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| <body id="backtotop"> | | <body id="backtotop"> |
| <div class="global"> | | <div class="global"> |
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− | <h1 class="text-center">Notebook</h1>
| + | <div class="container"><article class="col-md-11"><h1>Laboratory Notebook</h1> |
| + | <p class="introduction-text">A laboratory notebook is our real time record of our expriments. It porvides a detailled record of exactly what we do in the laboratory to obtain our experimental results. It documents our hypotheses, experiments and initial analysis or interpretation of our experiments. Moreover, we also mentionned the name of exprimenters and the place of our experiments. The protocols that we follow are available on protocols page: <a class="btn-sm" href="https://2018.igem.org/Team:Sorbonne_U_Paris/Protocols" role="button" style=" color:white; border-radius: 10px; background-color: #22D66C; text-decoration:none;"><i class="fas fa-book fa-1x"></i> Protocols </a> <br> |
| + | |
| + | |
| + | </p> </article></div> |
| + | |
| + | |
| + | |
| <h2 class="text-center" id="h2-calendar"> Calendars 2018</h2> | | <h2 class="text-center" id="h2-calendar"> Calendars 2018</h2> |
| <div class="container" > | | <div class="container" > |
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| <tr> | | <tr> |
| <td class="date"><a href="#jul9" class="pointer" title="Monday 9th July">9</a></td> | | <td class="date"><a href="#jul9" class="pointer" title="Monday 9th July">9</a></td> |
− | <td class="date"><a href="#jul10" class="pointer" title="Tuesday 10th Jult">10</a></td> | + | <td class="date"><a href="#jul10" class="pointer" title="Tuesday 10th July">10</a></td> |
| <td>11</td> | | <td>11</td> |
| <td>12</td> | | <td>12</td> |
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| <tr> | | <tr> |
| <td class="date"><a href="#s10" class="pointer" title="Monday 10th September">10</a></td> | | <td class="date"><a href="#s10" class="pointer" title="Monday 10th September">10</a></td> |
− | <td>11</td> | + | <td class="date"><a href="#s11" class="pointer" title="Tuesday 11th September">11</a></td> |
− | <td>12</td> | + | <td class="date"><a href="#s12" class="pointer" title="Wednesday 12th September">12</a></td> |
− | <td>13</td> | + | <td class="date"><a href="#s13" class="pointer" title="Monday 13th September">13</a></td> |
| <td>14</td> | | <td>14</td> |
| <td>15</td> | | <td>15</td> |
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| | | |
| <tr> | | <tr> |
− | <td>17</td> | + | <td class="date"><a href="#s17" class="pointer" title="Monday 17th September">17</a></td> |
| <td>18</td> | | <td>18</td> |
| <td>19</td> | | <td>19</td> |
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| </div> | | </div> |
| </div> </div> | | </div> </div> |
− | <p class="text-notebook"> <span style="font-weight:bold">Aim</span> : Extraction of plasmides from yesterday’s cultures and reactions of digestion/ligation p0universal/ pSAD and p0-B3/intron rubisco.</p> | + | <p class="text-notebook"> <span style="font-weight:bold">Aim</span> : Extraction of plasmides from <a href="#jun13" style="text-decoration: none;">yesterday’s cultures </a> and reactions of digestion/ligation p0universal/ pSAD and p0-B3/intron rubisco.</p> |
| <h5>Plasmid purification </h5> | | <h5>Plasmid purification </h5> |
| <p (p0universel=p0universel-pAGM9121)<br> | | <p (p0universel=p0universel-pAGM9121)<br> |
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| <div class="note"> | | <div class="note"> |
| <h2 class="text-center" id="jul10"> Thurday 10th July</h2> | | <h2 class="text-center" id="jul10"> Thurday 10th July</h2> |
− | <h4> Transformation of 𝝱10 with digestion/ligation products of GAG POL <br> (experiences of 07/09/18) </h4> | + | <h4> Transformation of 𝝱10 with digestion/ligation products of GAG POL <br> (<a href="#jul9">experiences of 07/09/18</a>) </h4> |
| <h6>Institut de biologie physico-chimique (IBPC) </h6> | | <h6>Institut de biologie physico-chimique (IBPC) </h6> |
| <div class="d-flex justify-content-end"> <div class="chip-icone"> <div class="chip"> | | <div class="d-flex justify-content-end"> <div class="chip-icone"> <div class="chip"> |
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| </div> </div> </div> | | </div> </div> </div> |
| <h5> Arrangement in the box iGEM 2018 </h5> | | <h5> Arrangement in the box iGEM 2018 </h5> |
− | <h5>Preparation of all the inserts in order to send them to sequecing </h5> | + | <h5>Preparation of all the inserts in order to send them to sequencing </h5> |
| <!-- --------------------------------------------FIGURE CAPTION B --------------------------------------------- --> | | <!-- --------------------------------------------FIGURE CAPTION B --------------------------------------------- --> |
| <a class="pointer" title="Click on the image for a larger view " data-toggle="modal" data-target=".Inserts1-180717"><div class="container-figurecaption figurecaptionB"> | | <a class="pointer" title="Click on the image for a larger view " data-toggle="modal" data-target=".Inserts1-180717"><div class="container-figurecaption figurecaptionB"> |
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| <div class="col-xs-12 col-sm-12 col-md-12 col-lg-12"> | | <div class="col-xs-12 col-sm-12 col-md-12 col-lg-12"> |
| <div class="note"> | | <div class="note"> |
− | <h2 class="text-center" id="jul19"> Thurday 19th July</h2> | + | <h2 class="text-center" id="jul19"> Thursday 19th July</h2> |
| | | |
| <h4> Analysis of sequencing results </h4> | | <h4> Analysis of sequencing results </h4> |
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| </div> </div> </div> | | </div> </div> </div> |
| <h5>1. Transplanting of a clamydomonas clone in 3ml of LB+ Spec </h5> | | <h5>1. Transplanting of a clamydomonas clone in 3ml of LB+ Spec </h5> |
− | <h5>2. Plasmid extraction from 𝝱 bacterias transformed the day before ( directly from dish).</h5> | + | <h5>2. Plasmid extraction from 𝝱 bacterias transformed <a href="#jul23">the day before</a> ( directly from dish).</h5> |
| <p class="text-notebook">Kit used = Nucleopsin Plasmid <br> | | <p class="text-notebook">Kit used = Nucleopsin Plasmid <br> |
| Elution volum= 40µL <br> | | Elution volum= 40µL <br> |
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| </div> </div> </div> | | </div> </div> </div> |
| | | |
− | <h5>Plasmid extraction from bacteria transformed </h5> | + | <h5>Plasmid extraction from <a href="#jul24">bacteria transformed</a> </h5> |
| <p class="text-notebook"> Put on liquid media the 24/07 <br> kit used : Nucleopsin plasmid | | <p class="text-notebook"> Put on liquid media the 24/07 <br> kit used : Nucleopsin plasmid |
| </p> | | </p> |
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| </div> </div> | | </div> </div> |
| <h5>1. Digestion/ ligation reaction of pSAD 2 Rb intron </h5> | | <h5>1. Digestion/ ligation reaction of pSAD 2 Rb intron </h5> |
− | <p class="text-notebook">see 06/14/2018 protocol</p> | + | <p class="text-notebook"> <a href="#jun14">see 06/14/2018 protocol</a></p> |
| <h5>2. Transformation </h5> | | <h5>2. Transformation </h5> |
| <p class="text-notebook">-90µl of DH5α +Ligation product +10µl CMR <br> | | <p class="text-notebook">-90µl of DH5α +Ligation product +10µl CMR <br> |
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| </div> | | </div> |
| <!-- -----------------------------------.\ One day of the notebook ------------------------------------------------------- --> | | <!-- -----------------------------------.\ One day of the notebook ------------------------------------------------------- --> |
− | <!-- ----------------------------------- Tuesday 29th Augus ------------------------------------------------------- --> | + | <!-- ----------------------------------- Tuesday 29th August ------------------------------------------------------- --> |
| <div class="container-fluid"> | | <div class="container-fluid"> |
| <div class="row text-center text-xs-center text-sm-center text-md-left text-lg-left "> | | <div class="row text-center text-xs-center text-sm-center text-md-left text-lg-left "> |
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| </div> | | </div> |
| <!-- -----------------------------------.\ One day of the notebook ------------------------------------------------------- --> | | <!-- -----------------------------------.\ One day of the notebook ------------------------------------------------------- --> |
− | <!-- ----------------------------------- Tuesday 30th Augus ------------------------------------------------------- --> | + | <!-- ----------------------------------- Tuesday 30th August ------------------------------------------------------- --> |
| <div class="container-fluid"> | | <div class="container-fluid"> |
| <div class="row text-center text-xs-center text-sm-center text-md-left text-lg-left "> | | <div class="row text-center text-xs-center text-sm-center text-md-left text-lg-left "> |
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| - otsB2 : 78.2ng/µl <br> | | - otsB2 : 78.2ng/µl <br> |
| </p> | | </p> |
− | <h5>4. Level 0 ligation protocol for GAGPOL parts : (see 09/07/2018)</h5> | + | <h5>4. Level 0 ligation protocol for GAGPOL parts : <a href="jul9">(see 09/07/2018)</a></h5> |
| <!-- --------------------------------------------FIGURE CAPTION B--------------------------------------------- --> | | <!-- --------------------------------------------FIGURE CAPTION B--------------------------------------------- --> |
| <a class="pointer" title="Click on the image for a larger view " data-toggle="modal" data-target=".Gagpolparts-180903"><div class="container-figurecaption figurecaptionB"> | | <a class="pointer" title="Click on the image for a larger view " data-toggle="modal" data-target=".Gagpolparts-180903"><div class="container-figurecaption figurecaptionB"> |
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| </div> | | </div> |
| </div> </div> | | </div> </div> |
− | <h5>1. Digestion of otsA and otsB ligation reaction of 30/08</h5> | + | <h5>1. Digestion of otsA and otsB ligation reaction of <a href="#a3">03/08/2018</a></h5> |
| <p class="text-notebook">Digestion reaction of otsA : <br> <br> | | <p class="text-notebook">Digestion reaction of otsA : <br> <br> |
| | | |
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| </p> | | </p> |
| | | |
− | <h5>2. Transformation of B10 bacteria with cloning reaction of 03/09 : p1-iGEM1 and p0-iGEM5 </h5> | + | <h5>2. Transformation of B10 bacteria with cloning reaction of <a href="#s3">03/09 </a>: p1-iGEM1 and p0-iGEM5 </h5> |
| <p class="text-notebook">25µl of B10 bacteria + 4µl of ligation product (4 different transformations) <br> | | <p class="text-notebook">25µl of B10 bacteria + 4µl of ligation product (4 different transformations) <br> |
| 30 min at 4°C <br> | | 30 min at 4°C <br> |
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| <h2 class="text-center" id="s5"> Wednesday 5th September</h2> | | <h2 class="text-center" id="s5"> Wednesday 5th September</h2> |
| | | |
− | <h4> PCR amplificication </h4> | + | <h4>Transformation of B10 bacteria with cloning reaction p1-iGEM1 and p0-iGEM5<br> Replanting of white colonies from p0-iGEM-GAGPO <br> Re-do of L1 ligation of p1-iGEM2 (Cargo) </h4> |
| <h6>Institut de biologie physico-chimique (IBPC) </h6> | | <h6>Institut de biologie physico-chimique (IBPC) </h6> |
| <div class="d-flex justify-content-end"> <div class="chip-icone"> <div class="chip"> | | <div class="d-flex justify-content-end"> <div class="chip-icone"> <div class="chip"> |
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| </div> | | </div> |
| </div> </div> | | </div> </div> |
− | <p class="text-notebook">- Lorem ipsum dolor sit amet, consectetur adipisicing elit, sed do eiusmod tempor incididunt ut labore et dolore magna aliqua. Ut enim ad minim veniam, quis nostrud exercitation ullamco laboris nisi ut aliquip ex ea commodo consequat.</p> | + | <h5>1. Transformation of B10 bacteria with cloning reaction of <a href="#s3">03/09 </a>: p1-iGEM1 and p0-iGEM5 </h5> |
− | <p class="text-notebook">-Lorem ipsum dolor sit amet, consectetur adipisicing elit, sed do eiusmod tempor incididunt ut labore et dolore magna aliqua. Ut enim ad minim veniam, quis nostrud exercitation ullamco laboris nisi ut aliquip ex ea commodo consequat.</p> </div> | + | <p class="text-notebook">Observation of plates from the day before <br> |
| + | - p1-iGEM2 (Cargo) : only blue colonies for + and - controle <br> |
| + | - p0-iGEM5- GagPol: only blue colonies for the positive (+) experiment , and both white and blue colonies for the negative (-) control |
| + | </p> |
| + | <h5>2. Replanting of white colonies from p0-iGEM-GAGPOL (-)on liquid media </h5> |
| + | <p class="text-notebook">Composition of the media :Amp+ Spec+ Xgal <br> |
| + | 4 colonies were replanted |
| + | </p> |
| + | <h5>Re-do of L1 ligation of p1-iGEM2 (Cargo) <a href="#s3"> (same experiment as the 09/03/2019)</a> </h5> </div> |
| </div> | | </div> |
| </div> | | </div> |
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| </div> | | </div> |
| </div> | | </div> |
− | <h5>3. 6 colonies from yesterday transformation p1igem2 in LB medium + amp </h5> | + | <h5>3. 6 colonies <a href="s6">from yesterday</a> transformation p1igem2 in LB medium + amp </h5> |
| | | |
| </div> | | </div> |
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| </div> | | </div> |
| </div> </div> | | </div> </div> |
− | <h5>1. DNA extraction of the 6 bacteria culture prepare on 7/09</h5> | + | <h5>1. DNA extraction of the 6 bacteria culture prepare on <a href="#s7">7/09</a></h5> |
| <p class="text-notebook">Used kit : NucleoSpin Plasmid (Macherey-Nagel)</p> | | <p class="text-notebook">Used kit : NucleoSpin Plasmid (Macherey-Nagel)</p> |
| <h5>2. Concentrations measurement at Nanodrop </h5> | | <h5>2. Concentrations measurement at Nanodrop </h5> |
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| <h5>Concentrations measurement at Nanodrop </h5> | | <h5>Concentrations measurement at Nanodrop </h5> |
| <p class="text-notebook">7.5µl of mix by tube + 2.5µl of DNA <br><br> | | <p class="text-notebook">7.5µl of mix by tube + 2.5µl of DNA <br><br> |
− | On 1% agarose gel, with otsB PCR from 7/09 : expected result : >800bp | + | On 1% agarose gel, with otsB PCR from <a href="#s7">7/09</a> : expected result : >800bp |
| </p> | | </p> |
| <!-- --------------------------------------------FIGURE CAPTION B--------------------------------------------- --> | | <!-- --------------------------------------------FIGURE CAPTION B--------------------------------------------- --> |
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| <!-- --------------------------------------------FIGURE CAPTION--------------------------------------------- --> | | <!-- --------------------------------------------FIGURE CAPTION--------------------------------------------- --> |
| | | |
− | <h5> 4. Transformation of B10 bacteria with ligation product from 07/09 </h5> | + | <h5> 4. Transformation of B10 bacteria with ligation product from <a href="#s7">07/09</a> </h5> |
| <p class="text-notebook">B10 bacteria + 3.5µl of ligation product <br> | | <p class="text-notebook">B10 bacteria + 3.5µl of ligation product <br> |
| - 30 min at 4°C <br> | | - 30 min at 4°C <br> |
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| - 1h at 37°C <br> | | - 1h at 37°C <br> |
| - Spreading of 200µl on plate with LB+spec+Xgal <br> | | - Spreading of 200µl on plate with LB+spec+Xgal <br> |
| + | </div> |
| + | </div> |
| + | </div> |
| + | </div> |
| + | <!-- -----------------------------------.\ One day of the notebook ------------------------------------------------------- --> |
| + | <!-- -----------------------------------Tuesday 11th September ------------------------------------------------------- --> |
| + | <div class="container-fluid"> |
| + | <div class="row text-center text-xs-center text-sm-center text-md-left text-lg-left "> |
| + | <div class="col-xs-12 col-sm-12 col-md-12 col-lg-12"> |
| + | <div class="note"> |
| + | <h2 class="text-center" id="s11"> Tuesday 11th September</h2> |
| + | |
| + | <h4>Digestion of p1-IGEM2 with bbsI <br> Transformation of bacteria with Gagpol </h4> |
| + | <h6> Muséum national d'histoire naturelle (MNHN) </h6> |
| + | <div class="d-flex justify-content-end"> <div class="chip-icone"> <div class="chip"> |
| + | <img src="https://static.igem.org/mediawiki/2018/1/1d/T--Sorbonne_U_Paris--Claude_avatar.png" alt="Person" width="96" height="96"> |
| + | Sara and Parisa |
| + | </div> |
| + | </div> </div> |
| + | <h5>1. Digestion of p1-IGEM2 with bbsI</h5> |
| + | <div class="d-flex justify-content-center"> |
| + | <div class="table-responsive-sm"> |
| + | <table class="text-center tablenotebook"> |
| + | <thead> |
| + | <tr> |
| + | <th class="th-notebook">Components</th> |
| + | <th class="th-notebook">1 reaction</th> |
| + | <th class="th-notebook">Mix (*6)</th> |
| + | </tr> |
| + | </thead> |
| + | <tbody> |
| + | <tr> |
| + | <td class="td-notebook">bbsI</td> |
| + | <td class="td-notebook">0.5µL </td> |
| + | <td class="td-notebook">3 µL</td> |
| + | </tr> |
| + | <tr> |
| + | <td class="td-notebook">Cutsmart buffer (10X)</td> |
| + | <td class="td-notebook">1 µL</td> |
| + | <td class="td-notebook">6 µL </td> |
| + | </tr> |
| + | <tr> |
| + | <td class="td-notebook">DNA</td> |
| + | <td class="td-notebook">2.5 µL</td> |
| + | <td class="td-notebook">6.5µl </td> |
| + | </tr> |
| + | <tr> |
| + | <td class="td-notebook">H2O</td> |
| + | <td class="td-notebook">6 µL</td> |
| + | <td class="td-notebook">36µL</td> |
| + | </tr> |
| + | </tbody> |
| + | </table> |
| + | </div> |
| + | </div> |
| + | |
| + | |
| + | <h5>2. Transformation of bacteria with Gagpol </h5> |
| + | <p class="text-notebook">2 white colonies were observed on the plate containing bacterias transformed with GAGPOL <br> |
| + | - Replanting on liquid media <br> |
| + | - Replanting on plate (not isolable) <br> |
| + | </p> |
| + | </div> |
| + | </div> |
| + | </div> |
| + | </div> |
| + | <!-- -----------------------------------.\ One day of the notebook ------------------------------------------------------- --> |
| + | <!-- -----------------------------------Wednesday 12th September ------------------------------------------------------- --> |
| + | <div class="container-fluid"> |
| + | <div class="row text-center text-xs-center text-sm-center text-md-left text-lg-left "> |
| + | <div class="col-xs-12 col-sm-12 col-md-12 col-lg-12"> |
| + | <div class="note"> |
| + | <h2 class="text-center" id="s12"> Wednesday 12th September</h2> |
| + | |
| + | <h4>Migration of the digestion products from the day before (pI-IGEM2) |
| + | <br> Plasmid extraction from the GAG clone culture <br> Purification of DNA contained in the migration gel for OtsB PCR products <br> Digestion reaction for Gag POL <br> Level 0 Otsb (digestion/ligation reaction) </h4> |
| + | <h6> Muséum national d'histoire naturelle (MNHN) </h6> |
| + | <div class="d-flex justify-content-end"> <div class="chip-icone"> <div class="chip"> |
| + | <img src="https://static.igem.org/mediawiki/2018/1/1d/T--Sorbonne_U_Paris--Claude_avatar.png" alt="Person" width="96" height="96"> |
| + | Sara and Parisa |
| + | </div> |
| + | <div class="chip"> |
| + | <img src="https://static.igem.org/mediawiki/2018/1/1d/T--Sorbonne_U_Paris--Claude_avatar.png" alt="Person" width="96" height="96"> |
| + | Victor |
| + | </div> |
| + | </div> </div> |
| + | <h5>1. Migration of the digestion products from the day before (pI-IGEM2)</h5> |
| + | <p class="text-notebook"> (0.1% agarose gel, 2-log ladder, 100V)<br> |
| + | We were expecting a 4.5kb band for the plasmid and a 2.6kb band for the insert. <br> |
| + | We do have the expected band for the plasmid but, we observe a band at 0.6kb for the insert (Lac Z maybe?)</p> |
| + | |
| + | <h5>2. Plasmid extraction from the GAG clone culture launched the day before </h5> |
| + | <p class="text-notebook">Kit used Nucleospin Plasmid </p> |
| + | |
| + | <h5>3. Purification of DNA contained in the migration gel for OtsB PCR products <a href="#s7">( from 09/07/2018)</a> |
| + | </h5> |
| + | <p class="text-notebook">Kit used : Nucleospin gel to PCR clean up </p> |
| + | |
| + | <h5>4. DNA concentration measurement on Nanodrop </h5> |
| + | <p class="text-notebook">Insert OtsB= 4ng/µL <br> |
| + | GAG palamsid = 48.1 ng/µl |
| + | </p> |
| + | |
| + | <h5>5. DNA concentration measurement on Nanodrop </h5> |
| + | <p class="text-notebook">Insert OtsB= 4ng/µL <br> |
| + | GAG palamsid = 48.1 ng/µl |
| + | </p> |
| + | |
| + | <h5>6. Level 0 Otsb (digestion/ligation reaction) </h5> |
| + | <p class="text-notebook">→ purification of PCR band and Launch of miniprep <br> |
| + | (To do next level 1 pI-Igem2)</p> |
| + | </div> |
| + | </div> |
| + | </div> |
| + | </div> |
| + | <!-- -----------------------------------.\ One day of the notebook ------------------------------------------------------- --> |
| + | <!-- -----------------------------------Tuesday 13th September ------------------------------------------------------- --> |
| + | <div class="container-fluid"> |
| + | <div class="row text-center text-xs-center text-sm-center text-md-left text-lg-left "> |
| + | <div class="col-xs-12 col-sm-12 col-md-12 col-lg-12"> |
| + | <div class="note"> |
| + | <h2 class="text-center" id="s13"> Tuesday 13th September</h2> |
| + | |
| + | <h4>Transformation of 𝛃10 bacterias with OtsB ligation products <br> DNA plamsid extraction of pO-IGEM5 <br> Digestion reaction </h4> |
| + | <h6> Muséum national d'histoire naturelle (MNHN) </h6> |
| + | <div class="d-flex justify-content-end"> <div class="chip-icone"> <div class="chip"> |
| + | <img src="https://static.igem.org/mediawiki/2018/1/1d/T--Sorbonne_U_Paris--Claude_avatar.png" alt="Person" width="96" height="96"> |
| + | Sara |
| + | </div> |
| + | <div class="chip"> |
| + | <img src="https://static.igem.org/mediawiki/2018/1/1d/T--Sorbonne_U_Paris--Claude_avatar.png" alt="Person" width="96" height="96"> |
| + | Victor |
| + | </div> |
| + | </div> </div> |
| + | <h5>1. Transformation of 𝛃10 bacterias with OtsB ligation products obtained the day before </h5> |
| + | <p class="text-notebook"> 𝛃10+ 4µL of OtsB ligation reaction products <br> |
| + | - 30min at 4°C <br> |
| + | - 55 sec at 42°C <br> |
| + | - 2 min at 4°C <br> |
| + | - Addition of 70µL of LB <br> <br> |
| + | 1 Hour at 37°C <br> |
| + | Spreading of 200µL on LB+Xgal + Spec plate <br> |
| + | 37°C O/N |
| + | </p> |
| + | |
| + | <h5>2. DNA plamsid extraction of pO-IGEM5 launch on liquid media yesterday |
| + | </h5> |
| + | <p class="text-notebook">Kit used Nucleospin Plasmid </p> |
| + | |
| + | <h5>3. Nanodrop measurement for p0-IGEM5 </h5> |
| + | <p class="text-notebook">26.4 ng/µL </p> |
| + | |
| + | <h5>4.Digestion reaction </h5> |
| + | <p class="text-notebook">bbsI =0.5µL <br> |
| + | buffer= 2µL<br> |
| + | DNA =10µL <br> |
| + | H2O= 6.5µL <br> |
| + | Expected result: 4,4kb + (?)</p> |
| + | |
| + | <h5>5. Gel migration of digestion reaction products </h5> |
| + | <p class="text-notebook">ast well = digestion reaction product of GagPOL from the day before |
| + | → Does not correspond to the expected lenght </p> |
| + | |
| + | </div> |
| + | </div> |
| + | </div> |
| + | </div> |
| + | <!-- -----------------------------------.\ One day of the notebook ------------------------------------------------------- --> |
| + | <!-- -----------------------------------Monday 17th September ------------------------------------------------------- --> |
| + | <div class="container-fluid"> |
| + | <div class="row text-center text-xs-center text-sm-center text-md-left text-lg-left "> |
| + | <div class="col-xs-12 col-sm-12 col-md-12 col-lg-12"> |
| + | <div class="note"> |
| + | <h2 class="text-center" id="s17"> Monday 17th September</h2> |
| + | |
| + | <h4>Ligation <br> Migration of the Gag Pol sample <br> Preculture of OTSB (7 white colonies) |
| + | </h4> |
| + | <h6> Muséum national d'histoire naturelle (MNHN) </h6> |
| + | <div class="d-flex justify-content-end"> <div class="chip-icone"> <div class="chip"> |
| + | <img src="https://static.igem.org/mediawiki/2018/1/1d/T--Sorbonne_U_Paris--Claude_avatar.png" alt="Person" width="96" height="96"> |
| + | Sara |
| + | </div> |
| + | <div class="chip"> |
| + | <img src="https://static.igem.org/mediawiki/2018/1/1d/T--Sorbonne_U_Paris--Claude_avatar.png" alt="Person" width="96" height="96"> |
| + | Victor |
| + | </div> |
| + | </div> </div> |
| + | <h5>1. Ligation </h5> |
| + | <p class="text-notebook">3 ligation tubes are prepared , T-, G, pre-mix of E, T- <br> |
| + | - Tube 1 : T- 1.2µl of blackbone +12.8 µL of H2O (14µL in total) <br> |
| + | - Tube 2 : G 2 µL of the 6 sub-parts for GagPol)+.0.8µl of H2O +1.2µL of backbone ( 14µl in total) |
| + | Tube 3: Master mix of enzymes |
| + | </p> |
| + | <div class="d-flex justify-content-center"> |
| + | <div class="table-responsive-sm"> |
| + | <table class="text-center tablenotebook"> |
| + | <thead> |
| + | <tr> |
| + | <th class="th-notebook">Components</th> |
| + | <th class="th-notebook">1 reaction</th> |
| + | </tr> |
| + | </thead> |
| + | <tbody> |
| + | <tr> |
| + | <td class="td-notebook">ATP</td> |
| + | <td class="td-notebook">4 µL </td> |
| + | </tr> |
| + | <tr> |
| + | <td class="td-notebook">Cutsmart buffer (10X)</td> |
| + | <td class="td-notebook">4 µL</td> |
| + | </tr> |
| + | <tr> |
| + | <td class="td-notebook">T4 ligase</td> |
| + | <td class="td-notebook">2 µL</td> |
| + | </tr> |
| + | <tr> |
| + | <td class="td-notebook">bbstI</td> |
| + | <td class="td-notebook">2 µL</td> |
| + | </tr> |
| + | </tbody> |
| + | </table> |
| + | </div> |
| + | </div> |
| + | <p class="text-notebook"> 12µL of mix in total dispatched in tubes 1 and 2 (6µL each)</p> |
| + | |
| + | <h5>2. 1% agarose gel preparation, in order to migrate the Gag Pol sample </h5> |
| + | <p class="text-notebook">- 0.5g of agarose <br> |
| + | - 50ml of TEA 1X <br> |
| + | - Cyber green <br> |
| + | |
| + | Gel plan: well 1 : 3µl of DNA ladder, well 2 and 3 10µl of Gagpol |
| + | </p> |
| + | |
| + | <h5>Preculture of OTSB (7 white colonies) </h5> |
| + | <p class="text-notebook">For each : <br> |
| + | - 4ml of LB media <br> |
| + | - 2µl of spectinomycin (100mg/ml) (in order to obtain 10µg/ml) <br> |
| + | - 1 white clone <br> |
| + | Incubation at 37°C overnight |
| + | |
| + | </p> |
| + | |
| + | <h5>4. To do next</h5> |
| + | <p class="text-notebook"> |
| + | - Otsb miniprep + digestion <br> |
| + | - Gag digestion <br> |
| + | - Gag transfo) |
| + | </p> |
| + | |
| + | |
| + | |
| </div> | | </div> |
| </div> | | </div> |
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