Team:Heidelberg/Tyrocidine

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             <!--Project Description-->
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                        <h1><span style="font-size:180%;color:#074E0B;">Tyrocidine.</span><span class="text-muted" style="font-family:Arial, sans-serif; font-size:100%"> Proving Modularity of NRPS by Shuffling Modules.</span></h1>
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                        <h1><span style="font-size:180%;color:#800000;">Novel NRPS</span> <span style="font-size:180%;color:#666666;">&</span> <span style="font-size:180%;color:#0B2161;">Indigoidine-Tag.</span><span class="text-muted" style="font-family:Arial, sans-serif; font-size:100%"> Exploring Modularity of NRPS by Shuffling Modules.</span></h1>
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                         <p>Lorem ipsum dolor sit amet, consetetur sadipscing elitr, sed diam nonumy eirmod tempor invidunt ut labore et dolore magna aliquyam erat, sed diam voluptua. At vero eos et accusam et justo duo dolores et ea rebum. Stet clita kasd gubergren, no sea takimata sanctus est Lorem ipsum dolor sit amet.</p>
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                     <!--<button type="button" class="btn btn-default">May</button>
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                                   <h1>Week 12</h1>
                                   <h1>Week 12</h1>
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<b> Module Shuffling </b> <br/>
Our strain <i>Brevibacillus Parabrevis</i> arrived from the Marahiel-lab. As preparation for the module shuffling experiments the strain was validated with test primers by colony PCR. The screening was positive, so we designed our Gibson compatible primers for amplification. </p>
Our strain <i>Brevibacillus Parabrevis</i> arrived from the Marahiel-lab. As preparation for the module shuffling experiments the strain was validated with test primers by colony PCR. The screening was positive, so we designed our Gibson compatible primers for amplification. </p>
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                                   <h1>Week 13</h1>
                                   <h1>Week 13</h1>
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">We started with the amplification of fragments for the module shuffling with Gibson Primers. Most fragments were amplified in the first attempt, however others needed protocol optimization. At the end of the week 12 out of 15 fragments were successfully amplified. The next step to take, is to amplify the remaining fragments and start with the Gibson Assembly. </p>
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">
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<b>Module Shuffling</b><br/>
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We started with the amplification of fragments for the module shuffling with Gibson Primers. Most fragments were amplified in the first attempt, however others needed protocol optimization. At the end of the week 12 out of 15 fragments were successfully amplified. The next step to take, is to amplify the remaining fragments and start with the Gibson Assembly. </p>
                                    
                                    
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                                   <h1>Week 14</h1>
                                   <h1>Week 14</h1>
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">After DNA concentration measurements, some of the previously amplified fragments had to be reamplified. The PCR protocols were optimized and the missing fragments were successfully obtained. We amplified all fragments with the necessary concentration to start with the Gibson assembly. However we noticed that we mixed up fragments during the assembly of Tripeptide-I-NRPS (pIK04)and resumed this experiment in the next week. </p>
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">
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<b> Module Shuffling </b> <br/>
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After DNA concentration measurements, some of the previously amplified fragments had to be reamplified. The PCR protocols were optimized and the missing fragments were successfully obtained. We amplified all fragments with the necessary concentration to start with the Gibson assembly. However we noticed that we mixed up fragments during the assembly of Tripeptide-I-NRPS (pIK04)and resumed this experiment in the next week. </p>
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                                   <h1>Week 15</h1>
                                   <h1>Week 15</h1>
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">The DNA concentration for all obtained fragments were measured and used for the calculation of the Gibson Assembly master mix. All five NRPS constructs producing the Dipeptide, Tripeptides I & II and Tetrapeptides I & II were assembled into a pSB1C3 backbone, electroporated into DH10β and spread on Chloramphenicol-LB plates. Several white colonies were picked and grown in 2x YT medium. Their mini-preps where validated through restriction digest. Positive samples were sent to sequencing. The results arrived in week 16.
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">
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<b> Module Shuffling </b> <br/>
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The DNA concentration for all obtained fragments were measured and used for the calculation of the Gibson Assembly master mix. All five NRPS constructs producing the Dipeptide, Tripeptides I & II and Tetrapeptides I & II were assembled into a pSB1C3 backbone, electroporated into DH10β and spread on Chloramphenicol-LB plates. Several white colonies were picked and grown in 2x YT medium. Their mini-preps where validated through restriction digest. Positive samples were sent to sequencing. The results arrived in week 16.<br/><br/>
For the detection of the short synthetic NRPs we decided on using Mass Spectrometry (MS) and contacted a MS facility on campus. </p>
For the detection of the short synthetic NRPs we decided on using Mass Spectrometry (MS) and contacted a MS facility on campus. </p>
                                   <p><a class="btn btn-large btn-primary" href="#">Learn more</a></p>
                                   <p><a class="btn btn-large btn-primary" href="#">Learn more</a></p>
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                                   <h1>Week 16</h1>
                                   <h1>Week 16</h1>
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;"><b>Module Shuffling</b>
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">
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Sequencing proved the successful assembly of the Tripeptide-I-NRPS (pIK04). All other NRPs had to be reconstructed through a new Gibson Assembly. For this purpose, we optimized the Gibson Assembly master mix, assuming that backbone religations were one of the main reasons for the failed assembly. We calculated a lower backbone-to-insert ratio and added fragment 12 in excess to the Tetrapeptide-I-fragment-mix. The assembled plasmids were transformed into electrocompetent DH10β and plated onto Cm-Lb. Afterwards white colonies were picked and grown overnight in 2x YT medium (Cm). Their mini-preps were analyzed with restriction digest. Two samples of each the Dipeptide (pIK03) and the Tetrapeptide-I (pPW01) plasmids were sent to sequencing. There was no positive restriction digest, neither for the Tetrapeptide-I-NRPS (pPW01) nor for Tetrapeptide-II-NRPS (pPW02). We decided not to reassemble the Tetrapeptide-II-construct (pPW02) and did not continue working on this NRP. Hence only colonies on the Tetrapeptide-I-construct (pPW01) plates were picked.
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<b>Module Shuffling</b> <br/>
 +
Sequencing proved the successful assembly of the Tripeptide-I-NRPS (pIK04). All other NRPs had to be reconstructed through a new Gibson Assembly. For this purpose, we optimized the Gibson Assembly master mix, assuming that backbone religations were one of the main reasons for the failed assembly. We calculated a lower backbone-to-insert ratio and added fragment 12 in excess to the Tetrapeptide-I-fragment-mix. The assembled plasmids were transformed into electrocompetent DH10β and plated onto Cm-Lb. Afterwards white colonies were picked and grown overnight in 2x YT medium (Cm).  
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<br/><br/>
 +
Their mini-preps were analyzed with restriction digest. Two samples of each the Dipeptide (pIK03) and the Tetrapeptide-I (pPW01) plasmids were sent to sequencing. There was no positive restriction digest, neither for the Tetrapeptide-I-NRPS (pPW01) nor for Tetrapeptide-II-NRPS (pPW02). We decided not to reassemble the Tetrapeptide-II-construct (pPW02) and did not continue working on this NRP. Hence only colonies on the Tetrapeptide-I-construct (pPW01) plates were picked.
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<br/><br/>
The positive Dipeptide- (pIK03), Tripeptide-I (pIK04) and Tetrapeptide-I (pPW01) NRPS constructs were chemically transformed into BAP I cells and plated onto Cm-LB. Furthermore colonies were picked and validated through restriction digest. Here only pIK03 (Dipeptide) and pIK04 (Tripeptide-I) were positive. The Tetrapeptide-I-NRPS (pPW01) was chemically transformed a second time into BAP I.
The positive Dipeptide- (pIK03), Tripeptide-I (pIK04) and Tetrapeptide-I (pPW01) NRPS constructs were chemically transformed into BAP I cells and plated onto Cm-LB. Furthermore colonies were picked and validated through restriction digest. Here only pIK03 (Dipeptide) and pIK04 (Tripeptide-I) were positive. The Tetrapeptide-I-NRPS (pPW01) was chemically transformed a second time into BAP I.
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<b>NRPS-Library</b>
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<br/><br/>
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For the standardization of the modules from the Tyrocidine cluster used in the shuffling we started amplification with the previously ordered Primers for Modules tycAdCom, tycB1dCom, tycC5, tycC6 introducing the RFC10 prefix and suffix. However, errors in the reverse Primers for tycC5 and tycC6 were noticed and re-ordered. Still the amplification of modules tycAdCom and tycB1dCom was started, but could not be amplified in the necessary concentrations.
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<b>Interspecies <br/> Module Shuffling</b><br/>
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<b>Interspecies Module Shuffling</b>
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The primers for the interspecies NRPS fusion of different Tyrocidine modules with the Indigoidine synthetase indC were designed and ordered.
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The primers for the interspecies NRPS fusion of different Tyrocidine modules with the Indigoidine synthetase indC were designed and ordered. </p>
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<br/><br/>
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<b>BioBrick Assembly</b><br/>
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For the standardization of the modules from the Tyrocidine cluster used in the shuffling we started amplification with the previously ordered Primers for Modules tycAdCom, tycB1dCom, tycC5, tycC6 introducing the RFC10 prefix and suffix. However, errors in the reverse Primers for tycC5 and tycC6 were noticed and re-ordered. Still the amplification of modules tycAdCom and tycB1dCom was started, but could not be amplified in the necessary concentrations. </p>
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                                   <h1>Week 17</h1>
                                   <h1>Week 17</h1>
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">Validation and characterization of BAP I cells transformed with the Dipeptide- (pIK03), Tripeptide-I- (pIK04) and Tetrapeptide-I-synthetase (pPW01) constructs through restriction digest. The pIK03 and pIK04 were positive and sent to sequencing.
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">
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<b>Module Shuffling</b><br/>
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Validation and characterization of BAP I cells transformed with the Dipeptide- (pIK03), Tripeptide-I- (pIK04) and Tetrapeptide-I-synthetase (pPW01) constructs through restriction digest. The pIK03 and pIK04 were positive and sent to sequencing.  
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<br/><br/>
The restriction digest for pPW01 was negative. I a new strategy it was therefore co-transformed with a plasmid (pRB15) carrying the PPTase sfp into electrocompetent DH10β. Again the restriction digest was negative and we decided to abandon this construct assuming it was too big for simple transformation.
The restriction digest for pPW01 was negative. I a new strategy it was therefore co-transformed with a plasmid (pRB15) carrying the PPTase sfp into electrocompetent DH10β. Again the restriction digest was negative and we decided to abandon this construct assuming it was too big for simple transformation.
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<br/><br/>
For the Mass Spectrometry (MS) we needed to find a clone strongly expressing the NRPS. Therefore we performed a SDS-PAGE, which failed due to systematic errors. This was resumed the following week.
For the Mass Spectrometry (MS) we needed to find a clone strongly expressing the NRPS. Therefore we performed a SDS-PAGE, which failed due to systematic errors. This was resumed the following week.
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The RFC10 standardization of the modules still showed to be difficult due to the total length of prefix/suffix + binding sequence (resulting in high annealing temperatures). To be efficient, we focused on the optimization of the amplification protocol for tycAdCom. We succeeded and adapted our protocols in the same manner for the other modules. Again the amplification for tycB1 and tycC5 failed, however we were able to amplify the module tycC6. After many attempts we redesigned the primers for tycB1dCom (fw and rv) and tycC5 (fw).
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<br/><br/>
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The experiments concerning the synthesis of the interspecies fusion of a Tyrocidine module and the Indigoigine synthetase were started with the amplification of the fragments needed for introduction of the three constructs (coding for Phe-/Asn-/Val-Ind-Synthetases) into their backbone pSB1C3 by Gibson Assembly. All of those fragments were obtained in the necessary concentrations after optimization of the protocols. </p>
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<b>Interspecies <br/>Module Shuffling</b><br/>
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The experiments concerning the synthesis of the interspecies fusion of a Tyrocidine module and the Indigoigine synthetase were started with the amplification of the fragments needed for introduction of the three constructs (coding for Phe-/Asn-/Val-Ind-Synthetases) into their backbone pSB1C3 by Gibson Assembly. All of those fragments were obtained in the necessary concentrations after optimization of the protocols.
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<br/><br/>
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<b>BioBrick Assembly</b><br/>
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The RFC10 standardization of the modules still showed to be difficult due to the total length of prefix/suffix + binding sequence (resulting in high annealing temperatures). To be efficient, we focused on the optimization of the amplification protocol for tycAdCom. We succeeded and adapted our protocols in the same manner for the other modules. Again the amplification for tycB1 and tycC5 failed, however we were able to amplify the module tycC6. After many attempts we redesigned the primers for tycB1dCom (fw and rv) and tycC5 (fw). </p>
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                                   <h1>Week 18</h1>
                                   <h1>Week 18</h1>
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">We started the week with a SDS-PAGE analyzing the expression capacity of several clones for the Dipeptide- and Tripeptide-I-NRPS. It showed a positive band for the Dipeptide synthetase (212 kDa) and an inconclusive band for the Tripeptide-I synthetase (381 kDa), because the top band of our ladder was at 260 kDa). Hence we interpreted this as a positive result for Tripeptide-I-synthetase as well.
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New primers for the tycB1dCom and tycC5 modules arrived and new protocols led to the successful amplification of the fragments. A restriction digest with EcoRI and PstI was executed to linearize the backbone pSB1C3 and to prepare the fragments for ligation. The Ligation was performed with T4 Ligase and then transformed into TOP10 cells. White clones where screened with a colony PCR (VF2 and VR primers) and one positive sample for each RFC10 compatible module-construct was sent to sequencing.
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<b>Module Shuffling</b><br/>
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Our fusion experiment was continued for all three constructs with the Gibson Assembly into pSB1C3. The mix was electroporated into DH10β and plated onto Cm-LB. The analytical restriction digest of picked colonies was positive for all constructs. Selected samples of each were proven to be positive by sequencing. Thereafter, the constructs were chemically transformed into our expression strain BAPI and spread onto Cm-LB plates. The colonies turned blue after less than two days, indicating the expression of Indigoidine. First a SDS-PAGE was executed showing that only the band for the Fusion NRPS producing Val-Ind was positive. For this clone purified Valine-Indigoidine from liquid culture was run next to native Indigoidine in a comparative TLC. Here it could be shown that the product from the Val-Ind-Synthetase runs slower than native Indigoidine. At this point it was already possible to assume that Indigoidine could be used to tag other NRP synthetase products by fusing it at the end of NRPS coding genes. To prove this assumption we designed a new strategy for the fusion of the indC to up to four Tyrocidine modules. For this plan new Gibson Assembly compatible primers were designed and ordered. </p>
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We started the week with a SDS-PAGE analyzing the expression capacity of several clones for the Dipeptide- and Tripeptide-I-NRPS. It showed a positive band for the Dipeptide synthetase (212 kDa) and an inconclusive band for the Tripeptide-I synthetase (381 kDa), because the top band of our ladder was at 260 kDa. We interpreted this as a positive result for Tripeptide-I-synthetase as well.
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<br/><br/>
 +
<b>Interspecies <br/>Module Shuffling</b><br/>
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 +
Our fusion experiment was continued for all three constructs with the Gibson Assembly into pSB1C3. The mix was electroporated into DH10β and plated onto Cm-LB. The analytical restriction digest of picked colonies was positive for all constructs. Selected samples of each were proven to be positive by sequencing. Thereafter, the constructs were chemically transformed into our expression strain BAPI and spread onto Cm-LB plates. The colonies turned blue after less than two days, indicating the expression of Indigoidine.  
 +
<br/><br/>
 +
First a SDS-PAGE was executed showing that only the band for the Fusion NRPS producing Val-Ind was positive. For this clone purified Valine-Indigoidine from liquid culture was run next to native Indigoidine in a comparative TLC. We were able to show that the product from the Val-Ind-Synthetase runs slower than native Indigoidine. As a result Indigoidine can be used to tag other NRP synthetase products by fusing it at the end of NRPS coding genes. To prove this assumption we designed a new strategy for the fusion of the indC to up to four Tyrocidine modules. For this experiment new Gibson Assembly compatible primers were designed and ordered.
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<br/><br/>
 +
<b>BioBrick Assembly</b><br/>
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New primers for the tycB1dCom and tycC5 modules arrived and new protocols led to the successful amplification of the fragments. A restriction digest with EcoRI and PstI was executed to linearize the backbone pSB1C3 and to prepare the fragments for ligation. The Ligation was performed with T4 Ligase and then transformed into TOP10 cells. White clones where screened with a colony PCR (VF2 and VR primers) and one positive sample for each RFC10 compatible module-construct was sent to sequencing.</p>
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                                   <h1>Week 19</h1>
                                   <h1>Week 19</h1>
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">Cras justo odio, dapibus ac facilisis in, egestas eget quam. Donec id elit non mi porta gravida at eget metus. Nullam id dolor id nibh ultricies vehicula ut id elit.</p>
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                                  <b>Module Shuffling</b><br/>
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Two months after the start of the tyrocidine project and after a lot of planning concerning the verifiability of the existence of small synthetic non-ribosomal peptides, the purification procedure for mass spectrometry was conducted. Since our backup strategies were rather complex, the simplest purification procedure was chosen to begin with. This procedure was performed in order to get a general idea of whether further desalting steps were needed. Purified samples were delievered to the neonate screening facility (tandem MS) at the university medical centre and the mass spectrometry facility at the Institute for Chemistry (HR-ESI MS). <br/><br/>
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After a first measurement with a tandem mass spectrometer (neonate screening facility) reasonable amino acid levels were observed, accounting for a well suited sample work up process. Therefore, samples of different constructs were taken at several time points after induction and delievered as well to assess time dependet expression. <br/><br/>
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<b>BioBrick Assembly</b><br/>
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<i>Module Shuffling </i><br/>
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For our RFC10 standardized modules we had to reamplify all fragments again and then prepared them by restriction digest with EcoRI and PstI for the standard Ligation. The standard shipment backbone pSB1C3 was linearized in this process. After Ligation with T4-Ligase and transformation into TOP10 cells white colonies were picked from the LB-Cm plates. The colonies were screened with VR and VF2 primers in a colony PCR. For each we could find a positive sample, of which we sent a sample to sequencing<br/><br/>
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 +
 
 +
<i>Interspecies Module Shuffling</i><br/>
 +
Since two illegal cutting sites of RFC-10 restriction enzymes were found, a CPEC approach was tried for the Asn-Indigoidine fusion (pPW04) to introduce a mutation at the targeted position. In the first instance this procedure did not result in visible colonies after transformation and is therefore planned to be repeated in the upcoming week.</p>
                                   <p><a class="btn btn-large btn-primary" href="#">Browse gallery</a></p>
                                   <p><a class="btn btn-large btn-primary" href="#">Browse gallery</a></p>
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                                   <h1>Week 20</h1>
                                   <h1>Week 20</h1>
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<b> Module Shuffling</b> <br/>
 +
In this week we sent two samples to the mass spectrometry facility of the Institute for Chemistry on campus. We have been offered only a couple of free measurements, so we decided to send two pellet samples containing the Dipeptide (pIK03) and Tripeptide-I (pIK04). Even though we did not receive a conclusive spectrum we can be sure that the salt concentrations were low enough to not overlap the signals of our peptides. We assume that either the solvent or cell lysis debris could be the reason for the unspecific profile. We now want to test samples of the supernatant, as well. <br/><br/>
 +
 
 +
<b>Interspecies Module Shuffling </b><br/>
 +
Because we could detect the Valin-Indigoidine NRP with comparative TLC and its synthetase by SDS-PAGE, we designed seven additional constructs adding up to four modules in front of the indC. We successfully amplified all fragments for the Gibson assembly and transformed the new constructs into electrocompetent DH10β.<br/><br/>
 +
 
 +
<b> BioBrick Assembly</b><br/>
 +
<i> Module Shuffling </i> <br/>
 +
The sequencing showed positive results for tycAdCom, tycB1dCom (silent mutations) and tycC6 (silent mutation). However the suspected tycC5 carying plasmid did NOT contain the right insert in the alignment. We tried to reamplify this fragment, however could not find the right protocol. We assume that, instead of tycC5, tycB1dCom (or similar) was the insert and that tycC5 was amplified with the same protocols as tycB1dCom because it was in fact tycB1dCom and not tycC5. Because of the amplification dificulties and the limited time we decided to cancel the standardization of tycC5.<br/>
 +
We started the preparation of the positive plasmids for shipping to the parts-registry.<br/><br/>
 +
<i>Interspecies Module Shuffling </i><br/>
 +
With regard to the week before, the CPEC approach was resumed with a mutation at the desired position. In parallel as an alternative approach the indC fragment of the domain shuffling experiments was used.<br/><br/></p>                
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                                   <h1>Week 21</h1>
                                   <h1>Week 21</h1>
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                                  <p><a class="btn btn-large btn-primary" href="#">Browse gallery</a></p>
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<b>Tyrocidine-Indigoidine-fusion</b><br/>
 +
During this week we proceeded with our work on the five Tyrocidine-Indigoidine fusion constructs (pPW06, pPW09, pPW10, pPW11, pPW12). The best result was achieved for the Orn-Val-Ind fusion. For plasmids pPW11 and pPW12 colony PCRs were prepared and positive samples were transformed into BAP-I.<br/><br/>
 +
 
 +
<b>ccdB-Indigoidine template</b><br/>
 +
We successfully amplified all necessary DNA fragments for Gibson assembly of the pJS01 plasmid. DNA concentrations were estimated via analytical gel electrophoresis and accordingly added to a common micro centrifuge tube. Afterwards plasmids were worked up by isopropanol purification and transformed by heat shock into ccdB resistant and non-resistant (Top10) cells. To assess transformation efficiency colony PCRs and restriction digests were prepared to obtain candidate plasmids for re-transformation and prepared for sequencing. Functional plasmids were submitted as BioBricks.<br/><br/>
 +
 
 +
<b>Linker variation</b><br/>
 +
Due to the fact, that there are a lot of different annotation resources predicting strongly deviating positions of domain borders, we decided to investigate different linker positions. We want to evaluate for which linker positions Val-Ind expression works best to support our Software and create standard linkers.
 +
In this week we focused on the preparation for this subproject. We amplified all of the domains with different linker positions, as well as the backbone and indC, and gained in all cases the concentrations necessary for Gibson assembly, which will be part of the week after.</p>
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                                   <h1>Week 22</h1>
                                   <h1>Week 22</h1>
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">Week of SUBMISSION DEADLINE (2013-09-25)
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+
Tyrocidine-Indigoidine-fusion extended<br/>
 +
As we focused mainly on the parts submission the week before, the Tyrocidine-Indigoidine fusion was picked up again this week. Four samples (pPW06, pPW09, pPW10 and pPW11) were transformed and colonies screened by colony PCRs. Except for pPW12G, all constructs showed expected cutting profiles after enzymatic digest. The sample pPW06 newC  was transformed into BAP-I cells. The liquid culture was induced with IPTG and turned blue. The indigoidine-tagged peptide was run on a TLC to proof the basic working principle of this tagging method.<br/>
 +
Linker variation<br/>
 +
Following up the week before, two of the constructs, which comprised the most wide apart linker positions, were assembled. <br/>
 +
Both plasmids were transformed via electroporation in competent DH10ß cells, spread on plates and picked for colony PCRs. As only LV1 showed appropriate bands, further colonies of LV7 were picked. In between, LV1 was chemically transformed into BAPI.<br/>
 +
At the end of the week we also assembled the other constructs. Three of these constructs ran on the expected heights on the gel and were also transformed into DH10ß.<br/></p>
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                                   <h1>Week 23</h1>
                                   <h1>Week 23</h1>
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;"><b>WIKIFREEZE (04.10.2013)</b><br/>
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                                  <p><a class="btn btn-large btn-primary" href="#">Browse gallery</a></p>
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<b>Linker variation</b><br/>
 +
In this week we aim to produce results out of our –putative- positive constructs. Therefore the left presumably positive samples induced and turned blue. Our goal was to evaluate, whether even through the variation of our Linkers our desired Val-Ind was expressed. Our samples were compared to native Indigoidine by TLC.</p>
 +
                                 
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                 <h2>Methods:</h2>
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                            <div class="tab-pane" id="b11">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                                    </html>{{:Team:Heidelberg/Templates/Del_week11_AE}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
                         
+
-
 
+
-
                            <div class="tab-pane" id="d11">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
 
+
-
                                </html>{{:Team:Heidelberg/Templates/Del_week11_AG}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
-
                            <div class="tab-pane" id="e11">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                              </html>{{:Team:Heidelberg/Templates/Del_week11_EG}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
-
                            <div class="tab-pane" id="f11">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                              </html>{{:Team:Heidelberg/Templates/Del_week11_G}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
-
                            <div class="tab-pane" id="j11">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                              </html>{{:Team:Heidelberg/Templates/Del_week11_LP}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
-
                            <div class="tab-pane" id="g11">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                              </html>{{:Team:Heidelberg/Templates/Del_week11_OP}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
-
                            <div class="tab-pane" id="h11">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                              </html>{{:Team:Heidelberg/Templates/Del_week11_L}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
-
                            <div class="tab-pane" id="i11">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                              </html>{{:Team:Heidelberg/Templates/Del_week11_pSB4K5}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
-
                      </div>
+
-
                  </div>
+
-
              </div>
+
-
            </div>
+
-
 
+
                     <!--Week 12-->
                     <!--Week 12-->
             <div class="labjournal-weekly">
             <div class="labjournal-weekly">
Line 378: Line 287:
                     <ul class="nav nav-tabs">
                     <ul class="nav nav-tabs">
                       <li class="active"><a href="#a12" data-toggle="tab">Overview</a></li>
                       <li class="active"><a href="#a12" data-toggle="tab">Overview</a></li>
-
                       <li><a href="#b12" data-toggle="tab">DelA-E</a></li>
+
                       <li><a href="#b12" data-toggle="tab">Module Shuffling</a></li>
-
                       <li><a href="#e12" data-toggle="tab">DelE-G</a></li>
+
                        
-
                      <li><a href="#f12" data-toggle="tab">DelG</a></li>
+
-
                      <li><a href="#h12" data-toggle="tab">DelL-P</a></li>
+
-
                      <li><a href="#g12" data-toggle="tab">DelO-P</a></li>
+
                        
                        
                     </ul>
                     </ul>
                 </div>
                 </div>
                     <div class="jumbotron weekly">
                     <div class="jumbotron weekly">
-
                     <div class="scrollContent nav navbar" data-spy="scroll" data-target="#navbarExample" data-offset="0">
+
                     <div class="nav navbar" data-spy="scroll" data-target="#navbarExample" data-offset="0">
   
   
Line 393: Line 299:
                             <div class="tab-pane active" id="a12">
                             <div class="tab-pane active" id="a12">
                                 <p style="font-size:12pt; text-align:justify;">
                                 <p style="font-size:12pt; text-align:justify;">
-
                             
+
                                </html>{{:Team:Heidelberg/Tyrocidine_week12_ov}}<html>
                                 </p>
                                 </p>
                             </div>
                             </div>
Line 399: Line 305:
                             <div class="tab-pane" id="b12">
                             <div class="tab-pane" id="b12">
                                 <p style="font-size:12pt; text-align:justify;">
                                 <p style="font-size:12pt; text-align:justify;">
-
                                     </html>{{:Team:Heidelberg/Templates/Del_week12_AE}}<html>
+
                                     </html>{{:Team:Heidelberg/Tyrocidine_week12_ms}}<html>
                                 </p>
                                 </p>
                             </div>
                             </div>
                              
                              
-
                            <div class="tab-pane" id="e12">
+
                         
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                              </html>{{:Team:Heidelberg/Templates/Del_week12_EG}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
-
                            <div class="tab-pane" id="f12">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                              </html>{{:Team:Heidelberg/Templates/Del_week12_G}}<html>
+
-
                                </p>
+
-
                            </div>
+
      
      
-
                            <div class="tab-pane" id="h12">
+
                         
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                              </html>{{:Team:Heidelberg/Templates/Del_week12_LP}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
-
                            <div class="tab-pane" id="g12">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                              </html>{{:Team:Heidelberg/Templates/Del_week12_OP}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
                         </div>
                         </div>
                     </div>
                     </div>
Line 438: Line 323:
                     <ul class="nav nav-tabs">
                     <ul class="nav nav-tabs">
                       <li class="active"><a href="#a13" data-toggle="tab">Overview</a></li>
                       <li class="active"><a href="#a13" data-toggle="tab">Overview</a></li>
-
                       <li><a href="#b13" data-toggle="tab">DelA-E</a></li>
+
                       <li><a href="#b13" data-toggle="tab">Module Shuffling</a></li>
-
                       <li><a href="#c13" data-toggle="tab">DelA-F</a></li>
+
                        
-
                      <li><a href="#d13" data-toggle="tab">DelA-G</a></li>
+
-
                      <li><a href="#h13" data-toggle="tab">DelE</a></li>
+
-
                      <li><a href="#e13" data-toggle="tab">DelE-G</a></li>
+
-
                      <li><a href="#f13" data-toggle="tab">DelG</a></li>
+
-
                      <li><a href="#g13" data-toggle="tab">DelO-P</a></li>
+
                     </ul>
                     </ul>
                 </div>
                 </div>
                 <div class="jumbotron weekly">
                 <div class="jumbotron weekly">
-
                     <div class="scrollContent nav navbar" data-spy="scroll" data-target="#navbarExample" data-offset="0">
+
                     <div class="nav navbar" data-spy="scroll" data-target="#navbarExample" data-offset="0">
                         <div class="tab-content">
                         <div class="tab-content">
Line 459: Line 339:
                             <div class="tab-pane" id="b13">
                             <div class="tab-pane" id="b13">
                                 <p style="font-size:12pt; text-align:justify;">
                                 <p style="font-size:12pt; text-align:justify;">
-
                                     </html>{{:Team:Heidelberg/Templates/Del_week13_AE}}<html>
+
                                     </html>{{:Team:Heidelberg/Tyrocidine_week13_ms}}<html>
                                 </p>
                                 </p>
                             </div>
                             </div>
-
                             <div class="tab-pane" id="c13">
+
                              
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                                </html>{{:Team:Heidelberg/Templates/Del_week13_AF}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
-
                            <div class="tab-pane" id="d13">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
 
+
-
                                </html>{{:Team:Heidelberg/Templates/Del_week13_AG}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
-
                            <div class="tab-pane" id="h13">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                                </html>{{:Team:Heidelberg/Templates/Del_week13_E}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
-
                            <div class="tab-pane" id="e13">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                              </html>{{:Team:Heidelberg/Templates/Del_week13_EG}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
-
                            <div class="tab-pane" id="f13">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                              </html>{{:Team:Heidelberg/Templates/Del_week13_G}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
-
                            <div class="tab-pane" id="g13">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                              </html>{{:Team:Heidelberg/Templates/Del_week13_OP}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
                         </div>
                         </div>
                     </div>
                     </div>
Line 509: Line 353:
                     <ul class="nav nav-tabs">
                     <ul class="nav nav-tabs">
                       <li class="active"><a href="#a14" data-toggle="tab">Overview</a></li>
                       <li class="active"><a href="#a14" data-toggle="tab">Overview</a></li>
-
                       <li><a href="#b14" data-toggle="tab">DelA-E</a></li>
+
                       <li><a href="#b14" data-toggle="tab">Module Shuffling</a></li>
-
                      <li><a href="#c14" data-toggle="tab">DelA-F</a></li>
+
             
-
                      <li><a href="#d14" data-toggle="tab">DelA-G</a></li>
+
-
                   
+
-
                      <li><a href="#f14" data-toggle="tab">DelG</a></li>
+
-
                      <li><a href="#g14" data-toggle="tab">DelO-P</a></li>
+
                        
                        
Line 520: Line 360:
                 </div>
                 </div>
                 <div class="jumbotron weekly">
                 <div class="jumbotron weekly">
-
                     <div class="scrollContent nav navbar" data-spy="scroll" data-target="#navbarExample" data-offset="0">
+
                     <div class="nav navbar" data-spy="scroll" data-target="#navbarExample" data-offset="0">
                         <div class="tab-content">
                         <div class="tab-content">
Line 532: Line 372:
                             <div class="tab-pane" id="b14">
                             <div class="tab-pane" id="b14">
                                 <p style="font-size:12pt; text-align:justify;">
                                 <p style="font-size:12pt; text-align:justify;">
-
                                 </html>{{:Team:Heidelberg/Templates/Del_week14_AE}}<html>
+
                                 </html>{{:Team:Heidelberg/Tyrocidine_week14_ms}}<html>
-
                                </p>
+
-
                            </div>
+
-
                           
+
-
                            <div class="tab-pane" id="c14">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                                </html>{{:Team:Heidelberg/Templates/Del_week14_AF}}<html>
+
                                 </p>
                                 </p>
                             </div>
                             </div>
 +
                                 
-
                            <div class="tab-pane" id="d14">
+
                         
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
 
+
-
                                </html>{{:Team:Heidelberg/Templates/Del_week14_AG}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
-
                            <div class="tab-pane" id="f14">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                              </html>{{:Team:Heidelberg/Templates/Del_week14_G}}<html>
+
-
                                </p>
+
-
                            </div>
+
-
 
+
-
                            <div class="tab-pane" id="g14">
+
-
                                <p style="font-size:12pt; text-align:justify;">
+
-
                              </html>{{:Team:Heidelberg/Templates/Del_week14_OP}}<html>
+
-
                                </p>
+
-
                            </div>
+
                         </div>
                         </div>
Line 571: Line 389:
                     <ul class="nav nav-tabs">
                     <ul class="nav nav-tabs">
                       <li class="active"><a href="#a15" data-toggle="tab">Overview</a></li>
                       <li class="active"><a href="#a15" data-toggle="tab">Overview</a></li>
-
                      <li><a href="#b15" data-toggle="tab">DelA-E</a></li>
+
                    <li><a href="#b15" data-toggle="tab">Module Shuffling</a></li>
-
                      <li><a href="#c15" data-toggle="tab">DelA-F</a></li>
+
                 
-
                      <li><a href="#d15" data-toggle="tab">DelA-G</a></li>
+
                   
-
                      <li><a href="#e15" data-toggle="tab">DelE-F</a></li>
+
-
                      <li><a href="#f15" data-toggle="tab">DelG</a></li>
+
-
                      <li><a href="#g15" data-toggle="tab">DelO-P</a></li>
+
-
                      <li><a href="#h15" data-toggle="tab">DelL</a></li>
+
-
                      <li><a href="#i15" data-toggle="tab">pSB4K5</a></li>
+
                     </ul>
                     </ul>
                 </div>
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                     <div class="nav navbar" data-spy="scroll" data-target="#navbarExample" data-offset="0">
                        
                        
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                                 <p style="font-size:12pt; text-align:justify;">
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                              </html>{{:Team:Heidelberg/Templates/Del_week15_EF}}<html>
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                                <p style="font-size:12pt; text-align:justify;">
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                              </html>{{:Team:Heidelberg/Templates/Del_week15_G}}<html>
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-
                       <li><a href="#b16" data-toggle="tab">DelA-F</a></li>                    
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                       <li><a href="#b16" data-toggle="tab">Module Shuffling</a></li>
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                       <li><a href="#d16" data-toggle="tab">DelA-G</a></li> 
+
                        
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                       <li><a href="#f16" data-toggle="tab">DelG</a></li>
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                       <li><a href="#d16" data-toggle="tab">BioBrick Assembly</a></li>
-
                      <li><a href="#g16" data-toggle="tab">DelO-P</a></li>
+
                   
-
                      <li><a href="#i16" data-toggle="tab">pSB4K5</a></li>
+
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                     <div class="nav navbar" data-spy="scroll" data-target="#navbarExample" data-offset="0">
                        
                        
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-
                             
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-
                                     </html>{{:Team:Heidelberg/Templates/Del_week16_AF}}<html>
+
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-
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                                 <p style="font-size:12pt; text-align:justify;">
                                 <p style="font-size:12pt; text-align:justify;">
-
                               </html>{{:Team:Heidelberg/Templates/Del_week16_G}}<html>
+
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                                <p style="font-size:12pt; text-align:justify;">
 
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-
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                 <div>
                 <div>
                     <ul class="nav nav-tabs">
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                       <li class="active"><a href="#a17" data-toggle="tab">Overview</a></li>
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                       <li><a href="#b17" data-toggle="tab">Module Shuffling</a></li>
-
                                           
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                       <li><a href="#d17" data-toggle="tab">BioBrick Assembly</a></li>
 +
                   
                     </ul>
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                       <div class="tab-content">
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-
                             <div class="tab-pane" id="i17">
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                                 <p style="font-size:12pt; text-align:justify;">
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 +
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                       </div>
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                 <div>
                 <div>
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                       <li class="active"><a href="#a18" data-toggle="tab">Overview</a></li>
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                       <li><a href="#b18" data-toggle="tab">Module Shuffling</a></li>
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 +
                       <li><a href="#d18" data-toggle="tab">BioBrick Assembly</a></li>
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                       <div class="tab-content">
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                             <div class="tab-pane" id="i18">
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-
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+
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 +
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 +
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 +
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 +
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                                <p style="font-size:12pt; text-align:justify;">
 +
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                 <div>
                 <div>
                     <ul class="nav nav-tabs">
                     <ul class="nav nav-tabs">
-
                       <li class="active"><a href="#a19" data-toggle="tab">Overview</a></li>
+
                   
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+
                       <li><a href="#b19" data-toggle="tab">Module Shuffling</a></li>
-
                       <li><a href="#i19" data-toggle="tab">pSB4K5</a></li>
+
   
 +
                       <li><a href="#d19" data-toggle="tab">BioBrick Assembly</a></li>
                     </ul>
                     </ul>
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                 </div>
                 <div class="jumbotron weekly">
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                     <div class="nav navbar" data-spy="scroll" data-target="#navbarExample" data-offset="0">
                        
                        
                       <div class="tab-content">
                       <div class="tab-content">
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                             <div class="tab-pane" id="i19">
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                                 <p style="font-size:12pt; text-align:justify;">
-
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+
                               </html>{{:Team:Heidelberg/Tyrocidine_week19_ms}}<html>
 +
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 +
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 +
                         
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 +
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                       <li class="active"><a href="#a20" data-toggle="tab">Overview</a></li>
-
                                           
+
                     
-
                       <li><a href="#i20" data-toggle="tab">pSB4K5</a></li>
+
                      <li><a href="#b20" data-toggle="tab">Module Shuffling</a></li>
 +
                      <li><a href="#c20" data-toggle="tab">Interspecies Module Shuffling</a></li>
 +
                       <li><a href="#d20" data-toggle="tab">BioBrick Assembly</a></li>
                     </ul>
                     </ul>
                 </div>
                 </div>
                 <div class="jumbotron weekly">
                 <div class="jumbotron weekly">
-
                     <div class="scrollContent nav navbar" data-spy="scroll" data-target="#navbarExample" data-offset="0">
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Latest revision as of 03:25, 29 October 2013

Novel NRPS & Indigoidine-Tag. Exploring Modularity of NRPS by Shuffling Modules.

Thanks to