Latest revision as of 02:15, 27 September 2012

iGEM TEAM ::: SDU-DENMARK

Laboratory Notebook

1st week	2nd week	3rd week	4th week
5th week	6th week	7th week	8th week
9th week	10th week	11th week	12th week

27-08-2012 to 02-09-2012

After 48 hours in the incubator, the 1-FFT colonies finaly reached a high enough concentration for sequencing.

Meanwhile, all the SST colonies had died out. To avoid unnecesary excess work, we simply ran PCR with all mutagenesis primers on an older 1-SST containing pJET plasmid. Miraculous, both gel band length and check digest on the resulting sequence yielded perfect results. Why had we not done this before?

In the following days 1-SST ligated into pJET, grown on ampicillin plates, transformed into Top10, transfered to liquid medium and miniprepped for sequencing.

@@ Line 293: / Line 293: @@
 <p> <b>27-08-2012  to  02-09-2012</b> </p>
-<p>DNA purification from FFT liquid cultures were made.<br/></br>
+<p>
-Nanodrop was performed on it:<br/>
+After 48 hours in the incubator, the 1-FFT colonies finaly reached a high enough concentration for sequencing.<br/><br/>
-: 83,6 ηg/μL<br/>
-: 17,2 ηg/μL<br/>
-: 121,1 ηg/μL<br/>
-: 48,1 ηg/μL<br/>
-: 99,1 ηg/μL<br/>
-: 59,6 ηg/μL<br/>
-: nothing(an error must have occurred)<br/>
-: 59,6 ηg/μL<br/></br>
-We made check-digest with EcoRI+SpeI to examine the plasmids in preparation of mutagenesis.
-The check digest showed that some had the appropriate digested sizes we would expect from a plasmid of 3kb and a gene of 2kb.<br/></br>
-Mutagenesis was run on these FFT colonies containing all primers.<br/>
-We made new SST cultures again and plated them on AMP-resistance plates. <br/>
-Isolated FFT and SST plasmids and sent them for sequencing.<br/>
-Afterwards we did a digest and transformation on FFT and plated them.<br/>
-We made liquid cultures of FFT and SST and incubated them over night. Later we made transformation on the three parts we chose from the iGEM kit.<br/>
-) R0010 <br/>
-) E0040<br/>
-) B0015<br/>
-Afterwards we plated them on AMP-resistance plates. <br/>
-We made liquid cultures of the three parts<br/></br>
-<h2>Purification of SST, FFT, B0015, E0040 and R0010 and following PCR</h2></br>
-<p>The O.N. cultures of SST, FFT and our 3 parts (B0015/terminator, E0040/GFP and R0010/LacL) showed promising results of growth. A miniprep was made from the 32 samples and a Nanodrop as well which gave the following results:
-</p>
-<TABLE border="1" width="100%">
+Meanwhile, all the SST colonies had died out. To avoid unnecesary excess work, we simply ran PCR with all mutagenesis primers on an older 1-SST containing pJET plasmid. Miraculous, both gel band length and check digest on the resulting sequence yielded perfect results. Why had we not done this before?<br/><br/>
-<CAPTION><EM>NanoDrop Results</EM></CAPTION>
-<TR><TH>1. R0010, culture 1 <TD>18,0 ng/ul<TH> <TD>
-<TR><TH>2. B0015, culture 3<TD>67,9 ng/ul<TH> <TD>
-<TR><TH>3. B0015, culture 5 <TD>62,9 ng/ul <TH> <TD>
-<TR><TH>4. R0010, culture 3 <TD>70,5 ng/ul <TH> <TD>
-<TR><TH>5. R0010, culture 5 <TD>69,2 ng/ul <TH> <TD>
-<TR><TH>6. E0040, culture 6  <TD>35,5 ng/ul <TH> <TD>
-<TR><TH>7. E0040, culture 1 <TD>66,2 ng/ul <TH> <TD>
-<TR><TH>8. E0040, culture 3  <TD>47,5 ng/ul <TH> <TD>
-<TR><TH>9. SST plate 1, culture 1 <TD>13,9 ng/ul <TH> <TD>
-<TR><TH>10. R0010, culture 2 <TD>22,3 ng/ul <TH> <TD>
-<TR><TH>11. E0040, culture 5 <TD>98,9 ng/ul <TH> <TD>
-<TR><TH>12. FFT plate 8, culture 5 <TD>22,4 ng/ul <TH> <TD>
-<TR><TH>13. FFT plate 4, culture 3 <TD>11,5 ng/ul <TH> <TD>
-<TR><TH>14. E0040, culture 2 <TD>50,2 ng/ul <TH> <TD>
-<TR><TH> <TD> <TH> <TD>
-<TR><TH> <TD> <TH> <TD>
-</TABLE>
+In the following days 1-SST ligated into pJET, grown on ampicillin plates, transformed into Top10, transfered to liquid medium and miniprepped for sequencing.<br/>
+</p>

Team:SDU-Denmark/labwork/Notebook/week9

From 2012.igem.org

Latest revision as of 02:15, 27 September 2012

Laboratory Notebook