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		+	{{HeaderGroningen2012}}
		+	<html>
		+	<body>
		+	<div style="position:absolute; right: 100px; top: 530px;">
-	Tom
-	Inoculation of E. coli containing LuxI and LuxR.	+	</div>
		+	</body>
		+	</html>
		+	<html>
		+	<head>
		+	<style type="text/css">
		+	p.margin{
		+	font-size:12pt;
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		+	margin-left:150px;
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		+	}
		+	</style>
		+	</head>
-	'''MicroArray experiment: preparations'''	+	<body>
		+	<p class="margin"><br><br><br><br>
		+	Tom <br> <br>
-	Arjan/Renske	+	Plasmid isolation of LuxR (BBa_R0062), LuxI (BBa_J37034) and backbone (BBa_090403) biobricks. <br> <br>
-	Made setup for the micro-array experiment:	+	Plasmid concentrations: LuxR (1) = 99.3 ng/ul, LuxR (2) = 164.3 ng/ul, LuxI (1) = 69.9 ng/ul , LuxI (2) = 130.6 ng/ul, backbone = 63.0 ng/ul. <br><br>
-	37 degrees room. Flask with 50 mL culture of Bacillus subtilis sp. 168, connected with tubes to 100 mL flask with rotting/fresh meat. Filters and peristaltic pump inbetween. Culture is stirred by a magnetic stirrer.	+
-	[[File:Groningen_RR_20120628_microarraysetup.jpg|thumb|400px|left|Micro-Array Setup]]	+
		+	Emeraldo/Nisa <br>
		+	<br>
		+	1.) Order SpeI and EcoRI FastDigest Fermentas<br>
		+	2.) Order Plamid High Pure purification kit Roche<br>
		+	3.) B. subtilis transformation with BBa_K090403 <br>
		+	4.) Digestion of pigment genes from their backbones with EcoRI and SpeI. Result: the pigments genes are in correct length. <br>
		+	5.) Digestion of BBa_K090403. Result: incorrect length.<br><br>
		+
		+
		+	MicroArray experiment: preparations <br><br>
		+
		+	Arjan/Renske <br><br>
		+
		+	Made setup for the micro-array experiment: <br>
		+	37 degrees room. Flask with 50 mL culture <br>
		+	of Bacillus subtilis sp. 168,<br>
		+	connected with tubes to 100 mL flask <br>
		+	with rotting/fresh meat. <br>
		+	Filters and peristaltic pump inbetween. <br>
		+	Culture is stirred by a magnetic stirrer.<br><br>
		+	<img src="https://static.igem.org/mediawiki/2012/9/9e/Groningen2012_RR_MicArraysetup.png" width="300" height="300">
		+	<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}}

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Latest revision as of 16:52, 25 September 2012

Tom

Plasmid isolation of LuxR (BBa_R0062), LuxI (BBa_J37034) and backbone (BBa_090403) biobricks.

Plasmid concentrations: LuxR (1) = 99.3 ng/ul, LuxR (2) = 164.3 ng/ul, LuxI (1) = 69.9 ng/ul , LuxI (2) = 130.6 ng/ul, backbone = 63.0 ng/ul.

Emeraldo/Nisa

1.) Order SpeI and EcoRI FastDigest Fermentas
2.) Order Plamid High Pure purification kit Roche
3.) B. subtilis transformation with BBa_K090403
4.) Digestion of pigment genes from their backbones with EcoRI and SpeI. Result: the pigments genes are in correct length.
5.) Digestion of BBa_K090403. Result: incorrect length.

MicroArray experiment: preparations

Arjan/Renske

Made setup for the micro-array experiment:
37 degrees room. Flask with 50 mL culture
of Bacillus subtilis sp. 168,
connected with tubes to 100 mL flask
with rotting/fresh meat.
Filters and peristaltic pump inbetween.
Culture is stirred by a magnetic stirrer.


Back to notebook