Latest revision as of 21:16, 25 September 2012

Plan for today:

1. plasmid isolation from E.coli Dh5A

2. ligate alsT promoter and GFP into pSB1C3 and pSac-Cm (B. subtilis backbone)

3. E.coli transformation for both

1. Plasmid isolation pSB1C3+insert from iGEM Groningen 2010

E.coli DH5a strong magenta = insert device OK!

plasmid concentration: 129,1 ng/ul

Purification of PCR product using gel DNA extraction kit

diluted in 50ul TE (elution buffer)

concentration: 35,6 ng.ul

Ligation pAlsT-GFP into backbone pSB1C3 (and pSac-Cm done next week 23/07)

Cut parts with restiction enzymes

alsT: EcoRI + SpeI

GFP: XbaI + PstI

backbone: EcoRI + PstI

Digestion reaction and subsequently ligation of:

1) alsT150-GFP-BB

2) alsT250-GFP-BB

3) alsT300-GFP-BB

4) alsT500-GFP-BB

3. Transformation of E.coli DH5a

4x promoter alsT testing devices

1x negative control

= 5x LB plate + 15 ug/ml Cm

Back to notebook

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+<head>
+<style type="text/css">
+p.margin
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-Plan for today:
+</style>
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-. plasmid isolation from E.coli Dh5A
+<body><br><br><br>
+<p class="margin">
-. ligate alsT promoter and GFP into pSB1C3 and pSac-Cm (B. subtilis backbone)
+Plan for today:<br>
+<br>
-. E.coli transformation for both
+. plasmid isolation from E.coli Dh5A<br>
+<br>
+. ligate alsT promoter and GFP into pSB1C3 and pSac-Cm (B. subtilis backbone)<br>
-. Plasmid isolation pSB1C3+insert from iGEM Groningen 2010
+<br>
+. E.coli transformation for both<br>
-E.coli DH5a strong magenta = insert device OK!
+<br>
+<br>
-plasmid concentration: 129,1 ng/ul
+. Plasmid isolation pSB1C3+insert from iGEM Groningen 2010<br>
+<br>
+E.coli DH5a strong magenta = insert device OK!<br>
-Purification of PCR product using gel DNA extraction kit
+<br>
+plasmid concentration: 129,1 ng/ul<br>
-diluted in 50ul TE (elution buffer)
+<br>
+<br>
-concentration: 35,6 ng.ul
+Purification of PCR product using gel DNA extraction kit<br>
+<br>
+diluted in 50ul TE (elution buffer)<br>
-Ligation pAlsT-GFP into backbone pSB1C3 (and pSac-Cm done next week 23/07)
+<br>
+concentration: 35,6 ng.ul<br>
-Cut parts with restiction enzymes
+<br>
+<br>
-alsT: EcoRI + SpeI
+Ligation pAlsT-GFP into backbone pSB1C3 (and pSac-Cm done next week 23/07)<br>
+<br>
-GFP: XbaI + PstI
+Cut parts with restiction enzymes<br>
+<br>
-backbone: EcoRI + PstI
+alsT: EcoRI + SpeI<br>
+<br>
-Digestion reaction and subsequently ligation of:
+GFP: XbaI + PstI<br>
+<br>
-) alsT150-GFP-BB
+backbone: EcoRI + PstI<br>
+<br>
-) alsT250-GFP-BB
+Digestion reaction and subsequently ligation of:<br>
+<br>
-) alsT300-GFP-BB
+) alsT150-GFP-BB<br>
+<br>
-) alsT500-GFP-BB
+) alsT250-GFP-BB<br>
+<br>
+) alsT300-GFP-BB<br>
-. Transformation of E.coli DH5a
+<br>
+) alsT500-GFP-BB<br>
-x promoter alsT testing devices
+<br>
+<br>
-x negative control
+. Transformation of E.coli DH5a<br>
+<br>
-= 5x LB plate + 15 ug/ml Cm
+x promoter alsT testing devices<br>
+<br>
-<html>
+x negative control<br>
+<br>
+= 5x LB plate + 15 ug/ml Cm<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}}

Team:Groningen/Notebook/Wetwork 20July2012

From 2012.igem.org

Latest revision as of 21:16, 25 September 2012

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