Team:Goettingen/week11-2

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#2 Speed Improvement - 10th week

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V07_02

V07_02_1 Preparative double digestion of 20E-flhDC, 2G-flhDC, 18O-flhDC and pSB1C3

Experiment:
In order to clone the flhDC-promoter constructs intro pSB1C3, all components were digested with EcoRI and PstI according to the protocol. The restriction products were subsequently separated on a gel in order to verify the digestions success and purification of the desired fragments.

Observations & Results:
The gel did not feature fragments of the expected size.Obviously, something was wrong with the digestion.

V07_02_2 Preparation of over night cultures

Experiment:
In order to gain more plasmid material of the flhDC-promoter constructs over night cultured were prepared for a subsequent plasmid isolation.
20E - #2
20G - #1
2G - #1
20I - #2
18M - #2
18O - #2
18K - #1
18C - #2

V07_03

V07_03_1 Miniprep of the flhDC-promoter constructs

Experiment:
Minipreps were conducted with PeqGOLD MiniPrep Kit (Peqlab) according to the user manual.

V07_03_2 Amplification of the genes fliC (DH10B), fliC (Salmonella), motA, motB and yhjH

Experiment:
The genes fliC (DH10B), fliC (Salmonella), motA, motB and yhjH were amplified by Pfu-Polymerase according to the following protocol. The success of the PCR was subsequently investigated preparing a 1% agarose gel.
Observations & Results:
The PCR failed for no bands were visible on the gel whereas the marker was clearly discernible.

V07_04

Repetition of the amplification of fliC (DH10B), fliC (Salmonella), motA, motB and yhjH

Experiment:
The genes fliC (DH10B), fliC (Salmonella), motA, motB and yhjH were amplified by Pfu-Polymerase according to the following protocol. Additionally, a negative control as well as a positive control were prepared this time. The success of the PCR was subsequently investigated preparing a 1% agarose gel.
Observations & Results:
The did not function again for no bands were visible on the gel; only the marker was clearly discernible. However, since also the positive control did not feature the slightest band, we assume that something might be wrong with our polymerase.

V07_05

V07_05_1 Repetition of the amplification of the genes fliC (DH10B), fliC (Salmonella), motA, motB and yhjH

Experiment:
To give it a last try the fliC (DH10B), fliC (Salmonella), motA, motB and yhjH were amplified by Pfu-Polymerase according to the following protocol one last time. Here again, a 1% agarose gel was prepared to investigate the PCRs outcome.

Observations & Results:
The gel of the PCR delivered the same picture as last time. No band could be observed except for the marker. Even the positive control does not work. Thus, we decided to buy a new polymerase.

V07_05_2 Repetition of the preparative double digestion of 20G-flhDC, 20I-flhDC, 18K-flhDC, and 18C-flhDC

Experiment:
The test digestion of the flhDC-promoter constructs EcoRI and PstI were applied according to the protocol. The restriction products were subsequently separated on a gel in order to verify the digestions success and purify the desired fragments.
Observations & Results:
The digestion was successful. Bands of the expected size could be observed and cut out.

V07_06

Repetition of the amplification of the fliC (DH10B), fliC (Salmonella), motA, motB and yhjH using the new polymerase

Experiment:
The genes fliC (DH10B), fliC (Salmonella), motA, motB and yhjH were amplified by Phusion-Polymerase according to the following protocol. We also prepared a negative control as well as a positive control. The success of the PCR was subsequently investigated preparing a 1% analytical agarose gel.
Observations & Results:
Finally,the PCR was successful! We were able to receive bands of the expected size for each construct. Obviously, the old Pfu-polymerase was not functional anymore and had caused the PCRs failure.

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@@ Line 520: / Line 520: @@
 <td style="padding: 0pt 20px 0pt 0pt;" width="900px">
 <font face="Verdana" size="-1">
-<h2><b><a name="week8#2">#2 Speed Improvement - 11th week</a></b></h2>
+<h2><b><a name="week10#2">#2 Speed Improvement - 10th week</a></b></h2>
 <a href="https://2012.igem.org/Team:Goettingen/Notebook">Back to overview</a><br>
 <br>
-<p align="justify" style="line-height:1.6em">
-</p>
-<p align="justify" style="line-height:1.6em">
-</p>
 <table cellpadding="20 px" border="1" bordercolor="black" valign="top">
 <tr bordercolor="black" valign="top">
 <td width="900" bordercolor="black" valign="top">
-<h2><b>Versuchsnummer </b></h2><br>
-<b>TITEL</i></b><br>
+<h2><b>V07_02 </b></h2><br>
+<b>V07_02_1 Preparative double digestion of 20E-<i>flhDC</i>, 2G-<i>flhDC</i>, 18O-<i>flhDC</i> and pSB1C3</b><br>
 <ul>
-<li>Experiment: <br>
+<li>Experiment:  <br>
-TEXT.<br>
+In order to clone the <i>flhDC</i>-promoter constructs intro pSB1C3, all components were digested with EcoRI and PstI according to the protocol. The restriction products were subsequently separated on a gel in order to verify the digestions success and purification of the desired fragments. </li><br>
+<li>Observations & Results: <br>
+The gel did not feature fragments of the expected size.Obviously, something was wrong with the digestion. </li>
+         </ul>
 <br>
-</li>
+<b>V07_02_2 Preparation of over night cultures</b><br>
+         <ul>
+                 <li>Experiment:  <br>
+In order to gain more plasmid material of the <i>flhDC</i>-promoter constructs over night cultured were prepared for a subsequent plasmid isolation.<br>
+E - #2 <br>
+G - #1 <br>
+G - #1 <br>
+I - #2 <br>
+M - #2 <br>
+O - #2 <br>
+K - #1 <br>
+C - #2 <br></li>
+    </ul>
+<br></td></tr>
 </table>
@@ Line 545: / Line 559: @@
 <td width="900" bordercolor="black" valign="top">
-<h2><b>Versuchsnummer </b></h2><br>
+<h2><b>V07_03 </b></h2><br>
-<b>TITEL</b><br>
+<b>V07_03_1 Miniprep of the <i>flhDC</i>-promoter constructs</b><br>
 <ul>
 <li>Experiment: <br>
-Text</li>
+Minipreps were conducted with PeqGOLD MiniPrep Kit (Peqlab) according to the user manual.</li></ul>
-</li></ul>
 <br>
+<b>V07_03_2 Amplification of the genes <i>fliC</i> (DH10B), <i>fliC</i> (<i>Salmonella</i>), <i>motA</i>, <i>motB</i> and <i>yhjH</i></b><br>
+<ul>
+<li>Experiment:  <br>
+The genes <i>fliC</i> (DH10B), <i>fliC</i> (<i>Salmonella</i>), <i>motA</i>, <i>motB</i> and <i>yhjH</i> were amplified by Pfu-Polymerase according to the following protocol. The success of the PCR was subsequently investigated preparing a 1% agarose gel.<br>
+<li>Observations & Results: <br>
+The PCR failed for no bands were visible on the gel whereas the marker was clearly discernible.</li>
+</ul><br>
 </td></tr>
 </table>
@@ Line 560: / Line 581: @@
 <tr bordercolor="black" valign="top">
 <td width="900" bordercolor="black" valign="top">
-<h2><b>Versuchsnummer </b></h2><br>
+<h2><b>V07_04 </b></h2><br>
-<b> Titel</i></i></b><br>
+<b> Repetition of the amplification of <i>fliC</i> (DH10B), <i>fliC</i> (<i>Salmonella</i>), <i>motA</i>, <i>motB</i> and <i>yhjH</i> </i></i></b><br>
 <ul>
 <li>Experiment: <br>
-Text<br>
+The genes <i>fliC</i> (DH10B), <i>fliC</i> (<i>Salmonella</i>), <i>motA</i>, <i>motB</i> and <i>yhjH</i> were amplified by Pfu-Polymerase according to the following protocol. Additionally, a negative control as well as a positive control were prepared this time. The success of the PCR was subsequently investigated preparing a 1% agarose gel.<br></li>
+<li>Observations & Results: <br>
+The did not function again for no bands were visible on the gel; only the marker was clearly discernible. However, since also the positive control did not feature the slightest band, we assume that something might be wrong with our polymerase.</li>
+<br></td></tr>
+</table>
+<br>
+<table cellpadding="20 px" border="1" bordercolor="black" valign="top">
+<tr bordercolor="black" valign="top">
+<td width="900" bordercolor="black" valign="top">
+<h2><b>V07_05 </b></h2><br>
+<b>V07_05_1 Repetition of the amplification of the genes <i>fliC</i> (DH10B), <i>fliC</i> (<i>Salmonella</i>), <i>motA</i>, <i>motB</i> and <i>yhjH</i></b><br>
+<ul>
+<li>Experiment: <br>
+To give it a last try the <i>fliC</i> (DH10B), <i>fliC</i> (<i>Salmonella</i>), <i>motA</i>, <i>motB</i> and <i>yhjH</i> were amplified by Pfu-Polymerase according to the following protocol one last time. Here again, a 1% agarose gel was prepared to investigate the PCRs outcome.</li><br>
+<li>Observations & Results: <br>
+The gel of the PCR delivered the same picture as last time. No band could be observed except for the marker. Even the positive control does not work. Thus, we decided to buy a new polymerase.</li>
+</ul>
+<br>
+<b>V07_05_2 Repetition of the preparative double digestion of 20G-<i>flhDC</i>, 20I-<i>flhDC</i>, 18K-<i>flhDC</i>, and 18C-<i>flhDC</i></b><br>
+<ul>
+<li>Experiment:  <br>
+The test digestion of the <i>flhDC</i>-promoter constructs EcoRI and PstI  were applied according to the protocol. The restriction products were subsequently separated on a gel in order to verify the digestions success and purify the desired fragments.<br>
+<li>Observations & Results: <br>
+The digestion was successful. Bands of the expected size could be observed and cut out.</li>
+</ul><br>
+</td></tr>
+</table>
+<br>
+<table cellpadding="20 px" border="1" bordercolor="black" valign="top">
+<tr bordercolor="black" valign="top">
+<td width="900" bordercolor="black" valign="top">
+<h2><b>V07_06 </b></h2><br>
+<b> Repetition of the amplification of the <i>fliC</i> (DH10B), <i>fliC</i> (<i>Salmonella</i>), <i>motA</i>, <i>motB</i> and <i>yhjH</i> using the new polymerase </b><br>
+<ul>
+<li>Experiment: <br>
+The genes <i>fliC</i> (DH10B), <i>fliC</i> (<i>Salmonella</i>), <i>motA</i>, <i>motB</i> and <i>yhjH</i> were amplified by Phusion-Polymerase according to the following protocol. We also prepared a negative control as well as a positive control. The success of the PCR was subsequently investigated preparing a 1% analytical agarose gel.<br></li>
+<li>Observations & Results: <br>
+Finally,the PCR was successful! We were able to receive bands of the expected size for each construct. Obviously, the old Pfu-polymerase was not functional anymore and had caused the PCRs failure. </li>
 <br></td></tr>
 </table>