Team:Bielefeld-CeBiTec/Project/Biosafety

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<h1> Biosafety </h1>
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<h1>Biosafety - Antibiotic-free Selection</h1>
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We work on two different biosafety systems.<br>
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An import aspect of biosafety discussion in the field of synthetic biology is the prevention of interactions between genetically modified bacteria and natural wild type strains. This prevents the uncontrolled distribution of sequences coding for genetically modified genes in the environment. Even if these sequences would be released from a laboratory it would be very unlikely that they are integrated in a bacterial genome. Most organisms protect themselves against foreign nucleic acids for example by expressing special RNases and DNases (Bertani and Weigle, 1953; Tock and Dryden, 2005). Further the genetically modified bacterial strains are adapted to the excellent conditions of the laboratory. It is highly unlikely that the natural bacteria will outlast these modified strains in nature due to the better adaptation of the wildtype strains to their environment conditions. But there is no guarantee that there is really no interaction and that the release does not affect the equilibrium of the environment.
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First of all we aim to implement an selection system without antibiotics. The target of this system is to perform two deletions in the KRX genome for two genes encoding the alanine racemase. The alanine racemase catalyses the reversible reaction from L-alanin into D-alanin. D-alanin is an important factor for the bacterial cell wall. Every plasmid which is used for the transformation should carry the alanine racemase to complement the deletion. Without the uptake of the plasmid the bacterial cells will die because of their lack of cell wall production.The advantage of this system is visible during the scientific research. It can be used for all cloning and selection purposes in labs all around the world. No antibiotics have to be used for fermentations for example. Therefor we work on a second biosafety system which is based on two steps.<br>
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So the question how a novel designed sequence or even a heterologous used sequence would affect the environment, can be divided into three cases. In the first scenario it is an artificial altered sequence of DNA or even the changed amino acid sequence of a protein. By introducting naturally not used building blocks in these sequences, like xenonucleotids (XNAs) one could reduce the risk of interaction with the environment.
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For second system the supplementation with L-rhamnose is essential. In the presence of L-rhamnose a rhamnose dependent promotor is activated which lead to the expression of araC and the alanine racemase. The protein of araC inhibits the expression of the P<sub>BAD</sub> promotor. In the absence of L-rhamnose two kill switches are activated. If the rhamnose dependent promotor is not activated D-alanine could not be produced which lead to the lysis of the cell wall. In addition araC is not expressed anymore. This leads to the expression of the RNase Ba (Barnase) which leads to the lysis of intracellular RNA.<br>
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By using a closed system and working with safety strains considering specifications our project fulfills regularities for an industrial application.
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The second case deals with sequences that are useless for the survival of an organisms in its natural enviroment. An example
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The question of biosecurity terms is manifold. The use of BioBricks enables an easy generation of modified organisms by combining different parts. The parts we are using during our project are taken from safety level 1 organisms. At this moment there are no hints for a possibility to abuse parts of our project for terroristic aspects (Dr. Arnold Sauter).<br><br>
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would be the RubisCO we introduced to <i>E.&nbsp;coli</i>. This enzyme is only useful to its host within high concentrations of carbon dioxide and the supply with ribulose-1,5-bisphosphate, which cannot be synthesized in most of the prokaryotes or Fumerate reductase, which also might be only useful under special conditions of an increasing electron supply and anaerobic conditions. So assumed that an intact sequence of one of these genes would integrate into the genome of a natural cell or would be plasmid based taken up, it might be lost even faster because of its higher burden to the cell.
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<a href="https://2014.igem.org/Team:Bielefeld-CeBiTec/Results/Biosafety"> Here</a> you will find the results of our biosafety.
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The third case is the type of genes that probably have an greater impact to the environment, like antibiotics and other bacterial or artificial toxins that entail an advantage in selection for the bacteria. Because of this, the uptake of a corresponding sequence will have an impact of the environment. Toxin encoding sequences are for example used in kill switches, which should prevent genetically modified bacteria from surviving in environment apart from laboratory conditions. If these systems fail there is the possibility of the distribution of such sequences in the environment. Also the probability is very low the consequences would be severely. An bacterium, which is able to produce a toxin, poses a great risk to its enviroment. The consequences could be even more striking when the organism is resistant to antibiotics.
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It is well known that antibiotic resistances are spreading out due to various reasons (Heuer et al., 2011; Lupo et al., 2012). This increases the risk of the formation of multi resistances, which causes problems in medical facilities. Especially in these institutes where a lot of weak, sick and immune suppressed peaple are hospitilized the threat of antibiotic resistant bacteria arises.
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Antibiotic resistances occur in nature in many species. The distribution of such resistances is a novel research field. Soil bacteria seem to be a reservoir of antibiotic resistance genes (Riesenfeld et al., 2004; Forsberg et al., 2012). All antibiotic resistances which are used in the laboratory were isolated from naturally occurring organisms. Nevertheless it is crucial to keep these genes from spreading out.
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To address this problem we implemented an antibiotic-free selection system by the complementation of a D-alanine auxotrophic <i>E.&nbsp;coli</i> strain. We have done this to reduce the need for antibiotic resistances as selection markers and enable an antibiotic-free plasmid selection.
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Further this sysem might be not only limited to <i>E.&nbsp;coli</i> since a D-alanine auxotrophy could be demonstrated also for other bacteria like <i>Listeria monocytes</i> (<a href="#Thompson1998">Thompson <i>et al.</i>, 1998</a>),  <i>Corynebacterium  glutamicum</i> (<a href="#Tauch2002">Tauch <i>et al.</i>, 2002</a>) or <i>Bacillus&nbsp;subtilis</i> (<a href="#Ferrari1985">Ferrari <i>et al.</i>, 1985</a>) as example. It is likely that the system is feasible with any bacteria where the cross-linkage of the peptidoglycane layer is realized with D-alanine.
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   Instruction manual GenTSV (S1)&nbsp; <a href = "https://static.igem.org/mediawiki/2014/e/ec/Bielefeld-CeBiTec_2014-07-20_2014-GenTSV-S1-CeBiTec.pdf" target="_blank"> <img src="https://static.igem.org/mediawiki/2014/b/bd/Bielefeld-CeBiTec_2014-08-12_pdf_Icon.png" height="30px"> </a>  
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    <h6>References</h6>
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      E. Ferrari, D. Henner und M. Yang (1985) Isolation of an alanine racemase gene from Bacillus subtilis and its use for plasmid maintenance in B.subtilis. <a href="http://www.nature.com/nbt/journal/v3/n11/pdf/nbt1185-1003.pdf" target="_blank"><i>Nature Biotechnology</i></a>, vol. 3, pp. 1003 - 1007.
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      A. Tauch, S. Götker, A. Pühler, J. Kalinowski, G. Thierbach (2002) The alanine racemase gene alr is an alternative to antibiotic resistance genes in cloning systems for industrial Corynebacterium glutamicum strains. <a href="http://ac.els-cdn.com/S0168165602001591/1-s2.0-S0168165602001591-main.pdf?_tid=770bd5ec-5570-11e4-9bc2-00000aacb361&acdnat=1413490405_6fec2c2bbb598b23bfd24b64748541b7" target="_blank"><i> Journal of Biotechnology</i></a>, vol. 99, pp. 79 - 91.
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      R. Thompson, H. Bouwer, D. Portnoy, F. Frankel (1998) Pathogenicity and and immunogenicity of a Listeria monocytogenes strain that requires D-alanine for growth. <a href="http://www.ncbi.nlm.nih.gov/pmc/articles/PMC108386/pdf/ii003552.pdf" target="_blank"><i> Infection and Immunity</i></a>, vol. 66, pp. 3552 - 3561.
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Lupo, A., Coyne, S. & Berendonk, T. U. Origin and Evolution of Antibiotic Resistance: The Common Mechanisms of Emergence and Spread in Water Bodies. Front Microbiol 3, (2012).<br>
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Heuer, H., Schmitt, H. & Smalla, K. Antibiotic resistance gene spread due to manure application on agricultural fields. Current Opinion in Microbiology 14, 236–243 (2011).<br>
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Forsberg, K. J. et al. The Shared Antibiotic Resistome of Soil Bacteria and Human Pathogens. Science 337, 1107–1111 (2012).
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Riesenfeld, C. S., Goodman, R. M. & Handelsman, J. Uncultured soil bacteria are a reservoir of new antibiotic resistance genes. Environmental Microbiology 6, 981–989 (2004).<br>
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Bertani, G. & Weigle, J. J. HOST CONTROLLED VARIATION IN BACTERIAL VIRUSES. J Bacteriol 65, 113–121 (1953).<br>
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Tock, M. R. & Dryden, D. T. The biology of restriction and anti-restriction. Current Opinion in Microbiology 8, 466–472 (2005).<br>
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Instruction manual GefStoffV &nbsp; <a href = "https://static.igem.org/mediawiki/2014/d/d6/Bielefeld-CeBiTec_2014-07-20_2014-GefStoffV-CeBiTec.pdf" target="_blank"> <img src="https://static.igem.org/mediawiki/2014/b/bd/Bielefeld-CeBiTec_2014-08-12_pdf_Icon.png" height="30px">  </a>
 
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Latest revision as of 04:00, 18 October 2014


Biosafety - Antibiotic-free Selection

An import aspect of biosafety discussion in the field of synthetic biology is the prevention of interactions between genetically modified bacteria and natural wild type strains. This prevents the uncontrolled distribution of sequences coding for genetically modified genes in the environment. Even if these sequences would be released from a laboratory it would be very unlikely that they are integrated in a bacterial genome. Most organisms protect themselves against foreign nucleic acids for example by expressing special RNases and DNases (Bertani and Weigle, 1953; Tock and Dryden, 2005). Further the genetically modified bacterial strains are adapted to the excellent conditions of the laboratory. It is highly unlikely that the natural bacteria will outlast these modified strains in nature due to the better adaptation of the wildtype strains to their environment conditions. But there is no guarantee that there is really no interaction and that the release does not affect the equilibrium of the environment. So the question how a novel designed sequence or even a heterologous used sequence would affect the environment, can be divided into three cases. In the first scenario it is an artificial altered sequence of DNA or even the changed amino acid sequence of a protein. By introducting naturally not used building blocks in these sequences, like xenonucleotids (XNAs) one could reduce the risk of interaction with the environment.
The second case deals with sequences that are useless for the survival of an organisms in its natural enviroment. An example would be the RubisCO we introduced to E. coli. This enzyme is only useful to its host within high concentrations of carbon dioxide and the supply with ribulose-1,5-bisphosphate, which cannot be synthesized in most of the prokaryotes or Fumerate reductase, which also might be only useful under special conditions of an increasing electron supply and anaerobic conditions. So assumed that an intact sequence of one of these genes would integrate into the genome of a natural cell or would be plasmid based taken up, it might be lost even faster because of its higher burden to the cell.
The third case is the type of genes that probably have an greater impact to the environment, like antibiotics and other bacterial or artificial toxins that entail an advantage in selection for the bacteria. Because of this, the uptake of a corresponding sequence will have an impact of the environment. Toxin encoding sequences are for example used in kill switches, which should prevent genetically modified bacteria from surviving in environment apart from laboratory conditions. If these systems fail there is the possibility of the distribution of such sequences in the environment. Also the probability is very low the consequences would be severely. An bacterium, which is able to produce a toxin, poses a great risk to its enviroment. The consequences could be even more striking when the organism is resistant to antibiotics. It is well known that antibiotic resistances are spreading out due to various reasons (Heuer et al., 2011; Lupo et al., 2012). This increases the risk of the formation of multi resistances, which causes problems in medical facilities. Especially in these institutes where a lot of weak, sick and immune suppressed peaple are hospitilized the threat of antibiotic resistant bacteria arises.
Antibiotic resistances occur in nature in many species. The distribution of such resistances is a novel research field. Soil bacteria seem to be a reservoir of antibiotic resistance genes (Riesenfeld et al., 2004; Forsberg et al., 2012). All antibiotic resistances which are used in the laboratory were isolated from naturally occurring organisms. Nevertheless it is crucial to keep these genes from spreading out.
To address this problem we implemented an antibiotic-free selection system by the complementation of a D-alanine auxotrophic E. coli strain. We have done this to reduce the need for antibiotic resistances as selection markers and enable an antibiotic-free plasmid selection.
Further this sysem might be not only limited to E. coli since a D-alanine auxotrophy could be demonstrated also for other bacteria like Listeria monocytes (Thompson et al., 1998), Corynebacterium glutamicum (Tauch et al., 2002) or Bacillus subtilis (Ferrari et al., 1985) as example. It is likely that the system is feasible with any bacteria where the cross-linkage of the peptidoglycane layer is realized with D-alanine.
References

  • E. Ferrari, D. Henner und M. Yang (1985) Isolation of an alanine racemase gene from Bacillus subtilis and its use for plasmid maintenance in B.subtilis. Nature Biotechnology, vol. 3, pp. 1003 - 1007.
  • A. Tauch, S. Götker, A. Pühler, J. Kalinowski, G. Thierbach (2002) The alanine racemase gene alr is an alternative to antibiotic resistance genes in cloning systems for industrial Corynebacterium glutamicum strains. Journal of Biotechnology, vol. 99, pp. 79 - 91.
  • R. Thompson, H. Bouwer, D. Portnoy, F. Frankel (1998) Pathogenicity and and immunogenicity of a Listeria monocytogenes strain that requires D-alanine for growth. Infection and Immunity, vol. 66, pp. 3552 - 3561.
  • Lupo, A., Coyne, S. & Berendonk, T. U. Origin and Evolution of Antibiotic Resistance: The Common Mechanisms of Emergence and Spread in Water Bodies. Front Microbiol 3, (2012).
  • Heuer, H., Schmitt, H. & Smalla, K. Antibiotic resistance gene spread due to manure application on agricultural fields. Current Opinion in Microbiology 14, 236–243 (2011).
  • Forsberg, K. J. et al. The Shared Antibiotic Resistome of Soil Bacteria and Human Pathogens. Science 337, 1107–1111 (2012). 1. Riesenfeld, C. S., Goodman, R. M. & Handelsman, J. Uncultured soil bacteria are a reservoir of new antibiotic resistance genes. Environmental Microbiology 6, 981–989 (2004).
    Bertani, G. & Weigle, J. J. HOST CONTROLLED VARIATION IN BACTERIAL VIRUSES. J Bacteriol 65, 113–121 (1953).
    Tock, M. R. & Dryden, D. T. The biology of restriction and anti-restriction. Current Opinion in Microbiology 8, 466–472 (2005).