From 2014.igem.org

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Revision as of 23:38, 16 October 2014

Imperial iGEM 2014

Parts

Featured Parts
Table of Parts

Overview

(INSERT BRIEF OVERVIEW HERE)

Key Achievements

Featured Parts

BBa_K1321340

N-terminal linker + double CBD

Double cellulose binding domain (dCBD) using two cellulose binding domains from Trichoderma reesei cellobiohydrolases, with an N-terminal linker and internal linker sequence between the two domains which are derived from the endogenous cellobiohydrolase linker sequence. This part is in RFC(25) Freiberg fusion format to allow for easy use in protein fusions.

BBa_K1321339

CBDcenA + Linker

Cellulose binding domain (CBD) of Endoglucanase A (cenA) from Cellulomonas fimi with an endogenous C-terminal linker. The part is in Freiburg format (RFC 25) for ease of use in protein fusions.

BBa_K1321014

CBDcipA with N and C-terminal linker

This CBD is from the Cellulosomal -scaffolding protein A (cipA) of Clostridium thermocellum including the endogenous linker sequences at the N and C-terminus. It is in RFC25 format to allow for easy use in protein fusions. At present the cloning for these constructs is still in progress to correct an illegal EcoRI site which was identified in the parts with this CBD. This can be achieved with a silent mutation via site-directed mutagenesis and we aim to send these parts to the registry once this is complete.

BBa_K1321005

Synthetic Phytochelatin (PC) EC20

A general heavy metal-binding peptide consisting of 20 Glu-Cys (EC) repeats in Freiburg format (RFC[25]) to allow for easy use in fusion proteins. We created a library of CBD fusions with this part and demonstrated [INSERT FINAL RESULTS SENTENCE HERE]

BBa_K1321200

Vitreoscilla haemoglobin (VhB)

This part is a haemoglobin isolated from Vitreoscilla (VHb) which increases cell metabolism. We used it as one technique to try and enhance cellulose production in G. xylinus .

BBa_K1321300, BBa_K1321301

pSEVA331 and pSEVA321 backbones

These are two broad host range vector backbones for which we have demonstrated use in E. coli and Gluconacetobacter xylinus .

BBa_K1321334, BBa_K1321335

Cellulose synthase operon AcsAB and AcsCD

Designed and refactored from G. xylinus, this operon was inserted into E.coli for cellulose synthesis.

BBa_K1321305, BBa_K1321306

Gluconacetobacter xylinus strains ATCC53582 and Kombucha Isolate

We created and characterised a library of parts for this organism, with the aim to increase the accessibility the chassis for future work in iGEM. By sharing these strains and their genomes on the registry we hope this will contribute to their ease of use and characterisation.

Table of Parts

<groupparts>iGEM014 Imperial</groupparts>

@@ Line 46: / Line 46: @@
                          <h2>Featured Parts</h2>
                          <div>
-                             <h3>Featured Part 1</h3>
+                             <h3><a href="http://parts.igem.org/BBa_K1321340">BBa_K1321340</a></h3>
                              <div>
                                  <div class="pure-g">
                                      <div class="pure-u-1-3">
-                                         <p>Part name/ID</p>
+                                         <p>N-terminal linker + double CBD</p>
                                      </div>
                                      <div class="pure-u-2-3">
-                                         <p>Part description</p>
+                                         <p>Double cellulose binding domain (dCBD) using two cellulose binding domains from <i>Trichoderma reesei</i> cellobiohydrolases, with an N-terminal linker and internal linker sequence between the two domains which are derived from the endogenous cellobiohydrolase linker sequence. This part is in RFC(25) Freiberg fusion format to allow for easy use in protein fusions.
+</p>
                                      </div>
                                  </div>
@@ Line 59: / Line 60: @@
                              </div>
-                         <h3>Featured Part 2</h3>
+                         <h3><a href="http://parts.igem.org/BBa_K1321339">BBa_K1321339</a></h3>
                              <div>
                                  <div class="pure-g">
                                      <div class="pure-u-1-3">
-                                         <p>Part name/ID</p>
+                                         <p>CBDcenA + Linker</p>
                                      </div>
                                      <div class="pure-u-2-3">
-                                         <p>Part description</p>
+                                         <p>Cellulose binding domain (CBD) of Endoglucanase A (cenA) from <i>Cellulomonas fimi</i> with an endogenous C-terminal linker. The part is in Freiburg format (RFC 25) for ease of use in protein fusions.</p>
                                      </div>
                                  </div>
@@ Line 72: / Line 73: @@
                              </div>
-                             <h3>Featured Part 3</h3>
+                             <h3><a href="http://parts.igem.org/BBa_K1321014"> BBa_K1321014</a></h3>
                              <div>
                                  <div class="pure-g">
                                      <div class="pure-u-1-3">
-                                         <p>Part name/ID</p>
+                                         <p>CBDcipA with N and C-terminal linker </p>
                                      </div>
                                      <div class="pure-u-2-3">
-                                         <p>Part description</p>
+                                         <p>This CBD is from the Cellulosomal -scaffolding protein A (cipA) of <i>Clostridium thermocellum </i> including the endogenous linker sequences at the N and C-terminus. It is in RFC25 format to allow for easy use in protein fusions. At present the cloning for these constructs is still in progress to correct an illegal EcoRI site which was identified in the parts with this CBD. This can be achieved with a silent mutation via site-directed mutagenesis and we aim to send these parts to the registry once this is complete.
+</p>
                                      </div>
                                  </div>
@@ Line 85: / Line 87: @@
                              </div>
-                             <h3>Featured Part 4</h3>
+                             <h3><a href="http://parts.igem.org/BBa_K1321005">BBa_K1321005</a></h3>
                              <div>
                                  <div class="pure-g">
                                      <div class="pure-u-1-3">
-                                         <p>Part name/ID</p>
+                                         <p>Synthetic Phytochelatin (PC) EC20</p>
                                      </div>
                                      <div class="pure-u-2-3">
-                                         <p>Part description</p>
+                                         <p>A general heavy metal-binding peptide consisting of 20 Glu-Cys (EC) repeats in Freiburg format (RFC[25]) to allow for easy use in fusion proteins. We created a library of CBD fusions with this part and demonstrated [INSERT FINAL RESULTS SENTENCE HERE]
+</p>
+                                    </div>
+                                </div>
+                                </div>
+                                <h3><a href="http://parts.igem.org/BBa_K1321200">BBa_K1321200</a></h3>
+                                <div>
+                                <div class="pure-g">
+                                    <div class="pure-u-1-3">
+                                        <p><i>Vitreoscilla</i> haemoglobin (VhB)</p>
+                                    </div>
+                                    <div class="pure-u-2-3">
+                                        <p>This part is a haemoglobin isolated from Vitreoscilla (VHb) which increases cell metabolism. We used it as one technique to try and enhance cellulose production in <i> G. xylinus </i>.
+</p>
                                      </div>
                                  </div>
                              </div>
+                            <h3><a href="http://parts.igem.org/BBa_K1321300">BBa_K1321300</a>, <a href="http://parts.igem.org/BBa_K1321301">BBa_K1321301</a> </h3>
+                            <div>
+                                <div class="pure-g">
+                                    <div class="pure-u-1-3">
+                                        <p>pSEVA331 and pSEVA321 backbones</p>
+                                    </div>
+                                    <div class="pure-u-2-3">
+                                        <p>These are two broad host range vector backbones for which we have demonstrated use in <i>E. coli</i> and <i>Gluconacetobacter xylinus </i>.
+</p>
+                                    </div>
+                                </div>
+                            </div>
+                            <h3><a href="http://parts.igem.org/BBa_K1321334"> BBa_K1321334</a>, <a href="http://parts.igem.org/BBa_K1321335">BBa_K1321335</a></h3>
+                            <div>
+                                <div class="pure-g">
+                                    <div class="pure-u-1-3">
+                                        <p>Cellulose synthase operon AcsAB and AcsCD</p>
+                                    </div>
+                                    <div class="pure-u-2-3">
+                                        <p>Designed and refactored from <i>G. xylinus</i>, this operon was inserted into <i>E.coli </i> for cellulose synthesis.
+</p>
+                                    </div>
+                                </div>
+</div>
+                            <h3><a href="http://parts.igem.org/BBa_K1321305">BBa_K1321305</a>,<a href="http://parts.igem.org/BBa_K1321306"> BBa_K1321306</a></h3>
+                            <div>
+                                <div class="pure-g">
+                                    <div class="pure-u-1-3">
+                                        <p><i>Gluconacetobacter xylinus</i> strains ATCC53582 and Kombucha Isolate</p>
+                                    </div>
+                                    <div class="pure-u-2-3">
+                                        <p>We created and characterised a library of parts for this organism, with the aim to increase the accessibility the chassis for future work in iGEM. By sharing these strains and their genomes on the registry we hope this will contribute to their ease of use and characterisation.
+</p>
+                                    </div>
+                                </div>
+                         </div>
                  </div>

Team:Imperial/Parts