font color>
<p><font size="3">
<p><font size="3">
-
  <p>  This is a sensor that RFP is expressed by particular temperature. We made two plasmids. One produces signaling molecule, the other receives the signaling molecule. The plasmids that produces signaling molecule have heat shock promoter(HSP). Transcription of luxI gene is regulated by a HSP. LuxI produces OHHL(3OC6HSL). The other plasmid has Ptet promoter and transcription of the luxR gene is constitutively regulated by the promoter. The luxR protein binds to OHHL and upregulated the luxpR promoter, causing transcription of the mCherry reporter.(ここにPlasmid map)</p>
+
  <p>  This is a sensor that promotes expression of RFP at a particular temperature. We made two plasmids. One produces a signaling molecule, and the other receives the signaling molecule. The plasmids that produces the signaling molecule has a heat shock promoter(HSP). Transcription of luxI gene is regulated by a HSP. LuxI produces OHHL(3OC6HSL). The other plasmid has Ptet promoter and transcription of the luxR gene is constitutively regulated by the promoter. The luxR protein binds to OHHL upregurates and upregulated the luxpR promoter, causing transcription of the mCherry reporter.</p>
<br>
<br>
<br>
<br>
<p><font size="3"><font color=red>・Cold Shock Sensor</font size> </font color>
<p><font size="3"><font color=red>・Cold Shock Sensor</font size> </font color>
-
  <p>This is a sensor that GFP is expressed by particular temperature. The sensor also consists two plasmids. The plasmids that produces signaling molecule have cold shock promoter(CSP). Transcription of lasI gene is regulated by a CSP. LasR produces 3OC12-HSL. The other plasmid has constitutive promoter, transcription of the lasR gene is regulated by the promoter. The lasR protein binds to 3OC12-HSL and upregulated the laspR promoter, causing transcription of the GFP.(ここにplasmid map)</p>
+
  <p>This is a sensor that promotes expression of GFP a particular temperature. The sensor also consists of two plasmids. The plasmid that produces signaling molecule has a cold shock promoter(CSP). Transcription of the lasI gene is regulated by a CSP. LasR produces 3OC12-HSL. The other plasmid has a constitutive promoter upstream, transcription of the lasR gene is regulated by the promoter. The lasR protein binds to 3OC12-HSL and upregulates the laspR promoter, causing transcription of the GFP.</p>
<br>
<br>
<br>
<br>
-
 
+
Figure1<td><img src="https://static.igem.org/mediawiki/2012/e/e8/HSP_luxI.jpg" width=250px></td>
-
'''Heat Shock Sensor'''<br>
+
Figure2<td><img src="https://static.igem.org/mediawiki/2012/c/cf/LuxR_RFP.jpg" width=250px></td>
-
PlasmidⅠ (Fig.1) was made for BBa_K338081 and BBa_C0261 by ligation.<br><br>
+
<BR>     PlasmidⅠ                       PlasmidⅡ<br>
-
'''Cold Shock Sensor'''<br>
+
Figure3<td><img src="https://static.igem.org/mediawiki/2012/c/c7/CSP_lasI.jpg" width=250px></td>
-
PlasmidⅡ(Fig.1 BBa_K794000) was made for BBa_S03878 and BBa_K328001 by ligation.<br>
+
Figure4<td><img src="https://static.igem.org/mediawiki/2012/b/bc/LasR_GFP.jpg" width=250px></td>
-
And we had to replace origin(rep(pMB1)) of PlasmidⅡ origin(p15A) of pPLPCB(S) by infusion.<br>
+
<BR>     PlasmidⅢ                       PlasmidⅣ<br><br>
-
PlasmidⅣ (Fig.1) was made for BBa_S03878 and BBa_K328001 by twice infusion (primer list 1~5).<br>
+
'''Heat Shock Sensor'''<br><br>
 +
Plasmid 1 (Fig.1) was made for BBa_K338081 and BBa_C0261 by ligation.<br><br>
 +
'''Cold Shock Sensor'''<br><br>
 +
Plasmid 2 (Fig.2 BBa_K794000) was made for BBa_S03878 and BBa_K328001 by ligation.<br><br>
 +
And we are planning to replace the origin(rep(pMB1)) of Plasmid 2 with the origin(p15A) of pPLPCB(S) by the InFusion system (Clontech).<br><br>
 +
Plasmid 4 (Fig.1) was made from BBa_S03878 and BBa_K328001 by repetition of the InFusion recombination
 +
(primer list 1~5).<br>
</p>
</p>

Latest revision as of 04:06, 27 September 2012

Ehime-Japan iGEM Team: Welcome




Principles



Light sensor genes

・Green light sensor :pJT118, pPLPCB(S) [1]  

Ho1 and PcyA synthesize 3z-phycocyanobirin (PCB) depending on ferredoxin (Fd). When PCB binds to Ccas, it catches light and affects the function of CcaS depending on the wavelength of the light. When the light is green, autophosphorylation of CcaS and phosphate transfer to CcaR increase. When CcaR is phosphorylated, it promotes the transcription from the PcpcG2 promoter. On the other hand, when the received light is red, CcaS responds reversely, to cause depression of the PcpcG2 promoter. In the original system, pPLPCB(S) provide Ho1 and PcyA, and pJT118 provides Ccas and CcaR in addition to the reporter lacZ gene under the control of PcpcG2.We replaced the LacZ gene in pJT118 with the gene coding for a fluorescent protein.




・Red light sensor :pCph8, pJT106b, pPLPCB(S)

Cph8 (a Cph1-EnvZ chimaeras) is expressed from PLTetO-1 promoter in the phosphorylated ground state. The Cph1 part of Cph8 is synthesized as the apo from, and holo Cph1 is formed when apo Cph1 ligates PCB. Holo Cph1 can absorb light. When far red light (705 nm) is absorbed, the rate of phosphotransfer from the EnvZ domain of Cph8 to OmpR and the affinity of the phosphorylated OmpR (OmpR-P) to the OmpC promoter is increased. This raises transcription of the cI gene downstream an OmpC promoter. The cI repressor represses transcription of a lacZ ORF under the control of the P&lamda; promoter. On the contrary, when red light (650 nm) is absorbed, the rate of phosphotransfer of the EnvZ part of Cph8 is decreased and less cI is expressed. As a result, the amount of transcription from P&lamda; promoter is increased.
[1] Tabor, J. J. et al. (2011) Multichromatic control of gene expression in Escherichia coli. J. Mol. Biol., 405, 315-324.
[2] Levskaya, A. et al. (2005) Engineering Escherichia coli to see light. Nature, 438, 441-442.
[3] Gambetta, G. A. and Lagarias, J. C. (2001) Genetic engineering of phytochrome biosynthesis in bacteria. Proc. Natl. Acad. Sci. USA, 98, 10566-10571
[4] Mattison, K. and Kenney, L.J. (2002) Phosphorylation Alters the Interaction of the Response Regulator OmpR with Its Sensor Kinase EnvZ. J. Biol. Chem., 277


Degradation system

In most bacteria, ssrA-tagged proteins are degraded by protease. In E. coli, the ssrA tag has 11-amino acid sequence that is recognized mainly by the ClpXP protease. The tag has been minimized into the three amino acid LVA tag, and this minimum tag is utilized widely in synthetic biology and in iGEM for temporal expression and degradation of stable protein, such as GFP and repressors. Mycoplasamas, however, do not have the ClpXP protease. The ssrA tag sequences are quite different from those of the other bacteria. It was found that the tag is degraded mainly by the Lon protease in Mesoplasma florum, a Mycoplasma species [1].So, we call the tag “Lon-tag”. The Lon-tagged proteins of M. florum are efficiently recognized and degraded by the M. florum Lon protease. M. florum Lon does not degrade proteins bearing the E. coli-ssrA tag, and E. coli Lon does not efficiently degrade proteins bearing the M. florum ssrA tag . In principle, Lon-tagged proteins in E. coli cells should be degraded more rapidly upon induction of the M.florum Lon protease.


[1] Gur, E. and Suer, R. T. (2008) Proc. Natl. Acad. Sci. USA, 105, 16113-16118. Evolution of the ssrA degradation tag in Mycoplasma: Specificity switch to a different protease.






Projects


E.co-mail


In order to make a circulatable communication system, we used the green and red light sensor plasmids: pJT122, pJT106b, and pPLPCB(S). The E.coli having these plasmids expresses lacZ when the E. coli absorbs the green or red light. First, we constructed the plasmids below.


Fig. 1 PcpcG2-GFP-mf-ssrA(pJT122)
Fig. 2 Pλ-mf.Lon-LVA(pJT106b)

We replaced the lacZ of pJT122 with GFP+ssrA tag (mf. lon) and the lacZ of pJT106b with mf.Lon+LVA. As a result, GFP+ssrA tag is synthesized when the E.coli is exposed green light and mf.Lon+LVA is expressed by red light. This mechanism is shown next.

1. Expose one of the two test tubes with E. coli (pJT122, pJT106b, and pPLPCB(S)) to green light.


The E. coli exposed to green light expresses GFP+ssrA tag.

2. GFP emits its green light byactivation with UV (364 nm) and the light is transferred to the other test tube through an optical fiber.


The other E. coli receives the green light and expresses GFP too.



3. Expose the E. coli to red light.


mf.Lon+LVA tag is expressed and GFP is degraded by the Lon protease.

4. mf.Lon+LVA tag is degraded by ClpX preexisting in E. coli


Return to No.1


Finally, we could construct an E-mail system by making this system smaller !!
Furthermore, the circulatable system could work well owing to the two degradation systems which are independent each other. The details are on "Degradation system".




Because it was difficult to regulate the quantitative control, we did not carry out the experiment to check if mf-ssrA tag is recognized by mf-Lon more speedily than the Lon and LVA tag from E. coli.





E.co-mail AssayⅠ



We made 6 E. coli samples harvoring a combination of 3 plasmids including pPLPCB(S) in common for studying "The effect of mf-Lon","The effect of LVA tag ", JW4092 (Lon-deficient) The combinations of the plasmids are as follows.


1. The effect of mf-Lon

pJT122 (GFP+mf-ssrA tag), pPLPCB(S)and either.



(1) pJT106b with the mf-Lon gene replacing the lacZ gene.

(2) pJT106b without lacZ.

2. The effect of mf-ssrA

pJT106b (mf-Lon) and pPLPCB(S), and either.



(3) pJT122 with the GFP+mf-ssrA tag gene replacing lacZ gene.

(4) pJT122 with the GFP gene (no mf-ssrA tag) replacing the lacZ gene.

3. The effect of LVA tag

pJT122 (GFP+mf-ssrA tag), pPLPCB(S), and either.



(5) pJT106b with the mf-Lon+LVA tag gene replacing the lacZ gene or.

(6) pJT106b with the mf-Lon gene (no LVA tag) replacing the lacZ gene.


E.co-mail ResultⅠ



1. The effect of mf-Lon

(1)
(2)
2. The effect of mf-ssrA

(3)
(4)
3. The effect of LVA tag

(5)
(6)

E.co-mail DiscussionⅠ



We could not tell based on Figures I and II whether the pair of mf-Lon and mf-ssrA tag worked. However, Figure III by itself could be interpreted as a result of degradation by mf-Lon: mf-Lon with the LVA tag should be less stable that without LVA, and the GFP with the mf-ssrA tag should be more slowly degraded by the LVA-tagged mf-Lon. It is possible that the expression of mf-Lon was lower in the cases of (1), (3), and (4).



E.co-mail AssayⅡ



Next, we constructed the simple device to confirm whether GFP is expressed by the green light of GFP through an optical fiber.





With an optical fiber, one test tube containing GFP protein emitting by UV (364 nm) was connected to the other containing the E.coli and shaded.


Because it was difficult to regulate the quantitative control, we did not carry out the experiment to check if mf-ssrA tag is recognized by mf-Lon more speedy than those from E.coli.





E.co-mail ResultⅡ


Light intensity 2
Dark 40.201
Green light 46.427




E.co-mail Discussion Ⅱ

Above picture shows that E.,coli lit GFP light develops more than that inhibited proteosynthesis and set a darkroom.



E.co-mail Refecence

Evolution of the ssrA degradation tag in Mycoplasma: Specificity switch to a different protease.




E.co-Domino


Let's make toppling dominoes with E.coli !

This project is based on an idea that, if E.coli transformants that emit green light when they catch green light are placed along a line on an agar plate, and if the end is activated with UV or blue light so that it emit green light, it would look like domino toppling with the green light moving along the line toward the other end. We planned to construct this light transfer system by using the red and green light sensor systems, the light receptor PCB catches light and activate transcription of a specific promoter upstream the lacZ reporter gene. So, we replaced the lacZ gene with the sequences coding for GFP and RFP.



Firework mechanism (using domino system)

 

We are trying to draw a movie of a firework that goes upward and bursts scattering light-emitting pieces. The basic green light sensor needs two plasmids.pPLPCB provides a light-sensing molecule that binds to CcaS molecule. pJT118 harbors the genes for CcaS and CcaR and the reporter lacZ gene under the control of the PcpcG2 promoter. CcaS activates PcpcG2,when the light-sensing molecule catches green light, by activating phosphorylation of CcaR. We will substitute the lacZ gene with the GFP gene. Therefore, our green sensor should produce GFP in reaponse to green light.

We will draw, with E. coli harboring pPLPCB and the GFP-substituted pJT118,a picture of a trajectory of a rising firework on an ager plate, and will “fire”with a pilot light at the bottom. Under the blue LED light(or weak UV light),the bottom part of the picture should begin to emit green light that should activate the neighboring bacteria. Because the GFP has a degradation tag, the emission will stop soon. It is exposed that, as a result, the green light will move upward along the trajectory until it reaches the top.

At the top, we put E.coli with pPLPCB and an RFP-substituted pJT118.This will sense the green light coming from the neighboring bacteria and emit red light.

At the last, we put E.coli with pPLPCB and an RFP-substituted pJT106b. This will sense the red light coming from the neighboring bacteria and emit red light.

=== Part 2 ===

=== The Experiments ===


Eco-Domino

pJT118 harbors the lacZ reporter gene in addition to the green sensor components. So, we replaced the lacZ sequence with the DNA coding for GFP.pJT106b contains the sequence for the lacZ reporter for the red light sensor. So, we replaced it with the gene for RFP. We also construct a pJT118 derivative containing the RFP gene.

With these plasmids, we believe that we could draw movie pictures on an ager plate canvas. Our first one would be that of a firework in which a ball of green light would go straight upward and burst, scattering lines of red light. The data for the plasmid construction experiments are shown below.



Plasmid construction

1.We amplified a sequence in pJT118 spanning almost all of the plasmid except the region of the lacZ ORF, by PCR with KOD Fx Neo. (using the primers GCGGCCGCTCGAGTCTAATTTTTTTG and ATCTATCATAGATAAAGTTAGTAATTAAAC). The 5780bp fragment was obtained and gel-purified.


2.We amplified the sequence of the GFP ORF from BioBrick (BBa-E0040) using the primers CTTTATCTATGATAGATATGCGTAAAGGAGAAGAACTT and GACCTGAGCGGCCGCTTTGTATAGTTCATCCATGCCAT.The 750bp fragment was gel-purified.


3.We put the fragment from 1 and 2 together by the InFusion svstem (Clontech). The miniprep plasmid sample from acolony was checked by agarose gel electrophoresis (Figure1,the middlelabeled as118+GFP). The other plasmids were constructed in almost the same way, and checked on agarose gels (Figures 1and 2).


figure1 figur2 figure3
figure4
figure5

figur1 figur2 figur3 figur4 figur5 fig. 1: An agarose gel separating the plasmids. center, 118+GFP; right, 118+RFP. fig. 2: An agarose gel separating plasmids. 106b+RFP is on the third lane. fig, 3: Schematic representation of plasmid 118+GFP. fig. 4: An illustration of 118+RFP. fig. 5: An illustration of 106b+RFP


Assay

The function of light sensor

・In liquid medium

In order to confirm if the light sensor system normally works, a control experiment (shown on Table1) was carried out.


Table1. The assay of light sensor
Under white light (42 hours) Dark (42 hours)
pJT118 (GFP), pPLPCB(S) No change No change
pJT118 (RFP), pPLPCB(S) No change No change
pJT106b (RFP), pCph8, pPLPCB(S) RFP was expressed RFP was expressed





We transformed JT2 (ΔEnvZ strain) with the plasmids and picked up an individual colony to put into liquid medium. Incubation with shaking at 37℃ was continued for 42 hours. We expected that the E. coli under white light will express GFP or RFP, and on the other hand, the E. coli under Dark will not express them. Unfortunately, we were not able to see that the E. coli having pJT118 (GFP and RFP) worked.

We wanted to try to find the best condition for GFP or RFP expression (green sensor), but time was running out, so we decided to use the red light sensor only for our project.


・On plate

To investigate the condition for expression of RFP, We incubated JT2 transformed with three plasmids (106b+RFP, cph8, and pPLPCB) with shaking at 37℃ for 16 hours, exposing white light to them. After centrifugation, the bacteria were plated on M9 agar and were incubated for 24 hours under three different conditions (at room temperature).
1. Red light
2. White light
3. Dark
Result → RFP was expressed under the all condition. 


・Make E.co-Domino


Purpose: To measure time required for activation of the red light sensor by RFP light.
We useed JT2 transformed with the plasmids(106b+RFP,cph8, and pPLPCB). It was first incubated with shaking incubate on 37℃ was constituted for 12 hours in LB medium. After centrifugation, the medium was replaced with 100μL of buffer(MQ). The samples were put into the wells of a microtiter plate. They were observed under a UV light. We tried this experiment under two different conditions.
1.Exposing UV
2.Dark
Result
RFP was expressed in 9 hours.



0hour→9hour


Result and Discussion

・Compare the time for expressing RFP from the different cells ( cell (1)-(3) ).

The cells are named (1)-(3) on above the picture.

(1) The E.coli on the top of E.coli expressing RFP (RFP-E.coli)
(2)The E.coli on the right of (1)
(3) The E.coli on the right of RFP-E.coli

RFP was expressed on the center of the cell.


Table2. The assay of E.co-Domino
(1) (2) (3)
7 hours 9 hours 10 hours


In comparison with the cell (2), the amount of RFP in the cell (3) was more. Also, the cell (1) and cell (2) expressed RFP. From the result above, we found that the red sensor genes are induced by UV (364 nm) and UV+RFP. Furthermore, the condition of RFP+UV is more effective for red sensor genes than UV only.



Therefore, E.co-Domino will be realized by the red light sensor system.











=== The Experiments ===


E.cold-heat Sensing System

・Heat Shock Sensor

This is a sensor that promotes expression of RFP at a particular temperature. We made two plasmids. One produces a signaling molecule, and the other receives the signaling molecule. The plasmids that produces the signaling molecule has a heat shock promoter(HSP). Transcription of luxI gene is regulated by a HSP. LuxI produces OHHL(3OC6HSL). The other plasmid has Ptet promoter and transcription of the luxR gene is constitutively regulated by the promoter. The luxR protein binds to OHHL upregurates and upregulated the luxpR promoter, causing transcription of the mCherry reporter.



・Cold Shock Sensor

This is a sensor that promotes expression of GFP a particular temperature. The sensor also consists of two plasmids. The plasmid that produces signaling molecule has a cold shock promoter(CSP). Transcription of the lasI gene is regulated by a CSP. LasR produces 3OC12-HSL. The other plasmid has a constitutive promoter upstream, transcription of the lasR gene is regulated by the promoter. The lasR protein binds to 3OC12-HSL and upregulates the laspR promoter, causing transcription of the GFP.



Figure1 Figure2
     PlasmidⅠ                    PlasmidⅡ
Figure3 Figure4
     PlasmidⅢ                    PlasmidⅣ

'''Heat Shock Sensor'''

Plasmid 1 (Fig.1) was made for BBa_K338081 and BBa_C0261 by ligation.

'''Cold Shock Sensor'''

Plasmid 2 (Fig.2 BBa_K794000) was made for BBa_S03878 and BBa_K328001 by ligation.

And we are planning to replace the origin(rep(pMB1)) of Plasmid 2 with the origin(p15A) of pPLPCB(S) by the InFusion system (Clontech).

Plasmid 4 (Fig.1) was made from BBa_S03878 and BBa_K328001 by repetition of the InFusion recombination (primer list 1~5).