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<h2 id="designrules">Design Rules For Genome Engineering Regarding Customization of Peroxisome Properties</h2>
 
<p>In order to reach the ultimate goal of creating a fully controllable artificial compartment, genome engineering can be utilized for customizing the compartment's properties,.These include aspects such as membrane permeability, size/number, or decoupling of peroxisomes from the cytoskeleton, the peroxisomal proteome or metabolome. In our project we used the Crispr Cas9 system for knocking out several genes (Pex9, Pex31&Pex32, INP1, POT1) at the same time in order to engineer the previously mentioned properties. Furthermore, we designed a yeast strain  with a completely replaced protein-import machinery for controlling the entire peroxisomal lumen.</p>
 
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<p>For the future one could think of much more radical strategies for peroxisomal engineering with a final goal of a “minimal peroxisome” by redirecting metabolic pathways through changing the protein-localization-signal in the yeast genome. Additionally, endogenous metabolic pathways could be redirected to our novel artificial compartment for establishing a customized metabolism specifically tailored for the user's application.</p>
 
  <h3>Introduction</h3>
 
<p>In order to achieve a fully controllable artificial compartment, the first step was to design a completely orthogonal import system. Next was the knockout of endogenous import systems. However, a few proteins are imported neither by the Pex5 nor the Pex7 import machinery. Therefore, specific genome engineering designs, such as knockouts, deleting or redirecting the protein localization could be utilized for the ultimate goal of creating a synthetic organelle.</p>
 
<p>Additionally, knockouts or genome integrations enable customization of the peroxisomal properties, such as membrane permeability, size/number, decoupling of peroxisomes from cytoskeleton and the peroxisomal metabolism.</p>
 
<p>All these strategies allow a rational design of an artificial compartment, which is fully engineerable regarding  the proteome, metabolome and the entire peroxisomal environment.</p>
 
<h3>Design of yeast multi -knockout strains</h3>
 
<h4>The Crispr Cas9 System</h4>
 
<p>The demands on yeast engineering have significantly increased with the design of more complex systems and extensive metabolic pathways. Genetic techniques that have historically relied on marker recycling are unable to keep up with the ambitions of synthetic biologists. In recent years the Crispr Cas9 system has been used for several strain-engineering purposes, including:</p>
 
<ul>
 
  <li>Markerless integration of multiple genetic cassettes into selected genomic loci</li>
 
  <li>Multiplexed and iterative gene knockouts without the need to recycle a marker</li>
 
  <li>Precise genome editing – nucleotide substitutions, etc.</li>
 
</ul>
 
<p>We utilized the Cas9 system as a tool for peroxisomal engineering and have adopted the existing toolbox from <abbr title="Lee, Michael E.; DeLoache, William C.; Cervantes, Bernardo; Dueber, John E. (2015): A Highly Characterized Yeast Toolkit for Modular, Multipart Assembly. In: ACS synthetic biology 4 (9), S. 975–986. DOI: 10.1021/sb500366v.">(Lee et al. 2015)</abbr> and the complete cloning system which also provides the possibilities for genome integration and gene editing by Cas9. For this, two oligonucleotides have to be designed for targeting the Cas protein to the gene of interest.</p>
 
 
 
<figure>
 
  <img src="https://static.igem.org/mediawiki/2017/3/3b/--T--cologne-duesseldorf--Cas9_1.PNG">
 
  <figcaption>Figure 1: Plasmid construction for the gRNA expression plasmid<br>Two oligos, containing the targeting sequence of the gRNA, have to be annealed and can then be integrated in the gRNA entry Vector by a Golden Gate reaction. Adapted from (<abbr title="Lee, Michael E.; DeLoache, William C.; Cervantes, Bernardo; Dueber, John E. (2015): A Highly Characterized Yeast Toolkit for Modular, Multipart Assembly. In: ACS synthetic biology 4 (9), S. 975–986. DOI: 10.1021/sb500366v.">Lee et al. 2015</abbr>)</figcaption>
 
</figure>
 
 
<p>Several gRNA vectors can subsequently be assembled into one vector with a Cas9 expression cassette and then be transformed into yeast. The expression of Cas9 together with gene specific gRNA´s leads to double strand breakage followed by non-homologous end joining repair or homologous recombination, in case of added repair DNA (figure 3).</p>
 
 
<figure>
 
  <img src="https://static.igem.org/mediawiki/2017/6/69/--T--cologne-duesseldorf--Cas9_2.PNG">
 
  <figcaption>Figure 2: Plasmid construction for the expression plasmid containing Cas9 and gRNA´s<br>Vector for Cas9 and gRNA expression, assembled by a Golden Gate reaction, containing a URA marker, Cen6 yeast origin and a kanamycin resistance. Adapted from (<abbr title="Lee, Michael E.; DeLoache, William C.; Cervantes, Bernardo; Dueber, John E. (2015): A Highly Characterized Yeast Toolkit for Modular, Multipart Assembly. In: ACS synthetic biology 4 (9), S. 975–986. DOI: 10.1021/sb500366v.">Lee et al. 2015</abbr>)</figcaption>
 
</figure>
 
 
<p>The combination of the Cas9 system with DNA repair sequences enables not only knockouts of peroxisomal proteins, but also allows redirecting protein localization by changing protein targeting signals or integration of linear DNA into yeast chromosomes. Genome engineering facilitates yeast strain development for customized peroxisomes.</p>
 
 
 
<figure>
 
  <img src="https://static.igem.org/mediawiki/2017/9/9b/--T--cologne-duesseldorf--Cas9_3.PNG">
 
  <figcaption><strong>Figure 3:</strong> Design of repair DNA sequences for homologous recombination after inducing double strand break by Cas9<br>
 
  Repair DNA sequences can be used to increase the efficiency for Cas9 guided knocking out of specific genes, but would also allow genomic integration of targeting signals or complete genes.  Adapted from (<abbr title="Lee, Michael E.; DeLoache, William C.; Cervantes, Bernardo; Dueber, John E. (2015): A Highly Characterized Yeast Toolkit for Modular, Multipart Assembly. In: ACS synthetic biology 4 (9), S. 975–986. DOI: 10.1021/sb500366v.">Lee et al. 2015</abbr>)</figcaption>
 
</figure>
 
 
<h3>The peroxisomal proteome of <i>Saccharomyces cerevisiae</i></h3>
 
<p>The peroxisomal proteome is studied extensively for saccharomyces cerevisiae and contains exactly 67 proteins (<abbr title="Kohlwein, Sepp D.; Veenhuis, Marten; van der Klei, Ida J. (2013): Lipid droplets and peroxisomes: key players in cellular lipid homeostasis or a matter of fat--store 'em up or burn 'em down. In: Genetics 193 (1), S. 1–50. DOI: 10.1534/genetics.112.143362.">Kohlwein et al. 2013</abbr>). The function is characterized for the most of those proteins and it is known, that yeast peroxisomes are expendable under optimal growth conditions. Nevertheless, some knockouts are lethal under oleate or stress conditions.</p>
 
 
 
 
 
 
 
<table>
 
  <thead>
 
    <tr>
 
      <th>Gene</th>
 
      <th>Required for growth on oleate</th>
 
      <th>Expression induced by oleate</th>
 
      <th>Enzyme/activity</th>
 
      <th>Molecular mass (kDa)</th>
 
      <th>Isoelectric point</th>
 
      <th>Molecules per cell </th>
 
      <th>Localization</th>
 
      <th>Function</th>
 
    </tr>
 
  </thead>
 
  <tbody>
 
    <tr>
 
      <td colspan=”9”>ß-Oxidation enzymes</td>
 
    </tr>
 
    <tr>
 
      <td>PCS60 (FAT2)</td>
 
      <td>No</td>
 
      <td>Yes</td>
 
      <td>Medium chain fatty acyl-CoA synthetase</td>
 
      <td>60.5</td>
 
      <td>9.98</td>
 
      <td>8.770</td>
 
      <td>Peripheral peroxisomal membrane and matrix</td>
 
      <td>Activates fatty acids with a preference for medium chain lengths, C9-C13</td>
 
    </tr>
 
    <tr>
 
      <td>FAT1</td>
 
      <td>No</td>
 
      <td>-</td>
 
      <td> Very long chain fatty acyl-CoA synthetase and long chain fatty acid transporter</td>
 
      <td>77.1</td>
 
      <td>8.47</td>
 
      <td>16,900</td>
 
      <td>Lipid droplet, ER, peroxisome Three predicted TM</td>
 
      <td>Activates fatty acids with a preference for very long chain lengths, C20–C26</td>
 
    </tr>
 
    <tr>
 
      <td>POX1</td>
 
      <td>Yes</td>
 
      <td>Yes</td>
 
      <td>Acyl-CoA- oxidase</td>
 
      <td>84.0</td>
 
      <td>8.73</td>
 
      <td>ND</td>
 
      <td>Peroxisomal matrix</td>
 
      <td>Oxidation of acyl-CoA</td>
 
    </tr>
 
    <tr>
 
      <td>CTA1</td>
 
      <td>No</td>
 
      <td>Yes</td>
 
      <td>Catalase</td>
 
      <td>58.6</td>
 
      <td>7.46</td>
 
      <td>623</td>
 
      <td>Peroxisomal matrix</td>
 
      <td>Degrades hydrogen peroxide produced by Pox1</td>
 
    </tr>
 
    <tr>
 
      <td>FOX2 (POX2)</td>
 
      <td>Yes</td>
 
      <td>Yes</td>
 
      <td>Multifunctional enzyme; 3-hydroxyacyl-CoA dehydrogenase and enoyl-CoA hydratase</td>
 
      <td>98.7</td>
 
      <td>9.75</td>
 
      <td>ND</td>
 
      <td>Peroxisomal matrix</td>
 
      <td>-</td>
 
    </tr>
 
    <tr>
 
      <td>POT1 (FOX3, POX3)</td>
 
      <td>Yes</td>
 
      <td>Yes</td>
 
      <td>3-Ketoacyl-CoA thiolase</td>
 
      <td>44.7</td>
 
      <td>7.56</td>
 
      <td>ND</td>
 
      <td>Peroxisomal matrix</td>
 
      <td>Cleaves 3-ketoacyl-CoA into acyl-CoA and acetyl-CoA</td>
 
    </tr>
 
    <tr>
 
      <td>DCI1 (ECI2)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td> Δ(3,5)-Δ(2,4)-dienoyl-CoA isomerase (putative)</td>
 
      <td>30.1</td>
 
      <td>8.83</td>
 
      <td>ND</td>
 
      <td>Peroxisomal matrix</td>
 
      <td>Auxiliary enzyme of fatty acid β-oxidation; role in β-oxidation debated</td>
 
    </tr>
 
    <tr>
 
      <td>SPS19 (SPX1)</td>
 
      <td>Yes</td>
 
      <td>Yes</td>
 
      <td>2,4-Dienoyl-CoA reductase</td>
 
      <td>31.1</td>
 
      <td>9.67</td>
 
      <td>ND</td>
 
      <td>Peroxisomal matrix</td>
 
      <td>Auxiliary enzyme of fatty acid β-oxidation</td>
 
    </tr>
 
    <tr>
 
      <td>ECI1</td>
 
      <td>Yes</td>
 
      <td>Yes</td>
 
      <td>Δ3, Δ2-enoyl-CoA isomerase</td>
 
      <td>31.7</td>
 
      <td>8.21</td>
 
      <td>ND</td>
 
      <td>Peroxisomal matrix</td>
 
      <td>Auxiliary enzyme of fatty acid β-oxidation</td>
 
    </tr>
 
    <tr>
 
      <td>TES1 (PTE1)</td>
 
      <td>Yes</td>
 
      <td>Yes</td>
 
      <td>Acyl-CoA thioesterase</td>
 
      <td>40.3</td>
 
      <td>9.58</td>
 
      <td>ND</td>
 
      <td>Peroxisomal matrix</td>
 
      <td>Auxiliary enzyme of fatty acid β-oxidation</td>
 
    </tr>
 
    <tr>
 
      <td>MDH3</td>
 
      <td>Yes</td>
 
      <td>Yes</td>
 
      <td>Malate dehydrogenase</td>
 
      <td>37.3</td>
 
      <td>10.00</td>
 
      <td>3,300</td>
 
      <td>Peroxisomal matrix</td>
 
      <td>Required for the malate-oxaloacetete shuttle, to exchange peroxisomal NADH for cytosolic NAD+, part of the glyoxylate cycle
 
      </td>
 
    </tr>
 
    <tr>
 
      <td>IDP3</td>
 
      <td>Yes</td>
 
      <td>Yes</td>
 
      <td>NADP+ dependent isocitrate dehydrogenase</td>
 
      <td>47.91</td>
 
      <td>10.02</td>
 
      <td>ND</td>
 
      <td>Peroxisomal matrix</td>
 
      <td>Required for the 2-ketoglutarate/isocitrate shuttle, exchanging peroxisomal NADP+ for cytosolic NADPH</td>
 
    </tr>
 
    <tr>
 
      <td>CAT2</td>
 
      <td>No</td>
 
      <td>No</td>
 
      <td>Carnitine acetyl-CoA transferase</td>
 
      <td>77.2</td>
 
      <td>8.34</td>
 
      <td>470</td>
 
      <td>Peroxisome mitochondria</td>
 
      <td>Transfers activated acetyl groups to carnitine to form acetylcarnitine which can be shuttled across membranes</td>
 
    </tr>
 
    <tr>
 
      <td colspan=”9”>Glyoxylate cycle</td>
 
    </tr>
 
    <tr>
 
      <td>CIT2</td>
 
      <td>No</td>
 
      <td>-</td>
 
      <td>Citrate synthase</td>
 
      <td>51.4</td>
 
      <td>6.34</td>
 
      <td>2,310</td>
 
      <td>Peroxisomal matrix</td>
 
      <td>Condensation of acetyl CoA and oxaloacetate to form citrate</td>
 
    </tr>
 
    <tr>
 
      <td>MDH3</td>
 
      <td>Yes</td>
 
      <td>Yes</td>
 
      <td>Malate dehydrogenase</td>
 
      <td>37.3</td>
 
      <td>10.00</td>
 
      <td>3,300</td>
 
      <td>Peroxisomal matrix</td>
 
      <td>Required for the malate–oxaloacetete shuttle, to exchange peroxisomal NADH for cytosolic NAD+</td>
 
    </tr>
 
    <tr>
 
      <td>MLS1</td>
 
      <td>Yes</td>
 
      <td>-</td>
 
      <td>Malate synthase</td>
 
      <td>62.8</td>
 
      <td>7.18</td>
 
      <td>ND</td>
 
      <td>Peroxisomal protein</td>
 
      <td>Required for utilization of nonfermentable carbon sources</td>
 
    </tr>
 
    <tr>
 
      <td colspan=”9”> Other peroxisome-associated enzyme activities</td>
 
    </tr>
 
    <tr>
 
      <td> GPD1 (DAR1, HOR1, OSG1, OSR5</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td> NAD-dependent glycerol-3-phosphate dehydrogenase</td>
 
      <td>42.9</td>
 
      <td>5.26</td>
 
      <td>807</td>
 
      <td>Peroxisome, cytosol, nucleus</td>
 
      <td> Key enzyme of glycerol synthesis, essential for growth under osmotic stress</td>
 
    </tr>
 
    <tr>
 
      <td>PNC1</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Nicotinamidase</td>
 
      <td>25.0</td>
 
      <td>6.23</td>
 
      <td>7,720</td>
 
      <td>Peroxisome, cytosol</td>
 
      <td>Converts nicotinamide to nicotinic acid as part of the NAD(+) salvage pathway</td>
 
    </tr>
 
    <tr>
 
      <td>NPY1</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>NADH diphosphatase</td>
 
      <td>43.5</td>
 
      <td>6.26</td>
 
      <td>846</td>
 
      <td>Peroxisome cytosol</td>
 
      <td>Hydrolyzes the pyrophosphate linkage in NADH and related nucleotides</td>
 
    </tr>
 
    <tr>
 
      <td>STR3</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td> Cystathionine β-lyase</td>
 
      <td>51.8</td>
 
      <td>7.96</td>
 
      <td>ND</td>
 
      <td>Peroxisome</td>
 
      <td>Converts cystathionine into homocysteine</td>
 
    </tr>
 
    <tr>
 
      <td>STR3</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Cystathionine ß-lyase</td>
 
      <td>51.8</td>
 
      <td>7.96</td>
 
      <td>ND</td>
 
      <td>Peroxisome</td>
 
      <td>Converts cystathionine into homocysteine</td>
 
    </tr>
 
    <tr>
 
      <td>GTO1</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td> ω-Class glutathione transferase </td>
 
      <td>41.3</td>
 
      <td>9.53</td>
 
      <td>-</td>
 
      <td>Peroxisome</td>
 
      <td>Induced under oxidative stress</td>
 
    </tr>
 
    <tr>
 
      <td>AAT2(ASP5)</td>
 
      <td>-</td>
 
      <td>Yes</td>
 
      <td>Aspartate aminotransferase</td>
 
      <td>46.1</td>
 
      <td>8.50</td>
 
      <td>7,700</td>
 
      <td>Cytosol, peroxisome</td>
 
      <td>Involved in nitrogen metabolism</td>
 
    </tr>
 
    <tr>
 
      <td>PCD1</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Nudix pyrophosphatase with specificity for coenzyme A and CoA derivatives</td>
 
      <td>39.8</td>
 
      <td>6.59</td>
 
      <td>238</td>
 
      <td>Peroxisome</td>
 
      <td>May function to remove potentially toxic oxidized CoA disulfide from peroxisomes</td>
 
    </tr>
 
    <tr>
 
      <td>LPX1</td>
 
      <td>-</td>
 
      <td>Yes</td>
 
      <td>Triacylglycerol lipase</td>
 
      <td>43.7</td>
 
      <td>8.16</td>
 
      <td>2,350</td>
 
      <td>Peroxisomal matrix</td>
 
      <td>-</td>
 
    </tr>
 
    <tr>
 
      <td colspan=”9”>Peroxisomal transporters</td>
 
    </tr>
 
    <tr>
 
      <td>PXA1 (LPI1, PAL1, PAT2, SSH2</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td> Subunit of a heterodimeric ATP-binding cassette transporter complex</td>
 
      <td>100.0</td>
 
      <td>10.34</td>
 
      <td>ND</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Import of long-chain fatty acids into peroxisomes</td>
 
    </tr>
 
    <tr>
 
      <td>PXA2 (PAT1)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Subunit of a heterodimeric ATP-binding cassette transporter complex</td>
 
      <td>97.1</td>
 
      <td>9.47</td>
 
      <td>ND</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Import of long-chain fatty acids into peroxisomes</td>
 
    </tr>
 
    <tr>
 
      <td>ANT1(YPR118C)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Adenine nucleotide transporter</td>
 
      <td>36.4</td>
 
      <td>10.6</td>
 
      <td>2,250</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Involved in β-oxidation of medium-chain fatty acids</td>
 
    </tr>
 
    <tr>
 
      <td colspan=”9”>Peroxins</td>
 
    </tr>
 
    <tr>
 
      <td>Pex1 (PAS1)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>AAA ATPase</td>
 
      <td>117.3</td>
 
      <td>6.93</td>
 
      <td>2,100</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Involved in recycling of Pex5, forms heterodimer with Pex6</td>
 
    </tr>
 
    <tr>
 
      <td>Pex2 (RT1, PAS5)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>E3 ubiquitin ligase</td>
 
      <td>30.8</td>
 
      <td>9.02</td>
 
      <td>339</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>RING finger protein, forms complex with Pex10 and Pex12. Involved in matrix protein import</td>
 
    </tr>
 
    <tr>
 
      <td>Pex3 (PAS3)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>50.7</td>
 
      <td>6.29</td>
 
      <td>1,400</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Required for proper localization of PMPs</td>
 
    </tr>
 
    <tr>
 
      <td>Pex4 (PAS2, UBC10)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Ubiquitin conjugating enzyme</td>
 
      <td>21.1</td>
 
      <td>5.36</td>
 
      <td>ND</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Involved in matrix protein import</td>
 
    </tr>
 
    <tr>
 
      <td>Pex5 (PAS10)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Soluble PTS1 receptor</td>
 
      <td>69.3</td>
 
      <td>4.79</td>
 
      <td>2,070</td>
 
      <td>Cytosol and peroxisomal matrix</td>
 
      <td>Required for import of PTS1-containing peroxisomal proteins, contains TPR domains</td>
 
    </tr>
 
    <tr>
 
      <td>Pex6 (PAS8)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>AAA ATPase</td>
 
      <td>115.6</td>
 
      <td>5.44</td>
 
      <td>1,630</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Involved in recycling of Pex5, forms heterodimer with Pex1</td>
 
    </tr>
 
    <tr>
 
      <td>Pex7 (PAS7, PEB1)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Soluble PTS2 receptor</td>
 
      <td>42.3</td>
 
      <td>8.34</td>
 
      <td>589</td>
 
      <td>Cytosol and peroxisomal matrix</td>
 
      <td>Requires Pex18 and Pex21 for association to the receptor docking site, contains WD40 repeat </td>
 
    </tr>
 
    <tr>
 
      <td>Pex8 (PAS6)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td> Intra peroxisomal organizer of the peroxisomal import machinery </td>
 
      <td>68.2</td>
 
      <td>7.62</td>
 
      <td>538</td>
 
      <td>Peroxisomal matrix and luminal membrane face</td>
 
      <td>Pex5-cargo dissociation</td>
 
    </tr>
 
    <tr>
 
      <td>Pex9</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>PTS-receptor</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>-</td>
 
    </tr>
 
    <tr>
 
      <td>Pex10</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>E3 ubiquitin ligase</td>
 
      <td>39.1</td>
 
      <td>9.88</td>
 
      <td>ND</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>RING finger protein involved in Ubc4-dependent Pex5 ubiquitination. Forms complex with Pex2 and Pex12 </td>
 
    </tr>
 
    <tr>
 
      <td>Pex11 (PMP24, PMP 27)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>26.9</td>
 
      <td>10.65</td>
 
      <td>1,630</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Involved in peroxisome fission, required for medium-chain fatty acid oxidation </td>
 
    </tr>
 
    <tr>
 
      <td>Pex12 (PAS11)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>E3 ubiquitin ligase</td>
 
      <td>46.0</td>
 
      <td>9.86</td>
 
      <td>907</td>
 
      <td>-</td>
 
      <td>RING finger protein, forms complex with Pex2 and Pex10</td>
 
    </tr>
 
    <tr>
 
      <td>Pex13 (PAS20)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Component of docking complex for Pex5 and Pex7</td>
 
      <td>42.7</td>
 
      <td>9.83</td>
 
      <td>7,900</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Forms complex with Pex14 and Pex17</td>
 
    </tr>
 
    <tr>
 
      <td>Pex14</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Central component of the receptor docking complex</td>
 
      <td>38.4</td>
 
      <td>4.61</td>
 
      <td>2,570</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Interacts with Pex13</td>
 
    </tr>
 
    <tr>
 
      <td>Pex15 (PAS21)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>43.7</td>
 
      <td>8.42</td>
 
      <td>1,070</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Recruitment of Pex6 to the peroxisomal membrane, tail anchored PMP</td>
 
    </tr>
 
    <tr>
 
      <td>Pex17 (PAS9)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Component of docking complex for Pex5 and Pex7</td>
 
      <td>23.2</td>
 
      <td>10.24</td>
 
      <td>656</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Forms complex with Pex13 and Pex14</td>
 
    </tr>
 
    <tr>
 
      <td>Pex18</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Required for PTS2 import</td>
 
      <td>32.0</td>
 
      <td>4.78</td>
 
      <td>ND</td>
 
      <td>Interacts with Pex7 partially redundant with Pex21</td>
 
    </tr>
 
    <tr>
 
      <td>Pex19 (PAS12)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Chaperone and import receptor for newly synthesized PMP</td>
 
      <td>38.7</td>
 
      <td>4.08</td>
 
      <td>5,350</td>
 
      <td>Cytosol, peroxisome, farnesylated</td>
 
      <td>Interacts with PMPs, involved in PMP sorting. Also interacts with Myo2 and contributes to peroxisome partitioning</td>
 
    </tr>
 
    <tr>
 
      <td>Pex21</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Required for PTS2 protein import</td>
 
      <td>33.0</td>
 
      <td>6.67</td>
 
      <td>ND</td>
 
      <td>Cytosol</td>
 
      <td>Interacts with Pex7, partially redundant with Pex18</td>
 
    </tr>
 
    <tr>
 
      <td>Pex22(YAF5)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Required for import of peroxisomal proteins</td>
 
      <td>19.9</td>
 
      <td>8.33</td>
 
      <td>259</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Recruits Pex4 to the peroxisomal membrane</td>
 
    </tr>
 
    <tr>
 
      <td>Pex25</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Involved in the regulation of peroxisome size and maintenance, required for re-introduction of peroxisomes in peroxisome deficient cells</td>
 
      <td>44.9</td>
 
      <td>9.77</td>
 
      <td>2,420</td>
 
      <td>Peripheral peroxisomal membrane</td>
 
      <td>Recruits GTPase RhoI to peroxisomes, interacts with homologous protein Pex27</td>
 
    </tr>
 
    <tr>
 
      <td>Pex27</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Involved in the regulation of peroxisome size and number</td>
 
      <td>44.1</td>
 
      <td>10.49</td>
 
      <td>382</td>
 
      <td>Peripheral peroxisomal membrane</td>
 
      <td>Interacts with homologous protein Pex25</td>
 
    </tr>
 
    <tr>
 
      <td>Pex28</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Involved in the regulation of peroxisome size, number and distribution</td>
 
      <td>66.1</td>
 
      <td>7.09</td>
 
      <td>ND</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>May act upstream of Pex30, Pex31 and Pex 32</td>
 
    </tr>
 
    <tr>
 
      <td>Pex29</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>63.5</td>
 
      <td>6.8</td>
 
      <td>5,040</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>May act upstream of Pex30, Pex31 and Pex32</td>
 
    </tr>
 
    <tr>
 
      <td>Pex30</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Involved in the regulation of peroxisome number</td>
 
      <td>59.5</td>
 
      <td>5.59</td>
 
      <td>4,570</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Negative regulator, partially functionally redundant with Pex31 and Pex32</td>
 
    </tr>
 
    <tr>
 
      <td>Pex31</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Involved in the regulation of peroxisome number</td>
 
      <td>52.9</td>
 
      <td>10.15</td>
 
      <td>238</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Negative regulator, partially functionally redundant with Pex30 and Pex32 </td>
 
    </tr>
 
    <tr>
 
      <td>Pex32</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Involved in the regulation of peroxisome number</td>
 
      <td>48.6</td>
 
      <td>9.14</td>
 
      <td>ND</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Negative regulator partially functionally redundant with Pex30 and Pex31</td>
 
    </tr>
 
    <tr>
 
      <td>Pex34</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Involved in the regulation of peroxisome number</td>
 
      <td>16.6</td>
 
      <td>10.30</td>
 
      <td>ND</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>-</td>
 
    </tr>
 
    <tr>
 
      <td colspan=”9”>Peroxisome fission and inheritance</td>
 
    </tr>
 
    <tr>
 
      <td>DYN2 (SLC1)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Light chain dynein</td>
 
      <td>10.4</td>
 
      <td>9.03</td>
 
      <td>1,310</td>
 
      <td>Cytosol</td>
 
      <td>Microtubule motor protein</td>
 
    </tr>
 
    <tr>
 
      <td>SEC20</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>v-SNARE</td>
 
      <td>43.9</td>
 
      <td>5.92</td>
 
      <td>4,910</td>
 
      <td>Golgi, ER</td>
 
      <td>Involved in retrograde transport from the Golgi to the ER, interacts with the Dsl1 complex through Tip20</td>
 
    </tr>
 
    <tr>
 
      <td>SEC39(DSL3)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Component of the Ds11p-tethering complex</td>
 
      <td>82.4</td>
 
      <td>4.65</td>
 
      <td>1,840</td>
 
      <td>ER, nuclear envelope</td>
 
      <td>Proposed to be involved in protein secretion</td>
 
    </tr>
 
    <tr>
 
      <td>DSL1 (RNS1)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Component of the ER target site that interacts with coatomer</td>
 
      <td>88.1</td>
 
      <td>4.69</td>
 
      <td>8,970</td>
 
      <td>Peripheral ER, Golgi membrane</td>
 
      <td>Forms a complex with Sec39 and Tip20 that interacts with ER SNAREs, Sec20 and Use1</td>
 
    </tr>
 
    <tr>
 
      <td>FIS1 (MDV2)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Required for peroxisome fission</td>
 
      <td>17.7</td>
 
      <td>9.87</td>
 
      <td>2,410</td>
 
      <td>Peroxisomal membrane mitochondria</td>
 
      <td>Tail anchored protein recruits Dnm1 via Mdv1/Caf4; also involved in mitochondrial fission</td>
 
    </tr>
 
    <tr>
 
      <td>DNM1</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>GTPase, dynamin like protein involved in peroxisome fission</td>
 
      <td>85.0</td>
 
      <td>5.25</td>
 
      <td>9,620</td>
 
      <td>-</td>
 
      <td>Also involved in mitochondrial fission</td>
 
    </tr>
 
    <tr>
 
      <td> VPS1 (GRD1, LAM1, SPO15, VPL1, VPT26)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>GTPase, dynamin like protein involved in peroxisome fission</td>
 
      <td>78.7</td>
 
      <td>8.15</td>
 
      <td>5,960</td>
 
      <td>-</td>
 
      <td>Also involved in vacuolar protein sorting</td>
 
    </tr>
 
    <tr>
 
      <td> VPS34 (END12, PEP15, VPL7, VPT29, STT8, VPS7)</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Phosphatidylinositol 3-kinase</td>
 
      <td>100.9</td>
 
      <td>7.79</td>
 
      <td>1,080</td>
 
      <td>-</td>
 
      <td>Forms complex with Vps15</td>
 
    </tr>
 
    <tr>
 
      <td>INP1</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Involved in retention of peroxisomes in mother cells</td>
 
      <td>47.3</td>
 
      <td>8.34</td>
 
      <td>639</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>Recruited to the peroxisome by binding to Pex3</td>
 
    </tr>
 
    <tr>
 
      <td>INP2</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>Myo2 receptor, involved in peroxisome inheritance</td>
 
      <td>81.5</td>
 
      <td>9.41</td>
 
      <td>736</td>
 
      <td>Peroxisomal membrane</td>
 
      <td>-</td>
 
    </tr>
 
    <tr>
 
      <td>RHO1</td>
 
      <td>-</td>
 
      <td>-</td>
 
      <td>GTP binding protein of the Rho subfamily of Ras like proteins, involved in actin assembly at the peroxisome</td>
 
      <td>23.2</td>
 
      <td>6.07</td>
 
      <td>ND</td>
 
      <td>-</td>
 
      <td>Involved in <em>de novo</em> peroxisome formation recruited to peroxisomes by Pex25</td>
 
    </tr>
 
  </tbody>
 
</table>
 
 
 
</article>
 
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Latest revision as of 10:12, 10 December 2017