Difference between revisions of "Team:Nankai/Parts"

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Parts Abstract

Number	Name	Type	Description	Creator	Length
BBa_K1628001	P_bca	Promoter	an original promoter of coding sequence pgsBCA operon	Tianyi Huang	364
BBa_K1628002	P_xyl	Promoter	a promoter of xylose operon	Tianyi Huang	217
BBa_K1628003	BJ27UP	Promoter	an artificially synthesized promoter	Xinhao Song	100
BBa_K1628004	C2up	Promoter	an artificially synthesized promoter	Xinhao Song	108
BBa_K1628005	A2up	Promoter	an artificially synthesized promoter	Yibing Wei	107
BBa_K1628006	P43	Promoter	a strong promoter in Bacillus subtilis 168	Yibing Wei	445
BBa_K1628007	P_amyA	Promoter	a strong promoter in Bacillus amyloliquefaciens LL3	Zhaoran Zhang	613
BBa_K1628101	pgsB	Coding	a gene responsible for γ-PGA synthesis in pgsBCA operon	Tianyi Huang	1182
BBa_K1628102	pgsCA	Coding	a coding gene in pgsBCA operon	Xinhao Song	1631
BBa_K1628201	P_lacI/lacI	Translational Unit	a promoter of lactose operon along with a repressor of lactose operon regulating the promoter	Yibing Wei	1386
BBa_K1628202	P_grac	Promoter	a promoter of lactose operon regulated by repressor LacI	Tianyi Huang	120
BBa_K1628203	xylR	Coding	a repressor of xylose operon regulating promoter P_xyl	Zhaoran Zhang	1167
BBa_K1628301	P1-GFP	Device	P3-GFP is a composite part used for the Measurement track of this year. This part consists of the promoter part of BBa_J23117, the official GFP device (with an RBS, GFP coding sequence and a set of double terminators) and a pSB1C3 backbone. We transformed this plasmid into E. coli cells and the fluorescence intensity of the GFP protein that was expressed by the bacteria was measured afterwards by a flow cytometry.	Tianyi Huang	?
BBa_K1628202	P2-GFP	Device	P2-GFP is a composite part used for the Measurement track of this year. This part consists of the promoter part of BBa_J23106, the official GFP device (with an RBS, GFP coding sequence and a set of double terminators) and a pSB1C3 backbone. We transformed this plasmid into E. coli cells and the fluorescence intensity of the GFP protein that was expressed by the bacteria was measured afterwards by a flow cytometry.	Xinhao Song	?
BBa_K1628303	P3-GFP	Device	P3-GFP is a composite part used for the Measurement track of this year. This part consists of the promoter part of BBa_J23117, the official GFP device (with an RBS, GFP coding sequence and a set of double terminators) and a pSB1C3 backbone. We transformed this plasmid into E. coli cells and the fluorescence intensity of the GFP protein that was expressed by the bacteria was measured afterwards by a flow cytometry.	Yibing Wei	?

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Difference between revisions of "Team:Nankai/Parts"

Latest revision as of 21:51, 18 September 2015

Team Parts

Parts Abstract

Team Parts

Basic Parts

Composite Parts

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 		<div class="parallax-overlay">
                      <p>Your place:&nbsp;<a href="https://2015.igem.org/Team:Nankai">Home</a>&nbsp;&gt;&nbsp;<a href="https://2015.igem.org/Team:Nankai/Parts">Parts</a></p>
@@ Line 115: / Line 33: @@
 			<div class="col-md-8 blog-posts">
 <h4>Parts Abstract</h4>
-<table width="544" border="1">
+<table width="544" border="1":font-family:"Gill Sans MT",Consolas,Constantia;>
    <tr>
      <th width="78" bgcolor="#999999" scope="col">Number</th>
@@ Line 126: / Line 44: @@
    <tr>
      <td bgcolor="#CCCCCC"><a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K1628001">BBa_K1628001</a></td>
-     <td bgcolor="#CCCCCC"><span class="zaq">Pbca</span></td>
+     <td bgcolor="#CCCCCC"><span class="zaq">P<sub>bca</sub></span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">Promoter</span></td>
-     <td bgcolor="#CCCCCC"><span class="zaq"> an original promoter of coding sequence pgsBCA</span></td>
+     <td bgcolor="#CCCCCC"><span class="zaq"> an original promoter of coding sequence <em>pgsBCA</em> operon</span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">Tianyi Huang</span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">364</span></td>
@@ Line 134: / Line 52: @@
    <tr>
      <td bgcolor="#CCCCCC"><a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K1628002">BBa_K1628002</a></td>
-     <td bgcolor="#FFFFFF"><span class="zaq">SPxyl </span></td>
+     <td bgcolor="#FFFFFF"><span class="zaq">P<sub>xyl</sub></span></td>
      <td bgcolor="#FFFFFF"><span class="zaq">Promoter</span></td>
-     <td bgcolor="#FFFFFF">&nbsp;</td>
+     <td bgcolor="#FFFFFF">a promoter of xylose operon</td>
      <td bgcolor="#FFFFFF"><span class="zaq">Tianyi Huang</span></td>
      <td bgcolor="#FFFFFF"><span class="zaq">217</span></td>
@@ Line 144: / Line 62: @@
      <td bgcolor="#CCCCCC"><span class="zaq">BJ27UP</span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">Promoter</span></td>
-     <td bgcolor="#CCCCCC"><span class="zaq">a synthetic promoter</span></td>
+     <td bgcolor="#CCCCCC">an artificially synthesized promoter</td>
      <td bgcolor="#CCCCCC"><span class="zaq">Xinhao Song</span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">100</span></td>
@@ Line 152: / Line 70: @@
      <td bgcolor="#FFFFFF"><span class="zaq">C2up</span></td>
      <td bgcolor="#FFFFFF"><span class="zaq">Promoter</span></td>
-     <td bgcolor="#FFFFFF">&nbsp;</td>
+     <td bgcolor="#FFFFFF">an artificially synthesized promoter</td>
      <td bgcolor="#FFFFFF"><span class="zaq">Xinhao Song</span></td>
      <td bgcolor="#FFFFFF"><span class="zaq">108</span></td>
@@ Line 158: / Line 76: @@
    <tr>
      <td bgcolor="#CCCCCC"><a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K1628005">BBa_K1628005</a></td>
-     <td bgcolor="#CCCCCC"><span class="zaq">A2cup</span></td>
+     <td bgcolor="#CCCCCC"><span class="zaq">A2up</span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">Promoter</span></td>
-     <td bgcolor="#CCCCCC">&nbsp;</td>
+     <td bgcolor="#CCCCCC">an artificially synthesized  promoter</td>
      <td bgcolor="#CCCCCC"><span class="zaq">Yibing Wei</span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">107</span></td>
@@ Line 168: / Line 86: @@
      <td><span class="zaq">P43</span></td>
      <td><span class="zaq">Promoter</span></td>
-     <td>&nbsp;</td>
+     <td>a strong promoter in <em>Bacillus subtilis </em>168</td>
      <td><span class="zaq">Yibing Wei</span></td>
      <td><span class="zaq">445</span></td>
@@ Line 174: / Line 92: @@
    <tr>
      <td bgcolor="#CCCCCC"><a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K1628007">BBa_K1628007</a></td>
-     <td bgcolor="#CCCCCC"><span class="zaq">PamyA</span></td>
+     <td bgcolor="#CCCCCC"><span class="zaq">P<sub>amyA</sub></span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">Promoter</span></td>
-     <td bgcolor="#CCCCCC">&nbsp;</td>
+     <td bgcolor="#CCCCCC">a strong promoter in <em>Bacillus amyloliquefaciens </em>LL3</td>
      <td bgcolor="#CCCCCC"><span class="zaq">Zhaoran Zhang</span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">613</span></td>
@@ Line 182: / Line 100: @@
    <tr bgcolor="#FFFFFF">
      <td bgcolor="#CCCCCC"><a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K1628101">BBa_K1628101</a></td>
-     <td><span class="zaq">pgsB</span></td>
+     <td><span class="zaq"><em>pgsB</em></span></td>
      <td><span class="zaq">Coding</span></td>
-     <td>&nbsp;</td>
+     <td>a gene responsible for  γ-PGA synthesis in <em>pgsBCA</em> operon</td>
      <td><span class="zaq">Tianyi Huang</span></td>
      <td><span class="zaq">1182</span></td>
@@ Line 190: / Line 108: @@
    <tr>
      <td bgcolor="#CCCCCC"><a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K1628102">BBa_K1628102</a></td>
-     <td bgcolor="#CCCCCC"><span class="zaq">pgsCA</span></td>
+     <td bgcolor="#CCCCCC"><span class="zaq"><em>pgsCA</em></span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">Coding</span></td>
-     <td bgcolor="#CCCCCC">&nbsp;</td>
+     <td bgcolor="#CCCCCC">a coding gene in <em>pgsBCA</em> operon</td>
      <td bgcolor="#CCCCCC"><span class="zaq">Xinhao Song</span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">1631</span></td>
@@ Line 198: / Line 116: @@
    <tr bgcolor="#FFFFFF">
      <td bgcolor="#CCCCCC"><a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K1628201">BBa_K1628201</a></td>
-     <td><span class="zaq">PlacI/lacI</span></td>
+     <td><span class="zaq">P<sub>lacI</sub>/lacI</span></td>
      <td><span class="zaq">Translational Unit </span></td>
-     <td>&nbsp;</td>
+     <td>a promoter of lactose operon along with a repressor of lactose operon regulating the promoter</td>
      <td><span class="zaq">Yibing Wei</span></td>
      <td><span class="zaq">1386</span></td>
@@ Line 206: / Line 124: @@
    <tr>
      <td bgcolor="#CCCCCC"><a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K1628202">BBa_K1628202</a></td>
-     <td bgcolor="#CCCCCC"><span class="zaq">Pgrac</span></td>
+     <td bgcolor="#CCCCCC"><span class="zaq">P<sub>grac</sub></span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">Promoter </span></td>
-     <td bgcolor="#CCCCCC">&nbsp;</td>
+     <td bgcolor="#CCCCCC">a promoter of lactose operon regulated by repressor LacI</td>
      <td bgcolor="#CCCCCC"><span class="zaq">Tianyi Huang</span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">120</span></td>
@@ Line 216: / Line 134: @@
      <td><span class="zaq">xylR</span></td>
      <td><span class="zaq">Coding </span></td>
-     <td>&nbsp;</td>
+     <td>a repressor of xylose operon regulating promoter <span class="zaq">P<sub>xyl</sub></span></td>
      <td><span class="zaq">Zhaoran Zhang</span></td>
      <td><span class="zaq">1167</span></td>
@@ Line 224: / Line 142: @@
      <td bgcolor="#CCCCCC"><span class="zaq">P1-GFP</span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">Device</span></td>
-     <td bgcolor="#CCCCCC">&nbsp;</td>
+     <td bgcolor="#CCCCCC">P3-GFP is a composite part used for the Measurement track of this year. This part consists of the promoter part of BBa_J23117, the official GFP device (with an RBS, GFP coding sequence and a set of double terminators) and a pSB1C3 backbone. We transformed this plasmid into E. coli cells and the fluorescence intensity of the GFP protein that was expressed by the bacteria was measured afterwards by a flow cytometry.</td>
      <td bgcolor="#CCCCCC"><span class="zaq">Tianyi Huang</span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">?</span></td>
@@ Line 232: / Line 150: @@
      <td><span class="zaq">P2-GFP</span></td>
      <td><span class="zaq">Device</span></td>
-     <td>&nbsp;</td>
+     <td>P2-GFP is a composite part used for the Measurement track of this year. This part consists of the promoter part of BBa_J23106, the official GFP device (with an RBS, GFP coding sequence and a set of double terminators) and a pSB1C3 backbone. We transformed this plasmid into <em>E. coli</em> cells and the fluorescence intensity of the GFP protein that was expressed by the bacteria was measured afterwards by a flow cytometry.</td>
      <td><span class="zaq">Xinhao Song</span></td>
      <td><span class="zaq">?</span></td>
@@ Line 240: / Line 158: @@
      <td bgcolor="#CCCCCC"><span class="zaq">P3-GFP </span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">Device</span></td>
-     <td bgcolor="#CCCCCC">&nbsp;</td>
+     <td bgcolor="#CCCCCC">P3-GFP is a composite part used for the Measurement track of this year. This part consists of the promoter part of BBa_J23117, the official GFP device (with an RBS, GFP coding sequence and a set of double terminators) and a pSB1C3 backbone. We transformed this plasmid into <em>E. coli </em>cells and the fluorescence intensity of the GFP protein that was expressed by the bacteria was measured afterwards by a flow cytometry.</td>
      <td bgcolor="#CCCCCC"><span class="zaq">Yibing Wei</span></td>
      <td bgcolor="#CCCCCC"><span class="zaq">?</span></td>
    </tr>
 </table>
-<p>&nbsp;</p>
-<p>&nbsp;</p>
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@@ Line 256: / Line 172: @@
 						<h6><a href="https://2015.igem.org/Team:Nankai/Basic_Part">Basic Parts</a></h6>
 						<h6><a href="https://2015.igem.org/Team:Nankai/Composite_Part">Composite Parts</a></h6>
-						<h6><a href="https://2015.igem.org/Team:Nankai/Part_Collection">Part Collection</a></h6>
+											</div> <!-- /.sidebar-widget -->
-						<ul id="flickr-feed" class="thumbs"></ul>
-					</div> <!-- /.sidebar-widget -->
 					<div class="sidebar-widget">
-						<img src="https://static.igem.org/mediawiki/2015/f/f2/Nankai_projectpic3.JPG">
+						<img src="https://static.igem.org/mediawiki/2015/d/de/Partsfigure_new1.jpeg">
-                                                 <p>Part-picture-1</p>
+                                                 <p>Have fun in iGEM 2015!</p>
-						<img src="https://static.igem.org/mediawiki/2015/6/6e/Nankai_projectpic1.JPG">
+						<img src="https://static.igem.org/mediawiki/2015/4/40/Partsfigure_new2.jpeg">
-                                                <p>Part-picture-2</p>
+                      <p>Have fun in iGEM 2015!</p>
-						<img src="https://static.igem.org/mediawiki/2015/2/2d/Nankai_projectpic2.jpg">
+						<img src="https://static.igem.org/mediawiki/2015/a/ad/Partsfigure_new3.jpeg">
-                       <p>Part-picture-3</p>
+                       <p>Have fun in iGEM 2015!</p>
 					</div> <!-- /.sidebar-widget -->
-<h6>References</h6>
+<h6>&nbsp;</h6>
-<p>1. Ashiuchi, M., Misono, H., 2002. Biochemistry and molecular genetics of poly-γ-glutamate synthesis. Appl. Biochem. Biotechnol. 59, 9–14.</br>
-. Kunioka, M., 1997. Biosynthesis and chemical reactions of poly(amino acid)s from
-microorganisms. Appl. Microbiol. Biotechnol. 47, 469–475.</br>
-. Shih, I.L., Van, Y.T., 2001. The production of poly(γ-glutamic acid) from microorganism and its various applications. Bioresour. Technol. 79, 207–225.</br>
-. Li, C., 2002. Poly(L-glutamic acid)--anticancer drug conjugates. Adv. Drug Deliver. Rev. 54, 695–713.</br>
-. Liang, H.F., Chen, C.T., Chen, S.C., Kulkarni, A.R., Chiu, Y.L., Chen, M.C., Sung, H.W., 2006. Paclitaxel-loaded poly(γ-glutamic acid)-poly(lactide) nanoparticles as a targeted drug delivery system for the treatment of liver cancer. Biomaterials. 27, 2051–2059.</br>
-. Richard, A., Margaritis, A., 2001. Poly (glutamic acid) for biomedical applications. Crit. Rev. Biotechnol. 21, 219–232.</br>
-. Park, Y.J., Liang, J., Yang, Z., Yang, V.C., 2001. Controlled release of clot-dissolving tissue-type plasmmogen activator from a poly(L-glutamic acid) semi-interpenetrating polymer network hydrogel. J. Control. Release. 74, 243–247.</br>
-. Cao, M.F., Geng, W.T., Liu, L., Song, C.J., Xie, H., Guo, W.B., Jin, Y.H., Wang, S.F., 2011. Glutamic acid independent production of poly-γ-glutamic acid by Bacillus amyloliquefaciens LL3 and cloning of pgsBCA genes. Bioresour. Technol. 102, 4251–4257.</br>
-. Geng, W.T., Cao, M.F., Song, C.J., Xie, H., Liu, L., Yang, C., Feng, J., Zhang, W., Jin, Y.H., Du, Y., Wang, S.F., 2011. Complete genome sequence of Bacillus amyloliquefaciens LL3, which exhibits glutamic acid-independent production of poly-γ-glutamic acid. J. Bacteriol. 193, 3393–3394.</br>
-. Feng, J., Gao, W.X., Gu, Y.Y., Zhang, W., Cao, M.F., Song, C.J., Zhang, P., Sun, M., Yang, C.,  Wang, S.F., 2014a. Functions of poly-gamma-glutamic acid (γ-PGA) degradation genes in γ-PGA synthesis and cell morphology maintenance. Appl. Microbiol. Biotechnol. 98, 6397–6407.</br>
-. Uy, D., Delaunay S., Germain, P., Engasser, J.M., Goergen, J.L. 2003. Instability of glutamate production by Corynebacterium glutamicum 2262 in continuous culture using the temperature-triggered process. J. Biotech. 104, 173-184.</p>
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+<p class="tail">&nbsp;<p>
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