Difference between revisions of "Team:Alverno CA/Basic Parts"

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	{{Alverno_CA}}		{{Alverno_CA}}
	<html>		<html>
−		+	<script src="http://wayou.github.io/SlipHover/js/jquery.sliphover.min.js">
		+	</script>
		+	<style type="text/css">
		+	#container{
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	<head>		<head>
	<title>Alverno iGEM 2016</title>		<title>Alverno iGEM 2016</title>
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	<br>		<br>
	<br>		<br>
−	<center><img src="https://static.igem.org/mediawiki/2016/thumb/5/58/T--Alverno_CA--Alverno_iGEM_2016_Logo.png/600px-T--Alverno_CA--Alverno_iGEM_2016_Logo.png" alt="Alverno iGEM Logo" style="width:300px;"></center>	+	<h2><center>Basic & Composite Parts</center></h2>
−	<h1><center>Basic Parts</center></h1>	+
−	<left><h2><a href="http://parts.igem.org/Part:BBa_K2145000">BBa_K2145000:</a></h2></left>	+	<div class="demo" id="container">
−	<p>This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part.</p>	+	<center>
		+	<ul>
		+	<li style="list-style: none"><br>
		+	<br>
		+	</li>
−	<left><h2>BBa_K2145000:</h2></left>	+	<li><img src=
		+	"https://static.igem.org/mediawiki/2016/1/15/T--Alverno_CA--asiasamsquare.jpg"
		+	style="height:215px;width:215px;" title=
		+	"Designing parts."/>
		+	</li>
		+	<li><img src=
		+	"https://static.igem.org/mediawiki/2016/7/78/T--Alverno_CA--samsquare.jpg"
		+	style="height:215px;width:215px;" title=
		+	"That's a good idea!">
		+	</li>
		+	<li><img src=
		+	"https://static.igem.org/mediawiki/2016/a/a4/T--Alverno_CA--asiasquareboard.jpg"
		+	style="height:215px;width:215px;" title=
		+	"Asia is thinking about parts. ">
		+	</li>
		+
		+	</ul>
		+	</center>
		+	</div>
		+	<br><br><br><br><br><br><br><br><br><br>
		+
		+	<left><h3><a href="http://parts.igem.org/Part:BBa_K2145000">BBa_K2145000(GG 95):</a></h3></left>
		+	<h5>This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part with a 500bp spacer in between.</h5>
		+	<h5>Direction of GFP: Forward, toward the spacer</h5>
		+	<h5>Direction of RFP: Forward, away from the spacer</h5>
		+
		+	<left><h3><a href="http://parts.igem.org/Part:BBa_K2145001">BBa_K2145001(GG 96):</a></h3></left>
		+	<h5>This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part with a 500bp spacer in between.</h5>
		+	<h5>Direction of GFP: Reverse, away from the spacer</h5>
		+	<h5>Direction of RFP: Forward, away from the spacer</h5>
		+
		+	<left><h3><a href="http://parts.igem.org/Part:BBa_K2145104">BBa_K2145104(GG 97):</a></h3></left>
		+	<h5>This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part with a 500bp spacer in between.</h5>
		+	<h5>Direction of GFP: Forward, toward the spacer</h5>
		+	<h5>Direction of RFP: Reverse, toward the spacer</h5>
		+
		+	<left><h3><a href="http://parts.igem.org/Part:BBa_K2145105">BBa_K2145105(GG 98):</a></h3></left>
		+	<h5>This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part with a 500bp spacer in between.</h5>
		+	<h5>Direction of GFP: Reverse, away from the spacer</h5>
		+	<h5>Direction of RFP: Reverse, toward the spacer</h5>
		+
		+	<left><h3><a href="http://parts.igem.org/Part:BBa_K2145124">BBa_K2145124(GG 99):</a></h3></left>
		+	<h5>This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part with a 500bp spacer in between.</h5>
		+	<h5>Direction of GFP: Forward, away from the spacer</h5>
		+	<h5>Direction of RFP: Reverse, away from the spacer</h5>
		+
		+	<left><h3><a href="http://parts.igem.org/Part:BBa_K2145107">BBa_K2145107(GG 100):</a></h3></left>
		+	<h5>This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part with a 500bp spacer in between.</h5>
		+	<h5>Direction of GFP: Reverse, toward the spacer</h5>
		+	<h5>Direction of RFP: Forward, toward the spacer</h5>
		+
		+	<left><h3><a href="http://parts.igem.org/Part:BBa_K2145126">BBa_K2145126(GG 101):</a></h3></left>
		+	<h5>This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part with a 500bp spacer in between.</h5>
		+	<h5>Direction of GFP: Forward, away from the spacer</h5>
		+	<h5>Direction of RFP: Reverse, away from the spacer</h5>
		+
		+	<left><h3><a href="http://parts.igem.org/Part:BBa_K2145127">BBa_K2145127(GG 102):</a></h3></left>
		+	<h5>This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part with a 500bp spacer in between.</h5>
		+	<h5>Direction of GFP: Reverse, toward the spacer</h5>
		+	<h5>Direction of RFP: Reverse, away from the spacer</h5>
		+
		+	<left><h3><a href="http://parts.igem.org/Part:BBa_K2145100">BBa_K2145100(GG 105):</a></h3></left>
		+	<h5>This plasmid contains a GFP and an RFP reporter separated by a 282-bp spacer containing three gRNA binding sites for dCas. The reporter is designed to demonstrate the effect, if any, of binding a dCas "clamp" between two genes (the idea being that such a clamp can limit propagation of supercoiling between the genes, functionally isolating them).</h5>
		+	<h5>Direction of GFP: Forward, toward the clamps</h5>
		+	<h5>Direction of RFP: Forward, away from the clamps</h5>
		+
		+	<left><h3><a href="http://parts.igem.org/Part:BBa_K2145101">BBa_K2145101(GG 106):</a></h3></left>
		+	<h5>This plasmid contains a GFP and an RFP reporter separated by a 282-bp spacer containing three gRNA binding sites for dCas. The reporter is designed to demonstrate the effect, if any, of binding a dCas "clamp" between two genes (the idea being that such a clamp can limit propagation of supercoiling between the genes, functionally isolating them).</h5>
		+	<h5>Direction of GFP: Reverse, away from the clamps</h5>
		+	<h5>Direction of RFP: Forward, away from the clamps</h5>
		+
		+	<left><h3><a href="http://parts.igem.org/Part:BBa_K2145102">BBa_K2145102(GG 107):</a></h3></left>
		+	<h5>This plasmid contains a GFP and an RFP reporter separated by a 282-bp spacer containing three gRNA binding sites for dCas. The reporter is designed to demonstrate the effect, if any, of binding a dCas "clamp" between two genes (the idea being that such a clamp can limit propagation of supercoiling between the genes, functionally isolating them).</h5>
		+	<h5>Direction of GFP: Forward, toward the clamps</h5>
		+	<h5>Direction of RFP: Reverse, toward the clamps</h5>
		+
		+	<left><h3><a href="http://parts.igem.org/Part:BBa_K2145103">BBa_K2145103(GG 108):</a></h3></left>
		+	<h5>This plasmid contains a GFP and an RFP reporter separated by a 282-bp spacer containing three gRNA binding sites for dCas. The reporter is designed to demonstrate the effect, if any, of binding a dCas "clamp" between two genes (the idea being that such a clamp can limit propagation of supercoiling between the genes, functionally isolating them).</h5>
		+	<h5>Direction of GFP: Reverse, away from the clamps</h5>
		+	<h5>Direction of RFP: Reverse, toward the clamps</h5>
		+
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		+
		+	<script>
		+	$("#container").sliphover();
		+	$(".sliphover-container").css('z-index','99');
		+	$("#menuContainer").css('z-index','99');
		+	</script>
	</html>		</html>

---

Latest revision as of 21:20, 2 December 2016

Basic & Composite Parts

BBa_K2145000(GG 95):

This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part with a 500bp spacer in between.

Direction of GFP: Forward, toward the spacer

Direction of RFP: Forward, away from the spacer

BBa_K2145001(GG 96):

This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part with a 500bp spacer in between.

Direction of GFP: Reverse, away from the spacer

Direction of RFP: Forward, away from the spacer

BBa_K2145104(GG 97):

This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part with a 500bp spacer in between.

Direction of GFP: Forward, toward the spacer

Direction of RFP: Reverse, toward the spacer

BBa_K2145105(GG 98):

This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part with a 500bp spacer in between.

Direction of GFP: Reverse, away from the spacer

Direction of RFP: Reverse, toward the spacer

BBa_K2145124(GG 99):

This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part with a 500bp spacer in between.

Direction of GFP: Forward, away from the spacer

Direction of RFP: Reverse, away from the spacer

BBa_K2145107(GG 100):

This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part with a 500bp spacer in between.

Direction of GFP: Reverse, toward the spacer

Direction of RFP: Forward, toward the spacer

BBa_K2145126(GG 101):

This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part with a 500bp spacer in between.

Direction of GFP: Forward, away from the spacer

Direction of RFP: Reverse, away from the spacer

BBa_K2145127(GG 102):

This part contains two fluorescent protein coding sites (for RFP and GFP) and was assembled using Golden Gate Assembly. To make plasmid, parts were taken from iGEM Registry (BBa_J04450 (RFP) and BBa_I13522 (GFP)) and assembled to make new part with a 500bp spacer in between.

Direction of GFP: Reverse, toward the spacer

Direction of RFP: Reverse, away from the spacer

BBa_K2145100(GG 105):

This plasmid contains a GFP and an RFP reporter separated by a 282-bp spacer containing three gRNA binding sites for dCas. The reporter is designed to demonstrate the effect, if any, of binding a dCas "clamp" between two genes (the idea being that such a clamp can limit propagation of supercoiling between the genes, functionally isolating them).

Direction of GFP: Forward, toward the clamps

Direction of RFP: Forward, away from the clamps

BBa_K2145101(GG 106):

This plasmid contains a GFP and an RFP reporter separated by a 282-bp spacer containing three gRNA binding sites for dCas. The reporter is designed to demonstrate the effect, if any, of binding a dCas "clamp" between two genes (the idea being that such a clamp can limit propagation of supercoiling between the genes, functionally isolating them).

Direction of GFP: Reverse, away from the clamps

Direction of RFP: Forward, away from the clamps

BBa_K2145102(GG 107):

This plasmid contains a GFP and an RFP reporter separated by a 282-bp spacer containing three gRNA binding sites for dCas. The reporter is designed to demonstrate the effect, if any, of binding a dCas "clamp" between two genes (the idea being that such a clamp can limit propagation of supercoiling between the genes, functionally isolating them).

Direction of GFP: Forward, toward the clamps

Direction of RFP: Reverse, toward the clamps

BBa_K2145103(GG 108):

This plasmid contains a GFP and an RFP reporter separated by a 282-bp spacer containing three gRNA binding sites for dCas. The reporter is designed to demonstrate the effect, if any, of binding a dCas "clamp" between two genes (the idea being that such a clamp can limit propagation of supercoiling between the genes, functionally isolating them).

Direction of GFP: Reverse, away from the clamps

Direction of RFP: Reverse, toward the clamps