Difference between revisions of "Team:Goettingen/Experiments"

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             </td>
 
             </td>
 
             <td valign="top" width="150">
 
             <td valign="top" width="150">
                 <p>ad. 1000mL</p>
+
                 <p>ad. 1000 mL</p>
 
             </td>
 
             </td>
 
         </tr>
 
         </tr>
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             <td valign="top" width="97">
 
             <td valign="top" width="97">
 
                 <p>
 
                 <p>
                     14mL
+
                     14 mL
 
                 </p>
 
                 </p>
 
             </td>
 
             </td>
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             <td valign="top" width="97">
 
             <td valign="top" width="97">
 
                 <p>
 
                 <p>
                     7.5mL
+
                     7.5 mL
 
                 </p>
 
                 </p>
 
             </td>
 
             </td>
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<p>1g Yeast extract</p>
 
<p>1g Yeast extract</p>
 
<p>3.5 ml 50% w/w Phytic acid</p>
 
<p>3.5 ml 50% w/w Phytic acid</p>
<p>0.2g CaCl2</p>
+
<p>0.2 g CaCl2</p>
<p>0.5g MgSO4</p>
+
<p>0.5 g MgSO4</p>
 
<p>Adjust the pH to 7.2 with NaOH</p>
 
<p>Adjust the pH to 7.2 with NaOH</p>
<p>Ad 2L of Millipore H2O</p>
+
<p>Ad 2 L of Millipore H2O</p>
<p>32g agar</p>
+
<p>32 g agar</p>
 
<p>Autoclave</p>
 
<p>Autoclave</p>
 
<p>&nbsp;</p>
 
<p>&nbsp;</p>
<p>After autoclaving the medium must cool down to ca. 50 ˚C. Now glycerol, IPTG, BCIP and the respective antiobiotic can be added.</p>
+
<p>After autoclaving the medium must cool down to ca. 50˚C. Now glycerol, IPTG, BCIP and the respective antiobiotic can be added.</p>
 
<p>&nbsp;</p>
 
<p>&nbsp;</p>
 
<p>For 2 L medium:</p>
 
<p>For 2 L medium:</p>
<p>2ml BCIP</p>
+
<p>2 ml BCIP</p>
<p>2ml 1M IPTG</p>
+
<p>2 ml 1M IPTG</p>
<p>2ml Ampicllin or Kanamycin</p>
+
<p>2 ml Ampicllin or Kanamycin</p>
<p>40mL Glycerol</p>
+
<p>40 mL Glycerol</p>
 
<p>The media is now ready for plating</p>
 
<p>The media is now ready for plating</p>
 
<p><br /> <strong>Result</strong>: On Sperber medium phosphatase-recombinant colonies should develop a distinct color blue after 2 days.</p>
 
<p><br /> <strong>Result</strong>: On Sperber medium phosphatase-recombinant colonies should develop a distinct color blue after 2 days.</p>
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<p style="text-align: center;"><span style="font-size: x-large; color: #888888;"><strong><span lang="EN-GB"></span></strong></span></p>
 
<p style="text-align: center;"><span style="font-size: x-large; color: #888888;"><strong><span lang="EN-GB"></span></strong></span></p>
 
<p><span lang="EN-GB">&nbsp;</span></p>
 
<p><span lang="EN-GB">&nbsp;</span></p>
<p><span lang="EN-GB">To 500ml of LB Media add 7.5g of Agar and 5ml of Tributyrin and homogenize with a mixer.</span></p>
+
<p><span lang="EN-GB">To 500 ml of LB Media add 7.5 g of Agar and 5 ml of Tributyrin and homogenize with a mixer.</span></p>
 
<p><span lang="EN-GB">This culture medium must be directly sterilized by autoclaving at 121˚C for 20 min.</span></p>
 
<p><span lang="EN-GB">This culture medium must be directly sterilized by autoclaving at 121˚C for 20 min.</span></p>
 
<p><span lang="EN-GB">If you wait too long it will be inhomogeneous again!</span></p>
 
<p><span lang="EN-GB">If you wait too long it will be inhomogeneous again!</span></p>
<p><span lang="EN-GB">When the medium cools down enough, the antibiotic can be added.</span></p>
+
<p><span lang="EN-GB">When the medium cools down to 50°C, the antibiotic can be added.</span></p>
 
<p><span lang="EN-GB">&nbsp;</span></p>
 
<p><span lang="EN-GB">&nbsp;</span></p>
 
<p><strong><span lang="EN-GB">Result:</span></strong><span lang="EN-GB"> Halo formation is visible around the positive clones.</span></p>
 
<p><strong><span lang="EN-GB">Result:</span></strong><span lang="EN-GB"> Halo formation is visible around the positive clones.</span></p>
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             </td>
 
             </td>
 
             <td valign="top" width="246">
 
             <td valign="top" width="246">
                 <p>10&micro;l</p>
+
                 <p>10 &micro;l</p>
 
             </td>
 
             </td>
 
         </tr>
 
         </tr>
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             </td>
 
             </td>
 
             <td valign="top" width="246">
 
             <td valign="top" width="246">
                 <p>125ng</p>
+
                 <p>125 ng</p>
 
             </td>
 
             </td>
 
         </tr>
 
         </tr>
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             </td>
 
             </td>
 
             <td valign="top" width="246">
 
             <td valign="top" width="246">
                 <p>50ng (1&micro;l)</p>
+
                 <p>50 ng (1&micro;l)</p>
 
             </td>
 
             </td>
 
         </tr>
 
         </tr>
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             </td>
 
             </td>
 
             <td valign="top" width="246">
 
             <td valign="top" width="246">
                 <p>1&micro;l</p>
+
                 <p>1 &micro;l</p>
 
             </td>
 
             </td>
 
         </tr>
 
         </tr>
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             </td>
 
             </td>
 
             <td valign="top" width="246">
 
             <td valign="top" width="246">
                 <p>x&micro;l</p>
+
                 <p>x &micro;l</p>
 
             </td>
 
             </td>
 
         </tr>
 
         </tr>
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             </td>
 
             </td>
 
             <td valign="top" width="246">
 
             <td valign="top" width="246">
                 <p>20&micro;l</p>
+
                 <p>20 &micro;l</p>
 
             </td>
 
             </td>
 
         </tr>
 
         </tr>

Revision as of 13:27, 18 September 2015



Media/Buffer

LB Medium

"Fat" LB Medium

Phosphatase Activity plates, Sperber media

Esterase Activity plates, with 1% Tributyrin

Cellulase activity plates

1x TAE Buffer

Cloning Methods

PCR product purification using QIAquick® PCR Purification Kit (QIAGEN)

PCR Gel extraction, peqGOLD Gel Extraction Kit

Blunt End Ligation in pJET1.2 vector –Clone JET PCR Cloning Kit– (Thermo Scientific)

Sticky End T4 Ligation (Thermo Scientific)

TOPO® Cloning protocol usingChampion™ pET Directional TOPO® Expression Kits (Thermo Fisher Scientific)

Plasmid transformation into chemically competent E. coli

Electroporation of BL21 cells with pJET_RFP

Plasmid Extraction - using QIAprep Spin Miniprep Kit (QIAGEN)

Plasmid Extraction - using peqGOLD Plasmid Miniprep Kit I (PEQLAB Technologies)

Competent Cells

Preparation of competent E.coli cells

Transformation Efficiency Kit, RFP construct (iGEM)

Protein Extraction and Purification

Protein Extraction (French Press) and Purification (Protino® Ni-IDA 2000 His-Tag protein purification, Macherey-Nagel)

Bradford Assay

Activity Screens

Esterase activity test

Phosphatase activity test

Cellulase activity screening

Restriction Controls

Aan I (Psi I ) - thermo fisher scientific - restriction control protocol

Double digestion restriction control

Restriction control using fast and slow digestion enzymes

Scafoldin Restriction control

Esterase Restriction Control

Phosphatase Restriction Control

PCR Preparation Methods

Colony PCR

Phusion PCR

Sequencing

Protocol for Sanger sequencing

Overnight Sanger Sequencing

Fluorescence Microscopy

RFP microscopy

Counting iGEM Goettingen2015.jpeg