Team:Heidelberg/Delftibactin/DelH

From 2013.igem.org

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                                   <h1>Week 11</h1>
                                   <h1>Week 11</h1>
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">Based on this week's experiments and in silico analysis to validate the fragments DelH F1a, F1b and F2, we discarded the restriction digest and ligation strategy for the assembly of the DelH plasmid. Instead, we chose Gibson assembly as alternative method, developed a strategy and designed primers accordingly. We are positive, to finally assemble pHM02.  
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">Based on this week's experiments and <i>in silico</i> analysis of the fragments DelH F1a, F1b and F2, we discarded the restriction digest and ligation strategy for the assembly of the DelH plasmid. Instead, we chose Gibson assembly as an alternative method, developed a strategy and designed primers accordingly.  
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                                   <h1>Week 12</h1>
                                   <h1>Week 12</h1>
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">The primers arrived and we started amplifying the Gibson fragments using different approaches. Since G1 could not be PCR amplified, we decided to divide G1 into sub fragments G1a and G1b, for which we had designed and ordered primers already. The amplification of fragment G2 worked well and was produced in reasonable amounts. Alternatively, we also produced the entire DelH as one fragment G0, as well as further sub fragments DelH G1/2a, G1b/2 and G2b. Amplification of G1b/2a did not work out. Due to the failure of the restriction digest strategy, we further analyzed the backbone pSB6A1-AraC-lacZ, which we decided to discard and instead, use pSB6A1 and BBa_J04450, which is already available in the parts registry. </p>
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">We started amplifying the Gibson fragments using different PCR approaches. Since we were not able to amplify G1 by PCR, we decided to divide G1 into the subfragments G1a and G1b, for which we had already designed and ordered primers. The amplification of fragment G2 worked well and yielded sufficient DNA amounts for subsequent steps. Alternatively, we also produced the entire DelH G0 as one fragment, as well as further subfragments DelH G1/2a, G1b/2 and G2b. Amplification of G1b/2a did not work out. Due to the failure of the restriction digest strategy, we further analyzed the backbone pSB6A1-AraC-lacZ, which we decided to discard. Instead, we choose to use pSB6A1 and BBa_J04450, which is already available in the parts registry. </p>
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                                   <h1>Week 13</h1>
                                   <h1>Week 13</h1>
                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">In order to realize the new strategy using the already existing backbone from the parts registry pSB6A1-lacZ-mRFP, we designed two new primers for the backbone amplification and created a map of pHM03.
                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">In order to realize the new strategy using the already existing backbone from the parts registry pSB6A1-lacZ-mRFP, we designed two new primers for the backbone amplification and created a map of pHM03.
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The plasmid for the backbone was obtained from the registry, transformed in E.coli and minipreped. The Gibson fragment of the backbone was successfully amplified, together with Gibson fragments DelH G0, G1 and G2b. </p>
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The plasmid for the backbone was obtained from the registry, transformed into <i>E.coli</i> and miniprepped. The Gibson fragment of the backbone was successfully amplified, together with Gibson fragments DelH G0, G1 and G2b. </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%;">In week 14, we've tested numerous colonies from last week's Gibson assembly 28-07 using DelH G0 as well as G1/2a and 2b by screening-PCR. None of the analyzed colonies carried a correct plasmid. We therefore performed another Gibson assembly 01-08 and again screened numerous clones. We found few possibly correct ones that will be further analyzed next week.
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">In week 14, we screened numerous colonies from last week's Gibson assembly (28-07) for plasmids containing DelH G0, G1/2a and 2b by screening-PCR. None of the analyzed colonies carried the correct plasmid. We performed another Gibson assembly (01-08) and screened numerous clones. We found few possibly correct ones that will be further analyzed next week.
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Additionally, the new D. acidovorans strain SPH1, whose sequence is available in GenBank, was ordered. We will have to amplify all fragments from this strain again as soon as it arrives. </p>
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Additionally, the new <i>D. acidovorans</i> strain SPH1, whose sequence is available in GenBank, was ordered. We will amplify all fragments from the genome of <i>D. acidovorans</i> SPH1 as soon as it arrives. </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%;">We further tested colonies from last weeks Gibson assemblies using DelH G0 as well as G1/2a and 2b. Unfortunately, they were all negative in the screening-PCR. Therefore, we amplified our Gibson fragments again and performed more Gibson assemblies. Yet again, there were no positive colonies in the colony-PCR. </p>
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                                   <p style="font-size:10pt; text-align:justify; position:relative; margin-left:6%;">We screened colonies from last weeks Gibson assemblies (01-08) for plasmids containing DelH G0 as well as G1/2a and 2b. None of the screening-PCRs yielded the expected DNA bands. Therefore, we amplified the Gibson fragments again and performed further Gibson assemblies. Yet again, we could not detect positive colonies by colony-PCR. </p>
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Revision as of 23:13, 2 October 2013

Del H. This bitchy 18 kbp fragment.

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Methods:

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