Team:NTU-Taida/Project/Stability

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(3. Post-Segregation Killing:srnBC toxin-antitoxin system)
(Abstract)
 
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{{:Team:NTU-Taida/Templates/BSHero|Title=Stability|Content=<p style="text-indent: 2em;">Every GM system that functions outside the laboratories will face two major problems: system stability and safety! Without selective pressure, we have to deal with plasmid instability; to make our ''E. coli'' colonized bowel we have to use recA+ strains which may cause plasmid multimer. Our genetically modified ''E. coli'' will also contact with many kinds of bacteria and is under the risk of horizontal gene transfer.</p><br />
+
{{:Team:NTU-Taida/Templates/BSHero|Title=Stability of Delivery System|Content=<p>Every GM system that functions outside the laboratories encounters two major problems: system stability and safety! Without selective pressure, we have to deal with plasmid instability. Besides, plasmid multimers may be produced in recA+ strains we used to make our ''E. coli'' colonize bowel. Lastly, with many kinds of bacteria in intestines, our genetically modified ''E. coli'' also lives under the risk of horizontal gene transfer.<p>
-
<p style="text-indent: 2em;">The following segment is our struggle against these obstacles.</p>}}
+
<p>The following segment depicts our struggle against these obstacles.</p>}}
-
==Stability of Delivery System==
+
==Abstract==
-
===Briefing===
+
<p style="text-indent: 2em;">Since our PepdEx system consists of several plasmids and will function in human gut, which lacks antibiotic selection pressure, plasmid segregation stability is critical for determining whether every single E. Coli in guts contains our original designed system after numerous generations. Inspired by natural plasmid and mobile gene element, we cope with segregation instability by incorporating three modules, namely <strong>partition system</strong>, <strong>Multimer resolution system</strong>, and <strong>toxin antitoxin system</strong> into our system. We suppose that the level of regulation would potentially benefit the entire synthetic biology community, as synthetic systems are becoming increasingly complex with fine controls (e.g. on low copy plasmids).</p>
-
<p style="text-indent: 2em;">As our PepdEx system consists of several plasmids and will function outside of the laboratory (human gut) which lacks of antibiotic selection pressure, plasmid segregation stability is critical that determines whether every single E. Coli cell contains the original system with the designated function. Inspired by natural plasmid &amp; mobile gene element, we cope with segregation instability by incorporating three modules, i.e. '''partition system''', '''Multimer resolution system''' and '''toxin antitoxin system''', on top of our system. We think that this layer of regulation will potentially benefit the entire synthetic biology community, as synthetic systems are becoming increasingly complex with fine controls (e.g. on low copy plasmids).</p>
+
-
===Obstacles===
+
==Stability Issues==
-
Plasmid instability problems come majorly from the segregational instability,the burden effect and the dimer catastrophe.
+
Problems of plamid instability mainly results from the segregational instability,the burden effect and the dimer catastrophe.
# Segregational instability <p style="text-indent: 2em;"> Plasmids are randomly (possibly uneven) distributed inside a bacterium. After cell division, one of the progenies may lose plasmids.</p>[[File:NTU-Taida-Par1.png|500px|center]]
# Segregational instability <p style="text-indent: 2em;"> Plasmids are randomly (possibly uneven) distributed inside a bacterium. After cell division, one of the progenies may lose plasmids.</p>[[File:NTU-Taida-Par1.png|500px|center]]
-
# Burden Effect <p style="text-indent: 2em;">Cells bearing our PepdEx system have to spend extra energy/resource, so will not grow as good as plasmid-free cells. This metabolic burden will cause our coli to gradually lose pieces of circuits, and the growth rate difference will eventually eliminate plasmid-bearing bacteria in the population.</p>[[File:NTU-Taida-Burden3.png|500px|center]]
+
# Burden Effect <p style="text-indent: 2em;">Cells bearing our PepdEx system have to spend extra energy/resource, so they won't grow as good as plasmid-free cells. This metabolic burden will cause our E.coli to gradually lose parts of our circuits, and the different growth rate will eventually bring about elimination of plasmid-bearing bacteria in the population.</p>[[File:NTU-Taida-Burden3.png|500px|center]]
-
# Dimer Catastrophe<p style="text-indent: 2em;">Homologues recombination may cause plasmid multimers which will increases segregational instability and burden[[#Ref1|[1] ]]. This is the reason why most lab coli are recA1 mutants. But since our coli must be able to colonize in the gut, it should be recA+ wild type strain. That's the problem!</p>[[File:NTU-Taida-Mrs-1.png|500px|center]]
+
# Dimer Catastrophe<p style="text-indent: 2em;">Homologues recombination may cause plasmid multimers which will increase segregational instability and burden[[#Ref|[1] ]]. This is the reason why most E.coli in lab are recA1 mutants. Since our E.coli must be able to colonize in the gut, it should be recA+ wild type strain. Therefore it's the problem we need to deal with right now!</p>[[File:NTU-Taida-Mrs-1.png|500px|center]]
-
===Stabilization Modules===
+
==1 Multimer Resolution System==
-
 
+
-
====1. Multimer Resolution System:Tn1000(gamma delta) resolution system====
+
[[FIle:NTU-Taida-Mrs-2.png|600px|center|structure of MRS]]
[[FIle:NTU-Taida-Mrs-2.png|600px|center|structure of MRS]]
-
:<p style="text-indent: 2em;">To deal with multimerization, we cloned an cassette (BBa_K817018) which encodes an autoregulated resolves (serine type recombinase) from E.coli F plasmid transposon tn1000 (tn3 family)[[#Ref2|[2] ]]. Its promoter region consists of 3 sub-sites(res site) and can process recombination[[#Ref3|[3] ]]. This cassette can resolve multimer that formed during replicative transposition[[#Ref4|[4] ]]. It can also resolve plasmid multimer to increase plasmid stability by avoiding dimer catastrophe. Multimer resolution system (MRS) provides analogous functions to E.coli chromosome XerCD/dif but acts independent of cell cycle, DNA localization and may have higher efficiency on plasmids compared with slow XerCD system[[#Ref5|[5] ]].</p>
+
:<p style="text-indent: 2em;">To deal with multimerization, we cloned a cassette (BBa_K817018) encoding an autoregulated resolvase (serine type recombinase) from E.coli F plasmid transposon tn1000 (tn3 family)[[#Ref|[2] ]]. Its promoter region consists of 3 sub-sites(res site) and can process recombination[[#Ref|[3] ]]. This cassette can resolve multimers that are formed during replicative transposition[[#Ref|[4] ]]. It can also increase plasmid stability by avoiding dimer catastrophe. Multimer resolution system (MRS) has analogous functions as chromosome XerCD/dif in E.coli; however, MRS seems more efficient due to its independence of cell cycle and DNA localization.[[#Ref|[5] ]].</p>
[[FIle:NTU-Taida-Mrs-4.png|200px|center]]
[[FIle:NTU-Taida-Mrs-4.png|200px|center]]
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[[FIle:NTU-Taida-Mrs-3.png|600px|center]]
[[FIle:NTU-Taida-Mrs-3.png|600px|center]]
-
====2. Partition System:from '''<em>Pseudomonas putida''' KT2440</em>====
+
==2 Partition System==
-
:<p style="text-indent: 2em;">Bacterium distributes chromosomes/plasmids evenly to its progenies by a dynamic system that includes SMC like proteins, type Ia partition system and so on[[#Ref6|[6] ]]]]. Type Ia partition system segregates chromosomes/plasmids in a process akin to Eukaryotic mitosis. It can be found on most eubacteria. However, E. coli is not the case.</p>
+
:<p style="text-indent: 2em;">Bacterium distributes chromosomes/plasmids evenly to its progenies by a dynamic system that includes SMC like proteins, type Ia partition system and so on[[#Ref|[6] ]]. Type Ia partition system segregates chromosomes/plasmids in a process akin to Eukaryotic mitosis. It can be found in most eubacteria. However, E. coli is not the case.</p>
[[FIle:NTU-Taida-Par2.png|700px|center]]
[[FIle:NTU-Taida-Par2.png|700px|center]]
-
:<p style="text-indent: 2em;">Previous study have shown that when providing parAB of P.putida in trans and carrying parS site in cis, segregation of low copy plasmids (mini F) can be stabilized in E. coli.[[#Ref7|[7] ]]]].The BioBrick vector pSB2K3 is a mini F plasmid, thus we expect we can stabilize its segregation this way. Our team have made a modified version of pSB2K3 with parS site (BBa_K817017), and plan to use it to harbor our PepdEx system (a low copy number plasmid allows us to fine tune our systems controls e.g. with smaller number of operator sites). We have also cloned the parAB operon (BBa_K817019), and provided the registry with the short 16bp parS site (BBa_K817016) for future applications.</p>
+
:<p style="text-indent: 2em;">Previous studies have shown that when putting parAB of P.putida in trans and setting parS site in cis, segregation of low copy plasmids (mini F) can be stabilized in E. coli.[[#Ref|[7] ]]]].The BioBrick vector pSB2K3 is a mini F plasmid, and thus we expect it can help stabilize the segregation of our system. Our team has made a modified version of pSB2K3 with parS site (BBa_K817017), and plans to use it to harbor our PepdEx system (a low copy number plasmid allows us to fine tune our systems controls e.g. with smaller number of operator sites). We have also cloned the parAB operon (BBa_K817019), and provided the registry with the short 16bp parS site (BBa_K817016) for future applications.</p>
[[FIle:NTU-Taida-Par3.png|500px|center]]
[[FIle:NTU-Taida-Par3.png|500px|center]]
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[[FIle:NTU-Taida-Par4.png|500px|center]]
[[FIle:NTU-Taida-Par4.png|500px|center]]
-
====3. Post-Segregation Killing:srnBC toxin-antitoxin system====
+
==3 Toxin-antitoxin System==
-
:No matter how well our partition system and multimer resolution system work, inevitably there will still be some bacteria losing plasmids (pieces of the circuit). These cells with incomplete system will not function as hoped. We sentence these cells to death to solve the problem.
+
:<p style="text-indent: 2em;">No matter how well our partition system and multimer resolution system work, inevitably there are still some bacteria losing their plasmids (parts of the circuit). These cells with incomplete system will not function as expected. Thus we sentence these cells to death to solve the problem.</p>
{| align="center"
{| align="center"
Line 47: Line 44:
|}
|}
-
:<p style="text-indent: 2em;">Type I toxin-antitoxin srnBC is an ideal executor which belongs to hok/sok homologues.[[#Ref8|[8] ]] It expresses stable toxin encoded RNA and short lived antitoxin RNA that can neutralize toxin RNA by RNA interaction and RNase III cleavage[[#Ref9|[9] ]]. It acts as post segregation killing system – a bacterial cell will get killed if it loses the DNA (genomic islands, plasmids, mobile gene elements) that contains the module[[#Ref10|[10] ]]. We plan to use it to reduce plasmid-lost cells in our coli population, in the hope to make applications without antibiotic selection more feasible. We have cloned the cassette with BioBrick standard (BBa_K817015). Following pictures show the mechanism (based on hok/sok).</p>
+
:<p style="text-indent: 2em;">Type I toxin-antitoxin srnBC is an ideal executor which belongs to hok/sok homologues. It expresses stable toxin encoding RNA and short-lived antitoxin RNA that can neutralize toxin RNA by RNA interaction and RNase III cleavage[[#Ref|[9] ]]. It acts as post segregation killing system – a bacterial cell will be killed if it loses the DNA (genomic islands, plasmids, mobile gene elements) containing the module[[#Ref|[10] ]]. We plan to use it to reduce plasmid-lost cells in our coli population, in the hope to make applications without antibiotic selection more feasible. We have cloned the cassette with BioBrick standard (BBa_K817015). Following pictures show the mechanism (based on hok/sok).</p>
-
 
+
-
[[FIle:NTU-Taida-SrnBC-Mechanism1.png|600px|thumb|center|<p style="text-indent: 2em;">TA loci express two kinds of RNA, namely srnB and srnC, respectively. Initially, srnB is inactive and stable (half-life in the order of 30 minutes [[#Ref11|[11] ]]) and will gradually be processed to active form producing hydrophobic toxic protein if srnC RNA does not exist; srnC is relative unstable and is degraded quickly, and it overlaps and compliments to 5’sequence of srnB.</p>]]
+
-
[[FIle:NTU-Taida-SrnBC-Mechanism2.png|600px|thumb|center|<p style="text-indent: 2em;">At normal condition (plasmid retained), srnC can pair with processed srnB and forms double stranded RNA that is susceptible to RNase III cleavage and thus prevents toxin production. If the plasmid loses, srnC will quickly disappear without replenishing and srnB will show its power[[#Ref12|[12] ]].</p>]]
+
[[FIle:NTU-Taida-SrnBC-Mechanism1.png|600px|thumb|center|<p style="text-indent: 2em;">TA loci express two kinds of RNA, namely srnB and srnC, respectively. Initially, srnB is inactive and stable (half-life in the order of 30 minutes [[#Ref|[11] ]]) and will gradually be processed to active form producing hydrophobic toxic protein if srnC RNA does not exist; srnC is relative unstable and is degraded quickly, and it overlaps and compliments to 5’sequence of srnB.</p>]]
-
====4. Reduce Burden Effect====
+
[[FIle:NTU-Taida-SrnBC-Mechanism2.png|600px|thumb|center|<p style="text-indent: 2em;">At normal condition (plasmid retained), srnC can pair with processed srnB and forms double stranded RNA that is susceptible to RNase III cleavage and thus prevents toxin production. If the plasmid loses, srnC will quickly disappear without replenishing and srnB will show its power[[#Ref|[12] ]].</p>]]
-
:Finally, beyond these modules, reducing the burden effect is in general important to the stability of complex artificial systems in an intact E. coli cell without antibiotic selection. We reason that a well designed system with a lower gene dosage will help.
+
==4 Reduce Burden Effect==
-
High level gene expression and gene dosage leads to burden effect. Therefore, if two systems are encoded in different plasmids with the same overall performance, low copy plasmids are preferred over high copy ones. And again if with the same overall outcome, stabilizing mRNA is preferred over overexpressing the gene (unless for regulatory purposes). Place yourselves in E. coli's position! Reduce its metabolic burden as much as possible then it will work for you!
+
:<p style="text-indent: 2em;">Finally, beyond these modules, reducing the burden effect is generally important to the stability of complex artificial systems in an intact E. coli cell without antibiotic selection. We reason that a well designed system with a lower gene dosage would help.</p>
 +
<p style="text-indent: 2em;">High level gene expression and gene dosage lead to burden effect. That is to say, if two systems are encoded in different plasmids with the same overall performance, bacteria with lower copy plasmids prevail over the ones with higher copy plasmids. Again if with the same overall outcome, stabilizing mRNA prevails over overexpressing the gene (unless for regulatory purposes). Put yourselves in E. coli's shoes! Reduce its metabolic burden as much as possible then it will work for you! </p>
[[FIle:NTU-Taida-Burden2.png|330px|center]]
[[FIle:NTU-Taida-Burden2.png|330px|center]]
-
=== Reference ===
 
-
<ol>
 
-
    <li>Field, C.M. and D.K. Summers, Multicopy plasmid stability: revisiting the dimer catastrophe. Journal of Theoretical Biology, 2011. 291: p. 119-27.
 
-
</li><li>Falvey, E. and N.D.F. Grindley, Contacts between Gamma-Delta-Resolvase and the Gamma-Delta-Res Site. Embo Journal, 1987. 6(3): p. 815-821.
 
-
</li><li>Grindley, N.D.F., et al., Transposon-Mediated Site-Specific Recombination - Identification of 3 Binding-Sites for Resolvase at the Res-Sites of Gamma-Delta and Tn3. Cell, 1982. 30(1): p. 19-27.
 
-
</li><li>Wells, R.G. and N.D.F. Grindley, Analysis of the Gamma-Delta Res Site - Sites Required for Site-Specific Recombination and Gene-Expression. Journal of Molecular Biology, 1984. 179(4): p. 667-687.
 
-
</li><li>Guhathakurta, A., I. Viney, and D. Summers, Accessory proteins impose site selectivity during ColE1 dimer resolution. Molecular Microbiology, 1996. 20(3): p. 613-620.
 
-
</li><li>Mullins, R.D., Bacterial Chromosome Segregation. Annu Rev Cell Dev Biol, 2009.
 
-
</li><li>Godfrin-Estevenon, A.M., F. Pasta, and D. Lane, The parAB gene products of Pseudomonas putida exhibit partition activity in both P. putida and Escherichia coli. Molecular Microbiology, 2002. 43(1): p. 39-49.
 
-
</li><li>Gerdes, K., et al., Mechanism of killer gene activation. Antisense RNA-dependent RNase III cleavage ensures rapid turn-over of the stable hok, srnB and pndA effector messenger RNAs. Journal of Molecular Biology, 1992. 226(3): p. 637-49.
 
-
</li><li>Thisted, T. and K. Gerdes, Mechanism of post-segregational killing by the hok/sok system of plasmid R1. Sok antisense RNA regulates hok gene expression indirectly through the overlapping mok gene. Journal of Molecular Biology, 1992. 223(1): p. 41-54.
 
-
</li><li>Szekeres, S., et al., Chromosomal toxin-antitoxin loci can diminish large-scale genome reductions in the absence of selection. Molecular Microbiology, 2007. 63(6): p. 1588-1605.
 
-
</li><li>Faridani, O.R., et al., Competitive inhibition of natural antisense Sok-RNA interactions activates Hok-mediated cell killing in Escherichia coli. Nucleic Acids Research, 2006. 34(20): p. 5915-5922.
 
-
</li><li=#Ref12>Gerdes, K. and E.G.H. Wagner, RNA antitoxins. Current Opinion in Microbiology, 2007. 10(2): p. 117-124.
 
-
</li>
+
===Reference===
 +
<ol id="Ref">
 +
<li >Field, C.M. and D.K. Summers, Multicopy plasmid stability: revisiting the dimer catastrophe. Journal of Theoretical Biology, 2011. 291: p. 119-27.</li>
 +
<li>Falvey, E. and N.D.F. Grindley, Contacts between Gamma-Delta-Resolvase and the Gamma-Delta-Res Site. Embo Journal, 1987. 6(3): p. 815-821.</li>
 +
<li>Grindley, N.D.F., et al., Transposon-Mediated Site-Specific Recombination - Identification of 3 Binding-Sites for Resolvase at the Res-Sites of Gamma-Delta and Tn3. Cell, 1982. 30(1): p. 19-27.</li>
 +
<li>Wells, R.G. and N.D.F. Grindley, Analysis of the Gamma-Delta Res Site - Sites Required for Site-Specific Recombination and Gene-Expression. Journal of Molecular Biology, 1984. 179(4): p. 667-687.</li>
 +
<li>Guhathakurta, A., I. Viney, and D. Summers, Accessory proteins impose site selectivity during ColE1 dimer resolution. Molecular Microbiology, 1996. 20(3): p. 613-620.</li>
 +
<li>Mullins, R.D., Bacterial Chromosome Segregation. Annu Rev Cell Dev Biol, 2009.</li>
 +
<li>Godfrin-Estevenon, A.M., F. Pasta, and D. Lane, The parAB gene products of Pseudomonas putida exhibit partition activity in both P. putida and Escherichia coli. Molecular Microbiology, 2002. 43(1): p. 39-49.</li>
 +
<li>Gerdes, K., et al., Mechanism of killer gene activation. Antisense RNA-dependent RNase III cleavage ensures rapid turn-over of the stable hok, srnB and pndA effector messenger RNAs. Journal of Molecular Biology, 1992. 226(3): p. 637-49.</li>
 +
<li>Thisted, T. and K. Gerdes, Mechanism of post-segregational killing by the hok/sok system of plasmid R1. Sok antisense RNA regulates hok gene expression indirectly through the overlapping mok gene. Journal of Molecular Biology, 1992. 223(1): p. 41-54.</li>
 +
<li>Szekeres, S., et al., Chromosomal toxin-antitoxin loci can diminish large-scale genome reductions in the absence of selection. Molecular Microbiology, 2007. 63(6): p. 1588-1605.</li>
 +
<li>Faridani, O.R., et al., Competitive inhibition of natural antisense Sok-RNA interactions activates Hok-mediated cell killing in Escherichia coli. Nucleic Acids Research, 2006. 34(20): p. 5915-5922.</li>
 +
<li>Gerdes, K. and E.G.H. Wagner, RNA antitoxins. Current Opinion in Microbiology, 2007. 10(2): p. 117-124.</li>
</ol>
</ol>
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Latest revision as of 21:25, 26 October 2012

Stability

Stability of Delivery System

Every GM system that functions outside the laboratories encounters two major problems: system stability and safety! Without selective pressure, we have to deal with plasmid instability. Besides, plasmid multimers may be produced in recA+ strains we used to make our ''E. coli'' colonize bowel. Lastly, with many kinds of bacteria in intestines, our genetically modified ''E. coli'' also lives under the risk of horizontal gene transfer.

The following segment depicts our struggle against these obstacles.

Contents

Abstract

Since our PepdEx system consists of several plasmids and will function in human gut, which lacks antibiotic selection pressure, plasmid segregation stability is critical for determining whether every single E. Coli in guts contains our original designed system after numerous generations. Inspired by natural plasmid and mobile gene element, we cope with segregation instability by incorporating three modules, namely partition system, Multimer resolution system, and toxin antitoxin system into our system. We suppose that the level of regulation would potentially benefit the entire synthetic biology community, as synthetic systems are becoming increasingly complex with fine controls (e.g. on low copy plasmids).

Stability Issues

Problems of plamid instability mainly results from the segregational instability,the burden effect and the dimer catastrophe.

  1. Segregational instability

    Plasmids are randomly (possibly uneven) distributed inside a bacterium. After cell division, one of the progenies may lose plasmids.

    NTU-Taida-Par1.png
  2. Burden Effect

    Cells bearing our PepdEx system have to spend extra energy/resource, so they won't grow as good as plasmid-free cells. This metabolic burden will cause our E.coli to gradually lose parts of our circuits, and the different growth rate will eventually bring about elimination of plasmid-bearing bacteria in the population.

    NTU-Taida-Burden3.png
  3. Dimer Catastrophe

    Homologues recombination may cause plasmid multimers which will increase segregational instability and burden[1] . This is the reason why most E.coli in lab are recA1 mutants. Since our E.coli must be able to colonize in the gut, it should be recA+ wild type strain. Therefore it's the problem we need to deal with right now!

    NTU-Taida-Mrs-1.png

1 Multimer Resolution System

structure of MRS

To deal with multimerization, we cloned a cassette (BBa_K817018) encoding an autoregulated resolvase (serine type recombinase) from E.coli F plasmid transposon tn1000 (tn3 family)[2] . Its promoter region consists of 3 sub-sites(res site) and can process recombination[3] . This cassette can resolve multimers that are formed during replicative transposition[4] . It can also increase plasmid stability by avoiding dimer catastrophe. Multimer resolution system (MRS) has analogous functions as chromosome XerCD/dif in E.coli; however, MRS seems more efficient due to its independence of cell cycle and DNA localization.[5] .

NTU-Taida-Mrs-4.png
NTU-Taida-Mrs-3.png

2 Partition System

Bacterium distributes chromosomes/plasmids evenly to its progenies by a dynamic system that includes SMC like proteins, type Ia partition system and so on[6] . Type Ia partition system segregates chromosomes/plasmids in a process akin to Eukaryotic mitosis. It can be found in most eubacteria. However, E. coli is not the case.

NTU-Taida-Par2.png

Previous studies have shown that when putting parAB of P.putida in trans and setting parS site in cis, segregation of low copy plasmids (mini F) can be stabilized in E. coli.[7] ]].The BioBrick vector pSB2K3 is a mini F plasmid, and thus we expect it can help stabilize the segregation of our system. Our team has made a modified version of pSB2K3 with parS site (BBa_K817017), and plans to use it to harbor our PepdEx system (a low copy number plasmid allows us to fine tune our systems controls e.g. with smaller number of operator sites). We have also cloned the parAB operon (BBa_K817019), and provided the registry with the short 16bp parS site (BBa_K817016) for future applications.

NTU-Taida-Par3.png
NTU-Taida-Par4.png

3 Toxin-antitoxin System

No matter how well our partition system and multimer resolution system work, inevitably there are still some bacteria losing their plasmids (parts of the circuit). These cells with incomplete system will not function as expected. Thus we sentence these cells to death to solve the problem.

NTU-Taida-TAgrenade.png Work hard or Die hard!!!

Type I toxin-antitoxin srnBC is an ideal executor which belongs to hok/sok homologues. It expresses stable toxin encoding RNA and short-lived antitoxin RNA that can neutralize toxin RNA by RNA interaction and RNase III cleavage[9] . It acts as post segregation killing system – a bacterial cell will be killed if it loses the DNA (genomic islands, plasmids, mobile gene elements) containing the module[10] . We plan to use it to reduce plasmid-lost cells in our coli population, in the hope to make applications without antibiotic selection more feasible. We have cloned the cassette with BioBrick standard (BBa_K817015). Following pictures show the mechanism (based on hok/sok).

TA loci express two kinds of RNA, namely srnB and srnC, respectively. Initially, srnB is inactive and stable (half-life in the order of 30 minutes [11] ) and will gradually be processed to active form producing hydrophobic toxic protein if srnC RNA does not exist; srnC is relative unstable and is degraded quickly, and it overlaps and compliments to 5’sequence of srnB.

At normal condition (plasmid retained), srnC can pair with processed srnB and forms double stranded RNA that is susceptible to RNase III cleavage and thus prevents toxin production. If the plasmid loses, srnC will quickly disappear without replenishing and srnB will show its power[12] .

4 Reduce Burden Effect

Finally, beyond these modules, reducing the burden effect is generally important to the stability of complex artificial systems in an intact E. coli cell without antibiotic selection. We reason that a well designed system with a lower gene dosage would help.

High level gene expression and gene dosage lead to burden effect. That is to say, if two systems are encoded in different plasmids with the same overall performance, bacteria with lower copy plasmids prevail over the ones with higher copy plasmids. Again if with the same overall outcome, stabilizing mRNA prevails over overexpressing the gene (unless for regulatory purposes). Put yourselves in E. coli's shoes! Reduce its metabolic burden as much as possible then it will work for you!

NTU-Taida-Burden2.png


Reference

  1. Field, C.M. and D.K. Summers, Multicopy plasmid stability: revisiting the dimer catastrophe. Journal of Theoretical Biology, 2011. 291: p. 119-27.
  2. Falvey, E. and N.D.F. Grindley, Contacts between Gamma-Delta-Resolvase and the Gamma-Delta-Res Site. Embo Journal, 1987. 6(3): p. 815-821.
  3. Grindley, N.D.F., et al., Transposon-Mediated Site-Specific Recombination - Identification of 3 Binding-Sites for Resolvase at the Res-Sites of Gamma-Delta and Tn3. Cell, 1982. 30(1): p. 19-27.
  4. Wells, R.G. and N.D.F. Grindley, Analysis of the Gamma-Delta Res Site - Sites Required for Site-Specific Recombination and Gene-Expression. Journal of Molecular Biology, 1984. 179(4): p. 667-687.
  5. Guhathakurta, A., I. Viney, and D. Summers, Accessory proteins impose site selectivity during ColE1 dimer resolution. Molecular Microbiology, 1996. 20(3): p. 613-620.
  6. Mullins, R.D., Bacterial Chromosome Segregation. Annu Rev Cell Dev Biol, 2009.
  7. Godfrin-Estevenon, A.M., F. Pasta, and D. Lane, The parAB gene products of Pseudomonas putida exhibit partition activity in both P. putida and Escherichia coli. Molecular Microbiology, 2002. 43(1): p. 39-49.
  8. Gerdes, K., et al., Mechanism of killer gene activation. Antisense RNA-dependent RNase III cleavage ensures rapid turn-over of the stable hok, srnB and pndA effector messenger RNAs. Journal of Molecular Biology, 1992. 226(3): p. 637-49.
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