Team:BNU-China/kill

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<h2>Kill Switch</h2>
<h2>Kill Switch</h2>
<p>We designed a kill switch to control "Prometheus" and to prevent potential contamination.</p>
<p>We designed a kill switch to control "Prometheus" and to prevent potential contamination.</p>
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<p>One difficulty we face is how to trigger the suicide progress spontaneously at a certain time. In the medium, the bacteria are easily controlled by adding or removing regulatory factors. However, after pouring E. coli into soil, it is hard for us to control. The suicide progress needs to be activated spontaneously. Moreover, the kill switch is supposed to be “off” for a certain time in the soil, so the bacteria will gain enough time to perform its function.</p>
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<p>One difficulty we face is how to trigger the suicide progress spontaneously at a certain time. In the medium, the bacteria are easily controlled by adding or removing regulatory factors. However, after pouring <i>E. coli</i> into soil, it is hard for us to control. The suicide progress needs to be activated spontaneously. Moreover, the kill switch is supposed to be “off” for a certain time in the soil, so the bacteria will gain enough time to perform its function.</p>
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<p>Considering the problems, toxin protein MazF is the best candidate to kill the “Prometheus” as well as to restrict the bacterial number under reasonable level.</p>
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<p>Considering the problems, toxin protein MazF is the best candidate for "Prometheus" to suicide with, as well as for us to restrict the bacterial number under reasonable level.</p>
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<h2>Background</h2>
<h2>Background</h2>
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     <p>MazEF is a toxin-antitoxin module composed of mazE and mazF locating on the chromosome of E. Coli and other pathogens (Hanna et al, 2005). The expression product of mazF is a stable toxin, while that of mazE is a labile antitoxin of MazF (Hazan et al, 2004; Schusteret al., 2013). MazF is a sequence-specific mRNA endoribonuclease that initiates a programmed cell death pathway in response to various stresses. The mazEF-mediated death pathway can act as a defense mechanism that prevents the spread of bacterial phage infection, allowing bacterial populations to behave like multicellular organisms.</p>
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     <p>MazEF is a toxin-antitoxin module comprising mazE and mazF locating on <i>E. coli</i> and other pathogens' chromosome (Hanna et al, 2005). The protein product of mazF expression is a stable toxin, while mazE a labile MazF antitoxin (Hazan et al, 2004; Schusteret al., 2013). MazF is a sequence-specific mRNA endo-ribonuclease that, when triggered in response to various stresses initiates programmed cell death. The mazEF-mediated death pathway initially acts as a defense mechanism to prevent the spread of bacterial phage infection, allowing bacterial populations to behave like multicellular organisms.</p>
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<a title="Background" href="https://static.igem.org/mediawiki/2014/3/3a/Bnu_safety04.png" rel="prettyPhoto"> <span class="overlay zoom" style="display: none;"></span><img style="opacity: 1; width:50%; margin-left: 200px;" src="https://static.igem.org/mediawiki/2014/3/3a/Bnu_safety04.png"> </a>
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<p>We also designed kill switch to control the death of <i>E. Coli</i>.</p>
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<p>With regard to mazEF system, we designed the kill switch for<i>E. coli</i>.</p>
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<h2>Design:</h2>
<h2>Design:</h2>
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<p>We plan to establish a new E.Coli strain without lacI and MazEF system gene to avoid the inference of cell itself. We will test cI background expression level to see if we need to knock out cI.</p>
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<p>We plan to establish a new <i>E.coli</i> strain without lacI and MazEF system gene to avoid the inference of cell itself. We will test cI background expression level to see if we need to knock out cI.</p>
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<p>As is shown in Fig.1, Fig.2, Fig.3 and Fig.4, in the “Stable State”, before poured into the soil, the E. Coli fertilizer is cultured in the medium with IPTG. Promoter 1 is a weak constitutive promoter, so lacI is transcribed and translated at a considerate low level. Therefore, high concentration of IPTG, which binds LacI and changes LacI’s conformation, is able to inactive LacI and open the promoter 2. Then, CI can be highly expressed to repress promoter3. Finally, mazF is inhibited. </p>
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<p>As is shown in Fig.1, 2, 3, and 4, in "Stable State", before poured into the soil, we culture the bacteria fertilizer in the medium with IPTG. Promoter 1 is a weak constitutive promoter, so lacI is transcribed and translated at a considerate low level. High concentration of IPTG, which inactivates LacI by changing its conformation, could turn on promoter 2. Then, CI can be highly expressed to repress promoter3. At this stage, mazF expression could be inhibited. </p>
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<p>After fertilizing, no more IPTG exists in the soil to bind LacI. As a result, LacI with a tag which stabilize the protein takes time to accumulate to a certain high concentration, which is the repression threshold of promoter 2, aiming to represses promoter 2 as well as the expression of cI. The time needed to finish this progress is the designed “memory time”. During this process, E. coli takes its own responsibility to deliver Mo. And after that, it can be killed to reduce the pollution to environment.</p>
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<p>Once poured into soil, the bacteria are no longer exposed to that level of IPTG. As a result, LacI with a stabilizing tag takes time to accumulate to the repression threshold of promoter 2. When lacI concentration exceeds the threshold, promoter 2, as well as the expression of cI, get repressed. Time needed to finish this progress is referred to as "memory time". Before lacI reaching the threshold, <i>E. coli</i> takes its own responsibility to deliver Mo. After that, suicide would be triggered.</p>
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<p>As is shown in table 1, all the biobricks in the design are from the top 10 most used parts of iGEM to guarantee the feasibility.</p>
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<p>As shown in Table 1, all the biobricks in the design are from the top 10 most used parts of iGEM to guarantee the feasibility.</p>
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<a title="Table 1 Biobricks used in the design" href="https://static.igem.org/mediawiki/2014/6/67/Bnu_safety09.png" rel="prettyPhoto"> <span class="overlay zoom" style="display: none;"></span><img style="opacity: 1; width:80%; margin-left: 80px;" src="https://static.igem.org/mediawiki/2014/6/67/Bnu_safety09.png"> </a>
<a title="Table 1 Biobricks used in the design" href="https://static.igem.org/mediawiki/2014/6/67/Bnu_safety09.png" rel="prettyPhoto"> <span class="overlay zoom" style="display: none;"></span><img style="opacity: 1; width:80%; margin-left: 80px;" src="https://static.igem.org/mediawiki/2014/6/67/Bnu_safety09.png"> </a>
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<p>Hazan R, Engelberg-Kulka H. mazEF: a chromosomal toxin-antitoxin module that triggers programmed cell death in bacteria. Journal of Cell Science 118:4327-4332</p>
<p>Hazan R, Engelberg-Kulka H. mazEF: a chromosomal toxin-antitoxin module that triggers programmed cell death in bacteria. Journal of Cell Science 118:4327-4332</p>
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<p>Hazan R, Sat B, Engelberg-Kulka H. Escherichia coli mazEF-Mediated Cell Death Is Triggered by Various Stressful Conditions. Journal of Bacterology 186(11):3663-3669.</p>
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<p>Hazan R, Sat B, Engelberg-Kulka H. <i>Escherichia coli</i> mazEF-Mediated Cell Death Is Triggered by Various Stressful Conditions. Journal of Bacterology 186(11):3663-3669.</p>
<p>Schuster CF, Park JH, Prax M.Characterization of a mazEF Toxin-Antitoxin Homologue from Staphylococcus equorum. Journal of Bacteriology 195:115-125</p>
<p>Schuster CF, Park JH, Prax M.Characterization of a mazEF Toxin-Antitoxin Homologue from Staphylococcus equorum. Journal of Bacteriology 195:115-125</p>
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Latest revision as of 02:34, 18 October 2014

1 2

Kill Switch

We designed a kill switch to control "Prometheus" and to prevent potential contamination.

One difficulty we face is how to trigger the suicide progress spontaneously at a certain time. In the medium, the bacteria are easily controlled by adding or removing regulatory factors. However, after pouring E. coli into soil, it is hard for us to control. The suicide progress needs to be activated spontaneously. Moreover, the kill switch is supposed to be “off” for a certain time in the soil, so the bacteria will gain enough time to perform its function.

Considering the problems, toxin protein MazF is the best candidate for "Prometheus" to suicide with, as well as for us to restrict the bacterial number under reasonable level.

Background

MazEF is a toxin-antitoxin module comprising mazE and mazF locating on E. coli and other pathogens' chromosome (Hanna et al, 2005). The protein product of mazF expression is a stable toxin, while mazE a labile MazF antitoxin (Hazan et al, 2004; Schusteret al., 2013). MazF is a sequence-specific mRNA endo-ribonuclease that, when triggered in response to various stresses initiates programmed cell death. The mazEF-mediated death pathway initially acts as a defense mechanism to prevent the spread of bacterial phage infection, allowing bacterial populations to behave like multicellular organisms.




With regard to mazEF system, we designed the kill switch forE. coli.



Design:



Fig 1. Stable State





Fig 3. Node Figure



Fig 2. Killing State





Fig 4. Truth Table



We plan to establish a new E.coli strain without lacI and MazEF system gene to avoid the inference of cell itself. We will test cI background expression level to see if we need to knock out cI.

As is shown in Fig.1, 2, 3, and 4, in "Stable State", before poured into the soil, we culture the bacteria fertilizer in the medium with IPTG. Promoter 1 is a weak constitutive promoter, so lacI is transcribed and translated at a considerate low level. High concentration of IPTG, which inactivates LacI by changing its conformation, could turn on promoter 2. Then, CI can be highly expressed to repress promoter3. At this stage, mazF expression could be inhibited.

Once poured into soil, the bacteria are no longer exposed to that level of IPTG. As a result, LacI with a stabilizing tag takes time to accumulate to the repression threshold of promoter 2. When lacI concentration exceeds the threshold, promoter 2, as well as the expression of cI, get repressed. Time needed to finish this progress is referred to as "memory time". Before lacI reaching the threshold, E. coli takes its own responsibility to deliver Mo. After that, suicide would be triggered.

As shown in Table 1, all the biobricks in the design are from the top 10 most used parts of iGEM to guarantee the feasibility.





Table 1 Biobricks used in the design



In the future, we plan to model the “memory time” and do more wet-experiments to confirm its feasibility. As for the modeling, we will test the expression level of promoter 1, the minimal stand of LacI to repress promoter 2 and the degradation speed of LacI. On the other hand, we will test the background expression of CI after removing IPTG to check if the CI concentration is low enough to open the promoter 3. Then we will strive to make this system more effective.



References

Hazan R, Engelberg-Kulka H. mazEF: a chromosomal toxin-antitoxin module that triggers programmed cell death in bacteria. Journal of Cell Science 118:4327-4332

Hazan R, Sat B, Engelberg-Kulka H. Escherichia coli mazEF-Mediated Cell Death Is Triggered by Various Stressful Conditions. Journal of Bacterology 186(11):3663-3669.

Schuster CF, Park JH, Prax M.Characterization of a mazEF Toxin-Antitoxin Homologue from Staphylococcus equorum. Journal of Bacteriology 195:115-125

Lewis D, Le P, Zurla C, Finzi L, Adhya S.Multilevel autoregulation of λ repressor protein CI by DNA looping in vitro. PNAS 108:14807-14812.

Wedler H, Wambutt R. A temperature-sensitive lambda cI repressor functions on a modified operator in yeast cells by masking the TATA element. NCBI 248:499-505.



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