"
Team:Tokyo Tech/Projects/Urea-cooler/index.htm
From 2011.igem.org
| Line 1: | Line 1: | ||
| + | <?xml version="1.0" encoding="Shift_JIS" ?> | ||
| + | <!DOCTYPE html PUBLIC "-//W3C//DTD XHTML 1.0 Transitional//EN" "http://www.w3.org/TR/xhtml1/DTD/xhtml1-transitional.dtd"> | ||
<html lang="english" xmlns="http://www.w3.org/1999/xhtml" xml:lang="english"> | <html lang="english" xmlns="http://www.w3.org/1999/xhtml" xml:lang="english"> | ||
<head> | <head> | ||
| Line 303: | Line 305: | ||
<ul> | <ul> | ||
<li> | <li> | ||
| - | <a href="# | + | <a href="#1abst">1. Abstruct</a> |
<ul> | <ul> | ||
<li><a href="#2.1Intro">2.1 Introduction</a></li> | <li><a href="#2.1Intro">2.1 Introduction</a></li> | ||
| Line 315: | Line 317: | ||
<!-- main contents --> | <!-- main contents --> | ||
<div class="main"> | <div class="main"> | ||
| - | <!-- ############ | + | <!-- ############ Write main contents here ############### --> |
<!-- page title --> | <!-- page title --> | ||
| Line 321: | Line 323: | ||
<p> | <p> | ||
| - | <h2 id=" | + | <h2 id="#1abst">1. Abstract</h2> |
<p> | <p> | ||
| - | We made urea cycle in E.coli by introducing of arginase encoded by | + | We made urea cycle in E.coli by introducing of arginase encoded by |
| - | and get urea to make urea cooler. To make urea cooler, | + | rocF gene and get urea to make urea cooler. To make urea cooler, |
we need large amount of urea. But just by introducing rocF, | we need large amount of urea. But just by introducing rocF, | ||
| - | only a little amount of urea can be produced because arginine biosynthesis | + | only a little amount of urea can be produced because arginine biosynthesis |
| - | repressed. Therefore, we tried to derepress the effect of repression.<br /> | + | is repressed. Therefore, we tried to derepress the effect of repression.<br /> |
| - | Furthermore, we researched flux to provide more urea. | + | Furthermore, we researched flux to provide more urea. As a result, |
| - | + | we found that the artificial urea production system, as well as natural one, | |
| - | + | is robust in a stoichometrically point of view. The analysis also | |
| - | + | found that supplementation of Arg, Glu and Asp would increase urea production rate.<br /> | |
| - | + | ||
<img src="https://static.igem.org/mediawiki/2011/c/cb/TokyoTech_urea-assay1.png" alt="Assay data" width="60%" height="60%" /> | <img src="https://static.igem.org/mediawiki/2011/c/cb/TokyoTech_urea-assay1.png" alt="Assay data" width="60%" height="60%" /> | ||
<div class="graph_title"> | <div class="graph_title"> | ||
| Line 342: | Line 344: | ||
<h3 id="2.1Intro">2.1 Introduction</h3> | <h3 id="2.1Intro">2.1 Introduction</h3> | ||
<p> | <p> | ||
| - | Coolers can be made by adding urea to water, since dissolving urea in water | + | Coolers can be made by adding urea to water, |
| - | + | since dissolving urea in water is an endothermic reaction (-57.8 cal/g). | |
| - | + | However, E. coli does not synthetize urea naturally, | |
| - | + | so we attempted to complete the urea cycle inside E. coli and get urea. <br /> | |
Originally, E.coli has all enzymes of the urea cycle except for the arginase. | Originally, E.coli has all enzymes of the urea cycle except for the arginase. | ||
In this work, introduction of the Bacillus subtilis rocF gene on a | In this work, introduction of the Bacillus subtilis rocF gene on a | ||
| Line 351: | Line 353: | ||
as reported by TUCHMAN et al., (1997) <br /> | as reported by TUCHMAN et al., (1997) <br /> | ||
(Fig.1). | (Fig.1). | ||
| - | + | </p> | |
| - | + | <img src="https://static.igem.org/mediawiki/2011/2/21/TokyoTech_urea-cycle1.png" alt="Urea cycle; Fig1" width="60%" height="60%"/> | |
| - | + | <div class="graph_title"> | |
| - | + | Fig.1 Addition of a gene which codes arginase completes urea cycle in E.coli | |
| + | </div> | ||
| + | |||
| + | <p> | ||
| + | However, just by introducing arginase , E.coli, has showed to produce | ||
| + | only a little amount of urea. TUCHMAN et al proposed that catabolite | ||
| + | repression in arginine biosynthesis pathway is the main reason for | ||
| + | the low production efficiency(TUCHMAN et al., 1997) The bacterial | ||
| + | arginine biosynthetic genes are all regulated via a common repressor | ||
| + | protein encoded by the argR gene and activated in the presence of arginine . | ||
| + | (Fig.3)They circumvented the arginine repression by introduction of | ||
| + | arginine operator sequences (Arg boxes), which bind the arginine repressor. | ||
| + | Upon arginine repressor binding to Arg boxes, the amount of the arginine | ||
| + | repressor which can repress arginine biosynthesis is reduced. | ||
| + | In this work, we tried two ways of solving this problem. One way | ||
| + | is introducing the Arg boxes as previous work. The other way is using an | ||
| + | E. coli that has an argR deletion genotype so that | ||
| + | the repressor is not synthetized. | ||
| + | </p> | ||
| - | + | <img src="https://static.igem.org/mediawiki/2011/9/98/TokyoTech_urea-arg-biosynth.png" alt="Fig2" /> | |
| - | + | <div class="graph_title"> | |
| - | + | Fig.2 Arginine biosynthesis is repressed by arginine repressor and its co-repressor | |
| - | + | </div> | |
| - | + | ||
| - | + | ||
| - | + | ||
| - | + | ||
| - | + | ||
| - | + | ||
| - | + | ||
| - | + | ||
| - | + | ||
| - | + | ||
| - | + | ||
| - | + | ||
| - | + | ||
| - | + | ||
| - | + | ||
<h3 id="2.2">2.2 Results</h3> | <h3 id="2.2">2.2 Results</h3> | ||
| Line 381: | Line 386: | ||
Bacterial strains and plasmids | Bacterial strains and plasmids | ||
The bacterial strains and plasmids used in this study are listed in Table 1 and Table 2, and the constructions are shown in Fig.3. | The bacterial strains and plasmids used in this study are listed in Table 1 and Table 2, and the constructions are shown in Fig.3. | ||
| - | + | ||
<table> | <table> | ||
<caption>TABLE 1. E.coli strains used in this study</caption> | <caption>TABLE 1. E.coli strains used in this study</caption> | ||
| Line 392: | Line 397: | ||
<td>+</td> | <td>+</td> | ||
</tr> | </tr> | ||
| - | + | <tr> | |
| - | + | <td>JD24293</td> | |
| - | + | <td>-</td> | |
</tr> | </tr> | ||
</table> | </table> | ||
| - | |||
JD24293 was obtained from National Institute of Genetics. | JD24293 was obtained from National Institute of Genetics. | ||
| Line 406: | Line 410: | ||
<th>vector</th> | <th>vector</th> | ||
<th>rocF</th> | <th>rocF</th> | ||
| - | <th>Arg | + | <th>Arg box</th> |
</tr> | </tr> | ||
<tr> | <tr> | ||
| - | <td> | + | <td>pTrc-rocF</td> |
<td>pSB3K3</td> | <td>pSB3K3</td> | ||
<td>+</td> | <td>+</td> | ||
| Line 415: | Line 419: | ||
</tr> | </tr> | ||
<tr> | <tr> | ||
| - | <td> | + | <td>pTrc-rocF-Arg Box</td> |
<td>pSB3K3</td> | <td>pSB3K3</td> | ||
<td>+</td> | <td>+</td> | ||
| Line 421: | Line 425: | ||
</tr> | </tr> | ||
</table> | </table> | ||
| - | + | </p> | |
| - | + | ||
| - | + | <img src="https://static.igem.org/mediawiki/2011/6/67/TokyoTech_urea-parts-design.png" alt="plasmid map" /> | |
| - | + | <div class="graph_title"> | |
| - | + | Fig.3 Plasmids used in this study<br /> | |
| - | + | The details of the constructions are here. | |
| - | + | </div> | |
| + | |||
| + | <p> | ||
MG1655 and JD24293 were transformed separately with pSB3K3, | MG1655 and JD24293 were transformed separately with pSB3K3, | ||
pTrc-rocF or pTRC-rocF-Arg box. A detailed method is described here. | pTrc-rocF or pTRC-rocF-Arg box. A detailed method is described here. | ||
| - | + | </p> | |
| - | Urea concentrations detected in growth media of bacterial samples | + | <p> |
| - | after IPTG induction are shown in Fig.5.Detialed procedure is described here | + | Urea concentrations detected in growth media of bacterial samples |
| - | + | 1 hour after IPTG induction are shown in Fig.5. | |
| - | + | Detialed procedure is described here | |
| - | + | </p> | |
| - | + | ||
| - | + | <img src="https://static.igem.org/mediawiki/2011/c/cb/TokyoTech_urea-assay1.png" alt="fig4 Assay data" width="60%" height="60%" /> | |
| - | + | <div class="graph_title"> | |
| - | In MG1655(ArgR+), addition of Trc promoter-rocF led to more production | + | Fig.4 Urea concentration in growth media 1 hour after IPTG induction |
| - | urea compared to the bare backbone pSB3K3 as expected. | + | </div> |
| - | show that insertion of rocF resulted in arginase production as expected, | + | |
| - | + | <p> | |
| - | + | In MG1655(ArgR+), addition of Trc promoter-rocF led to more production | |
| - | + | of urea compared to the bare backbone pSB3K3 as expected. | |
| - | + | These results show that insertion of rocF resulted in arginase | |
| - | + | production as expected, therefore completing the urea cycle in E.coli. | |
| - | + | In the same strain, however, addition of Arg box sequence led | |
| - | + | to little change in urea production. The reason why the effect of | |
| - | + | Arg boxes was not apparent is probably that pSB3K3 is a | |
| - | + | low-copy-number plasmid, in contrast to high-copy number used in the | |
| + | previous report. A low-copy-number plasmid is not capable of introducing | ||
| + | enough number of Arg boxes to effectively deactivate the arginine repressor. | ||
| + | Both of the plasmids containing rocF gene in the stain | ||
| + | JD24293(Arg-) produce urea more efficiently than those in MG1655. | ||
| + | </p> | ||
| + | <p> | ||
These results are in line with the fact that JD24293 carries argR | These results are in line with the fact that JD24293 carries argR | ||
| - | (a gene which codes arginine repressor) loss-of-function mutant, | + | (a gene which codes arginine repressor) loss-of-function mutant, |
| - | means deactivation of arginine repressor by Arg boxes is not needed and | + | which means deactivation of arginine repressor by Arg boxes |
| - | + | is not needed and addition of the Arg box does not result in a | |
| + | significant increase of urea production. | ||
| + | </p> | ||
</p> | </p> | ||
| - | |||
<!-- ############ End of main contents ############ --> | <!-- ############ End of main contents ############ --> | ||
</div> | </div> | ||
Revision as of 09:34, 3 October 2011
<?xml version="1.0" encoding="Shift_JIS" ?> <!DOCTYPE html PUBLIC "-//W3C//DTD XHTML 1.0 Transitional//EN" "http://www.w3.org/TR/xhtml1/DTD/xhtml1-transitional.dtd">
Urea cooler
1. Abstract
We made urea cycle in E.coli by introducing of arginase encoded by
rocF gene and get urea to make urea cooler. To make urea cooler,
we need large amount of urea. But just by introducing rocF,
only a little amount of urea can be produced because arginine biosynthesis
is repressed. Therefore, we tried to derepress the effect of repression.
Furthermore, we researched flux to provide more urea. As a result,
we found that the artificial urea production system, as well as natural one,
is robust in a stoichometrically point of view. The analysis also
found that supplementation of Arg, Glu and Asp would increase urea production rate.
2.1 Introduction
Coolers can be made by adding urea to water,
since dissolving urea in water is an endothermic reaction (-57.8 cal/g).
However, E. coli does not synthetize urea naturally,
so we attempted to complete the urea cycle inside E. coli and get urea.
Originally, E.coli has all enzymes of the urea cycle except for the arginase.
In this work, introduction of the Bacillus subtilis rocF gene on a
standardized plasmid completed urea cycle and enabled E.coli to produce urea
as reported by TUCHMAN et al., (1997)
(Fig.1).
However, just by introducing arginase , E.coli, has showed to produce only a little amount of urea. TUCHMAN et al proposed that catabolite repression in arginine biosynthesis pathway is the main reason for the low production efficiency(TUCHMAN et al., 1997) The bacterial arginine biosynthetic genes are all regulated via a common repressor protein encoded by the argR gene and activated in the presence of arginine . (Fig.3)They circumvented the arginine repression by introduction of arginine operator sequences (Arg boxes), which bind the arginine repressor. Upon arginine repressor binding to Arg boxes, the amount of the arginine repressor which can repress arginine biosynthesis is reduced. In this work, we tried two ways of solving this problem. One way is introducing the Arg boxes as previous work. The other way is using an E. coli that has an argR deletion genotype so that the repressor is not synthetized.
2.2 Results
Bacterial strains and plasmids The bacterial strains and plasmids used in this study are listed in Table 1 and Table 2, and the constructions are shown in Fig.3.
| Strain | argR |
|---|---|
| MG1655 | + |
| JD24293 | - |
| Designation | vector | rocF | Arg box |
|---|---|---|---|
| pTrc-rocF | pSB3K3 | + | - |
| pTrc-rocF-Arg Box | pSB3K3 | + | + |
The details of the constructions are here.
MG1655 and JD24293 were transformed separately with pSB3K3, pTrc-rocF or pTRC-rocF-Arg box. A detailed method is described here.
Urea concentrations detected in growth media of bacterial samples 1 hour after IPTG induction are shown in Fig.5. Detialed procedure is described here
In MG1655(ArgR+), addition of Trc promoter-rocF led to more production of urea compared to the bare backbone pSB3K3 as expected. These results show that insertion of rocF resulted in arginase production as expected, therefore completing the urea cycle in E.coli. In the same strain, however, addition of Arg box sequence led to little change in urea production. The reason why the effect of Arg boxes was not apparent is probably that pSB3K3 is a low-copy-number plasmid, in contrast to high-copy number used in the previous report. A low-copy-number plasmid is not capable of introducing enough number of Arg boxes to effectively deactivate the arginine repressor. Both of the plasmids containing rocF gene in the stain JD24293(Arg-) produce urea more efficiently than those in MG1655.
These results are in line with the fact that JD24293 carries argR (a gene which codes arginine repressor) loss-of-function mutant, which means deactivation of arginine repressor by Arg boxes is not needed and addition of the Arg box does not result in a significant increase of urea production.
