Team:Warsaw/Project

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                <li rel="whyThis"><a href="https://2012.igem.org/Team:Warsaw/Project#whyThis">why this?</a></li>
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                <li rel="steps"><a href="https://2012.igem.org/Team:Warsaw/Project#steps">steps</a></li>
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                <li rel="measurement"><a href="https://2012.igem.org/Team:Warsaw/Project#measurement">measurement</a></li></ul>
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<span><b>Why this project?</b><hr/></span><br clear="all" />
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<p>    <i>Escherichia coli</i>, which is by far the greatest model for iGEM projects, is a gram-negative bacterium. Because of that, the expression of some proteins, which came from gram-positive bacteria, is sometimes hard to achieve in <i>E. coli</i>. Even if we managed to express proteins from gram-positive bacteria in a gram-negative model, the proteins could for example have different localization in the cell and behave differently from how they did in the original cell they came from.</p><br />
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<p>   <i>Bacillus subtilis</i> is a great model of gram-positive bacteria; it was also used by some iGEM teams in previous years. We were curious, why only a few teams used that model. When we began searching partsregistry for some BioBricks especially for <i>Bacillus subtilis</i>, we realized that there is only a very limited number of them. It could be the reason why this model isn't so popular, but it is also the reason why we found working with <i>Bacillus subtilis</i> so interesting and at the same time so daring and challenging.</p><br />
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<p>  Of course, we wanted to make a functional project, but we also thought that it is a great challenge to work with another model than <i>E. coli</i>. We truly believed, that making some new BioBricks for <i>Bacillus subtilis</i>, even such basic ones like promoters and rbs, is important because it would help the iGEM community to work with this great model of gram-positive bacteria in the future.</p><br /><hr />
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<p>Our goal this year was to create a bacteria strain which could carry certain genes into eucaryotic cells. For safety reasons, and also to keep the work more coherent, we divided our task into two separate steps:</p><br />
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        <li><a href="https://2012.igem.org/Team:Warsaw">HOME</a></li>
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    <li><a href="https://2012.igem.org/Team:Warsaw/Project">PROJECT</a>
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                <li rel="Team"><a href="#">part: 1</a></li>
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<li><p>The first one was creating an 'invasive' <i>Bacillus subtilis</i> strain. <i>B. subtilis</i> is a non-pathogenic bacteria living peacefully in the soil. However, there are many bacteria species that have the ability to invade animal as well as human cells. We had an idea to create a plasmid for <i>B. subtilis</i> carrying listerolysin gene as to enable the bacteria to enter the eucaryotic cells just as <i>Listeria monocytogenes</i> from which the gene was taken does. <i>L. monocytogenes</i> is a dangerous pathogen; however, <i>B. subtilis</i> is a safe bacterium. With the lysis device installed in it, <i>B. subtilis</i> cells lyse after entering the eucaryotic cells. Since both of the bacteria are gram-positive, gene expression should undergo without obstructions. The plasmid also carries the GFP coding device which will help us to determine the success of our experiment. After the lysis of <i>B. subtilis</i> cells, GFP will be released and the measurement of its fluorescence will give us the idea of how the experiment worked out.
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<center><a href="https://static.igem.org/mediawiki/2012/a/ac/Masterschemat.png"><img src="https://static.igem.org/mediawiki/2012/a/ac/Masterschemat.png" width="400" alt="Invasion diagram" style="float:center;border:none;" /></center></a>
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<small><b>The mechanism of invasion of mammalian cells by bacteria leading to delivered gene expression</b><br clear="all" />
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1. Adhesion<br clear="all" />
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2. Internalization of the bacteria by the cell and subsequent phagocytosis<br clear="all" />
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3. Expression of listeriolysin present on the <i>B. subtilis</i> construct lyses the phagosomal membrane and bacteria escape from the phagosome <br clear="all" />
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4. Release of the vector due to the installed lysis device in the bacteria<br clear="all" />
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5. Replication and expression of the mammalian vector induced by oriP<br clear="all" /></small><br clear="all" />
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<li><p>The next step was creating a vector capable of replication and gene expression in mammalian cells. After the lysis of <i>B. subtilis</i> cells, the vector would be released directly into the cytoplasm, and then act just as mammalian DNA molecule. The EBNA1 gene from Epstein-Barr virus is essential for oriP to work properly. The vector would carry RFP, whose fluorescent activity measurement would prove the success of the presence, replication and expression of the vector within the mammalian cells. Due to safety measures, we never placed this plasmid in the bacteria cells. </p></li><br clear="all" /><br clear="all" />
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                <li rel="Team"><a href="#" >part: 1</a></li>
 
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<li><p>The last step was creating a shuttle vector which would be capable of replication and gene expression inside the eucaryotic cells. The vector will carry RFP coding device, and it will be RFP flourescence measurement which will confirm the presence of the vector in  mammalian cells and GFP in bacterial cells. However, due to safety reasons, we did not combine the two steps of our experiment. Each of the systems is tested separately, with all the safety precautions. In the future, when all the safety issues are resolved, these systems might be able to help a great deal in gene therapy. Delivering certain genes right into the malfunctioning cells would be a tremendous help in treatment of complicated diseases.  </p></li></ul>
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    1. If any one ensnare another, putting a ban upon him, but he can not prove it, then he that ensnared him shall be put to death.<br clear="all" />
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2. If any one bring an accusation against a man, and the accused go to the river and leap into the river, if he sink in the river his accuser shall take possession of his house. But if the river prove that the accused is not guilty, and he escape unhurt, then he who had brought the accusation shall be put to death, while he who leaped into the river shall take possession of the house that had belonged to his accuser. <br clear="all" />
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3. If any one bring an accusation of any crime before the elders, and does not prove what he has charged, he shall, if it be a capital offense charged, be put to death. <br clear="all" />
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4. If he satisfy the elders to impose a fine of grain or money, he shall receive the fine that the action produces. <br clear="all" />
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5. If a judge try a case, reach a decision, and present his judgment in writing; if later error shall appear in his decision, and it be through his own fault, then he shall pay twelve times the fine set by him in the case, and he shall be publicly removed from the judge's bench, and never again shall he sit there to render judgement. <br clear="all" />
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6. If any one steal the property of a temple or of the court, he shall be put to death, and also the one who receives the stolen thing from him shall be put to death. <br clear="all" />
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7. If any one buy from the son or the slave of another man, without witnesses or a contract, silver or gold, a male or female slave, an ox or a sheep, an ass or anything, or if he take it in charge, he is considered a thief and shall be put to death. <br clear="all" />8. If any one steal cattle or sheep, or an ass, or a pig or a goat, if it belong to a god or to the court, the thief shall pay thirtyfold therefor; if they belonged to a freed man of the king he shall pay tenfold; if the thief has nothing with which to pay he shall be put to death. <br clear="all" />
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9. If any one lose an article, and find it in the possession of another: if the person in whose possession the thing is found say "A merchant sold it to me, I paid for it before witnesses," and if the owner of the thing say, "I will bring witnesses who know my property," then shall the purchaser bring the merchant who sold it to him, and the witnesses before whom he bought it, and the owner shall bring witnesses who can identify his property. The judge shall examine their testimony -- both of the witnesses before whom the price was paid, and of the witnesses who identify the lost article on oath. The merchant is then proved to be a thief and shall be put to death. The owner of the lost article receives his property, and he who bought it receives the money he paid from the estate of the merchant. <br clear="all" />
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10. If the purchaser does not bring the merchant and the witnesses before whom he bought the article, but its owner bring witnesses who identify it, then the buyer is the thief and shall be put to death, and the owner receives the lost article.<br clear="all" />
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    11. If the owner do not bring witnesses to identify the lost article, he is an evil-doer, he has traduced, and shall be put to death. <br clear="all" />
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12. If the witnesses be not at hand, then shall the judge set a limit, at the expiration of six months. If his witnesses have not appeared within the six months, he is an evil-doer, and shall bear the fine of the pending case. <br clear="all" />
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14. If any one steal the minor son of another, he shall be put to death. <br clear="all" />
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15. If any one take a male or female slave of the court, or a male or female slave of a freed man, outside the city gates, he shall be put to death. <br clear="all" />
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16. If any one receive into his house a runaway male or female slave of the court, or of a freedman, and does not bring it out at the public proclamation of the major domus, the master of the house shall be put to death. <br clear="all" />
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17. If any one find runaway male or female slaves in the open country and bring them to their masters, the master of the slaves shall pay him two shekels of silver. <br clear="all" />
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18. If the slave will not give the name of the master, the finder shall bring him to the palace; a further investigation must follow, and the slave shall be returned to his master. <br clear="all" />
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19. If he hold the slaves in his house, and they are caught there, he shall be put to death. <br clear="all" />
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20. If the slave that he caught run away from him, then shall he swear to the owners of the slave, and he is free of all blame. <br clear="all" />
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<b>First step</b><hr /><br clear="all" />
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<p>    In the first step of our project we designed a few BioBricks adapted for <i>Bacillus subtilis</i>. We decided, that even if some basic parts are available in partsregistry, we would create a few more to expand the amount of BioBricks for this bacterium. Therefore, we designed:</p><br />
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  <li>     Two new promoters for <i>Bacillus subtilis</i></li>
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  <li>    Three new RBSes for <i>Bacillus subtilis</i></li>
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  <li>      One terminator for <i>Bacillus subtilis</i></li>
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<p>  We believed that these parts will be useful for creating constructs designed for <i> Bacillus subtilis</i> in this year's project of ours and in the future projects based on this bacterium.<br />
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We performed all designing work in Clone Manager software, which we found easy and useful.</p><br />
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<p>    Then, we designed parts especially devoted to our project. Our goal was to create two main constructs:
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the first one should allow <i>Bacillus subtilis</i> to enter mammalian cell. To give <i>Bacillus</i> this ability, we decided to use listeriolysin, a protein naturally existing in <i>Listeria monocytogenes</i>. To confirm that <i>Bacillus</i> entered the mammalian cell we used GFP protein, which would give us a fluorescent signal, easy to notice by using fluorescent microscopy.
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We designed our construct like this:</p><br />
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<center><a href="https://static.igem.org/mediawiki/2012/5/50/Bacillusowy.png"><img src="https://static.igem.org/mediawiki/2012/5/50/Bacillusowy.png" width="300" alt="Bacillus plasmid" style="float:center;border:none;" /></a></center>
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<p>  The listeriolysin gene was taken from the <a href="http://partsregistry.org/Part:BBa_K177026">BioBrick BBa_K177026</a>. Listeriolysin is a protein considered to be the virulence factor of <i>Listeria monocytogenes</i>, because of its pivotal role is the process of pathogenesis of these bacteria. Since both <i>L. monocytogenes</i> and <i>B. subtilis</i> are gram-positive bacteria, we believed that the expression of listeriolysin will be much better in <i> B. subtilis</i> than in the gram-negative <i>E. coli</i>.  </p><br />
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     Our plan was to test all our basic parts in this construct, by creating few parallel versions, using different promoters and RBSes and choose the best version.<br /><br clear="all" />
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<p>While doing that, we were also preparing construct which could replicate and be expressed in both bacterial (<i>E. coli</i>) and mammalian cell. We based our plasmid on pSB1A3 plasmid backbone and ligated into it the <a href="http://partsregistry.org/wiki/index.php?title=Part:BBa_J52034">CMV mammalian promoter</a> (designed and sent to us by Slovenia iGEM Team) with mammalian RBSes (we wanted to test both <a href="http://partsregistry.org/Part:BBa_J63003">J63003</a> and <a href="http://partsregistry.org/Part:BBa_K165002">K165002</a> Kozak sequence) and <a href="http://partsregistry.org/wiki/index.php?title=Part:BBa_J06504">RFP</a> (to confirm expression in mammalian cells). To confirm expression in <i>E. coli</i> cells, we used the construct with <a href="http://partsregistry.org/Part:BBa_I746916">SF-GFP</a></p><br />
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<p>  Another main construct was devoted for using directly in mammalian cells. It was based on BioBricks from partregistry with our new part containing oriP. To allow the plasmid to replicate in a mammalian cell, we prepared a BioBrick containing oriP and coding sequence of EBNA1 gene (which is essential for oriP to work properly) from Epstein-Barr virus. We got the sequence of oriP from <a href="http://tools.invitrogen.com/content/sfs/manuals/pcep4_man.pdf">pCep4</a> commercial plasmid available from Invitrogen. We had been trying to receive this BioBrick using PCR method.</p><br />
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<p>    Unfortunately, the original oriP sequence had a restriction site of SpeI enzyme in the middle of the sequence. We decided to amplify this in two separate parts, because in this situation we could modify enzyme site by placing it in the middle of the primer for one of the parts. After amplification, we planned to ligate these two parts into one full BioBrick. Unluckily, we didn't manage to fulfill our plan. When we realized that we fail with preparing this part that way, we tried to get this BioBrick even with this illegal restriction site and just clone it without using SpeI enzyme. After several attempts, we got this BioBrick and ligated it with the construct containing CMV, RBS and RFP. Unfortunately when we received it, we were already running out of time and didn't manage to confirm the sequence of this part and test it in mammalian cells.</p><br />
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<p>    The design of the constructs looked like this:</p>
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<a href="https://static.igem.org/mediawiki/2012/e/eb/Mammalian.png"><img src="https://static.igem.org/mediawiki/2012/e/eb/Mammalian.png" width="300" alt="Mammalian plasmid" style="float:center;border:none;" /></a>
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<a href="https://static.igem.org/mediawiki/2012/a/aa/Shuttle.png"><img src="https://static.igem.org/mediawiki/2012/a/aa/Shuttle.png" width="300" alt="Shuttle vector" style="float:right;border:none;" /></a>
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<b>Second step</b><hr /><br clear="all" />
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Then we entered the wet lab and started preparing our BioBricks made of DNA, not only pixels on the computer screen ;)<br />
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We decided to achieve our promoters, RBS and terminator parts with method called in our laboratory “PCR without template”. It goes like this:<br />
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  <li>  For each part we designed two starters that covered each other in about 20bp on 3' ends</li>
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  <li>    Each primer had prefix or suffix (depending on the primer) on its 5' end</li>
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  <li>    Then we prepared PCR reaction mixture</li>
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  <li>  We used Taq polymerase MasterMix and primers in different concentrations</li>
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  <li>    We didn't add any DNA template</li>
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  <li>    We calculated the annealing temperature by oligocalculator </li>
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  <li>    For first three cycles of PCR reaction temperature was calculated for primer without overhang</li>
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  <li>    Then for thirty more cycles temperature of annealing was calculated for the whole long primer with overhang – that is because from this moment there was enough product of the reaction in the reaction mix to become a template for the next cycles</li>
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  <li>    And that's it!</li></ul>
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<center><a href="https://static.igem.org/mediawiki/2012/8/82/PCR_3.png"><img src="https://static.igem.org/mediawiki/2012/8/82/PCR_3.png" width="300" alt="PCR without template" style="float:center;border:none;" /></a></center>
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<p>Then we cloned our PCR product into pJet plasmid, using special <a href="http://www.fermentas.com/en/products/all/molecular-cloning/kits/k123-clonejet-pcr-cloning">kit for cloning PCR products</a>, and transformed with it <i>E. coli</i> TOP10. After isolation of the plasmid, we confirmed the sequence of received product by DNA sequencing (traditional Sanger sequencing). From this step, our parts were ready to digest and clone with procedures recommended by iGEM :)</p></br>
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<p>We managed to optimize reaction conditions and received all of ours parts by PCR reaction. Unfortunately, then we faced some problems and weren't as successful as we hoped. We didn't manage to confirm all our products' sequences by DNA sequencing. Finally we received a full BioBrick part:</p><br />
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  <li><a href="http://partsregistry.org/Part:BBa_K780003">Promoter</a></li>
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  <li>Two RBS, <a href="http://partsregistry.org/Part:BBa_K780001">BBa_K780001</a> and <a href="http://partsregistry.org/Part:BBa_K780002">BBa_K780002</a></li>
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  <li><a href="http://partsregistry.org/Part:BBa_K780000">Terminator</a></li></ul>
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<b>Third step</b><hr /><br clear="all" />
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<p>    As soon as we received our first full and confirmed BioBrick part, we started preparing our construct for <i>Bacillus subtilis</i>. We began from ligation of this part with GFP, because that would allow us to check if our promoter and RBSes work. We used 3A assembly procedure, which we found on iGEM website. We followed the set pattern:</p><br clear="all"/>
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<center><a href="https://static.igem.org/mediawiki/2012/e/e0/3a_3.png"><img src="https://static.igem.org/mediawiki/2012/e/e0/3a_3.png" width="400" alt="3a diagram" style="float:center;border:none;" /></center></a>
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<br/><br clear="all"/>
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We knew that we had still a long way ahead to receive our full construct in <i>Bacillus subtilis</i>, and so we decided to start measuring our parts in <i>E. Coli</i> for the start. Measurement in <i>E. Coli</i> is the most common standard of measurement in iGEM community. We predicted that our parts will be working also in <i>E. coli</i>, but with lower efficiency than in <i>Bacillus subtilis</i>.
<br clear="all" /><br clear="all" />
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  21. If any one break a hole into a house (break in to steal), he shall be put to death before that hole and be buried. <br clear="all" />
 
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22. If any one is committing a robbery and is caught, then he shall be put to death. <br clear="all" />
 
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23. If the robber is not caught, then shall he who was robbed claim under oath the amount of his loss; then shall the community, and ... on whose ground and territory and in whose domain it was compensate him for the goods stolen. <br clear="all" />
 
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24. If persons are stolen, then shall the community and ... pay one mina of silver to their relatives. <br clear="all" />
 
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25. If fire break out in a house, and some one who comes to put it out cast his eye upon the property of the owner of the house, and take the property of the master of the house, he shall be thrown into that self-same fire. <br clear="all" />
 
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26. If a chieftain or a man (common soldier), who has been ordered to go upon the king's highway for war does not go, but hires a mercenary, if he withholds the compensation, then shall this officer or man be put to death, and he who represented him shall take possession of his house. <br clear="all" />
 
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27. If a chieftain or man be caught in the misfortune of the king (captured in battle), and if his fields and garden be given to another and he take possession, if he return and reaches his place, his field and garden shall be returned to him, he shall take it over again. <br clear="all" />
 
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28. If a chieftain or a man be caught in the misfortune of a king, if his son is able to enter into possession, then the field and garden shall be given to him, he shall take over the fee of his father. <br clear="all" />
 
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29. If his son is still young, and can not take possession, a third of the field and garden shall be given to his mother, and she shall bring him up. <br clear="all" />
 
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30. If a chieftain or a man leave his house, garden, and field and hires it out, and some one else takes possession of his house, garden, and field and uses it for three years: if the first owner return and claims his house, garden, and field, it shall not be given to him, but he who has taken possession of it and used it shall continue to use it. <br clear="all" />
 
 +
We successfully measured our RBS37 (BBa_K780002) comparing to RBS Bba_B0034, and we obtained result 10,13%.<br clear="all" /><br clear="all" />
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 +
We also tried to measure our other parts, but we didn't manage to put together full constructs with them, so the measurement was impossible.</p></br> <br /><br clear="all"/><br clear="all"/>
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<b>Step four</b><hr /><br clear="all" />
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<p>    When we had a ready construct consisting of promoter + RBS + GFP we cloned it on <a href="http://partsregistry.org/Part:BBa_I742103">pTG262 vector</a>. This plasmid, which was constructed and sent to us by Edinburgh iGEM Team, is the only autoreplicating plasmid meeting iGEM standards designed for <i>Bacillus subtilis</i>. We managed to successfully clone our insert to the vector, what we confirmed by digesting with EcoRI and PstI and gel electrophoresis of the vector and insert.<br />
 +
In the same time we had been improving our constructs by adding the terminator to them.</p><br />
 +
<br clear="all" />
 +
 +
<b>Step five</b><hr /><br /><br clear="all" />
 +
 +
<p>Finally, in order to confirm the functionality of our construct, we intended to make series of measurements using fluorometry. We tried to transform two different strains of <i>Bacillus subtilis</i>: 168 and 979 and used two different transforming procedures which you can see <a href="https://static.igem.org/mediawiki/2012/3/32/Transformation_Bsu.pdf">here</a> and <a href=" http://wiki.biol.uw.edu.pl/t/img_auth.php/b/b5/Bacillus_subtilis_competent_cells.pdf">here</a>.</p><br /><br clear="all" />
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 +
<p>First of all, we tried to select our transformants on plates with LB agar with chloramphenicol. Unfortunately, after several trials we didn't received desirable colonies. Bacteria that grow on dishes with chloramphenicol do not carry our plasmid. We thought that something could be wrong with the concentration of the antibiotic, so we tried few different ones, but none worked. Then, we tried to select bacteria using neomycin resistance, since pTG626 plasmid also carries a resistance gene for this antibiotic. Unfortunately, it didn’t work either.</p><br /><br clear="all" />
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<p> - Bielecki J., Youngman P., Connelly P., Portnoy D., '<i>Bacillus subtilis expressing a haemolysin gene from Listeria monocytogenes can grow in mammalian cells.</i>', Nature, 1990. </p> <br clear="all" />
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<p> - Stewart C. et all, '<i> Genes and Regulatory Sites of the "Host Takeover Module" in the Terminal Redundancy of Bacillus subtilis Bacteriophage SPO1.'</i>, Virology, 1998.</p><br clear="all" />
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<b>Measurement</b><hr/><br clear="all" /><br clear="all" />
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<b>General info</b><br clear="all" /><br clear="all" />
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We designed two new RBSes for <i>Bacillus subtilis</i>. We managed to successfully measure one of them comparing to RBS BBa_B0034. Our measurement was performed in <i>E. coli</i>. Our reasults are presented below.<br clear="all" /><br clear="all" />
 +
 
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We also planned to measure our part in <i>Bacillus subtilis</i>, but unfortunately we didn't manage to successfully prepare and transform our measuring construct into that bacteria.<br clear="all" /><br clear="all" />
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<b>Sample preparation</b><br clear="all" /><br clear="all" />
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To measure the fluorescence of samples of 3 milliliters of LB with KAN were inoculated with a colony from the plate. Cultures were vigorously shaken in 37°C overnight. The next step was to centrifuge 1,5 milliliters of liquid culture in an 1,5 ml tube. The pellet was resuspended in 200 microliters of RF. Finally, the prepared samples were placed in the fluorimeter plate. We used Corning 96 deep well plates with clear UV transparent bottom. Measurements were carried out using Tecan HS2000 pro fluorimeter with bottom read mode and using active gain optimization function.<br clear="all" /><br clear="all" />
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<tr><th>Wavelength value</th> <th> GFP </th> </tr>
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<tr><td> Excitation [nm]</td><td> 488 </td> </tr>
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<tr><td> Emission [nm]  </td><td> 509 </td> </tr>
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<b> Results</b><br clear="all" /><br clear="all" /><br clear="all" />
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Latest revision as of 00:53, 27 September 2012

Warsaw Team






Why this project?

Escherichia coli, which is by far the greatest model for iGEM projects, is a gram-negative bacterium. Because of that, the expression of some proteins, which came from gram-positive bacteria, is sometimes hard to achieve in E. coli. Even if we managed to express proteins from gram-positive bacteria in a gram-negative model, the proteins could for example have different localization in the cell and behave differently from how they did in the original cell they came from.


Bacillus subtilis is a great model of gram-positive bacteria; it was also used by some iGEM teams in previous years. We were curious, why only a few teams used that model. When we began searching partsregistry for some BioBricks especially for Bacillus subtilis, we realized that there is only a very limited number of them. It could be the reason why this model isn't so popular, but it is also the reason why we found working with Bacillus subtilis so interesting and at the same time so daring and challenging.


Of course, we wanted to make a functional project, but we also thought that it is a great challenge to work with another model than E. coli. We truly believed, that making some new BioBricks for Bacillus subtilis, even such basic ones like promoters and rbs, is important because it would help the iGEM community to work with this great model of gram-positive bacteria in the future.




Our goal this year was to create a bacteria strain which could carry certain genes into eucaryotic cells. For safety reasons, and also to keep the work more coherent, we divided our task into two separate steps:


  • The first one was creating an 'invasive' Bacillus subtilis strain. B. subtilis is a non-pathogenic bacteria living peacefully in the soil. However, there are many bacteria species that have the ability to invade animal as well as human cells. We had an idea to create a plasmid for B. subtilis carrying listerolysin gene as to enable the bacteria to enter the eucaryotic cells just as Listeria monocytogenes from which the gene was taken does. L. monocytogenes is a dangerous pathogen; however, B. subtilis is a safe bacterium. With the lysis device installed in it, B. subtilis cells lyse after entering the eucaryotic cells. Since both of the bacteria are gram-positive, gene expression should undergo without obstructions. The plasmid also carries the GFP coding device which will help us to determine the success of our experiment. After the lysis of B. subtilis cells, GFP will be released and the measurement of its fluorescence will give us the idea of how the experiment worked out.



  • Invasion diagram


    The mechanism of invasion of mammalian cells by bacteria leading to delivered gene expression
    1. Adhesion
    2. Internalization of the bacteria by the cell and subsequent phagocytosis
    3. Expression of listeriolysin present on the B. subtilis construct lyses the phagosomal membrane and bacteria escape from the phagosome
    4. Release of the vector due to the installed lysis device in the bacteria
    5. Replication and expression of the mammalian vector induced by oriP


  • The next step was creating a vector capable of replication and gene expression in mammalian cells. After the lysis of B. subtilis cells, the vector would be released directly into the cytoplasm, and then act just as mammalian DNA molecule. The EBNA1 gene from Epstein-Barr virus is essential for oriP to work properly. The vector would carry RFP, whose fluorescent activity measurement would prove the success of the presence, replication and expression of the vector within the mammalian cells. Due to safety measures, we never placed this plasmid in the bacteria cells.



  • The last step was creating a shuttle vector which would be capable of replication and gene expression inside the eucaryotic cells. The vector will carry RFP coding device, and it will be RFP flourescence measurement which will confirm the presence of the vector in mammalian cells and GFP in bacterial cells. However, due to safety reasons, we did not combine the two steps of our experiment. Each of the systems is tested separately, with all the safety precautions. In the future, when all the safety issues are resolved, these systems might be able to help a great deal in gene therapy. Delivering certain genes right into the malfunctioning cells would be a tremendous help in treatment of complicated diseases.




First step

In the first step of our project we designed a few BioBricks adapted for Bacillus subtilis. We decided, that even if some basic parts are available in partsregistry, we would create a few more to expand the amount of BioBricks for this bacterium. Therefore, we designed:


  • Two new promoters for Bacillus subtilis
  • Three new RBSes for Bacillus subtilis
  • One terminator for Bacillus subtilis

We believed that these parts will be useful for creating constructs designed for Bacillus subtilis in this year's project of ours and in the future projects based on this bacterium.
We performed all designing work in Clone Manager software, which we found easy and useful.


Then, we designed parts especially devoted to our project. Our goal was to create two main constructs: the first one should allow Bacillus subtilis to enter mammalian cell. To give Bacillus this ability, we decided to use listeriolysin, a protein naturally existing in Listeria monocytogenes. To confirm that Bacillus entered the mammalian cell we used GFP protein, which would give us a fluorescent signal, easy to notice by using fluorescent microscopy. We designed our construct like this:


Bacillus plasmid


The listeriolysin gene was taken from the BioBrick BBa_K177026. Listeriolysin is a protein considered to be the virulence factor of Listeria monocytogenes, because of its pivotal role is the process of pathogenesis of these bacteria. Since both L. monocytogenes and B. subtilis are gram-positive bacteria, we believed that the expression of listeriolysin will be much better in B. subtilis than in the gram-negative E. coli.


Our plan was to test all our basic parts in this construct, by creating few parallel versions, using different promoters and RBSes and choose the best version.

While doing that, we were also preparing construct which could replicate and be expressed in both bacterial (E. coli) and mammalian cell. We based our plasmid on pSB1A3 plasmid backbone and ligated into it the CMV mammalian promoter (designed and sent to us by Slovenia iGEM Team) with mammalian RBSes (we wanted to test both J63003 and K165002 Kozak sequence) and RFP (to confirm expression in mammalian cells). To confirm expression in E. coli cells, we used the construct with SF-GFP


Another main construct was devoted for using directly in mammalian cells. It was based on BioBricks from partregistry with our new part containing oriP. To allow the plasmid to replicate in a mammalian cell, we prepared a BioBrick containing oriP and coding sequence of EBNA1 gene (which is essential for oriP to work properly) from Epstein-Barr virus. We got the sequence of oriP from pCep4 commercial plasmid available from Invitrogen. We had been trying to receive this BioBrick using PCR method.


Unfortunately, the original oriP sequence had a restriction site of SpeI enzyme in the middle of the sequence. We decided to amplify this in two separate parts, because in this situation we could modify enzyme site by placing it in the middle of the primer for one of the parts. After amplification, we planned to ligate these two parts into one full BioBrick. Unluckily, we didn't manage to fulfill our plan. When we realized that we fail with preparing this part that way, we tried to get this BioBrick even with this illegal restriction site and just clone it without using SpeI enzyme. After several attempts, we got this BioBrick and ligated it with the construct containing CMV, RBS and RFP. Unfortunately when we received it, we were already running out of time and didn't manage to confirm the sequence of this part and test it in mammalian cells.


The design of the constructs looked like this:


Mammalian plasmid Shuttle vector


Second step

Then we entered the wet lab and started preparing our BioBricks made of DNA, not only pixels on the computer screen ;)
We decided to achieve our promoters, RBS and terminator parts with method called in our laboratory “PCR without template”. It goes like this:

  • For each part we designed two starters that covered each other in about 20bp on 3' ends
  • Each primer had prefix or suffix (depending on the primer) on its 5' end
  • Then we prepared PCR reaction mixture
  • We used Taq polymerase MasterMix and primers in different concentrations
  • We didn't add any DNA template
  • We calculated the annealing temperature by oligocalculator
  • For first three cycles of PCR reaction temperature was calculated for primer without overhang
  • Then for thirty more cycles temperature of annealing was calculated for the whole long primer with overhang – that is because from this moment there was enough product of the reaction in the reaction mix to become a template for the next cycles
  • And that's it!

PCR without template



Then we cloned our PCR product into pJet plasmid, using special kit for cloning PCR products, and transformed with it E. coli TOP10. After isolation of the plasmid, we confirmed the sequence of received product by DNA sequencing (traditional Sanger sequencing). From this step, our parts were ready to digest and clone with procedures recommended by iGEM :)


We managed to optimize reaction conditions and received all of ours parts by PCR reaction. Unfortunately, then we faced some problems and weren't as successful as we hoped. We didn't manage to confirm all our products' sequences by DNA sequencing. Finally we received a full BioBrick part:



Third step

As soon as we received our first full and confirmed BioBrick part, we started preparing our construct for Bacillus subtilis. We began from ligation of this part with GFP, because that would allow us to check if our promoter and RBSes work. We used 3A assembly procedure, which we found on iGEM website. We followed the set pattern:


3a diagram


We knew that we had still a long way ahead to receive our full construct in Bacillus subtilis, and so we decided to start measuring our parts in E. Coli for the start. Measurement in E. Coli is the most common standard of measurement in iGEM community. We predicted that our parts will be working also in E. coli, but with lower efficiency than in Bacillus subtilis.

We successfully measured our RBS37 (BBa_K780002) comparing to RBS Bba_B0034, and we obtained result 10,13%.

We also tried to measure our other parts, but we didn't manage to put together full constructs with them, so the measurement was impossible.





Step four

When we had a ready construct consisting of promoter + RBS + GFP we cloned it on pTG262 vector. This plasmid, which was constructed and sent to us by Edinburgh iGEM Team, is the only autoreplicating plasmid meeting iGEM standards designed for Bacillus subtilis. We managed to successfully clone our insert to the vector, what we confirmed by digesting with EcoRI and PstI and gel electrophoresis of the vector and insert.
In the same time we had been improving our constructs by adding the terminator to them.



Step five


Finally, in order to confirm the functionality of our construct, we intended to make series of measurements using fluorometry. We tried to transform two different strains of Bacillus subtilis: 168 and 979 and used two different transforming procedures which you can see here and here.



First of all, we tried to select our transformants on plates with LB agar with chloramphenicol. Unfortunately, after several trials we didn't received desirable colonies. Bacteria that grow on dishes with chloramphenicol do not carry our plasmid. We thought that something could be wrong with the concentration of the antibiotic, so we tried few different ones, but none worked. Then, we tried to select bacteria using neomycin resistance, since pTG626 plasmid also carries a resistance gene for this antibiotic. Unfortunately, it didn’t work either.





- Bielecki J., Youngman P., Connelly P., Portnoy D., 'Bacillus subtilis expressing a haemolysin gene from Listeria monocytogenes can grow in mammalian cells.', Nature, 1990.


- Stewart C. et all, ' Genes and Regulatory Sites of the "Host Takeover Module" in the Terminal Redundancy of Bacillus subtilis Bacteriophage SPO1.', Virology, 1998.



Measurement


General info

We designed two new RBSes for Bacillus subtilis. We managed to successfully measure one of them comparing to RBS BBa_B0034. Our measurement was performed in E. coli. Our reasults are presented below.

We also planned to measure our part in Bacillus subtilis, but unfortunately we didn't manage to successfully prepare and transform our measuring construct into that bacteria.

Sample preparation

To measure the fluorescence of samples of 3 milliliters of LB with KAN were inoculated with a colony from the plate. Cultures were vigorously shaken in 37°C overnight. The next step was to centrifuge 1,5 milliliters of liquid culture in an 1,5 ml tube. The pellet was resuspended in 200 microliters of RF. Finally, the prepared samples were placed in the fluorimeter plate. We used Corning 96 deep well plates with clear UV transparent bottom. Measurements were carried out using Tecan HS2000 pro fluorimeter with bottom read mode and using active gain optimization function.

Wavelength value GFP
Excitation [nm] 488
Emission [nm] 509


Results