Team:Goettingen/week20-2

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#2 Speed Improvement - 20th week

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V09_10

V09_10_1 Miniprep of pSB1C3 (including motA, motB or yhjH)

Experiment:
Plasmids were prepped using PeqGOLD MiniPrep Kit (Peqlab) accirding to the manual.

V09_10_2 Test digestion of pSB1C3 (including motA, motB or yhjH)

Experiment:
Test digestion of pSB1C3 (including motA, motB or yhjH) with the restriction enzymes EcoRI and PstI. Afterwards, the product was loaded in a 1% analytical gel in order to verify its success.
Observations & Results:
The digestion worked for all clones since fragments with the appropriate size were produced over all.

V09_10_3 Digestion of motA, motB, yhjH and the promoters 20E, 20I and 18C

Experiment:
motA, motB or yhjH were digested with XbaI and PstI. The plasmids with the different promoters were treated with SpeI and PstI. The digestion was then controlled via gel-electrophoresis.
Observations & Results:
Since for all clones band of the expected size could be obtained these were isolated from the gel and purified using PeqGOLD Gelextraction Kit (Peqlab) according to the manual.

V09_10_4 Repetition of the Quikchange of fliC

Experiment:
This the Quikchange PCR was performed using the designed primers and a new PfuTurbo polymerase (see Quick Change protocol in "protocols"). 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. Whether the primers, the enzyme or anything else cause the QC PCRs failure is not clear to us yet.

V09_11

V09_11_1 Insertion motA, motB and yhjH into J61002

Experiment:
motA, motB and yhjH were ligated nto the plasmid J61002 with different promoters (20E, 20I and 18C) according to the protocol.

V09_11_2 Chemical transformation of motA, motB and yhjH into E. coli DH10B

Experiment:
The ligation products were transformed into the E. coli DH10B as described in the standard protocol.
Observations & Results:
The transformation was successful since numerous colonies were grown on all plates except for the negative control.

V09_11_3 Repetition of the Quikchange of fliC part 1

Experiment:
After consultation with our supervisor we decided to give the QC PCR another try using Phusion polymerase this time. The first reaction round resulting in the production of the four short fragments was prepared according to the protocol and subsequently analyzed on gel.
Observations & Results:
This time the QC PCR was successful! The gel showed stron bands of the expected size. Obviously the PfuTurbo polymerase, which is known to be perfect for Quikchange was the reason for the previous failures.

V09_12

V09_12_1 Repetition of the Quikchange of FliC part 2

Experiment:
Since the first round of amplifications was successful, the samples 1 and 2 as well as 3 and 4 were combined via overlapping PCR. Afterwards, the samples 1+2 and 3+4 were combined as well. For all reaction the new Phusion polymerase was used. The success of both reactions was investigated via agarose gel electrophoresis.
Observations & Results:
Both reactions were successful. We were able to receive fragments of a reasonable size.

V09_12_2 Preparative double digestion of yhjH

Experiment:
In order to clone yhjH behind different promoter a digestion with XbaI and PstI was performed according to the protocol. The restriction product was subsequently loaded on a 1% agarose gel, cut out and purified using the PeqGOLD Gelextraction Kit (Peqlab).
Observations & Results:
The digestion was successful for bands of the correct size could be observed.

V09_12_3 Insertion of yhjH into J61002 including the promoters 20E, 20I and 18C

Experiment:
yhjH was ligated into the plasmid J61002 behind the promoters 20E, 20I and 18C according to the protocol.

V09_12_4 Preparative double digestion of RFP-promoter constructs and pSB1C3

Experiment:
In order to bring the promoters of the BioBrick library we used for our experiments on the new BioBrick standard the parts as well as pSB1C3 were digested with EcoRI and PstI as described in the protocol. The restriction products were subsequently loaded on a 1% agarose gel, cut out and purified using the PeqGOLD Gelextraction Kit (Peqlab).
Observations & Results:
The digestion was successful for bands of the correct size could be observed.

V09_12_5 Insertion of the RFP-promoter constructs into pSB1C3

Experiment:
The eight RFP-promoter constructs were ligated into the vector pSB1C3 according to the protocol.

V09_12_6 Miniprep of motA, motB and RFP

Experiment:
Minipreps of motA, motB and RFP in pSB1C3 were conducted using the PeqGOLD MiniPrep Kit (Peqlab) according to the user manual.

V09_13

V09_13_1 Chemical transformation of the RFP-promoter constructs (in pSB1C3) into E. coli DH10B

Experiment:
The transformation was performed as described in the protocol.
Observations & Results:
successful?

V09_13_2 Preparative double digestion of fliC

Experiment:
In order to clone fliC into pSB1C3 the product of the QC PCR was digested with EcoRI and PstI according to the protocol. The restriction products were subsequently leaded on a 1% agarose gel, cut out and purified using the PeqGOLD MiniPrep Kit (Peqlab) according to the user manual.
Observations & Results:
The digestion was successful since fragments of the expected size could be obtained.

V09_13_3 Insertion of fliC into pSB1C3

Experiment:
For the ligation of fliC into the vector pSB1C3 the protocol was followed.

V09_13_4 Preparation of over night cultures

Experiment:
The following over night cultures were prepared:
PSB1C3-MotA in DH10B and BL21
PSB1C3-motB in DH10B and BL21

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@@ Line 543: / Line 543: @@
 <b>V09_10_2 Test digestion of pSB1C3 (including <i>motA</i>, <i>motB</i> or <i>yhjH</i>)</b><br>
 <ul>
-<li>Experiment: <br>Test digestion of pSB1C3 (including <i>motA</i>, <i>motB</i> or <i>yhjH</i>) with the restriction enzymes EcoRI and PstI. Afterwards, the product was loaded in a 1% analytical gel in order to verify its success.<br> </li>
+<li>Experiment: <br>Test digestion of pSB1C3 (including <i>motA</i>, <i>motB</i> or <i>yhjH</i>) with the restriction enzymes <i>EcoRI</i> and <i>PstI</i>. Afterwards, the product was loaded in a 1% analytical gel in order to verify its success.<br> </li>
 <li>Observations & Results: <br>
   The digestion worked for all clones since fragments with the appropriate size were produced over all. </li>
@@ Line 550: / Line 550: @@
 <b>V09_10_3 Digestion of <i>motA</i>, <i>motB</i>, <i>yhjH</i> and the promoters 20E, 20I and 18C</b><br>
 <ul>
-<li>Experiment: <br> <i>motA</i>, <i>motB</i> or <i>yhjH</i> were digested with XbaI and PstI. The plasmids with the different promoters were treated with SpeI and PstI. The digestion was then controlled via gel-electrophoresis.<br> </li>
+<li>Experiment: <br> <i>motA</i>, <i>motB</i> or <i>yhjH</i> were digested with <i>XbaI</i> and <i>PstI</i>. The plasmids with the different promoters were treated with <i>SpeI</i> and <i>PstI</i>. The digestion was then controlled via gel-electrophoresis.<br> </li>
 <li>Observations & Results: <br>
 Since for all clones band of the expected size could be obtained these were isolated from the gel and purified using PeqGOLD Gelextraction Kit (Peqlab) according to the manual.</li>
@@ Line 557: / Line 557: @@
 <b> V09_10_4 Repetition of the Quikchange of <i>fliC</i></b><br>
 <ul>
-<li>Experiment: <br> This the Quikchange PCR was performed using the designed primers and a new Pfu Turbo polymerase (see Quick Change protocol in "protocols"). Also this time four short fragments were produced first and subsequently combined to a complete final DNA fragment. <br></li>
+<li>Experiment: <br> This the Quikchange PCR was performed using the designed primers and a new <i>PfuTurbo</i> polymerase (see Quick Change protocol in "protocols"). 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. Whether the primers, the enzyme or anything else cause the QC PCRs failure is not clear to us yet.  </li>
@@ Line 586: / Line 586: @@
 After consultation with our supervisor we decided to give the QC PCR another try using Phusion polymerase this time. The first reaction round resulting in the production of the four short fragments was prepared according to the protocol  and subsequently analyzed on gel. <br></li>
 <li>Observations & Results: <br>
-This time the QC PCR was successful! The gel showed stron bands of the expected size. Obviously the Pfu Turbo polymerase, which is known to be perfect for Quikchange was the reason for the previous failures. </li>
+This time the QC PCR was successful! The gel showed stron bands of the expected size. Obviously the <i>PfuTurbo</i> polymerase, which is known to be perfect for Quikchange was the reason for the previous failures. </li>
 </ul>
 <br></td></tr>
@@ Line 598: / Line 598: @@
 <ul>
 <li>Experiment: <br>
-Since the first round of amplifications was successful, the samples 1 and 2 as well as 3 and 4 were combined via overlapping PCR. Afterwards, the samples 1+2 and 3+4 were combined as well. The success of both reactions was investigated via agarose gel electrophoresis. </li>
+Since the first round of amplifications was successful, the samples 1 and 2 as well as 3 and 4 were combined via overlapping PCR. Afterwards, the samples 1+2 and 3+4 were combined as well. For all reaction the new Phusion polymerase was used. The success of both reactions was investigated via agarose gel electrophoresis. </li>
 <li>Observations & Results: <br>
 Both reactions were successful. We were able to receive fragments of a reasonable size. </li>
@@ Line 606: / Line 606: @@
 <ul>
 <li>Experiment: <br>
-In order to clone <i>yhjH</i> behind different promoter a digestion with XbaI and PstI was performed according to the protocol. The restriction product was subsequently loaded on a 1% agarose gel, cut out and purified using the PeqGOLD Gelextraction Kit (Peqlab).</li>
+In order to clone <i>yhjH</i> behind different promoter a digestion with <i>XbaI</i> and <i>PstI</i> was performed according to the protocol. The restriction product was subsequently loaded on a 1% agarose gel, cut out and purified using the PeqGOLD Gelextraction Kit (Peqlab).</li>
 <li>Observations & Results: <br>
 The digestion was successful for bands of the correct size could be observed. </li>
@@ Line 618: / Line 618: @@
 <ul>
 <li>Experiment: <br>
-In order to bring the promoters of the BioBrick library we used for our experiments on the new BioBrick standard the parts as well as pSB1C3 were digested with EcoRI and PstI  as described in the protocol. The restriction products were subsequently loaded on a 1% agarose gel, cut out and purified using the PeqGOLD Gelextraction Kit (Peqlab).  </li>
+In order to bring the promoters of the BioBrick library we used for our experiments on the new BioBrick standard the parts as well as pSB1C3 were digested with <i>EcoRI</i> and <i>PstI</i>  as described in the protocol. The restriction products were subsequently loaded on a 1% agarose gel, cut out and purified using the PeqGOLD Gelextraction Kit (Peqlab).  </li>
 <li>Observations & Results: <br>
 The digestion was successful for bands of the correct size could be observed.</li>
@@ Line 651: / Line 651: @@
 <ul>
 <li>Experiment: <br>
-In order to clone <i>fliC</i> into pSB1C3 the product of the QC PCR was digested with EcoRI and PstI according to the protocol. The restriction products were subsequently leaded on a 1% agarose gel, cut out and purified using the PeqGOLD MiniPrep Kit (Peqlab) according to the user manual.  </li>
+In order to clone <i>fliC</i> into pSB1C3 the product of the QC PCR was digested with <i>EcoRI</i> and <i>PstI</i> according to the protocol. The restriction products were subsequently leaded on a 1% agarose gel, cut out and purified using the PeqGOLD MiniPrep Kit (Peqlab) according to the user manual.  </li>
 <li>Observations & Results: <br>
 The digestion was successful since fragments of the expected size could be obtained. </li>
@@ Line 663: / Line 663: @@
 <ul>
 <li>Experiment: <br> The following over night cultures were prepared:<br>
-Psb1c3-MotA in DH10B and BL21<br>
+PSB1C3-<i>MotA</i> in DH10B and BL21<br>
-Psb1c3-MotB in DH10B and BL21<br>
+PSB1C3-<i>motB</i> in DH10B and BL21<br>
 </li>
 </ul>