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	{{HeaderGroningen2012}}		{{HeaderGroningen2012}}
		+	<html>
		+	<head>
		+	<style type="text/css">
		+	p.margin
		+	{
		+	font-size:12pt;
		+	line-height:14pt;
		+	color:white;
-	Nisa	+	margin-top:0px;
		+	margin-bottom:20px;
		+	margin-left:150px;
		+	margin-right:250px;
		+	}
		+	</style>
		+	</head>
-	PCR of GFP with the recieved primers	+	<body><br><br><br>
-	T melting Fwd= 57C	+	<p class="margin">
-	T melting Rev = 61C	+	Nisa<br>
-	Therefore, make a gradient from 55-65C	+	<br>
		+	PCR of GFP (optimized for B. subtilis) with the recieved primers<br>
		+	T melting Fwd= 57C <br>
		+	T melting Rev = 61C<br>
		+	Therefore, make a gradient from 55C-65C (55, 57, 59,61,63,65)<br>
		+	<br>
		+	<br>
		+	Ligation primer<br>
		+	<br>
		+	idea: ligate mulitple fragments of DNA without T4 ligase, but using the PCR method.<br>
		+	<br>
		+	<br>
		+	<A HREF="https://2012.igem.org/Team:Groningen/Notebook"><FONT COLOR=#ff6700>Back to notebook</FONT></A>
		+	</p><br><br>
		+	</body>
		+	</html>
-		+	{{Template:SponsorsGroningen2012}}
-	Ligation primer	+
-		+
-	idea: ligate mulitple fragments of DNA without T4 ligase, but using PCR	+

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Latest revision as of 21:09, 25 September 2012

Nisa

PCR of GFP (optimized for B. subtilis) with the recieved primers
T melting Fwd= 57C
T melting Rev = 61C
Therefore, make a gradient from 55C-65C (55, 57, 59,61,63,65)


Ligation primer

idea: ligate mulitple fragments of DNA without T4 ligase, but using the PCR method.


Back to notebook