Team:Bielefeld-Germany/Labjournal/July

From 2013.igem.org

(Difference between revisions)
Line 109: Line 109:
Size:1800 bp
Size:1800 bp
<br>Program: <a href="https://2013.igem.org/Team:Bielefeld-Germany/Labjournal/ProtocolsPrograms#cyt_frag1">PhusionPCR</a>
<br>Program: <a href="https://2013.igem.org/Team:Bielefeld-Germany/Labjournal/ProtocolsPrograms#cyt_frag1">PhusionPCR</a>
-
<br>mtrC_fwd:
+
<br>Gradient: 54°C - 71°C over 8 steps
-
<br>mtr_Frag1_rev:  
+
<br>Primer: mtrC_fwd & mtr_Frag1_rev
 +
<br>Template: S. oneidensis PCR Template from genomic DNA
 +
<br>Notes: Annealing temperature has no significant impact on the PCR
</blockquote>
</blockquote>
</div>
</div>
Line 119: Line 121:
Size:330 bp
Size:330 bp
<br>Program: <a href="https://2013.igem.org/Team:Bielefeld-Germany/Labjournal/ProtocolsPrograms#cyt_frag2">PhusionPCR</a>
<br>Program: <a href="https://2013.igem.org/Team:Bielefeld-Germany/Labjournal/ProtocolsPrograms#cyt_frag2">PhusionPCR</a>
-
<br>mtr_Frag2_fwd:
+
<br>Primer: mtr_Frag2_fwd & mtr_Frag2_rev
-
<br>mtr_Frag2_rev:  
+
<br>Template: S. oneidensis PCR Template from genomic DNA
 +
<br>Notes:  
</blockquote>
</blockquote>
</div>
</div>
Line 129: Line 132:
Size:3000 bp
Size:3000 bp
<br>Program: <a href="https://2013.igem.org/Team:Bielefeld-Germany/Labjournal/ProtocolsPrograms#cyt_frag3">PhusionPCR</a>
<br>Program: <a href="https://2013.igem.org/Team:Bielefeld-Germany/Labjournal/ProtocolsPrograms#cyt_frag3">PhusionPCR</a>
-
<br>mtr_Frag3_fwd:
+
<<br>Gradient: 54°C - 71°C over 8 steps
-
<br>mtr_B_rev:  
+
<br>Primer: mtr_Frag3_fwd & mtrB_rev
 +
<br>Template: S. oneidensis PCR Template from genomic DNA
 +
<br>Notes: Annealing temperature has no significant impact on the PCR
</blockquote>
</blockquote>
</div>
</div>

Revision as of 20:33, 2 September 2013





July

Milestones


1.Week

MFC

Mediators

Cytochromes

Design and order of new Primer

The mtrCAB fragment has two illegal PstI restriction sites at x xbp and yy bp, so we had to design new primers to remove them. We replaced one base in each restriction site, without affecting the coding triplett, by respective primer overlaps . We ended up with three different fragments, which will be ligated back together via Gibson Assembly.
mtrCAB_Frag1_rev:
mtrCAB_Frag2_fwd:
mtrCAB_Frag2_rev:
mtrCAB_Frag3_fwd:

Biosafety

Porines









2.Week

MFC

Mediators

Cytochromes

Biosafety

Porines









3.Week

MFC

Mediators

Cytochromes

Amplification of Fragment 1

Size:1800 bp
Program: PhusionPCR
Gradient: 54°C - 71°C over 8 steps
Primer: mtrC_fwd & mtr_Frag1_rev
Template: S. oneidensis PCR Template from genomic DNA
Notes: Annealing temperature has no significant impact on the PCR

Amplification of Fragment 2

Size:330 bp
Program: PhusionPCR
Primer: mtr_Frag2_fwd & mtr_Frag2_rev
Template: S. oneidensis PCR Template from genomic DNA
Notes:

Amplification of Fragment 3

Size:3000 bp
Program: PhusionPCR <
Gradient: 54°C - 71°C over 8 steps
Primer: mtr_Frag3_fwd & mtrB_rev
Template: S. oneidensis PCR Template from genomic DNA
Notes: Annealing temperature has no significant impact on the PCR

Biosafety

Porines









4.Week

MFC

Mediators

Cytochromes

Biosafety

Porines









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