Difference between revisions of "Team:Tec-Chihuahua/Design"

 
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<h2 align="center"> Design Overview</h2>
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<h2 align="center">Design Overview</h2>
<div class="a">
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<h4 align="justify"><b>Considerations</b></h4>  
<p align="justify">Team Tec-Chihuahua’s main objective is to prevent (and treat) both the American Foulbrood and European Foulbrood, as well as to increase the general defenses of the bees and its larvae. The way in which we are planning to accomplish this purpose is by using synthetic biology techniques. Our project can be divided into two parts: first characterizing that our proteins will have an effect on P. larvae and M. plutonius and then having them ready as a product for sale. </p></div>
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<ol>
<h2 align="center">Proof of Concept</h2>
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  <li>In order to obtain the antimicrobial peptides of interest (apidaecin, abaecin, defensin 1 and defensin 2) and to be able to use them against both pathogens (<i>Paenibacillus larvae</i> and <i>Melissococcus plutonius</i>) an appropriate design is required; specialized in expressing heterologous proteins that are meant to be purified.</li><br>
<div class="a">
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  <li>Given that the peptides will be exposed to the hive's environment, it is essential to provide them protection which can increase their half-life.</li>
<p align="justify">The first step in making our dream of saving the bees possible was to design the genetic device that would later on give us our recombinant proteins. In order to express successfully a considerable amount of proteins, we had to create one genetic design for each of the peptides (Figure 1). The main part of this characterization was to prove that these peptides, individually or combined, have antimicrobial activity against both pathogens. </p></div>
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</ol>  
<div class="a">
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<br>
<p align="justify">Before even thinking of transforming any E. coli, we got to make sure we have a structured plan on what to do for it to work. The basic idea around the genetic device was having a strong promoter, such as the T7 phage one, plus an RBS, our genes of interest, and finally an efficient terminator, such as the rrnB T1 terminator. Later on, we started thinking ahead, realizing that a secretion signal and a way in which it could be purified might be needed. </p></div>
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<h4 align="justify"><b>Genetic Design</b></h4>
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<br>
 
<div class="row">
 
<div class="row">
 
   <div class="col-md-12">
 
   <div class="col-md-12">
       <img src="https://static.igem.org/mediawiki/2018/f/fc/T--Tec-Chihuahua--DiagramaIncompleto.png"></div></div>
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       <img src="https://static.igem.org/mediawiki/2018/b/bf/T--Tec-Chihuahua--Dise%C3%B1o.png"></div></div><br>
        <h4 align="center"><b>Figure 1: </b>First design created based on just expressing the proteins inside the bacteria.</h4>  
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<div class="a">
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<p align="justify">The need for an efficient peptide production led to the use of a strong promoter. The answer was the T7 promoter which possesses a high specificity to the T7 RNA polymerase; only DNA cloned downstream from T7 promoter can serve as a template for T7 RNA Polymerase-directed RNA synthesis<sup>1</sup>. The choice of this promoter was the first step to create the genetic design. The iGEM registry already had a T7 promoter, which also included an RBS <a href="http://parts.igem.org/Part:BBa_K525998">(BBa_K525998)</a> and this part was elected for the experimentation.</p></div>
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<br>
  
<div class="row">
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<div class="a">
  <div class="col-md-6">
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<p align="justify"><i>E. coli</i> BL21(DE3), a chassis specialized in high-level expression of recombinant proteins, harbors a prophage DE3 derived from a bacteriophage λ, which carries the T7 RNA polymerase gene under the control of the lacUV5 promoter.<sup>2</sup> Given that expression control was sought out, and that the peptide expression depended on the presence of T7 RNA polymerase, this strain was chosen. When IPTG is added, RNA polymerase is produced.
      <h3 align="center">Bronze</h3>
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</p></div>
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<br>
        <p align="justify"></p></div></div>
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      <h3 align="center">Silver</h3>
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        <div class="a">
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        <p align="justify"></p></div></div>
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</div>
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<h2 align="center">Final Product</h2>
 
 
<div class="a">
 
<div class="a">
<p align="justify">Even if the genes worked as they should and the proteins were expressed as we wanted them to, we still needed a way to eliminate inclusion bodies, get the proteins to the periplasmic space for an easier purification and adding a tag to assure the proteins could be purified. The solutions we came up with were 2 main additions. The first one consists of adding a secretion leader sequence, the pelB leader sequence. This secretion signal helps our proteins of interest get to the periplasmic space once they are synthesized by the bacteria, but it has another amazing feature, it prevents the inclusion bodies from forming. The second addition was to add a 6xHis-tag that allows us to purify the proteins easily. Information related to these additions is found in the <b>PARTS</b> section of our wiki. </p></div>
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<p align="justify">Looking for better expression of proteins, further evaluation of reported parts was carried; the pelB leader sequence found in the iGEM registry <a href="http://parts.igem.org/Part:BBa_J32015">(BBa_J32015)</a> was selected. It directs the protein to the bacterial periplasmic membrane and reduces or even eliminates inclusion body formation<sup>3</sup>.
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</p></div>
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<br>
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<div class="a">
 
<div class="a">
<p align="justify">After solving these problems we finally got to a final version of the plasmids we would use to transform our <i>E. coli</i>´s (Figure 2). This final version contained all the parts previously described for the proteins to be produced as planned. </p></div>
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<p align="justify">In order to be able to purify the peptides of interest, a 6X his-tag downstream the antimicrobial peptide sequence was considered, in addition an efficient terminator of transcription from the iGEM registry was selected <a href="http://parts.igem.org/Part:BBa_B0010">(BBa_B0010)</a>.
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</p></div>
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<br>
  
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<div class="a">
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<p align="justify">Finally the complete composite is obtained: (T7 promoter + RBS) + (PelB) + (antimicrobial peptide) + (6x His-Tag) + (T1 terminator)
 +
</p></div>
 +
<br>
 +
<h4 align="justify"><b>Experimental plan to test the genetic design</b></h4>
 +
 +
<ol>
 +
  <li>Synthesis of the complete composite, flanked by the iGEM prefix and suffix.</li>
 +
  <li>Digestion with EcoRI and PstI of both the synthesized composite and the pSB1C3 linearized vector.</li>
 +
  <li>Ligation of the pSB1C3 backbone to the composite.</li>
 +
  <li>Transformation of chemically competent BL21 (DE3) cells.</li>
 +
  <li>Plasmidic extraction of transformed BL21(DE3) cells.</li>
 +
  <li>Electrophoresis gel.</li>
 +
  <li>Induction with IPTG of BL21 (DE3) transformed cells.</li>
 +
  <li>Extraction of soluble and insoluble proteins.</li>
 +
  <li>Affinity chromatography purification.</li>
 +
  <li>SDS-PAGE and antibiograms.</li>
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 +
 +
</ol>   
 +
<br>
 +
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<h4 align="justify"><b>Final application</b></h4>
 
<div class="row">
 
<div class="row">
 
   <div class="col-md-12">
 
   <div class="col-md-12">
       <img src="https://static.igem.org/mediawiki/2018/3/32/T--Tec-Chihuahua--DiagramaCompleto.png"></div></div>
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       <img src="https://static.igem.org/mediawiki/2018/5/5a/T--Tec-Chihuahua--Hive.png"></div></div><br>
        <h4 align="center"><b>Figure 2: </b>Finished genetic design considering AMP extraction and purification. </h4>
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<h2 align="center">Prototype Design</h2>
 
 
<div class="a">
 
<div class="a">
<p align="justify">Once we have pure peptides we need to find out a way for them to reach safely to the larva without denaturalizing or losing its contemplated effect. The way we would do this is by microencapsulation protocols. In simple terms, the process would go as follows.</p></div>
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<p align="justify">The final application implements the proteins produced (after performing the antibiograms with different combinations of AMP's and selecting the best option) in a product that is suitable for beekeepers to apply to their hives.
 +
</p></div>
 +
<br>
 +
 
 
<div class="a">
 
<div class="a">
<p align="justify">The materials we will use are PLGA, a biodegradable copolymer whose degradation is pH dependent, and Dichloromethane, (DCM) used as a solvent for the PLGA. The solution both of these substances create is used as the oil phase in the microencapsulation process. The next step is getting our peptides in the form of a powder. Using a centrifuge we’ll combine both substances, the DCM/PLGA solution and the powdered peptides. This last combination is then passed through a membrane using pressurized nitrogen, thanks to its inert properties. After passing through the membrane tiny PLGA capsules containing our peptides are created. After letting the microcapsules dry out, they are ready to use and to be given to the bees. </p></div>
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<p align="justify">We knew that the peptides required a cover to extend their half-life, so methods for peptide protection were investigated, and thanks to the characteristics PLGA conferred to the covering, the usage of this copolymer was chosen. Poly Lactic-co-Glycolic Acid (PLGA) is biocompatible and a biodegradable FDA approved polymer that has been extensively studied as a delivery vehicle for drugs, proteins, and various other macromolecules<sup>4</sup>. PLGA nanoparticles are reported to control drug release, to protect the compounds from inactivation before reaching their site of action<sup>5</sup>, and they also exhibit a wide range of pH-dependent erosion times<sup>4</sup>.
<div class="a">
+
 
<p align="justify">Now the beekeeper has the microcapsules available, now what? They will be able to add them to the diet they commonly feed them with. It can either be added to a solid diet, which consists of powdered sugar or in a liquid form, which consists of a water and sugar mixture. In either case, these microcapsules won´t be affected nor will the peptides inside them, they won´t lose they antimicrobial activity, plus the microcapsule will keep them viable longer.<br></p></div>
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</div>
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</div>
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</p></div>
 +
<br>
 +
<div class="a"><p align="justify">The choice of the final method of application was possible thanks to our integrated human practices. <a href="https://2018.igem.org/Team:Tec-Chihuahua/Human_Practices#Basis">(You can see the exact trajectory on how the application method was changing in base to our human practices.)</a>
 +
 
 +
</p></div>
 +
<div class="a"><p align="justify"> After considering applying the nanocapsules in the bee bread, the idea of using powder or sprinkler to apply the product in the hive was contemplated, however studying the best option, it was finally concluded that the application method would consist in adding the nanoencapsulated peptides to the liquid food beekeepers give to their hives.
 +
 
 +
<h3>References</h3>
 +
 
 +
</p></div>
 +
<ol><li>Promega. (2018). T7 RNA Polymerase. Retrieved from https://worldwide.promega.com/products/cloning-and-dna-markers/molecular-biology-enzymes-and-reagents/t7-rna-polymerase/?catNum=P2075</li>
 +
<li>Promega. (2018). T7 RNA Polymerase. Retrieved from https://worldwide.promega.com/products/cloning-and-dna-markers/molecular-biology-enzymes-and-reagents/t7-rna-polymerase/?catNum=P2075</li>
 +
<li>Kovalskaya, N., & Hammond, R. W. (2009). Expression and functional characterization of the plant antimicrobial snakin-1 and defensin recombinant proteins. Protein Expression and Purification, 63(1), 12–17. doi:10.1016/j.pep.2008.08.013</li>
 +
<li>Makadia, H. & Siegel, S. (2011). Poly Lactic-co-Glycolic Acid (PLGA) as Biodegradable Controlled Drug Delivery Carrier. Retrieved from https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3347861/</li>
 +
<li>Teixeira, M., Alonso, M., Pinto, M. & Barbosa, C. (2004). Development and characterization of PLGA nanospheres and nanocapsules containing xanthone and 3-methoxyxanthone. Retrieved from https://pdfs.semanticscholar.org</li>
 +
</ol> <br><br>
 +
 
 +
</div></div>
 
</div>
 
</div>
  

Latest revision as of 03:35, 18 October 2018

Erwinions












Design Overview

Considerations

  1. In order to obtain the antimicrobial peptides of interest (apidaecin, abaecin, defensin 1 and defensin 2) and to be able to use them against both pathogens (Paenibacillus larvae and Melissococcus plutonius) an appropriate design is required; specialized in expressing heterologous proteins that are meant to be purified.

  2. Given that the peptides will be exposed to the hive's environment, it is essential to provide them protection which can increase their half-life.

Genetic Design



The need for an efficient peptide production led to the use of a strong promoter. The answer was the T7 promoter which possesses a high specificity to the T7 RNA polymerase; only DNA cloned downstream from T7 promoter can serve as a template for T7 RNA Polymerase-directed RNA synthesis1. The choice of this promoter was the first step to create the genetic design. The iGEM registry already had a T7 promoter, which also included an RBS (BBa_K525998) and this part was elected for the experimentation.


E. coli BL21(DE3), a chassis specialized in high-level expression of recombinant proteins, harbors a prophage DE3 derived from a bacteriophage λ, which carries the T7 RNA polymerase gene under the control of the lacUV5 promoter.2 Given that expression control was sought out, and that the peptide expression depended on the presence of T7 RNA polymerase, this strain was chosen. When IPTG is added, RNA polymerase is produced.


Looking for better expression of proteins, further evaluation of reported parts was carried; the pelB leader sequence found in the iGEM registry (BBa_J32015) was selected. It directs the protein to the bacterial periplasmic membrane and reduces or even eliminates inclusion body formation3.


In order to be able to purify the peptides of interest, a 6X his-tag downstream the antimicrobial peptide sequence was considered, in addition an efficient terminator of transcription from the iGEM registry was selected (BBa_B0010).


Finally the complete composite is obtained: (T7 promoter + RBS) + (PelB) + (antimicrobial peptide) + (6x His-Tag) + (T1 terminator)


Experimental plan to test the genetic design

  1. Synthesis of the complete composite, flanked by the iGEM prefix and suffix.
  2. Digestion with EcoRI and PstI of both the synthesized composite and the pSB1C3 linearized vector.
  3. Ligation of the pSB1C3 backbone to the composite.
  4. Transformation of chemically competent BL21 (DE3) cells.
  5. Plasmidic extraction of transformed BL21(DE3) cells.
  6. Electrophoresis gel.
  7. Induction with IPTG of BL21 (DE3) transformed cells.
  8. Extraction of soluble and insoluble proteins.
  9. Affinity chromatography purification.
  10. SDS-PAGE and antibiograms.

Final application


The final application implements the proteins produced (after performing the antibiograms with different combinations of AMP's and selecting the best option) in a product that is suitable for beekeepers to apply to their hives.


We knew that the peptides required a cover to extend their half-life, so methods for peptide protection were investigated, and thanks to the characteristics PLGA conferred to the covering, the usage of this copolymer was chosen. Poly Lactic-co-Glycolic Acid (PLGA) is biocompatible and a biodegradable FDA approved polymer that has been extensively studied as a delivery vehicle for drugs, proteins, and various other macromolecules4. PLGA nanoparticles are reported to control drug release, to protect the compounds from inactivation before reaching their site of action5, and they also exhibit a wide range of pH-dependent erosion times4.


The choice of the final method of application was possible thanks to our integrated human practices. (You can see the exact trajectory on how the application method was changing in base to our human practices.)

After considering applying the nanocapsules in the bee bread, the idea of using powder or sprinkler to apply the product in the hive was contemplated, however studying the best option, it was finally concluded that the application method would consist in adding the nanoencapsulated peptides to the liquid food beekeepers give to their hives.

References

  1. Promega. (2018). T7 RNA Polymerase. Retrieved from https://worldwide.promega.com/products/cloning-and-dna-markers/molecular-biology-enzymes-and-reagents/t7-rna-polymerase/?catNum=P2075
  2. Promega. (2018). T7 RNA Polymerase. Retrieved from https://worldwide.promega.com/products/cloning-and-dna-markers/molecular-biology-enzymes-and-reagents/t7-rna-polymerase/?catNum=P2075
  3. Kovalskaya, N., & Hammond, R. W. (2009). Expression and functional characterization of the plant antimicrobial snakin-1 and defensin recombinant proteins. Protein Expression and Purification, 63(1), 12–17. doi:10.1016/j.pep.2008.08.013
  4. Makadia, H. & Siegel, S. (2011). Poly Lactic-co-Glycolic Acid (PLGA) as Biodegradable Controlled Drug Delivery Carrier. Retrieved from https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3347861/
  5. Teixeira, M., Alonso, M., Pinto, M. & Barbosa, C. (2004). Development and characterization of PLGA nanospheres and nanocapsules containing xanthone and 3-methoxyxanthone. Retrieved from https://pdfs.semanticscholar.org