Difference between revisions of "Team:York/Parts"

Revision as of 12:49, 16 September 2015 (view source) Lizalexianu (Talk | contribs) ← Older edit		Latest revision as of 23:16, 18 September 2015 (view source) Ab1443 (Talk | contribs)
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	<div class="col-md-10 layer">		<div class="col-md-10 layer">
	<!-- CONTENT GOES HERE :D -->		<!-- CONTENT GOES HERE :D -->
−		+	<br>
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	<div class="col-md-1"></div>		<div class="col-md-1"></div>
−	<div class="col-md-7">	+	<div class="col-md-10">
−	<table >	+	<table width="100%">
		+	<col style="width:30%">
		+	<col style="width:10%">
		+	<col style="width:10%">
		+	<col style="width:35%">
		+	<col style="width:5%">
		+	<col style="width:5%">
		+	<col style="width:5%">
	<tr>		<tr>
−	<td>Source Organism</td>	+	<td><b>Source Organism</b></td>
−	<td>Gene</td>	+	<td><b>Gene</b></td>
−	<td>Part Name</td>	+	<td><b>Part Name</b></td>
−	<td>Function</td>	+	<td class="width"><b>Function</b></td>
−	<td>Characterised?</td>	+	<td><b>Characterised</b></td>
−	<td>Sequenced?</td>	+	<td><b>Sequenced</b></td>
−	<td>Submitted?</td>	+	<td><b>Submitted</b></td>
	</tr>		</tr>
−	<tr>	+	<tr>
−	<td><i>Escherichia coli</i></td>	+	<td><b>Expression vector “pAdapt” in pSB1C3</b></td>
−	<td>EcPPK</td>	+	<td>lacZalpha</td>
−	<td></td>	+	<td><a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K1807000">BBa_K1807000</a></td>
−	<td>Phosphate Kinase</td>	+	<td class="width">Used as cloning vector</td>
		+	<td>✔</td>
		+	<td>✔</td>
		+	<td>✔</td>
		+	</tr>
		+	<tr>
		+	<td><i><b>Escherichia coli</b></i></td>
		+	<td>EcPPX</td>
		+	<td><a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K1807001">BBa_K1807001</a></td>
		+	<td class="width">Phosphate Kinase</td>
	<td></td>		<td></td>
	<td>✔</td>		<td>✔</td>
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	</tr>		</tr>
	<tr>		<tr>
−	<td></td>	+	<td><i><b>Escherichia coli</b></i></td>
−	<td>EcPhoE</td>	+	<td>EcPPK</td>
−	<td></td>	+	<td><a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K1807002">BBa_K1807002</a></td>
−	<td>Phosphoporin</td>	+	<td class="width">Phosphate Kinase</td>
	<td></td>		<td></td>
	<td>✔</td>		<td>✔</td>
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	</tr>		</tr>
	<tr>		<tr>
−	<td></td>	+	<td><i><b>Escherichia coli</b></i></td>
	<td>EcPstSCAB</td>		<td>EcPstSCAB</td>
	<td></td>		<td></td>
−	<td>Phosphate specific transporter</td>	+	<td class="width">Phosphate specific transporter</td>
	<td></td>		<td></td>
	<td>✔</td>		<td>✔</td>
−	<td>✔</td>	+	<td></td>
	</tr>		</tr>
	<tr>		<tr>
−	<td><i>Kingella oralis</i></td>	+	<td><i><b>Kingella oralis</b></i></td>
	<td>KoPPK</td>		<td>KoPPK</td>
−	<td></td>	+	<td><a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K1807006">BBa_K1807006</a></td>
−	<td>PolyPhosphate Kinase</td>	+	<td class="width">PolyPhosphate Kinase</td>
−	<td></td>	+	<td>✔</td>
	<td>✔</td>		<td>✔</td>
	<td>✔</td>		<td>✔</td>
	</tr>		</tr>
	<tr>		<tr>
−	<td><i>Sinorhizobium meliloti</i></td>	+	<td><i><b>Sinorhizobium meliloti</b></i></td>
	<td>SmPstSCAB</td>		<td>SmPstSCAB</td>
	<td></td>		<td></td>
−	<td>Phosphate specific transporter</td>	+	<td class="width">Phosphate specific transporter</td>
−	<td></td>	+
	<td>✔</td>		<td>✔</td>
−	<td>✔</td>
−	</tr>
−	<tr>
−	<td><i>Candidatus accumulibacter phosphatis</i></td>
−	<td>ApPstSCAB</td>
−	<td></td>
−	<td>Phosphate specific transporter</td>
−	<td></td>
	<td>✔</td>		<td>✔</td>
	<td>✔</td>		<td>✔</td>
	</tr>		</tr>
	<tr>		<tr>
−	<td></td>	+	<td><i><b>Candidatus Accumulibacter phosphatis</b></i></td>
	<td>ApPPK BA-91</td>		<td>ApPPK BA-91</td>
−	<td></td>	+	<td><a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K1807003">BBa_K1807003</a></td>
−	<td>PolyPhosphate kinase</td>	+	<td class="width">PolyPhosphate kinase</td>
−	<td></td>	+	<td>✔</td>
	<td>✔</td>		<td>✔</td>
	<td>✔</td>		<td>✔</td>
	</tr>		</tr>
	<tr>		<tr>
−	<td></td>	+	<td><i><b>Candidatus Accumulibacter phosphatis</b></i></td>
	<td>ApPPK SK-12</td>		<td>ApPPK SK-12</td>
−	<td></td>	+	<td><a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K1807004">BBa_K1807004</a></td>
−	<td>PolyPhosphate kinase</td>	+	<td class="width">PolyPhosphate kinase</td>
−	<td></td>	+	<td>✔</td>
	<td>✔</td>		<td>✔</td>
	<td>✔</td>		<td>✔</td>
	</tr>		</tr>
	<tr>		<tr>
−	<td></td>	+	<td><i><b>Candidatus Accumulibacter phosphatis</b></i></td>
	<td>ApPPK UW-1</td>		<td>ApPPK UW-1</td>
−	<td></td>	+	<td><a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K1807005">BBa_K1807005</a></td>
−	<td>PolyPhosphate kinase</td>	+	<td class="width">PolyPhosphate kinase</td>
−	<td></td>	+	<td>✔</td>
	<td>✔</td>		<td>✔</td>
	<td>✔</td>		<td>✔</td>
	</tr>		</tr>
−	<tr>	+	<tr>
−	<td>Expression vector “pAdapt” in pSB1C3</td>	+	<td><i><b>Candidatus Accumulibacter phosphatis</b></i></td>
−	<td></td>	+	<td>ApPstSCAB</td>
−	<td>BBa_K1807000</td>	+	<td><a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K1807007">BBa_K1807007</a></td>
−	<td>Used as cloning vector</td>	+	<td class="width">Phosphate specific transporter</td>
	<td></td>		<td></td>
	<td>✔</td>		<td>✔</td>
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	</tr>		</tr>
	</table>		</table>
−	</div>
−	<div class="col-md-4"></div>
−
	</div>		</div>
	<div class="col-md-1"></div>		<div class="col-md-1"></div>
−	</body>
−	<!--	+	<div class="col-md-12">
−	<p>Each team will make new parts during iGEM and will submit them to the Registry of Standard Biological Parts. The iGEM software provides an easy way to present the parts your team has created. The <code>&lt;groupparts&gt;</code> tag (see below) will generate a table with all of the parts that your team adds to your team sandbox.</p>	+	<h1>So what do all of these parts do?</h1>
−	<p>Remember that the goal of proper part documentation is to describe and define a part, so that it can be used without needing to refer to the primary literature. Registry users in future years should be able to read your documentation and be able to use the part successfully. Also, you should provide proper references to acknowledge previous authors and to provide for users who wish to know more.</p>	+
		+	<div class="col-md-3">
		+	<div class="navbar">
		+	<ul>
		+	<li style="display:block;">Click to view:</li>
		+	<li style="display:block;" onclick="toggleSection('BBa_K1807000')">BBa_K1807000</li>
		+	<li style="display:block;" onclick="toggleSection('BBa_K1807001')">BBa_K1807001</li>
		+	<li style="display:block;" onclick="toggleSection('BBa_K1807002')">BBa_K1807002</li>
		+	<li style="display:block;" onclick="toggleSection('BBa_K1807003')">BBa_K1807003</li>
		+	<li style="display:block;" onclick="toggleSection('BBa_K1807004')">BBa_K1807004</li>
		+	<li style="display:block;" onclick="toggleSection('BBa_K1807005')">BBa_K1807005</li>
		+	<li style="display:block;" onclick="toggleSection('BBa_K1807006')">BBa_K1807006</li>
		+	<li style="display:block;" onclick="toggleSection('BBa_K1807007')">BBa_K1807007</li>
		+	</ul>
		+	</div>
		+	</div>
−	<div class="highlightBox">	+	<div class="col-md-9">
−	<h4>Note</h4>	+	<div class="section" id="BBa_K1807000">
−	<p>Note that parts must be documented on the <a href="http://parts.igem.org/Main_Page"> Registry</a>. This page serves to <i>showcase</i> the parts you have made. Future teams and other users and are much more likely to find parts by looking in the Registry than by looking at your team wiki.</p>	+	<h3>BBa_K1807000</h3>
		+	<ul>
		+	<li>This device allows for the IPTG-inducible expression of lacZα peptide which in the presence of Xgal in the medium and chromosomal lacZΔM15 produces blue-coloured colonies. The device was used as an expression vector. SmaI restriction sites flank the lacZ alpha coding sequence. Cutting the part with this enzyme allows for the in-frame insertion of any desired protein coding sequence that contains the splice-in flanking sequences (they can be found in the design section). </li>
		+	<li>BBa_K1807000 was designed as a blue-white screening device that would also be easily used in Gibson Assembly. Surrounding the lacZ alpha coding sequence are two SmaI restriction sites (CCC/GGG). SmaI is a blunt-end endonuclease- we used it to simulatenously linearize our vector and remove the lacZ alpha coding sequence. Our BioBricks contained overhangs that make them compatible with the SmaI-digested BBa_K1807000.
		+	The overhang sequences used to make this part are as follows:
		+	<br>- BBa_K1807000 Assembly 5'end Overhang (complementary to pSB1C3): cgctaaggatgatttctgGAATTCGCGGCCGCTTCTAGAG
		+	<br>- BBa_K1807000 Assembly 3'end Overhang (complementary to pSB1C3): TACTAGTAGCGGCCGCTGCAGtccggcaaaaaagggcaag
		+	The subparts of the device are as follows: BBa_R0011, BBa_B0034, BBa_E0038, BBa_B0015.</li>
		+	</ul>
		+	</div>
	</div>		</div>
		+	<div class="col-md-9">
		+	<div class="section" id="BBa_K1807001">
		+	<h3>BBa_K1807001</h3>
		+	<ul>
		+	<li>This part codes for the exopolyphosphatase (PPX) enzyme of <i>Escherichia coli</i>. PPX is able to release phosphate residues from the ends of a polyphosphate chain.</li>
		+	</ul>
		+	</div>
		+	</div>
		+	<div class="col-md-9">
		+	<div class="section" id="BBa_K1807002">
		+	<h3>BBa_K1807002</h3>
		+	<ul>
		+	<li>This part is a protein coding device containing the Polyphosphate Kinase (PPK) gene from <i>Escherichia coli</i>. PPK produces polyphosphate, more specifically PPK catalyzes the reversible conversion of the γ-phosphate of ATP to the end of the polyphosphate chain (Akiyama et al., 1992). This enzyme is responsible for the formation of long chain polyphosphate molecules (up to a thousand orthophosphate residues long).</li>
		+	</ul>
		+	</div>
		+	</div>
−	<h4>Adding parts to the registry</h4>	+	<div class="col-md-9">
−	<p>You can add parts to the Registry at our <a href="http://parts.igem.org/Add_a_Part_to_the_Registry">Add a Part to the Registry</a> link.</p>	+	<div class="section" id="BBa_K1807003">
−	<p>We encourage teams to start completing documentation for their parts on the Registry as soon as you have it available. The sooner you put up your parts, the better you will remember all the details about your parts. Remember, you don't need to send us the DNA sample before you create an entry for a part on the Registry. (However, you <b>do</b> need to send us the DNA sample before the Jamboree. If you don't send us a DNA sample of a part, that part will not be eligible for awards and medal criteria.)</p>	+	<h3>BBa_K1807003</h3>
−		+	<ul>
−		+	<li>This part is a protein coding device containing the Polyphosphate Kinase (PPK) gene from <i>Candidatus Accumulibacter phosphatis</i> strain BA-91. PPK produces polyphosphate, more specifically PPK catalyzes the reversible conversion of the γ-phosphate of ATP to the end of the polyphosphate chain. This enzyme is responsible for the formation of long chain polyphosphate molecules (up to a thousand orthophosphate residues long).</li>
−	<h4>What information do I need to start putting my parts on the Registry?</h4>	+	</ul>
−	<p>The information needed to initially create a part on the Registry is:</p>	+	</div>
−	<ul>	+	</div>
−	<li>Part Name</li>	+
−	<li>Part type</li>	+
−	<li>Creator</li>	+
−	<li>Sequence</li>	+
−	<li>Short Description (60 characters on what the DNA does)</li>	+
−	<li>Long Description (Longer description of what the DNA does)</li>	+
−	<li>Design considerations</li>	+
−	</ul>	+
−		+
−	<p>	+
−	We encourage you to put up <em>much more</em> information as you gather it over the summer. If you have images, plots, characterization data and other information, please also put it up on the part page. </p>	+
−		+
−		+
−		+
−		+
−		+
−		+
−	<h4>Inspiration</h4>	+
−	<p>We have a created  a <a href="http://parts.igem.org/Well_Documented_Parts">collection of well documented parts</a> that can help you get started.</p>	+
−		+
−	<p> You can also take a look at how other teams have documented their parts in their wiki:</p>	+
−	<ul>	+
−	<li><a href="https://2014.igem.org/Team:MIT/Parts"> 2014 MIT </a></li>	+
−	<li><a href="https://2014.igem.org/Team:Heidelberg/Parts"> 2014 Heidelberg</a></li>	+
−	<li><a href="https://2014.igem.org/Team:Tokyo_Tech/Parts">2014 Tokyo Tech</a></li>	+
−	</ul>	+
−	-->	+
		+	<div class="col-md-9">
		+	<div class="section" id="BBa_K1807004">
		+	<h3>BBa_K1807004</h3>
		+	<ul>
		+	<li>This part is a protein coding device containing the Polyphosphate Kinase (PPK) gene from <i>Candidatus Accumulibacter phosphatis</i> strain Sk-12. PPK produces polyphosphate, more specifically PPK catalyzes the reversible conversion of the γ-phosphate of ATP to the end of the polyphosphate chain. This enzyme is responsible for the formation of long chain polyphosphate molecules (up to a thousand orthophosphate residues long).</li>
		+	</ul>
		+	</div>
		+	</div>
		+	<div class="col-md-9">
		+	<div class="section" id="BBa_K1807005">
		+	<h3>BBa_K1807005</h3>
		+	<ul>
		+	<li>This part is a protein coding device containing the Polyphosphate Kinase (PPK) gene from <i>Candidatus Accumulibacter phosphatis</i> strain UW-1. PPK produces polyphosphate, more specifically PPK catalyzes the reversible conversion of the γ-phosphate of ATP to the end of the polyphosphate chain. This enzyme is responsible for the formation of long chain polyphosphate molecules (up to a thousand orthophosphate residues long).</li>
		+	</ul>
		+	</div>
		+	</div>
		+	<div class="col-md-9">
		+	<div class="section" id="BBa_K1807006">
		+	<h3>BBa_K1807006</h3>
		+	<ul>
		+	<li>This part is a protein coding device containing the Polyphosphate Kinase (PPK) gene from <i>Kingella oralis</i>. PPK produces polyphosphate, more specifically PPK catalyzes the reversible conversion of the γ-phosphate of ATP to the end of the polyphosphate chain. This enzyme is responsible for the formation of long chain polyphosphate molecules (up to a thousand orthophosphate residues long).</li>
		+	</ul>
		+	</div>
		+	</div>
		+	<div class="col-md-9">
		+	<div class="section" id="BBa_K1807007">
		+	<h3>BBa_K1807007</h3>
		+	<ul>
		+	<li>This part is a protein coding device containing the Phosphate Specific Transporter (Pst) gene from <i>Candidatus Accumulibacter phosphatis</i>SCAB. This transporter consists of 4 individual genes- pstA, pstC, pstB and pstS. PstA and pstC are phosphate transporter permeases, pstB is a phosphate transporter ATPase and pstS is a phosphate transporter periplasmic binding protein. </li>
		+	</ul>
		+	</div>
		+	</div>
		+	</div>
		+	</div>
		+	<div class="col-md-1"></div>
		+	</body>
		+	<script>
		+	function toggleSection(sectionID) {
		+	$('.section').hide(); // this hides all currently open div of class(if any);
		+	$('#' + sectionID).fadeIn(500); // show desired div
		+	}
		+	$('.section').hide(); //All div start hidden
		+	$(document).ready(function(){
		+	$("img").click(function() {
		+	$(this).toggleClass("bigger");
		+	});
		+	});
		+	</script>
	</html>		</html>

---

Latest revision as of 23:16, 18 September 2015

• Home
• Project
  • Description
  • Project Breakdown
  • Modeling
• Parts
  • Parts
  • Basic Parts
  • Composite Parts
  • Part Collection
  • Part Guide
• Human Practices
  • Outreach
  • Survey
  • Collaborations
  • Business Plan
• Notebooks
  • Team Notebook
  • Protocols
• About Us
  • Team Bios
  • Attributions
  • Acknowledgements
  • Sponsors

Part Table

Source Organism	Gene	Part Name	Function	Characterised	Sequenced	Submitted
Expression vector “pAdapt” in pSB1C3	lacZalpha	BBa_K1807000	Used as cloning vector	✔	✔	✔
Escherichia coli	EcPPX	BBa_K1807001	Phosphate Kinase		✔	✔
Escherichia coli	EcPPK	BBa_K1807002	Phosphate Kinase		✔	✔
Escherichia coli	EcPstSCAB		Phosphate specific transporter		✔
Kingella oralis	KoPPK	BBa_K1807006	PolyPhosphate Kinase	✔	✔	✔
Sinorhizobium meliloti	SmPstSCAB		Phosphate specific transporter	✔	✔	✔
Candidatus Accumulibacter phosphatis	ApPPK BA-91	BBa_K1807003	PolyPhosphate kinase	✔	✔	✔
Candidatus Accumulibacter phosphatis	ApPPK SK-12	BBa_K1807004	PolyPhosphate kinase	✔	✔	✔
Candidatus Accumulibacter phosphatis	ApPPK UW-1	BBa_K1807005	PolyPhosphate kinase	✔	✔	✔
Candidatus Accumulibacter phosphatis	ApPstSCAB	BBa_K1807007	Phosphate specific transporter		✔	✔

So what do all of these parts do?

• Click to view:
• BBa_K1807000
• BBa_K1807001
• BBa_K1807002
• BBa_K1807003
• BBa_K1807004
• BBa_K1807005
• BBa_K1807006
• BBa_K1807007

BBa_K1807000

• This device allows for the IPTG-inducible expression of lacZα peptide which in the presence of Xgal in the medium and chromosomal lacZΔM15 produces blue-coloured colonies. The device was used as an expression vector. SmaI restriction sites flank the lacZ alpha coding sequence. Cutting the part with this enzyme allows for the in-frame insertion of any desired protein coding sequence that contains the splice-in flanking sequences (they can be found in the design section).
• BBa_K1807000 was designed as a blue-white screening device that would also be easily used in Gibson Assembly. Surrounding the lacZ alpha coding sequence are two SmaI restriction sites (CCC/GGG). SmaI is a blunt-end endonuclease- we used it to simulatenously linearize our vector and remove the lacZ alpha coding sequence. Our BioBricks contained overhangs that make them compatible with the SmaI-digested BBa_K1807000. The overhang sequences used to make this part are as follows:
  - BBa_K1807000 Assembly 5'end Overhang (complementary to pSB1C3): cgctaaggatgatttctgGAATTCGCGGCCGCTTCTAGAG
  - BBa_K1807000 Assembly 3'end Overhang (complementary to pSB1C3): TACTAGTAGCGGCCGCTGCAGtccggcaaaaaagggcaag The subparts of the device are as follows: BBa_R0011, BBa_B0034, BBa_E0038, BBa_B0015.

BBa_K1807001

• This part codes for the exopolyphosphatase (PPX) enzyme of Escherichia coli. PPX is able to release phosphate residues from the ends of a polyphosphate chain.

BBa_K1807002

• This part is a protein coding device containing the Polyphosphate Kinase (PPK) gene from Escherichia coli. PPK produces polyphosphate, more specifically PPK catalyzes the reversible conversion of the γ-phosphate of ATP to the end of the polyphosphate chain (Akiyama et al., 1992). This enzyme is responsible for the formation of long chain polyphosphate molecules (up to a thousand orthophosphate residues long).

BBa_K1807003

• This part is a protein coding device containing the Polyphosphate Kinase (PPK) gene from Candidatus Accumulibacter phosphatis strain BA-91. PPK produces polyphosphate, more specifically PPK catalyzes the reversible conversion of the γ-phosphate of ATP to the end of the polyphosphate chain. This enzyme is responsible for the formation of long chain polyphosphate molecules (up to a thousand orthophosphate residues long).

BBa_K1807004

• This part is a protein coding device containing the Polyphosphate Kinase (PPK) gene from Candidatus Accumulibacter phosphatis strain Sk-12. PPK produces polyphosphate, more specifically PPK catalyzes the reversible conversion of the γ-phosphate of ATP to the end of the polyphosphate chain. This enzyme is responsible for the formation of long chain polyphosphate molecules (up to a thousand orthophosphate residues long).

BBa_K1807005

• This part is a protein coding device containing the Polyphosphate Kinase (PPK) gene from Candidatus Accumulibacter phosphatis strain UW-1. PPK produces polyphosphate, more specifically PPK catalyzes the reversible conversion of the γ-phosphate of ATP to the end of the polyphosphate chain. This enzyme is responsible for the formation of long chain polyphosphate molecules (up to a thousand orthophosphate residues long).

BBa_K1807006

• This part is a protein coding device containing the Polyphosphate Kinase (PPK) gene from Kingella oralis. PPK produces polyphosphate, more specifically PPK catalyzes the reversible conversion of the γ-phosphate of ATP to the end of the polyphosphate chain. This enzyme is responsible for the formation of long chain polyphosphate molecules (up to a thousand orthophosphate residues long).

BBa_K1807007

• This part is a protein coding device containing the Phosphate Specific Transporter (Pst) gene from Candidatus Accumulibacter phosphatisSCAB. This transporter consists of 4 individual genes- pstA, pstC, pstB and pstS. PstA and pstC are phosphate transporter permeases, pstB is a phosphate transporter ATPase and pstS is a phosphate transporter periplasmic binding protein.