Team:Goettingen/week19-2

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Latest revision as of 17:18, 22 September 2012


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#2 Speed Improvement - 19th week

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V09_03

Overlapping PCR of fliC

Experiment:
In order to eliminate undesired restriction sites inside of our fliC part a Overlapping PCR was performed using especially designed primers that will cause a point mutation and PfuTurbo polymerase (protocol). Since four unwanted restriction sites are localized in our part four reactions were prepared producing overlapping fragments. Subsequently samples 1 and 2 as well as 3 and 4 were combined via overlapping PCR reducing the number of fragments at two. Finally sample 1+2 and 3+4 were combined as well and one final DNA fragment is obtained.
Observations & Results:
The QC PCR was not successful. We were not able to observe any PCR product.

V09_04

V09_04_1 Test digestion of pSB1C3 (including flHDC under the control of different promoters)

Experiment:
The test digestion of pSB1C3 including flHDC under the expression of 8 different promoters was performed with the restriction enzymes EcoRI and PstI according to the protocol. The product was subsequently analyzed on an 1% analytical agarose gel.
Observations & Results:
Since fragments of the expected size could be obtained for all clones the test digestion worked for all.

V09_04_2 Biobrick Standardization of motA,motB and yhjH

Experiment:
PCR of motA, motB and yhjH using primers containing the standard BioBrick sequences. Procedure was succesful and the PCR products were purified via PeqGOLD Gelextraction Kit (Peqlab).

V09_05

V09_05_1 Preparative double digestion of motA, motB, yhjH and pSB1C3

Experiment:
motA, motB, yhjH and pSB1C3 were digested with EcoRI and PstI. The prodcuts were seperated via gel electrophoresis and purified using PeqGOLD Gelextraction Kit (Peqlab).

V09_05_2 Repetition of the Overlapping PCR of fliC

Experiment:
Here again the Overlapping PCR was performed using designed primers and PfuTurbo polymerase (protocol). However, this time a lower annealing temperature was chosen. Also this time four short fragments were produced first and subsequently combined to a complete final DNA fragment.
Observations & Results:
Once again the QC PCR failed for no PCR product was observed. Since we already had problems with enzymes during our experiments we consider an non-functionable polymerase.

V09_06

V09_06_1 Ligation of motA, motB and yhjH into pSB1C3

Experiment:
The ligation of motA, motB and yhjH with pSB1C3 was conducted as described in the protocol.

V09_06_2 Chemical transformation of motA, motB and yhjH to E. coli DH10B

Experiment:
The transformation was performed as described in the standard protocol.
Observations & Results:
The transformation was successful since numerous colonies has formed whereas the negative control remained clear.

V09_09

Preparation of over night cultures

Experiment:
Over night cultures were prepared:

pSB1C3-motA
pSB1C3-motB
pSB1C3-yhjH

Back to overview

@@ Line 25: / Line 25: @@
 <td width="900" bordercolor="black" valign="top">
 <h2><b>V09_03 </b></h2><br>
-<b>Quikchange of <i>fliC</i></b><br>
+<b>Overlapping PCR of <i>fliC</i></b><br>
 <ul>
-<li>Experiment: <br> In order to eliminate undesired restriction sites inside of our part a Quikchange PCR was performed using especially designed primers that will cause a point mutation and <i>PfuTurbo</i> polymerase (see Quick Change protocol in "protocols"). Since four unwanted restriction sites are localized in our part four reactions were prepared producing overlapping fragments. Subsequently samples 1 and 2 as well as 3 and 4 were combined via overlapping PCR reducing the number of fragments at two. Finally smaple 1+2 and 3+4 were combined as well and one final DNA fragment is obtained. <br></li>
+<li>Experiment: <br> In order to eliminate undesired restriction sites inside of our <i>fliC</i> part a Overlapping PCR was performed using especially designed primers that will cause a point mutation and <i>PfuTurbo</i> polymerase (<a href="https://2012.igem.org/Team:Goettingen/Project/Methods">protocol</a>). Since four unwanted restriction sites are localized in our part four reactions were prepared producing overlapping fragments. Subsequently samples 1 and 2 as well as 3 and 4 were combined via overlapping PCR reducing the number of fragments at two. Finally sample 1+2 and 3+4 were combined as well and one final DNA fragment is obtained. <br></li>
 <li>Observations & Results: <br>
   The QC PCR was not successful. We were not able to observe any PCR product.</li>
@@ Line 40: / Line 40: @@
 <b>V09_04_1 Test digestion of pSB1C3 (including <i>flHDC</i> under the control of different promoters)</b><br>
 <ul>
-<li>Experiment: <br>The test digestion of pSB1C3 including <i>flHDC</i> under the expression of 8 different promoters was performed with the restriction enzymes <i>EcoRI</i> and <i>PstI</i> according to the protocol. The product was subsequently analyzed on an 1% analytical agarose gel.<br> </li>
+<li>Experiment: <br>The test digestion of pSB1C3 including <i>flHDC</i> under the expression of 8 different promoters was performed with the restriction enzymes <i>EcoRI</i> and <i>PstI</i> according to the <a href="https://2012.igem.org/Team:Goettingen/Project/Methods">protocol</a>. The product was subsequently analyzed on an 1% analytical agarose gel.<br> </li>
 <li>Observations & Results: <br>
 Since fragments of the expected size could be obtained for all clones the test digestion worked for all.</li>
@@ Line 61: / Line 61: @@
 </ul>
 <br>
-<b>V09_05_2 Repetition of the Quikchange of <i>fliC</i></b><br>
+<b>V09_05_2 Repetition of the Overlapping PCR of <i>fliC</i></b><br>
 <ul>
-<li>Experiment: <br> Here again the Quikchange PCR was performed using designed primers and <i>PfuTurbo</i> polymerase (see Quick Change protocol in "protocols"). However, this time a lower annealing temperature was chosen. Also this time four short fragments were produced first and subsequently combined to a complete final DNA fragment. <br></li>
+<li>Experiment: <br> Here again the Overlapping PCR was performed using designed primers and <i>PfuTurbo</i> polymerase (<a href="https://2012.igem.org/Team:Goettingen/Project/Methods">protocol</a>). However, this time a lower annealing temperature was chosen. Also this time four short fragments were produced first and subsequently combined to a complete final DNA fragment. <br></li>
 <li>Observations & Results: <br>
   Once again the QC PCR failed for no PCR product was observed. Since we already had problems with enzymes during our experiments we consider an non-functionable polymerase. </li>
@@ Line 76: / Line 76: @@
 <td width="900" bordercolor="black" valign="top">
 <h2><b>V09_06 </b></h2><br>
-<b>V09_06_1 Insertion of <i>motA</i>, <i>motB</i> and <i>yhjH</i> into pSB1C3 </b><br>
+<b>V09_06_1  Ligation of <i>motA</i>, <i>motB</i> and <i>yhjH</i> into pSB1C3 </b><br>
 <ul>
 <li>Experiment: <br>
-The ligation of <i>motA</i>, <i>motB</i> and <i>yhjH</i> with pSB1C3 was conducted as described in the protocol. <br></li>
+The ligation of <i>motA</i>, <i>motB</i> and <i>yhjH</i> with pSB1C3 was conducted as described in the <a href="https://2012.igem.org/Team:Goettingen/Project/Methods">protocol</a>. <br></li>
 </ul>
 <br>
@@ Line 102: / Line 102: @@
 <ul>
 <li>Experiment: <br>Over night cultures were prepared:<br>
+<br>
 pSB1C3-<i>motA</i><br>
-pSB1C3-<i>motB</i></li>
+pSB1C3-<i>motB</i><br>
+pSB1C3-<i>yhjH</i><br>
+</li>
+<br>
 </ul>
 <br></td></tr>