Team:Paris Bettencourt/Project/Infiltrate

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     <img src="https://static.igem.org/mediawiki/2013/6/6c/PB_infiltrate.gif" style="height:80px;margin-top:-10px" />
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     <img src="https://static.igem.org/mediawiki/2013/3/3a/PB_logoParis.gif" width="122px" style="position:absolute;top:40px;right:30px;"/>
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    INFILTRATE
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  <img src="https://static.igem.org/mediawiki/2013/0/00/PB_infiltratetitle.png" style="margin-bottom:15px"/>
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      <h2>Background</h2>
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      <p>Latent tuberculosis persists inside macrophages, where it is partially protected from both the host immune system and conventional antibiotics.</p>
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    </div>
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    <div class="results">
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      <h2>Results</h2>
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      <ul>
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        <li>We expressed the enzyme Trehalose Dimycolate Hydrolase (TDMH) in <i>E. coli</i> and showed that it is highly toxic to mycobacteria in culture.</li>
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        <li>We expressed the listeriolyin O (LLO) gene in <i>E. coli</i> and showed that it is capable of entering the macrophage cytosol.</li>
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        <li>We co-infected macrophages with both mycobacteria and our engineered <i>E. coli</i> to characterize the resulting phagocytosis and killing.</li>
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        <li> We measured the effect of a range of pH (from 3 to 8,8) on <i>M. smegmatis</i> and the TDMH enzyme activity.</li>
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      </ul>
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    </div>
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    <div class="biocriks">
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      <h2>BioBricks</h2>
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      <ol>
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        <li><a href="http://parts.igem.org/Part:BBa_K1137008" target="_blank">BBa_K1137008 (TDMH)</a></li>
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      </ol>
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    </div>
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    <div style="clear: both;"></div>
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    <div class="aims">
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      <h2>Aim</h2>
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      <p>To create an <i>E. coli</i> strain capable of entering the macrophage cytosol and delivering a lytic enzyme to kill mycobacteria.</p>
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    </div>
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    <a href="#Introduction">
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      <div class="hlink">
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<h2>Skip to Introduction</h2>
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      </div>
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    </a>
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    <a href="#Design">
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      <div class="hlink">
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<h2>Skip to Design</h2>
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      </div>
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    </a>
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    <a href="#Killing">
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      <div class="hlink">
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<h2>Skip to Killing Assay</h2>
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      </div>
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    </a>
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    <a href="#Macrophages">
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      <div class="hlink" style="margin-right:0px">
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<h2>Skip to Drug Delivery</h2>
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      </div>
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    </a>
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  </div>
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    <div id="Introduction"></div>
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    <h2>Introduction</h2>
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    <div class="leftparagraph">
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      <p> &nbsp;&nbsp;
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<i>Mycobacterium tuberculosis</i> (Mtb), the bacterium responsible for tuberculosis (TB), spreads by aerosol and infects its host through the airways. The bacterium is phagocytosed by macrophages in the lung, yet often evades death in the lysosome. Mtb can persist for years or even decades inside macrophages by inhibiting phagosome/lysosome fusion and supressing the normal acidification of the lysosome.</p>
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      <p>An efficient treatment for persistent TB must enter infected macrophages and kill the pathogen there. In our system, <i>E. coli</i> is both the vector and the therapeutic agent agent by expressing the listeriolyin O gene LLO to enter macrophages and TDMH to kill mycobacteria.  Additionally we thought about how we could deliver the E. coli to the lungs and decided that the most effective way would be through an inhaler.
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      </p>
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    </div>
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    <div class="rightparagraph">
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      <div style="width:90%;margin-left:5%;border:2px solid;">
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<h4>&nbsp;BOX 1: Why is it difficult to treat tuberculosis?</h4>
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<ul style="width:90%">
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  <li>Mtb can survive and replicate for years inside the macrophages by supressing the normal process of phagocytosis.</li>
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  <li>The cell wall of <i>M. tuberculosis</i> is thick, waxy and rich in mycolic acids. It it difficult to penetrate with a small-molecule drug.</li>
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  <li>The pathogen grows very slowly inside macrophages. Most conventional antibiotics target processes like DNA replication that are specific to growing cells.</li>
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</ul>
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    <center><a href="https://static.igem.org/mediawiki/2013/1/1d/PB_inhalorinfiltrate.png" target="_blank"><img src="https://static.igem.org/mediawiki/2013/1/1d/PB_inhalorinfiltrate.png" width="1100"/></a></center>
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<br><br>
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    <div id="Design"></div>
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    <h2>TDMH and the mycobacterial cell wall</h2>
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    <div class="leftparagraph">
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      <p>&nbsp;&nbsp;Mycobacterium species share a characteristic cell wall: thick, waxy, hydrophobic, and rich in mycolic acids. The low permeability of the envelope to hydrophilic solutes contributes to the intrinsic drug tolerance in mycobacteria.</p>
       <p>
       <p>
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<b>
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&nbsp;&nbsp;Trehalose Dimycolate Hydrolase (TDMH) is a cutinase-like serine esterase that triggers rapid lysis of the mycobacterial cell wall by degrading the mycolate layer. The enzyme was first isolated from <i>Mycobacterium smegmatis</i> and subsequently shown to hydrolyze purified TDM from various mycobacterial species. Exposure to TDMH triggers an immediate release of free mycolic acids, ultimately leading to lysis of many mycobacteria including Mtb (Yang et al. 2012).
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Bacterial vectors offer a biological route to gene and protein delivery to cells such as macrophages. We want to investigate the potential use of <i>Escherichia coli</i> as a drug delivery system  to kill <i>Mycobacerium tuberculosis</i> inside of the infected macrophages. In our system <i>E. coli</i> contains two expression systems enabeling Listeriolysin O (LLO) and Trechalose Dimycolate Hydrolase (TDMH) production. Subsequent to phagocytosis the <i>E. coli</i> are degraded within the phagosomes, causing the release of LLO and TDMH from the bacteria. LLO acts by forming large pores in the phagosomal membrane, thus releasing TDMH into the cytosol. TDMH can then trigger lysis of the mycobacterial cell wall.
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      </p>
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</p> <br>
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    <div class="rightparagraph">
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<p>
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      <p>&nbsp;&nbsp;We have used <i>M. smegmatis</i> as a model system because Mtb are highly pathogenic and difficult to culture in the lab. <i>M. smegmatis</i> is a close relative of Mtb, shares many of its membrane properties, and is commonly used as a stand-in for Mtb physiology in the lab.</p>
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<i>Mycobacterium tuberculosis</i> (Mtb) is the bacterium responsible for tuberculosis (TB). For decades, it was believed that TB was a disease of the past, but the onset of the HIV epidemic, the emergence of antibiotic resistant Mtb, and the relative ineffectiveness of the BCG vaccine have put TB back on the agenda.<br>
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      <p>&nbsp;&nbsp;In our system, described in the methods below, we used <i>E. coli</i> BL21 (DE3) as a chassis to express TDMH from an IPTG-inducible strong T7 promoter.</p>
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    </div>
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One of the main problems in treating TB is reaching its causer, which could evade the drug in use and survive in the cells of the immune system. Mtb infects its host through the airways. The bacterium is phagocytosed by resident macrophages in the lung and is able to replicate inside them. Its able to evade macrophage responses in part by inhibiting the fusion between the phagosome in which it resides and bactericidal lysosomes, as well as by dampening the acidification of the vacuole.<br>
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    <div style="clear: both;"></div>
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<br />
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A more efficient treatment of TB should contain a drug which rapidly kills mycobacteria and a delivery system for such drug, which could enable the killing of mycobacteria inside the infected macrophages. In our system the rapid drug is Trehalose Dimycolate Hydrolase (TDMH), while the delivery system is LLO carrying strain of <i>E. coli</i>.<br>
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</p>
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<h3>Background </h3>
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<br />
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<p>
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<b>Why is it so difficult to treat tuberculosis? </b>
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<p>
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This is due to several parameters linked to the nature of the pathogen, <i>Mycobacterium tuberculosis</i>:
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<br />•This bacterium has the power to replicate or remain dormant for years inside the macrophages. It happens by many complex mechanisms including prevention of the phagosomal maturation.
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<br />•The cell wall of <i>M.tuberculosis</i> is very complex and it's difficult for drugs to get inside.
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<br />•The growth of the bacteria is very slow and majority of drugs can reach only bacteria which are dividing.
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</p>
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<p>
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<b>Trehalose Dimycolate Hydrolase</b>
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<p>
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Mycobacterium species share a characteristic cell wall, which consists of the hydrophobic mycolate layer and a peptidoglycan layer held together by a polysaccharide arabinogalactan. The hydrophobicity of the envelope contributes to a high level of intrinsic drug tolerance in mycobacteria. All this makes mycolic components of the mycobacterial cell wall important as targets in drug design, where one such component is trehalose-6,6-dimycolate (TDM).<br>
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<br />
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TDM molecule comprises trehalose sugar esterified into two mycolic acid residues which range from 20–80 carbons in length. It’s the main virulence factor for the <i> M. tuberculosis </i> that makes it resistance to anti-tuberculosis medications, blocks macrophage activation by interferones and induces secretion of tumor necrosis factors. <br>
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<br />
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Trehalose Dimycolate Hydrolase (TDMH) is a cutinase-like serine esterase that triggers rapid lysis of the mycobacterial cell wall. This enzyme was first isolated form <i> M. smegmatis </i> mutant strain and it could hydrolyze purified TDM from various mycobacterial species. It was shown that exposure to TDMH triggers an immediate release of free mycolic acids from noncovalently associated mycolyl-containing glycolipids, ultimately leading to rapid and extensive lysis of pathogenic species, such as <i> M. tuberculosis </i>, <i> M. bovis </i>, and <i> M. marinum </i>, as well as to a lesser extent of <i> M. smegmatis </i> and <i> M. avium </i> (Yang <i> et al. </i> 2012).<br>
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<br />
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In our system a gene which encodes TDMH is driven under the T7 promoter in the pET21b(+) expression system. The plasmid was kindly provided by  Dr. Anil Ojha from the University of Pittsburgh.
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a. <br>
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<br>
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</p>
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<p>
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<b> <i> E. coli </i> expressing LLO as a drug delivery system </b>
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<p>
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<i> Listeria monocytogenes </i> is a bacterial pathogen that replicates within the cytosol of mammalian cells. After internalization into host cells, bacteria are initially contained within host phagosomes which they subsequently lyse  to gain access to the cytosol. The ability of <i> L. monocytogenes </i> to lyse the phagosome is primarily mediated by listeriolysin O (LLO). This protein is activated by the low pH in the lysosme. By causing large pore formation in the lysosomal membrane, it could provide protein delivery to the cytosol of macrophages. Higgins <i> et al. </i> reported that <i> E.coli </i> expressing cytoplasmic LLO can be used to efficiently and rapidly deliver b-galactosidase and chicken ovalbumin to the cytosol of macrophages. In our system we use the LLO carrying plasmid described in this paper - a pACYC184 vector where the LLO encoding gene, <i> hly </i>, is driven under the tetracycline promoter. <br>
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    <div id="Killing"></div>
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<br />
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    <h2>Killing mycobacteria with TDMH</h2>
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The advantages of using <i> E. coli </i> as a protein delivery system is that no TDMH isolation and purification is needed. As well, the delivery system is efficient and specific, because of the natural tendency of the macrophages to phagocytose the bacteria and the drug which they contain. <br>
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    <div class="leftparagraph">
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<br />
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However, dangerous factors are involved in using live bacteria as a drug delivery system. The act of releasing the drug from the burst cell also involves releasing the rest of intracellular contents.  There are also complications arising from the possible interactions between the the bacteria and the immune system. <br>
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</p>
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<br>
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<h3>Experimental design </h3>
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<p>
<p>
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<b> The killing assay in liquid media </b>
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&nbsp;&nbsp;Figure 1 describes how we performed the setup of our experience by making a coculture of <i>M.smegmatis</i> and <i>E.coli</i>.</p>
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<p>
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<p>Figure 2(below) shows the killing of <i>M. smegmatis</i> with TDMH expressed by <i>E. coli</i>. We mixed liquid cultures of <i>E. coli</i> and <i>M. smegmatis</i> at equal cell densities as determined by plating assays. When expression of TMDH was induced with IPTG, nearly 99% of the <i>M. smegmatis</i> were killed within six hours. We saw no change in viability in cultures of <i>M. smegmatis</i> alone or when mixed with uninduced <i>E. coli</i>.</p>
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At first we wanted to investigate how TDMH producing <i> E. coli </i> is efficient in killing mycobacteria. <i> E. coli </i> BL21 was transformed with the TDMH carrying plasmid (pET21b) and with the pColA Duet plasmid carrying an RFP cassette with a constitutive Anderson promoter (BBa_J23102). The killing efficiency was tested on <i> Mycobacterium smegmatis </i> MC2, a non-phatogenic rapidly growing strain of mycobacteria. We cultivated <i> E. coli </i> BL21 and <i> M. smegmatis </i> MC2 in LB media, with different ratios of the two strains:
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      <p>
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<br />
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&nbsp;&nbsp;We next sought to quantify the effectiveness of TDMH killing. We mixed induced<i> E. coli</i> and mycobacteria in different ratios and used plating assays to measure viability. As shown in figure 3 mycobacterial killing displayed dose dependence on the <i>E. coli</i> cell density. Small numbers of <i>E. coli</i> could kill many mycobacteria. For example, in mixed populations with 100 mycobactera for each <i>E. coli</i>, we still observed >50% mycobacterial killing after 2 hours. This indicates that, on average, each <i>E. coli</i> produced enough TDMH to kill 50 mycobacteria. We reason that this killing may be even more effective inside macrophages, where constrained volumes will increase the effective TDMH concentration.</p>
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    </div>
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<br />• 1 <i> E. coli </i> for 1 <i> M. smegmatis </i>  
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    <div class="rightparagraph">
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<br />• 1 <i> E. coli </i> for 10 <i> M. smegmatis </i>  
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      <center><a href="https://static.igem.org/mediawiki/2013/d/d9/PB_FigIva.png" target="_blank"><img src="https://static.igem.org/mediawiki/2013/d/d9/PB_FigIva.png" width="70%" style="margin-top:-50px"/></a></center>
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<br />1 <i> E. coli </i> for 100 <i> M. smegmatis </i>
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      <p><b>Figure 1</b> Experimental setup of the <i>M. smegmatis</i> killing assay.<div style="font-size:90%"> <i>M. smegmatis</i> and <i>E.coli</i> cells (Uninduced and induced with various concentrations of IPTG) were cultured up to OD 1,then serially diluted. Equal volumes of <i>E.coli</i> and <i>M. smegmatis</i> cultures of the same dilutions were mixed, incubated for 6 hours, and plated at 0,3 and 6 hours. </div></p>
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    </div>
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In these cultures <i> E. coli </i> was induced with 10 mM IPTG, which led to overexpression and release of TDMH in the media. The growth of both strains was measured for different time points (0, 1, 2, 3 and 6 h) by standard dilution series procedure and was expressed in CFUs/mL. Nalidixic acid plates (3 µg/mL) were used for following the growth of <i> M. smegmatis </i>m while the growth of <i> E. coli </i> was followed on kanamycin plates. For each time point the total amount of proteins was followed by the Bradford assay. Different control groups were also designed – a group where <i> M. smgematis </i> is grown without <i> E. coli </i>, a group where <i> E. coli </i> is induced and grown without <i> M. smegmatis </i>, and a group where <i> M. smegmatis </i> is was cultivated with the un-induced strain of <i> E. coli </i>.
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    <div style="clear: both;"></div>
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<br></p>
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    <div class="leftparagraph">
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<br>
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      <a href="https://static.igem.org/mediawiki/2013/a/a7/PB_Fig1_Myco_Kill_Curve.png" target="_blank"><img src="https://static.igem.org/mediawiki/2013/a/a7/PB_Fig1_Myco_Kill_Curve.png" width="100%"/></a>
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<p>
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      <p><b>Figure 2</b> TDMH-expressing <i>E.coli</i> kill mycobacteria in culture.<div style="font-size:90%"> We mixed TDMH-expressing <i>E.coli</i> and WT <i>M. smegmatis</i> in LB media at an initial cell density of 107 cells/ml each. Plating assays were used to count specifically <i>M. smegmatis</i> after the indicated times. When TDMH-expression was fully induced with 1 mM IPTG, more than 98% of mycobacteria were killed after 6 hours (red line). Populations of mycobacteria alone (black line) and mycobacteria mixed with uninduced <i>E.coli</i> (blue line) were stable.</div></p>
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<b>The killing assay inside the macrophages</b>
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    </div>
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<p>
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    <div class="rightparagraph">
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To test if <i> E. coli </i> carrying TDMH could kill mycobacteria which are inside of the macrophages a J774 macrophage cell line was used. <i> M. smegmatis </i> MC2 was transformed with pMyco-gfp plasmid (Alibaud <i> et al. </i> 2011). <i> E. coli </i> BL21 was transformed with 3 plasmids: pET21b + TDMH, pACYC184 + <i> hly </i> and pColA + BBa_J23102. The macrophages were grown in 24 well plates in RPMI 1640 media supplemented with 1 % glutamine, 10% of fetal bovine serum, 1% HEPES, 1% sodium  pyruvate. When around 90 % of confluence was reached, the cells were infected with <i> M. smegmatis </i>. Mycobacteria from an overnight culture were resuspended in RPMI and set to the final O.D. of 0.1. After infection, cells were incubated for 1 h (37 <sup>o</sup>C, 5% CO<sub>2</sub>) and then washed 10 times with PBS. After washing the cells new RPMI media was added and the cells were infected with an overnight culture of <i> E. coli </i> which was induced with 10 µM IPTG. <i> E. coli </i> were resuspended in RPMI where the final O.D. was set to 0.1. Then the infected cells were incubated for 1 h (37 oC, 5% CO2), washed 10 times with PBS and fresh RPMI media was added. Macrophages were then observed under the fluorescent microscope and after 3 h of incubation. We counted and compared the percentage of the macrophages which were infected with mycobacteria for these two time points. We also formed control groups: macrophages which were infected only with mycobacteria or only with <i> E. coli </i> so we could see the infection rate for these two strains; macrophages which were infected with <i> M. smegmatis </i> and with <i> E. coli </i> which wasn’t induced with IPTG. We also performed the same experiment where in the first infection step the cells were infected with <i> E. coli </i> and in the second one they were infected with mycobacteria.  
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      <center><a href="https://static.igem.org/mediawiki/2013/e/e0/PB_Fig2_Coli_Kill_Ratios.png" target="_blank"><img src="https://static.igem.org/mediawiki/2013/e/e0/PB_Fig2_Coli_Kill_Ratios.png" width="100%"/></a></center>
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<br>
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      <p><b>Figure 3</b> Dose-dependence in killing of mycobacteria by <i>E. coli.</i><div style="font-size:90%">We mixed <i>M. smegmatis</i> at a density of 10<sup>7</sup> cells/ml with <i>E. coli</i> at densities of 10<sup>5</sup> cells/ml (blue line) 10<sup>6</sup> cells/ml (green line) or 10<sup>7</sup> cells/ml to produce the ratios above. Even low densities of <i>E. coli</i> produced significant killing. Uninduced <i>E. coli</i> produced no significant killing.</div></p>
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    </div>
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    <div style="clear: both;"></div>
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<h3>Main results</h3>
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<p>
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    <h2></h2>
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<b>Killing assay outside the macrophages</b><br>
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    <div class="leftparagraph">
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<p>
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      <p>&nbsp;&nbsp;We investigated further the mechanism of TDMH-mediated cell killing. The TDMH enzyme in our system does not carry a secretion tag. Therefore, lysis of the <i>E. coli</i> membrane is probably required for the protein to reach (and lyse) <i>M. smegmatis</i>. We used plating assays to investigate the effect of TDMH induction on <i>E. coli</i> viability and Bradford assays to measure released protein. The results are presented in figure 4.</p>
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2 ratios were successful regarding the killing of M.smegmatis:<br>
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      <p>Figure 4A shows that inducing TDMH-expressing <i>E. coli</i> with IPTG rapidly kills the <i>E. coli.</i> In figure 4B, we show that inducing TDMH expression increases the concentration of free protein in the media. In our model, TDMH induction leads to spontaneous lysis of TDMH-expressing <i>E. coli</i>. This could be simply due to the extremely high protein expression levels driven by the T7 promoter, or it may be partially due to the esterase activities of the TDMH enzyme. Once the TDMH is released from the <i>E. coli</i> it is free to act on mycobacterial membranes, causing lysis and the release of additional proteins.
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1 to 10 and 1 to 1.Whereas in the 1 to 100 ratio we observed a recovery of M.smegmatis. <br>
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      </p>
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In the figure 1 you can see in blue the behavior of M.smegmatis alone, in red the behavior of M.smegmatis when we add E.coli uninduced and in green the behavior of M.smegmatis when we add E.coli and we induced to produce TDMH.<br>
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    </br>
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We decided that we will use the 1/1 ratio for the rest of our experiments. <br>
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      <p><b>Figure 4</b> Induction of TDMH kills <i>E. coli</i> and releases protein to the media.<div style="font-size:90%"><b>A)</b>Plating assays were used to determine <i>E. coli</i> viability in LB media after the indicated times. TDMH-induced <i>E. coli</i> rapidly lost viability (red line) Uninduced <i>E. coli</i> grew normally following a lag phase (black line).<b>B)</b>Bradford assays were used to measure free protein concentrations in mixed and induced bacterial cultures. When <i>E. coli</i> and mycobacteria are mixed and TDMH-expression is induced, free protein concentrations increase. This is consistent with a model in which TDMH induction leads to the lysis of the <i>E. coli</i> membrane. Action of TDMH on mycobacteria leads to further lysis and protein release.</div></p>
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<br>
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    </div>
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<b>Killing assay inside the macrophages: microscopy and video movie</b><br>
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    <div class="rightparagraph">
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<br>
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      </br></br></br></br></br>
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<h3>Discussion</h3>
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      <center><a href="https://static.igem.org/mediawiki/2013/7/74/PB_Fig3_Coli_Protein_Curve.png" target="_blank"><img width="100%" src="https://static.igem.org/mediawiki/2013/7/74/PB_Fig3_Coli_Protein_Curve.png"/></a></center>  
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    </div>
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    <div id="Macrophages"></div>
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    <h2>Programmed drug delivery with LLO</h2>
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    <div class="leftparagraph">
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      <p>&nbsp;&nbsp;<i>Listeria monocytogenes</i> is a bacterial pathogen that replicates in the cytosol of mammalian cells. The pathogen is initially internalized in host phagosomes, then lyses them to obtain access to the cytosol. A single gene, LLO, is responsible for this activity and is sufficient to convey the phenotype to <i>E. coli</i>.
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      </p>
 +
      <p>The LLO protein is activated by the low pH of the lysosme. By forming large pores in the lysosomal membrane, it allows protein delivery to the cytosol of macrophages (Higgins et al. 1999). Using <i>E. coli</i> as a protein vector means we don't need to isolate and purify the TDMH enzyme. </p>
 +
      <p>We hypothesized that a bacterial delivery system could be efficient and specific in targeting mycobacterial-infected macrophages. In effect, we might take advantage of the natural tendency of macrophages to phagocytose <i>E. coli</i> and their enzymatic payload.</p>
 +
      <p>Because LLO expression is known to be associated with Listeria pathogenicity, we took extra precautions in our cloning and experiments. These measures are detailed on our team safety page. Briefly, we worked in a Biosafety Level 2 lab under the supervision of two full-time lab managers. We researched and complied with French national and insitutional biosafety rules as they apply to this gene.</p>
 +
    </div>
 +
    <div class="rightparagraph">
 +
      <center><img src="https://static.igem.org/mediawiki/2013/b/b7/PB_Killing_assay_macrophages1.png" width="80%"/></center>
 +
      <p><b>Figure 5</b> Experimental design of the killing assay inside the macrophages. We infected them with <i>M. smegmatis</i> and washed after 1 hour. Then, we infected them with <i>E. coli</i> and washed after 1 hour. The end of this final infection step refers to the time 0 on our graphs. At this time we started the observation under the microscope</p>
 +
    </div>
 +
    <div style="clear: both;"></div>
-
<p>Our results show an indeniable role of the protein TDMH in the lysis of M.smegmatis. This target is independant of the Mycobacteria’s growth making it a molecule of choice in the war against tuberculosis.<br>
+
    <h2><i>E. coli</i> and <i>M. smegmatis</i> coinfections</h2>
-
<br>
+
    <div class="leftparagraph">
-
Using E.coli as a vector allows us to target the macrophages using a natural process: the phagocytosis. We showed that E.coli can enter a macrophage where there is already M.smegmatis. They didn’t seem to be in the same phagosome but the TDMH produced by E.coli can reach M.smegmatis. This is possible thanks to the lysteriolysin that lysed E.coli’s phagosome. <br>
+
      <p> &nbsp;&nbsp;Figure 6 displays J774 macrophages one hour after coinfection with <i>E. coli</i> and <i>M. smegmatis</i>. As described in the methods, the <i>E. coli</i> express TDMH and LLO and fluorescent mRFP as a label. The <i>M. smegmatis</i> express GFP as a label, but are otherwise wild type.</p>
-
<br>
+
      <p>The two movies displayed in figure 7 are time-lapse microscopy of live coinfected macrophages collected over a period of 6 hours. Fluorescence patterns revealing the localization of <i>E. coli</i> and <i>M. smegmatis</i> within the macrophages are relatively stable over this time period.</p>
-
<h3>Perspectives</h3>
+
    </div>
-
<p>It will be interesting to study the stability of TDMH at the phagosome’s pH and to imagine a protein delivery system that can target the macrophages without using a living organism (for example like they do with imiglucerase). The problem is our protein is not glycosylated so it will not be that easy. </p>
+
    <div class="rightparagraph">
-
<br>
+
      <p> We next applied quantitative microscopy to characterize the behavior of our system inside live macrophages. We imaged macrophage populations under several conditions and time points and scored their rates of infection with <i>E. coli</i>, <i>M. smegmatis</i> or both. In all we scored over 13,000 individual cells collected from more than 100 separate images.</p>
-
<h3>Bibliography</h3>
+
    </div>
-
<p>
+
    <div style="clear: both;"></div>
-
1. Yang Y, Bhatti A, Ke D, Gonzalez-Juarrero M, Lenaerts A, Kremer L, Guerardel Y, Zhang P, Ojha AK (2012) : Exposure to a cutinase-like serine esterase triggers rapid lysis of multiple mycobacterial species. J Biol Chem. 2013 Jan 4;288(1):382-92.<br>
+
    <div class="leftparagraph">
-
2. Rajesh Jayachandran, Varadharajan Sundaramurthy, Benoit Combaluzier , Philipp Mueller, Hannelie Korf, Kris Huygen, Toru Miyazaki, Imke Albrecht, Jan Massner, Jean Pieters (2007) : Survival of Mycobacteria in Macrophages Is Mediated by Coronin 1-Dependent Activation of Calcineurin. Cell, Volume 130, Issue 1, 13 July 2007, Pages 12-14 <br>
+
      <center><a href="https://static.igem.org/mediawiki/2013/5/52/PB_Fig4_Fresh_coinfection.png" target="_blank"><img src="https://static.igem.org/mediawiki/2013/5/52/PB_Fig4_Fresh_coinfection.png" width="100%"/></a></center>
 +
      </br>
 +
      <a href="https://static.igem.org/mediawiki/2013/5/51/PB_Fig4_Fresh_coinfection_zoom1.png" target="_blank"><img src="https://static.igem.org/mediawiki/2013/5/51/PB_Fig4_Fresh_coinfection_zoom1.png" width="48%"/></a>
 +
      <a href="https://static.igem.org/mediawiki/2013/c/c1/PB_Fig4_Fresh_coinfection_zoom2.png" target="_blank"><img src="https://static.igem.org/mediawiki/2013/c/c1/PB_Fig4_Fresh_coinfection_zoom2.png" width="48%" style="margin-left:3%"/></a>
 +
     
 +
      <p><b>Figure 6</b> Coinfection of J774 macrophages with mycobacteria and <i>E. coli</i> expressing TDMH and LLO<div style="font-size:90%"> <i>E. coli</i> (red) express mRFP as a marker and <i>M. smegmatis</i> (green) express GFP as a marker. Macrophages are observed to take up Mycobateria, <i>E. coli</i>, neither or both. This image was collected one hour after introducing the bacteria to the macrophage culture and following extensive washing to remove free bacteria.</div></p>
 +
    </div>
 +
    <div class="rightparagraph">
 +
      <iframe frameborder="0" style="margin-bottom:20px;" width="535" height="300" src="http://www.dailymotion.com/embed/video/x15jnu6"></iframe>
 +
      <iframe frameborder="0" width="535" height="300" src="http://www.dailymotion.com/embed/video/x15jnv8"></iframe>
 +
      <p><b>Figure 7</b> Temporal dynamics of macrophages coinfected with <i>E. coli</i> and <i>M. smegmatis.</i><div style="font-size:90%"><i>E. coli</i> and <i>M. smegmatis</i>, expressing mRFP and GFP respectively, were introduced to J774 macrophages. Fluorescent and bright field images were collected every 15 minutes for 6 hours. In these movies, the <i>E. coli</i> also express TDMH and LLO. Macrophages are observed to uptake <i>E. coli</i>, <i>M. smegmatis</i>, neither or both. The fluorescence patterns appear stable for these conditions and time period.</div></p>
 +
    </div>
 +
    <h2>pH influence </h2>
 +
<div class="leftparagraph">
 +
<p> &nbsp;&nbsp;We wanted to study the pH influence on <i>M. smegmatis</i> growth and on TDMH enzyme activity. We know that the phagosomal pH is usually acid (around 6) but can reach 4,5. We wondered if TDMH enzyme was working at this range of pH.</p>
 +
<p>We studied 7 different buffers :  3 ; 4,5 ; 5,1 ; 6,4 ; 7,35 ; 8,2 and 8,8. </p>
 +
<p>Figure 8 shows the activity of TDMH enzyme at various pH levels.</p>
 +
<p>Mycobacteria was unable to grow at pH 3 with or without the presence of TDMH.  Therefore we are unable to make any conclusions regarding the activity of the enzyme at very low pH values.</p>
 +
<p>TDMH activity was active across a large range of pH from 4.5 to 8.8, though there was a small decrease in efficiency observed at pH 8.2.  This is a promising result due to the difference in pH between the phagosome and the cytosol.  Additionally, the high activity of TDMH even at low pH is promising as it will be required to function at low pH inside the phagosome.
 +
</p>
-
       </p>
+
 
 +
</div>
 +
<div class="rightparagraph">
 +
 
 +
<center> <img src="https://static.igem.org/mediawiki/2013/e/e4/PB_TBC_PH_indepedence.png" width="60%"/></center> <p><b>Figure 8</b> pH influence on  TDMH enzyme activity <div style="font-size:90%"> We add to <i>M.smegmatis</i> the proteins of an induced control, the uninduced strain of Bl21 and the induced strain producing TDMH.</div></p>
 +
</div>
 +
 
 +
 
 +
    <div style="clear: both;"></div>
 +
 
 +
    <h2>Conclusions and continuing work</h2>
 +
    <div class="leftparagraph">
 +
       <p>&nbsp;&nbsp;We have shown that <i>E. coli</i> can effectively kill mycobacteria in culture by expressing the TDMH enzyme, now a BioBrick. We have further shown that <i>E. coli</i> and mycobateria may co-localize within macrophages, where LLO-based systems can effectively deliver protein payloads.</p>
 +
      <p>In the coming weeks, we will continue to refine our cell culture techniques to precisely characterize the effectiveness of our system <i>in situ</i>, within the living macrophage.</p>
 +
      <p><b>Figure 9</b> The effect of TDMH-induced <i>E. coli</i> on macrophage infection rates after 3 hours.<div style="font-size:90%">We scored fluorescence microscopy images of macrophages exposed to both <i>E. coli</i> and <i>M. smegmatis</i> expressing fluorescent protein markers.  The <i>E. coli</i> expressed LLO and were induced or uninduced for TDMH expression. For both treatments, we observed an increase in the infection rates of both bacteria after 3 hours. We attribute this to combination of the media with free bacteria, which macrophages continue to consume over the course of the experiment. TDMH induction slowed the increase in <i>E. coli</i> infection rates, which is likely due to the toxic effects of TDMH expression on <i>E. coli</i>, as shown in figure 4.</div></p>
     </div>
     </div>
-
     <div class="pageimgs">
+
     <div class="rightparagraph">
-
       <img width="100%" src="https://static.igem.org/mediawiki/2013/0/0f/TB_Ception_Figure.png" />
+
       <center><img src="https://static.igem.org/mediawiki/2013/1/15/PB_Fig6_Image_Counts.png" width="80%"/></center>
     </div>
     </div>
 +
    <div style="clear: both;">
 +
 +
    <h2>Bibliography</h2>
 +
    <ul>
 +
      <li>Yang Y, Bhatti A, Ke D, Gonzalez-Juarrero M, Lenaerts A, Kremer L, Guerardel Y, Zhang P, Ojha AK (2012) : Exposure to a cutinase-like serine esterase triggers rapid lysis of multiple mycobacterial species. J Biol Chem. 2013 Jan 4;288(1):382-92.</li>
 +
      <li>Rajesh Jayachandran, Varadharajan Sundaramurthy, Benoit Combaluzier , Philipp Mueller, Hannelie Korf, Kris Huygen, Toru Miyazaki, Imke Albrecht, Jan Massner, Jean Pieters (2007) : Survival of Mycobacteria in Macrophages Is Mediated by Coronin 1-Dependent Activation of Calcineurin. Cell, Volume 130, Issue 1, 13 July 2007, Pages 12-14 </li>
 +
    </ul>
-
<div class="pageimgs"><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br><br>
 
-
<img width="100%" src="https://static.igem.org/mediawiki/2013/e/e5/Figure_1_M.smeg.png"/>
 
-
</div>
 
   </div>
   </div>
-
  <div style="clear: both;"></div>
+
<div style="clear: both;"></div>
-
</div>
+
 
-
 
+
    <h2>Attributions</h2>  
 +
 
 +
<p>pET21 1519 plasmid was kindly provided by Anil Ojha of the University of Pittsburgh.</p>
 +
<p> Murine cell line macrophages J774 were a gift from Nicole Guiso and Nicolas Hegerle from Pasteur institute (Unit of Molecular Prevention and Therapy of Human Diseases. </p>
 +
<p> <i>Mycobacterium smegmatis</i> was a gift from Brigitte Gicquel from Pasteur institute (Unit Mycobacterial genetics). </p>
 +
<p> <i>Mycobacterium smegmatis</i> expressing GFP was kindly provided by Stephane Canaan from CNRS (Laboratory of Enzymology at Interfaces and Physiology of Lipolysis). </p>
 +
<p>The project itself was designed and accomplished by Camélia Bencherif and Iva Atanaskovic with consultation with Edwin Wintermute, Mathias Toulouze and Ariel Lindner.</p>
 +
<p> We also discussed the project with Christopher Anderson from Berkeley University (Synthetic biology Anderson lab) about the feasibility, good points and critical points of the project. </p>
 +
<p> We want to thank all these people that made Infiltrate project happen !</p>
 +
 
 +
 
 +
   
 +
</div>
</html>
</html>
{{:Team:Paris_Bettencourt/footer}}
{{:Team:Paris_Bettencourt/footer}}

Latest revision as of 03:44, 29 October 2013

Background

Latent tuberculosis persists inside macrophages, where it is partially protected from both the host immune system and conventional antibiotics.

Results

  • We expressed the enzyme Trehalose Dimycolate Hydrolase (TDMH) in E. coli and showed that it is highly toxic to mycobacteria in culture.
  • We expressed the listeriolyin O (LLO) gene in E. coli and showed that it is capable of entering the macrophage cytosol.
  • We co-infected macrophages with both mycobacteria and our engineered E. coli to characterize the resulting phagocytosis and killing.
  • We measured the effect of a range of pH (from 3 to 8,8) on M. smegmatis and the TDMH enzyme activity.

Aim

To create an E. coli strain capable of entering the macrophage cytosol and delivering a lytic enzyme to kill mycobacteria.

Introduction

   Mycobacterium tuberculosis (Mtb), the bacterium responsible for tuberculosis (TB), spreads by aerosol and infects its host through the airways. The bacterium is phagocytosed by macrophages in the lung, yet often evades death in the lysosome. Mtb can persist for years or even decades inside macrophages by inhibiting phagosome/lysosome fusion and supressing the normal acidification of the lysosome.

An efficient treatment for persistent TB must enter infected macrophages and kill the pathogen there. In our system, E. coli is both the vector and the therapeutic agent agent by expressing the listeriolyin O gene LLO to enter macrophages and TDMH to kill mycobacteria. Additionally we thought about how we could deliver the E. coli to the lungs and decided that the most effective way would be through an inhaler.

 BOX 1: Why is it difficult to treat tuberculosis?

  • Mtb can survive and replicate for years inside the macrophages by supressing the normal process of phagocytosis.
  • The cell wall of M. tuberculosis is thick, waxy and rich in mycolic acids. It it difficult to penetrate with a small-molecule drug.
  • The pathogen grows very slowly inside macrophages. Most conventional antibiotics target processes like DNA replication that are specific to growing cells.


TDMH and the mycobacterial cell wall

  Mycobacterium species share a characteristic cell wall: thick, waxy, hydrophobic, and rich in mycolic acids. The low permeability of the envelope to hydrophilic solutes contributes to the intrinsic drug tolerance in mycobacteria.

  Trehalose Dimycolate Hydrolase (TDMH) is a cutinase-like serine esterase that triggers rapid lysis of the mycobacterial cell wall by degrading the mycolate layer. The enzyme was first isolated from Mycobacterium smegmatis and subsequently shown to hydrolyze purified TDM from various mycobacterial species. Exposure to TDMH triggers an immediate release of free mycolic acids, ultimately leading to lysis of many mycobacteria including Mtb (Yang et al. 2012).

  We have used M. smegmatis as a model system because Mtb are highly pathogenic and difficult to culture in the lab. M. smegmatis is a close relative of Mtb, shares many of its membrane properties, and is commonly used as a stand-in for Mtb physiology in the lab.

  In our system, described in the methods below, we used E. coli BL21 (DE3) as a chassis to express TDMH from an IPTG-inducible strong T7 promoter.

Killing mycobacteria with TDMH

  Figure 1 describes how we performed the setup of our experience by making a coculture of M.smegmatis and E.coli.

Figure 2(below) shows the killing of M. smegmatis with TDMH expressed by E. coli. We mixed liquid cultures of E. coli and M. smegmatis at equal cell densities as determined by plating assays. When expression of TMDH was induced with IPTG, nearly 99% of the M. smegmatis were killed within six hours. We saw no change in viability in cultures of M. smegmatis alone or when mixed with uninduced E. coli.

  We next sought to quantify the effectiveness of TDMH killing. We mixed induced E. coli and mycobacteria in different ratios and used plating assays to measure viability. As shown in figure 3 mycobacterial killing displayed dose dependence on the E. coli cell density. Small numbers of E. coli could kill many mycobacteria. For example, in mixed populations with 100 mycobactera for each E. coli, we still observed >50% mycobacterial killing after 2 hours. This indicates that, on average, each E. coli produced enough TDMH to kill 50 mycobacteria. We reason that this killing may be even more effective inside macrophages, where constrained volumes will increase the effective TDMH concentration.

Figure 1 Experimental setup of the M. smegmatis killing assay.

M. smegmatis and E.coli cells (Uninduced and induced with various concentrations of IPTG) were cultured up to OD 1,then serially diluted. Equal volumes of E.coli and M. smegmatis cultures of the same dilutions were mixed, incubated for 6 hours, and plated at 0,3 and 6 hours.

Figure 2 TDMH-expressing E.coli kill mycobacteria in culture.

We mixed TDMH-expressing E.coli and WT M. smegmatis in LB media at an initial cell density of 107 cells/ml each. Plating assays were used to count specifically M. smegmatis after the indicated times. When TDMH-expression was fully induced with 1 mM IPTG, more than 98% of mycobacteria were killed after 6 hours (red line). Populations of mycobacteria alone (black line) and mycobacteria mixed with uninduced E.coli (blue line) were stable.

Figure 3 Dose-dependence in killing of mycobacteria by E. coli.

We mixed M. smegmatis at a density of 107 cells/ml with E. coli at densities of 105 cells/ml (blue line) 106 cells/ml (green line) or 107 cells/ml to produce the ratios above. Even low densities of E. coli produced significant killing. Uninduced E. coli produced no significant killing.

  We investigated further the mechanism of TDMH-mediated cell killing. The TDMH enzyme in our system does not carry a secretion tag. Therefore, lysis of the E. coli membrane is probably required for the protein to reach (and lyse) M. smegmatis. We used plating assays to investigate the effect of TDMH induction on E. coli viability and Bradford assays to measure released protein. The results are presented in figure 4.

Figure 4A shows that inducing TDMH-expressing E. coli with IPTG rapidly kills the E. coli. In figure 4B, we show that inducing TDMH expression increases the concentration of free protein in the media. In our model, TDMH induction leads to spontaneous lysis of TDMH-expressing E. coli. This could be simply due to the extremely high protein expression levels driven by the T7 promoter, or it may be partially due to the esterase activities of the TDMH enzyme. Once the TDMH is released from the E. coli it is free to act on mycobacterial membranes, causing lysis and the release of additional proteins.


Figure 4 Induction of TDMH kills E. coli and releases protein to the media.

A)Plating assays were used to determine E. coli viability in LB media after the indicated times. TDMH-induced E. coli rapidly lost viability (red line) Uninduced E. coli grew normally following a lag phase (black line).B)Bradford assays were used to measure free protein concentrations in mixed and induced bacterial cultures. When E. coli and mycobacteria are mixed and TDMH-expression is induced, free protein concentrations increase. This is consistent with a model in which TDMH induction leads to the lysis of the E. coli membrane. Action of TDMH on mycobacteria leads to further lysis and protein release.






Programmed drug delivery with LLO

  Listeria monocytogenes is a bacterial pathogen that replicates in the cytosol of mammalian cells. The pathogen is initially internalized in host phagosomes, then lyses them to obtain access to the cytosol. A single gene, LLO, is responsible for this activity and is sufficient to convey the phenotype to E. coli.

The LLO protein is activated by the low pH of the lysosme. By forming large pores in the lysosomal membrane, it allows protein delivery to the cytosol of macrophages (Higgins et al. 1999). Using E. coli as a protein vector means we don't need to isolate and purify the TDMH enzyme.

We hypothesized that a bacterial delivery system could be efficient and specific in targeting mycobacterial-infected macrophages. In effect, we might take advantage of the natural tendency of macrophages to phagocytose E. coli and their enzymatic payload.

Because LLO expression is known to be associated with Listeria pathogenicity, we took extra precautions in our cloning and experiments. These measures are detailed on our team safety page. Briefly, we worked in a Biosafety Level 2 lab under the supervision of two full-time lab managers. We researched and complied with French national and insitutional biosafety rules as they apply to this gene.

Figure 5 Experimental design of the killing assay inside the macrophages. We infected them with M. smegmatis and washed after 1 hour. Then, we infected them with E. coli and washed after 1 hour. The end of this final infection step refers to the time 0 on our graphs. At this time we started the observation under the microscope

E. coli and M. smegmatis coinfections

  Figure 6 displays J774 macrophages one hour after coinfection with E. coli and M. smegmatis. As described in the methods, the E. coli express TDMH and LLO and fluorescent mRFP as a label. The M. smegmatis express GFP as a label, but are otherwise wild type.

The two movies displayed in figure 7 are time-lapse microscopy of live coinfected macrophages collected over a period of 6 hours. Fluorescence patterns revealing the localization of E. coli and M. smegmatis within the macrophages are relatively stable over this time period.

We next applied quantitative microscopy to characterize the behavior of our system inside live macrophages. We imaged macrophage populations under several conditions and time points and scored their rates of infection with E. coli, M. smegmatis or both. In all we scored over 13,000 individual cells collected from more than 100 separate images.


Figure 6 Coinfection of J774 macrophages with mycobacteria and E. coli expressing TDMH and LLO

E. coli (red) express mRFP as a marker and M. smegmatis (green) express GFP as a marker. Macrophages are observed to take up Mycobateria, E. coli, neither or both. This image was collected one hour after introducing the bacteria to the macrophage culture and following extensive washing to remove free bacteria.

Figure 7 Temporal dynamics of macrophages coinfected with E. coli and M. smegmatis.

E. coli and M. smegmatis, expressing mRFP and GFP respectively, were introduced to J774 macrophages. Fluorescent and bright field images were collected every 15 minutes for 6 hours. In these movies, the E. coli also express TDMH and LLO. Macrophages are observed to uptake E. coli, M. smegmatis, neither or both. The fluorescence patterns appear stable for these conditions and time period.

pH influence

  We wanted to study the pH influence on M. smegmatis growth and on TDMH enzyme activity. We know that the phagosomal pH is usually acid (around 6) but can reach 4,5. We wondered if TDMH enzyme was working at this range of pH.

We studied 7 different buffers : 3 ; 4,5 ; 5,1 ; 6,4 ; 7,35 ; 8,2 and 8,8.

Figure 8 shows the activity of TDMH enzyme at various pH levels.

Mycobacteria was unable to grow at pH 3 with or without the presence of TDMH. Therefore we are unable to make any conclusions regarding the activity of the enzyme at very low pH values.

TDMH activity was active across a large range of pH from 4.5 to 8.8, though there was a small decrease in efficiency observed at pH 8.2. This is a promising result due to the difference in pH between the phagosome and the cytosol. Additionally, the high activity of TDMH even at low pH is promising as it will be required to function at low pH inside the phagosome.

Figure 8 pH influence on TDMH enzyme activity

We add to M.smegmatis the proteins of an induced control, the uninduced strain of Bl21 and the induced strain producing TDMH.

Conclusions and continuing work

  We have shown that E. coli can effectively kill mycobacteria in culture by expressing the TDMH enzyme, now a BioBrick. We have further shown that E. coli and mycobateria may co-localize within macrophages, where LLO-based systems can effectively deliver protein payloads.

In the coming weeks, we will continue to refine our cell culture techniques to precisely characterize the effectiveness of our system in situ, within the living macrophage.

Figure 9 The effect of TDMH-induced E. coli on macrophage infection rates after 3 hours.

We scored fluorescence microscopy images of macrophages exposed to both E. coli and M. smegmatis expressing fluorescent protein markers. The E. coli expressed LLO and were induced or uninduced for TDMH expression. For both treatments, we observed an increase in the infection rates of both bacteria after 3 hours. We attribute this to combination of the media with free bacteria, which macrophages continue to consume over the course of the experiment. TDMH induction slowed the increase in E. coli infection rates, which is likely due to the toxic effects of TDMH expression on E. coli, as shown in figure 4.

Bibliography

  • Yang Y, Bhatti A, Ke D, Gonzalez-Juarrero M, Lenaerts A, Kremer L, Guerardel Y, Zhang P, Ojha AK (2012) : Exposure to a cutinase-like serine esterase triggers rapid lysis of multiple mycobacterial species. J Biol Chem. 2013 Jan 4;288(1):382-92.
  • Rajesh Jayachandran, Varadharajan Sundaramurthy, Benoit Combaluzier , Philipp Mueller, Hannelie Korf, Kris Huygen, Toru Miyazaki, Imke Albrecht, Jan Massner, Jean Pieters (2007) : Survival of Mycobacteria in Macrophages Is Mediated by Coronin 1-Dependent Activation of Calcineurin. Cell, Volume 130, Issue 1, 13 July 2007, Pages 12-14

Attributions

pET21 1519 plasmid was kindly provided by Anil Ojha of the University of Pittsburgh.

Murine cell line macrophages J774 were a gift from Nicole Guiso and Nicolas Hegerle from Pasteur institute (Unit of Molecular Prevention and Therapy of Human Diseases.

Mycobacterium smegmatis was a gift from Brigitte Gicquel from Pasteur institute (Unit Mycobacterial genetics).

Mycobacterium smegmatis expressing GFP was kindly provided by Stephane Canaan from CNRS (Laboratory of Enzymology at Interfaces and Physiology of Lipolysis).

The project itself was designed and accomplished by Camélia Bencherif and Iva Atanaskovic with consultation with Edwin Wintermute, Mathias Toulouze and Ariel Lindner.

We also discussed the project with Christopher Anderson from Berkeley University (Synthetic biology Anderson lab) about the feasibility, good points and critical points of the project.

We want to thank all these people that made Infiltrate project happen !

Centre for Research and Interdisciplinarity (CRI)
Faculty of Medicine Cochin Port-Royal, South wing, 2nd floor
Paris Descartes University
24, rue du Faubourg Saint Jacques
75014 Paris, France
+33 1 44 41 25 22/25
team2013@igem-paris.org
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