Team:Goettingen/week19-2

(Difference between revisions)

Revision as of 12:03, 18 September 2012

Language:

English,

Deutsch

Quikchange of fliC

Experiment:
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 Pfu Turbo 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 DNA fragment is obtained.
Observations & Results:
The QC PCR was not successful. We were not able to observe any PCR product.

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_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 Quickchange of fliC

Experiment:
Quick Change overlapping PCR was performed using designed primers and Pfu Turbo polymerase (see Quick Change protocol in "protocols").
Observations & Results:
The QC PCR was not successful again. We were not able to observe any PCR product.

V09_06_1 Insertion 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.

Preparation of over night cultures

Important pages:
Home; Team; Official Team Profile; Project; Parts submitted to the Registry; Modeling; Notebook; Saftey; Attributions

@@ Line 536: / Line 536: @@
 <td width="900" bordercolor="black" valign="top">
 <h2><b>V09_03 </b></h2><br>
-<b>Quickchange of <i>fliC</i></b><br>
+<b>Quikchange of <i>fliC</i></b><br>
 <ul>
-<li>Experiment: <br>Quick Change overlapping PCR was performed using designed primers and Pfu Turbo polymerase (see Quick Change protocol in "protocols").<br></li>
+<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 Pfu Turbo 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 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>