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| + | #Notes{ |
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| <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> | | <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> |
| <header class="entry-header"> | | <header class="entry-header"> |
− | <div class="entry-title" align="center" >General Protocols</div> | + | <div class="entry-title" align="center" style="font-size:42px;margin-top:30px" >General Protocols</div> |
| </header><!-- .entry-header --> | | </header><!-- .entry-header --> |
| <h2 class="entry-title">1.Plasmid Extraction</h2> | | <h2 class="entry-title">1.Plasmid Extraction</h2> |
| <div class="entry-content"> | | <div class="entry-content"> |
| <div class="note-content"> | | <div class="note-content"> |
− |
| + | |
| We use the<b> TIANprep Mini Plasmid Kit </b>made by <b>TIANGEN Biotech Co.,Ltd.</b> to extract plasmid. Here is the protocol.<br/> | | We use the<b> TIANprep Mini Plasmid Kit </b>made by <b>TIANGEN Biotech Co.,Ltd.</b> to extract plasmid. Here is the protocol.<br/> |
| Add <b>ethanol (96-100%)</b> to Buffer <b>PW </b>before use, check bottle tag for the adding volume.<br/> | | Add <b>ethanol (96-100%)</b> to Buffer <b>PW </b>before use, check bottle tag for the adding volume.<br/> |
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| 6. Transfer the supernatant from step 5 to the Spin Column <b>CP3</b> (place <b>CP3 </b>in a collection tube) by decanting or pipetting. Centrifuge for <b>30-60 s </b>at <b>12,000 rpm (~13,400 × g)</b>. Discard the flow-through and set the Spin Column <b>CP3 </b>back into the Collection Tube.<br/> | | 6. Transfer the supernatant from step 5 to the Spin Column <b>CP3</b> (place <b>CP3 </b>in a collection tube) by decanting or pipetting. Centrifuge for <b>30-60 s </b>at <b>12,000 rpm (~13,400 × g)</b>. Discard the flow-through and set the Spin Column <b>CP3 </b>back into the Collection Tube.<br/> |
| 7. (Optional, actually we hardly ever use) Wash the Spin Column <b>CP3 </b>by adding <b>500 μl</b> Buffer <b>PD </b>and centrifuge for <b>30-60 s</b> at <b>12,000 rpm (~13,400 × g)</b>. Discard the flow-through and put Spin Column <b>CP3 </b>back to the collection tube.<br/> | | 7. (Optional, actually we hardly ever use) Wash the Spin Column <b>CP3 </b>by adding <b>500 μl</b> Buffer <b>PD </b>and centrifuge for <b>30-60 s</b> at <b>12,000 rpm (~13,400 × g)</b>. Discard the flow-through and put Spin Column <b>CP3 </b>back to the collection tube.<br/> |
− | This step is recommended to remove trace nuclease activity when using <b>endA+</b> strains such as the<b> JM series</b>, <b>HB101</b> and its derivatives, or any wild-type strain, which have high levels of nuclease activity or high carbohydrate content.<br/> | + | This step is recommended to remove trace nuclease activity when using <b><i>endA+</i></b> strains such as the<b><i> JM series</i></b>, <b><i>HB101</i></b> and its derivatives, or any wild-type strain, which have high levels of nuclease activity or high carbohydrate content.<br/> |
| 8. Wash the Spin Column <b>CP3 </b>by adding <b>600 μl</b> Buffer <b>PW</b> (ensure that <b>ethanol (96%-100%)</b> has been added) and centrifuge for <b>30-60 s </b>at <b>12,000 rpm (~13,400 × g)</b>. Discard the flow-through, and put the Spin Colum<b> CP3</b> back into the Collection Tube.<br/> | | 8. Wash the Spin Column <b>CP3 </b>by adding <b>600 μl</b> Buffer <b>PW</b> (ensure that <b>ethanol (96%-100%)</b> has been added) and centrifuge for <b>30-60 s </b>at <b>12,000 rpm (~13,400 × g)</b>. Discard the flow-through, and put the Spin Colum<b> CP3</b> back into the Collection Tube.<br/> |
| 9. Repeat Step 8.<br/> | | 9. Repeat Step 8.<br/> |
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| 11. Place the Spin Column <b>CP3 </b>in a clean <b>1.5 ml </b>microcentrifuge tube. To elute DNA, add <b>50-100 μl</b> Buffer <b>EB </b>to the center of the Spin Column <b>CP3</b>, incubate for <b>2 min</b>, and centrifuge for <b>2 min</b> at <b>12,000 rpm (~13,400 × g)</b>.<br/> | | 11. Place the Spin Column <b>CP3 </b>in a clean <b>1.5 ml </b>microcentrifuge tube. To elute DNA, add <b>50-100 μl</b> Buffer <b>EB </b>to the center of the Spin Column <b>CP3</b>, incubate for <b>2 min</b>, and centrifuge for <b>2 min</b> at <b>12,000 rpm (~13,400 × g)</b>.<br/> |
| Note: If the volume of eluted buffer is less than <b>50 μl</b>, it may affect recovery efficiency. The pH value of eluted buffer will have some influence in eluting; Buffer <b>EB</b> or distilled water (<b>pH 7.0-8.5</b>) is suggested to elute plasmid DNA. For long-term storage of DNA, eluting in Buffer<b> EB</b> and storing at<b> -20°C</b> is recommended, since DNA stored in water is subject to acid hydrolysis. Repeat step 11 to increase plasmid recovery efficiency. | | Note: If the volume of eluted buffer is less than <b>50 μl</b>, it may affect recovery efficiency. The pH value of eluted buffer will have some influence in eluting; Buffer <b>EB</b> or distilled water (<b>pH 7.0-8.5</b>) is suggested to elute plasmid DNA. For long-term storage of DNA, eluting in Buffer<b> EB</b> and storing at<b> -20°C</b> is recommended, since DNA stored in water is subject to acid hydrolysis. Repeat step 11 to increase plasmid recovery efficiency. |
| + | |
| </div> | | </div> |
| <a class="expand-btn">Show More</a> | | <a class="expand-btn">Show More</a> |
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| Note: Residual ethanol from Buffer <b>PW</b> will influence the subsequent enzymatic reaction (enzyme digestion, PCR etc). <br/> | | Note: Residual ethanol from Buffer <b>PW</b> will influence the subsequent enzymatic reaction (enzyme digestion, PCR etc). <br/> |
| 8. Transfer the Spin Column<b> CA2</b> to a clean <b>1.5 ml</b> microcentrifuge tube. Add appropriate volume of Buffer<b> EB </b>to the center of the membrane, incubate at room temperature (<b>15-25°C</b>) for <b>2 min</b>, then centrifuge at <b>12,000 rpm (~13,400 × g)</b> for <b>2 min</b>. <br/> | | 8. Transfer the Spin Column<b> CA2</b> to a clean <b>1.5 ml</b> microcentrifuge tube. Add appropriate volume of Buffer<b> EB </b>to the center of the membrane, incubate at room temperature (<b>15-25°C</b>) for <b>2 min</b>, then centrifuge at <b>12,000 rpm (~13,400 × g)</b> for <b>2 min</b>. <br/> |
− | Note: The elution volume should not be less than <b>30 μl</b> since smaller volume will affect recovery efficiency. The pH value of eluted buffer will affect eluting. If purified DNA is used for sequencing, it is recommended to choose ddH2O (<b>pH 7.0-8.5</b>) to elute DNA, <b>pH<7.0</b> will decrease the elution efficiency. Obtained DNA should be stored at<b> -20°C</b> to prevent degradation. Buffer (<b>10 mM Tris-Cl, pH 8.0</b>) could also be used for DNA elution. For higher yield, pipette the eluate to the center of the membrane again, incubate <b>2 min</b> and centrifuge at <b>12,000 rpm (~13,400 × g)</b> for <b>2 min</b>. | + | Note: The elution volume should not be less than <b>30 μl</b> since smaller volume will affect recovery efficiency. The pH value of eluted buffer will affect eluting. If purified DNA is used for sequencing, it is recommended to choose ddH<sub>2</sub>O (<b>pH 7.0-8.5</b>) to elute DNA, <b>pH<7.0</b> will decrease the elution efficiency. Obtained DNA should be stored at<b> -20°C</b> to prevent degradation. Buffer (<b>10 mM Tris-Cl, pH 8.0</b>) could also be used for DNA elution. For higher yield, pipette the eluate to the center of the membrane again, incubate <b>2 min</b> and centrifuge at <b>12,000 rpm (~13,400 × g)</b> for <b>2 min</b>. |
| | | |
| </div> | | </div> |
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| <div class="note-content4"> | | <div class="note-content4"> |
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− | 1. Preparation of <b>TAE buffer</b>: Add <b>242g Tris, 37.2g Na2EDTA·2H2O, 800mL ddH2O</b>, after all the solute dissolve, add <b>57.1mL acetic acid </b>and add <b>ddH2O</b> to make the total volume <b>1L</b>.<br/> | + | 1. Preparation of <b>TAE buffer</b>: Add <b>242g Tris, 37.2g Na2EDTA·2H2O, 800mL ddH<sub>2</sub>O</b>, after all the solute dissolve, add <b>57.1mL acetic acid </b>and add <b>ddH<sub>2</sub>O</b> to make the total volume <b>1L</b>.<br/> |
| 2. Preparation of sample: Add <b>DNA loading buffer</b> to the DNA solution according to the dilution ratio of particular buffer.<br/> | | 2. Preparation of sample: Add <b>DNA loading buffer</b> to the DNA solution according to the dilution ratio of particular buffer.<br/> |
| 3. Preparation of agarose gel: Add <b>agarose powder 10g/L, 1×TAE buffer 100mL </b>(variable, according to need), heat the mixture by microwave oven until the agarose was dissolved. After the solution cool down to touchable temperature, add <b>50-100μL/L Goldenview Nucleic acid dye</b> to the solution. Then pour the solution to the gel mould with gel comb inserted and wait for its concretion.<br/> | | 3. Preparation of agarose gel: Add <b>agarose powder 10g/L, 1×TAE buffer 100mL </b>(variable, according to need), heat the mixture by microwave oven until the agarose was dissolved. After the solution cool down to touchable temperature, add <b>50-100μL/L Goldenview Nucleic acid dye</b> to the solution. Then pour the solution to the gel mould with gel comb inserted and wait for its concretion.<br/> |
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| <li>10×Cut Smart Buffer:<b> 5μL</b></li> | | <li>10×Cut Smart Buffer:<b> 5μL</b></li> |
| <li>DNA to be cut: <b>30μL</b></li> | | <li>DNA to be cut: <b>30μL</b></li> |
− | <li>ddH2O:<b> 13μL</b></li> | + | <li>ddH<sub>2</sub>O:<b> 13μL</b></li> |
| <br/> | | <br/> |
| <li>Reaction time: <b>2h</b></li> | | <li>Reaction time: <b>2h</b></li> |
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| <li>5×Ligase Buffer:<b> 4μL</b></li> | | <li>5×Ligase Buffer:<b> 4μL</b></li> |
| <li>DNA to be linked: <b>(c1V1/L1): (c2V2/L2)=5:1</b>. (c1: Concentration of cut DNA fragments; c2: Concentration of cut plasmid; V1: Volume of cut DNA fragments; V2: Volume of cut plasmid; L1: Length of cut DNA fragments; L2: Length of cut plasmid)</li> | | <li>DNA to be linked: <b>(c1V1/L1): (c2V2/L2)=5:1</b>. (c1: Concentration of cut DNA fragments; c2: Concentration of cut plasmid; V1: Volume of cut DNA fragments; V2: Volume of cut plasmid; L1: Length of cut DNA fragments; L2: Length of cut plasmid)</li> |
− | <li>ddH2O: add to make the total volume <b>20μL</b></li> | + | <li>ddH<sub>2</sub>O: add to make the total volume <b>20μL</b></li> |
| <br/> | | <br/> |
| <li>Reaction time:<b> 2h</b></li> | | <li>Reaction time:<b> 2h</b></li> |
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| <li>Template: <b>1μL</b></li> | | <li>Template: <b>1μL</b></li> |
| <li>dNTP:<b> 1μL</b></li> | | <li>dNTP:<b> 1μL</b></li> |
− | <li>Primer: Sense Primer and Anti-sense Primer, respectively <b>2.5μL</b></li> | + | <li>Primers: Sense Primer and Anti-sense Primer, respectively <b>2.5μL</b></li> |
− | <li>ddH2O: <b>32.5μL</b></li> | + | <li>ddH<sub>2</sub>O: <b>32.5μL</b></li> |
| <br/> | | <br/> |
| <li>Cycles: <b>25-35</b></li> | | <li>Cycles: <b>25-35</b></li> |
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| <li>Total volume: <b>20μL</b></li> | | <li>Total volume: <b>20μL</b></li> |
| <li>Colony PCR System: 2×Taq Master Mix (Dye added) <b>10μL</b></li> | | <li>Colony PCR System: 2×Taq Master Mix (Dye added) <b>10μL</b></li> |
− | <li>ddH2O: <b>10μL</b></li> | + | <li>Primers: Sense Primer and Anti-sense Primer, respectively <b>1μL</b></li> |
| + | <li>ddH<sub>2</sub>O: <b>8μL</b></li> |
| <li>select single colony with stick and immerse the stick into the system for <b>1 min</b>. Preparing the bacterial liquid and then add 1μL of it is also feasible. | | <li>select single colony with stick and immerse the stick into the system for <b>1 min</b>. Preparing the bacterial liquid and then add 1μL of it is also feasible. |
| </li><br/> | | </li><br/> |
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| Prepare the system: | | Prepare the system: |
| <li>Total volume: <b>50μL</b></li> | | <li>Total volume: <b>50μL</b></li> |
− | <li>ddH2O: <b>50μL</b></li> | + | <li>ddH<sub>2</sub>O: <b>50μL</b></li> |
| <li>select single colony with stick and immerse the stick into the system for <b>1 min</b> | | <li>select single colony with stick and immerse the stick into the system for <b>1 min</b> |
| </li><br/> | | </li><br/> |
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| <div class="note-content9"> | | <div class="note-content9"> |
| | | |
− | 1. Mix 50μL competent E.coli cell with 10μL plasmids, and place them in ice bath for 30 min. | + | 1. Mix <b>50μL</b> competent <i>E.coli</i> cell with <b>10μL</b> plasmids, and place them in ice bath for <b>30 min</b>.<br/> |
− | 2. Heat shock at 42℃ for 30 s. | + | 2. Heat shock at <b>42℃</b> for <b>30 s</b>.<br/> |
− | 3. Put the system back on ice for 2 min. | + | 3. Put the system back on ice for <b>2 min</b>.<br/> |
− | 4. Add 500 μl of LB without antibiotics and incubate at 37 ℃ for 30-60 min with the shaking speed of 200rpm. | + | 4. Add <b>500 μl</b> of LB without antibiotics and incubate at <b>37 ℃</b> for <b>30-60 min</b> with the shaking speed of <b>200rpm</b>.<br/> |
− | 5. Centrifuge the culture medium at 4000 rpm for 3min. | + | 5. Centrifuge the culture medium at <b>4000 rpm</b> for <b>3min</b>.<br/> |
| 6. Discard the supernatant and resuspend the sediment, use this resuspending liquid to spread the plate with antibiotics. | | 6. Discard the supernatant and resuspend the sediment, use this resuspending liquid to spread the plate with antibiotics. |
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| </div><!-- .entry-content --> | | </div><!-- .entry-content --> |
| <br/><br/> | | <br/><br/> |
− | <div class="entry-title" align="center" >Protocols for Microbial Consortia</div> | + | <div class="entry-title" align="center" style="font-size:42px">Protocols for Microbial Consortia</div> |
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| <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> | | <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> |
| <header class="entry-header"> | | <header class="entry-header"> |
− | <h2 class="entry-title">1.Culture Medium of E.coli-Sc Microbial consortia</h2> | + | <h2 class="entry-title">1.16s-DNA </h2> |
| </header><!-- .entry-header --> | | </header><!-- .entry-header --> |
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| <div class="entry-content"> | | <div class="entry-content"> |
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− | <div class="note-content10"> | + | <div class="note-content11"> |
| | | |
− | <li>13.3 g/L KH2PO4</li> | + | Prepare the system: |
− | <li>4 g/L (NH4)2HPO4 </li> | + | <li>Total volume: <b>20μL</b></li> |
− | <li>1.7 g/L citric acid </li> | + | <li>Colony PCR System: 2×Taq Master Mix (Dye added) <b>10μL</b></li> |
− | <li>0.0084 g/L EDTA </li> | + | <li>ddH<sub>2</sub>O: <b>8.2μL</b></li> |
− | <li>0.0025 g/L CoCl2</li> | + | <li>primer: <b>0.4μL </b> each</li> |
− | <li>0.015 g/L MnCl2 </li> | + | <li>bacteria liquid:<b>1μL</b></li> |
− | <li>0.0015 g/L CuCl2</li> | + | <li>The primer could copy the special 16s-DNA from this kind of bacteria.</li> |
− | <li>0.003 g/L H3BO3</li> | + | <li>The bacteria liquid is pretreatment. </li> |
− | <li>0.0025 g/L Na2MoO4</li> | + | <br/> |
− | <li>0.008 g/L Zn(CH3COO)2) </li> | + | <li>Cycles:<b> 25-35</b></li> |
− | <li>0.06 g/L Fe(III) citrate </li> | + | <li>Pre-denaturation: <b>94℃,2min</b></li> |
− | <li>0.0045 g/L thiamine</li> | + | <li>Denaturation: <b>94℃,30s</b></li> |
− | <li>1.3 g/L MgSO4 </li> | + | <li>Annealing: Depend on the primers, generally <b>45-65℃,20-60s</b></li> |
− | <li>40 g/L glucose </li> | + | <li>Extension: <b>72℃</b>, depend on the length of amplified fragment, generally <b>20-60s</b></li> |
− | <li>5 g/L yeast extract</li> | + | <li>Fully extension: <b>72℃,4min</b></li> |
− | <li>20 g/L xylose</li> | + | <li>Product Storage:<b> 4℃</b></li> |
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| </div> | | </div> |
− | <a class="expand-btn10">Show More</a> | + | <a class="expand-btn11">Show More</a> |
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| </div><!-- .entry-content --> | | </div><!-- .entry-content --> |
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| <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> | | <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> |
| <header class="entry-header"> | | <header class="entry-header"> |
− | <h2 class="entry-title">2.16s-DNA </h2> | + | <h2 class="entry-title">2. Preparation of W medium </h2> |
| </header><!-- .entry-header --> | | </header><!-- .entry-header --> |
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| <div class="entry-content"> | | <div class="entry-content"> |
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− | <div class="note-content11"> | + | <div class="note-content15"> |
| + | |
| + | Initial medium |
| + | <b><li>KH<sub>2</sub>PO<sub>4</sub>: 1.7 g/L</li> |
| + | <li>Na<sub>2</sub>HPO<sub>4</sub>: 9.8 g/L</li> |
| + | <li>(NH<sub>4</sub>)<sub>2</sub>SO<sub>4</sub>: 1.0 g/L</li> |
| + | <li>MgSO<sub>4</sub>·7H<sub>2</sub>O: 0.1 g/L</li> |
| + | <li>FeSO<sub>4</sub>·7H<sub>2</sub>O: 0.95 mg/L</li> |
| + | <li>MgO: 10.75 mg/L</li> |
| + | <li>CaCO<sub>3</sub>: 2.0 mg/L</li> |
| + | <li>ZnSO<sub>4</sub>·7H<sub>2</sub>O: 1.44 mg/L</li> |
| + | <li>CuSO<sub>4</sub>·5H<sub>2</sub>O: 0.25 mg/L</li> |
| + | <li>CoSO<sub>4</sub>·7H<sub>2</sub>O: 0.25 mg/L</li> |
| + | <li>H<sub>3</sub>BO<sub>3</sub>: 0.06 mg/L</li> |
| + | <li>HCl: 51.3ml/L</li></b> |
| + | <br/> |
| + | |
| + | We modify initial formula for convenience, and modified formula is shown as following table: |
| + | |
| + | <b><li>KH<sub>2</sub>PO<sub>4</sub>: 1.7 g/L</li> |
| + | <li>Na<sub>2</sub>HPO<sub>4</sub>: 9.8 g/L</li> |
| + | <li>(NH<sub>4</sub>)<sub>2</sub>SO4: 1.0 g/L</li> |
| + | <li>NH<sub>4</sub>Cl: 0.865 g/L</li> |
| + | <li>MgSO<sub>4</sub>·7H<sub>2</sub>O: 0.1 g/L</li> |
| + | <li>MgCl<sub>2</sub>: 0.025 g/L</li> |
| + | <li>Mother solution: 1 ml/L</li></b> |
| + | <br/> |
| + | Formula of mother solution |
| + | <b><li>FeSO<sub>4</sub>·7H<sub>2</sub>O: 0.95 g/L</li> |
| + | <li>CoCl<sub>2</sub>·6H<sub>2</sub>O: 0.236 g/L</li> |
| + | <li>CaCl<sub>2</sub>: 2.22 g/L</li> |
| + | <li>ZnSO<sub>4</sub>·7H<sub>2</sub>O: 1.44 g/L</li> |
| + | <li>CuSO<sub>4</sub>: 0.16 g/L</li> |
| + | <li>H<sub>3</sub>BO<sub>3</sub>: 0.06 g/L</li></b> |
| + | |
| + | |
| + | |
| + | </div> |
| + | <a class="expand-btn15">Show More</a> |
| + | |
| + | </div><!-- .entry-content --> |
| + | |
| + | |
| + | |
| + | |
| + | <div class="entry-title" align="center" style="font-size:42px">Protocols for Protein Engineering</div> |
| + | |
| + | |
| + | <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> |
| + | <header class="entry-header"> |
| + | <h2 class="entry-title">1.Preparation of the optimized yeast culture medium </h2> |
| + | </header><!-- .entry-header --> |
| + | |
| + | <div class="entry-content"> |
| + | |
| + | <div class="note-content23"> |
| + | |
| + | <b><li>Glucose:22g/L</li> |
| + | <li>Yeast Nitrogen Base:6.7g/L</li> |
| + | <li>Dispense mixture:1.224g/L</li> |
| + | <li>Agar:15g/L</li> |
| + | <li>His/Trp/Leu mixed solution:10ml/L</li></b> |
| + | |
| + | |
| + | |
| + | </div> |
| + | <a class="expand-btn23">Show More</a> |
| + | |
| + | </div><!-- .entry-content --> |
| + | |
| + | |
| + | |
| + | <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> |
| + | <header class="entry-header"> |
| + | <h2 class="entry-title">2.pNPA assay</h2> |
| + | </header><!-- .entry-header --> |
| + | |
| + | <div class="entry-content"> |
| + | |
| + | <div class="note-content24"> |
| + | A Buffer |
| + | <b><li>Glycerol:400μl</li> |
| + | <li> Gal:1000μl</li> |
| + | <li>SC-Ura:3600μl</li></b> |
| + | B Buffer: |
| + | <b><li>10mM pNPA Buffer:50μl</li> |
| + | <li> PBS(pH=7.4):98μl</li></b> |
| + | |
| + | |
| + | |
| + | </div> |
| + | <a class="expand-btn24">Show More</a> |
| + | |
| + | </div><!-- .entry-content --> |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | <div class="entry-title" align="center" style="font-size:42px">Protocols for Cell-Free Protein Synthesis</div> |
| + | |
| + | |
| + | <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> |
| + | <header class="entry-header"> |
| + | <h2 class="entry-title">1.Cell-free protein synthesis system(50 µL) </h2> |
| + | </header><!-- .entry-header --> |
| + | |
| + | <div class="entry-content"> |
| + | |
| + | <div class="note-content12"> |
| + | |
| + | <li>ddH<sub>2</sub>O:<b>7.9µL</b></li> |
| + | <li>Feeding buffer : <b>25µL</b></li> |
| + | <li>Mg<sup>2+</sup> solution : <b>1.1µL</b></li> |
| + | <li>Gene( plasmid as template) :<b> 1µL</b></li> |
| + | <li>Lysate : <b>15µL</b></li> |
| + | |
| + | |
| + | |
| + | </div> |
| + | <a class="expand-btn12">Show More</a> |
| + | |
| + | </div><!-- .entry-content --> |
| + | |
| + | |
| + | |
| + | <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> |
| + | <header class="entry-header"> |
| + | <h2 class="entry-title">2.Preparation of pNPA degradation reaction system </h2> |
| + | </header><!-- .entry-header --> |
| + | |
| + | <div class="entry-content"> |
| + | |
| + | <div class="note-content13"> |
| + | |
| + | Substrate: <b>0.2mM pNPA </b>water solution (<b>0.0362g pNPA </b>dissolving in ddH<sub>2</sub>O)<br/> |
| + | Reaction system: <b>10 times</b> diluted Enzyme solution(unpurified) mixed with the equal volume substrate. (<b>pH=7</b>)<br/> |
| + | After static reaction at <b>39℃ </b>for <b>8 hours</b>, we detected the characteristic adsorption peak of the product ,pNP, which has no other characteristic adsorption peak except in <b>400nm</b>. |
| + | |
| + | |
| + | </div> |
| + | <a class="expand-btn13">Show More</a> |
| + | |
| + | </div><!-- .entry-content --> |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> |
| + | <header class="entry-header"> |
| + | <h2 class="entry-title">3.Preparation of PET degradation reaction system </h2> |
| + | </header><!-- .entry-header --> |
| + | |
| + | <div class="entry-content"> |
| + | |
| + | <div class="note-content14"> |
| + | |
| + | Reaction system: PET was put into <b>20 times </b>diluted Enzyme solution(unpurified).(<b>pH=7</b>)<br/> |
| + | After static reaction at <b>39℃</b> for <b>2 days</b>, we detected the characteristic adsorption peak of the product ,MHET, which has no other characteristic adsorption peak except in <b>260nm</b>. And detect it every other day in the future 3-4 days. |
| + | |
| + | |
| + | </div> |
| + | <a class="expand-btn14">Show More</a> |
| + | |
| + | </div><!-- .entry-content --> |
| + | |
| + | |
| + | |
| + | <div class="entry-title" align="center" style="font-size:42px">Protocols for Cyanobacteria</div> |
| + | |
| + | |
| + | |
| + | <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> |
| + | <header class="entry-header"> |
| + | <h2 class="entry-title">1.Restriction Endonuclease Cutting and Dephosphorylation </h2> |
| + | </header><!-- .entry-header --> |
| + | |
| + | <div class="entry-content"> |
| + | |
| + | <div class="note-content16"> |
| | | |
| Prepare the system: | | Prepare the system: |
− | <li>Total volume: 20μL</li> | + | <li>Total volume: <b>100μL</b></li> |
− | <li>Colony PCR System: 2×Taq Master Mix (Dye added) 10μL</li> | + | <li>Restriction endonuclease :<b> 3μL respectively</b></li> |
− | <li>ddH2O: 8.2μL</li> | + | <li>10×fastdigest Buffer:<b> 10μL</b></li> |
− | <li>primer: 0.4μL each</li> | + | <li>Plasmids to be cut: <b>2μg</b></li> |
− | <li>bacteria liquid:1μL</li> | + | <li>ddH<sub>2</sub>O: add to make the total volume <b>100μL</b></li> |
− | <li>The primer could copy the special 16s-DNA from this kind of bacteria.</li> | + | |
− | <li>The bacteria liquid is pretreatment. </li> | + | |
| <br/> | | <br/> |
− | <li>Cycles: 25-35</li> | + | <li>fast AP: add when reacting for <b>1.5h</b></li> |
− | <li>Pre-denaturation: 94℃,2min</li> | + | <li>Total reaction time: <b>2h</b></li> |
− | <li>Denaturation: 94℃,30s</li> | + | <li>Reaction temperature:<b> 37℃</b></li> |
− | <li>Annealing: Depend on the primers, generally 45-65℃,20-60s</li> | + | |
− | <li>Extension: 72℃, depend on the length of amplified fragment, generally 20-60s</li> | + | |
− | <li>Fully extension: 72℃,4min</li>
| + | |
− | <li>Product Storage: 4℃</li>
| + | |
| | | |
| + | |
| + | </div> |
| + | <a class="expand-btn16">Show More</a> |
| + | |
| + | </div><!-- .entry-content --> |
| + | |
| + | |
| + | <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> |
| + | <header class="entry-header"> |
| + | <h2 class="entry-title">2.Phosphorylation </h2> |
| + | </header><!-- .entry-header --> |
| + | |
| + | <div class="entry-content"> |
| + | |
| + | <div class="note-content17"> |
| + | |
| + | Prepare the system: |
| + | <li>Total volume: <b>20μL</b></li> |
| + | <li>ATP:<b>2μL</b></li> |
| + | <li>10×Buffer A:<b>2μL</b></li> |
| + | <li>PNK:<b>1μL</b></li> |
| + | <li>ddH<sub>2</sub>O: add to make the total volume<b> 200μL</b></li> |
| + | <br/> |
| + | <li>Reaction time:<b>0.5h</b></li> |
| + | <li>Reaction temperature:<b> 37℃</b></li> |
| | | |
| | | |
| </div> | | </div> |
− | <a class="expand-btn11">Show More</a> | + | <a class="expand-btn17">Show More</a> |
| | | |
| </div><!-- .entry-content --> | | </div><!-- .entry-content --> |
| + | |
| + | |
| + | |
| + | <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> |
| + | <header class="entry-header"> |
| + | <h2 class="entry-title">3.Ligation of Phosphorylated DNA Fragments and Dephosphorylated Plasmids </h2> |
| + | </header><!-- .entry-header --> |
| + | |
| + | <div class="entry-content"> |
| | | |
− |
| + | <div class="note-content18"> |
| + | |
| + | Prepare the system: |
| + | <li>Total volume: <b>20μL</b></li> |
| + | <li>DNA fragment: <b>3μL</b></li> |
| + | <li>Plasmids to be ligase : <b>1μL</b></li> |
| + | <li>T4 Buffer:<b> 2μL</b></li> |
| + | <li>PEG4000:<b>2μL</b></li> |
| + | <li>T4 DNA ligase: <b>1μL </b></li> |
| + | <li>PCR H<sub>2</sub>O:<b>11μL</b></li> |
| + | <br/> |
| + | <li>Reaction time:<b> >1h</b></li> |
| + | <li>Reaction temperature:<b> 22℃</b></li> |
| + | |
| + | |
| + | |
| + | </div> |
| + | <a class="expand-btn18">Show More</a> |
| + | |
| + | </div><!-- .entry-content --> |
| + | |
| + | |
| + | |
| + | |
| + | <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> |
| + | <header class="entry-header"> |
| + | <h2 class="entry-title">4.A-Tailing Reaction </h2> |
| + | </header><!-- .entry-header --> |
| + | |
| + | <div class="entry-content"> |
| | | |
| + | <div class="note-content19"> |
| | | |
| + | Prepare the system: |
| + | <li>Total volume:<b> 20μL</b></li> |
| + | <li>Talling-A reaction Buffer:<b> 4μL</b></li> |
| + | <li>DNA fragment: <b>15μL</b></li> |
| + | <li>Taq DNA Polymerase: <b>1μL</b></li> |
| + | <br/> |
| + | <li>Reaction time: <b>>0.5h</b></li> |
| + | <li>Reaction temperature: <b>72℃</b></li> |
| | | |
| | | |
| | | |
| | | |
| + | </div> |
| + | <a class="expand-btn19">Show More</a> |
| + | |
| + | </div><!-- .entry-content --> |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> |
| + | <header class="entry-header"> |
| + | <h2 class="entry-title">5.TA cloning </h2> |
| + | </header><!-- .entry-header --> |
| + | |
| + | <div class="entry-content"> |
| + | |
| + | <div class="note-content20"> |
| + | |
| + | Prepare the system: |
| + | <li>Total volume:<b> 10μL</b></li> |
| + | <li>5×Buffer:<b>2μL</b></li> |
| + | <li>Vector:<b>0.5μL</b></li> |
| + | <li>DNA fragment:<b> 7μL</b></li> |
| + | <li>T4 DNA ligase:<b> 0.5μL</b> </li> |
| + | <br/> |
| + | <li>Reaction time: <b>0.5-1h</b></li> |
| + | <li>Reaction temperature:<b> 22℃</b></li> |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | </div> |
| + | <a class="expand-btn20">Show More</a> |
| + | |
| + | </div><!-- .entry-content --> |
| + | |
| + | |
| + | |
| + | |
| + | <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> |
| + | <header class="entry-header"> |
| + | <h2 class="entry-title">6.Electroporation </h2> |
| + | </header><!-- .entry-header --> |
| + | |
| + | <div class="entry-content"> |
| + | |
| + | <div class="note-content21"> |
| + | |
| + | 1.Cultures (<b>OD630=0.6–0.7</b>) which grow approaching the plateau are harvested.<br/> |
| + | 2.According to the quantity of transformation, one plasmid need <b>8-10mL</b> cultures. Cells are harvested by centrifugation at<b>3500rpm</b> for <b>13min</b> at<b> 4°C</b>. <br/> |
| + | 3.Discard the supernatant, resuspend with <b>20mL</b> sterilized ultrapure water. Then, centrifuge at <b>3500rpm</b> for <b>13min</b> at <b>4°C</b>.<br/> |
| + | 4.Repeat step3.<br/> |
| + | 5.Add <b>200mL </b>sterilized ultrapure water for each plasmid.<br/> |
| + | 6. Plasmid(<b>2μg</b>) is added to <b>200mL</b> condensed cultures in a sterilized EP tube. Then transfer the mixture into a <b>2mm</b>-gap electroporation cuvette.<br/> |
| + | 7.Place them on the ice for<b> 1-3min</b>.<br/> |
| + | 8. Bacteria are pulsed at <b>2.5kV(1.8kV)</b>.<br/> |
| + | 9. <b>200μL </b>BG-11 medium(without antibiotics) is added into the electroporation mixture and incubate for <b>5h</b>.<br/> |
| + | 10. Use the liquid to spread the plate with antibiotics. |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | </div> |
| + | <a class="expand-btn21">Show More</a> |
| + | |
| + | </div><!-- .entry-content --> |
| + | |
| + | |
| + | |
| + | <article id="post-4252" class="post-4252 post type-post status-publish format-standard has-post-thumbnail hentry category-150 tag-174 tag-xinjiang tag-173"> |
| + | <header class="entry-header"> |
| + | <h2 class="entry-title">7.Preparation of BG-11 medium </h2> |
| + | </header><!-- .entry-header --> |
| + | |
| + | <div class="entry-content"> |
| + | |
| + | <div class="note-content22"> |
| + | |
| + | <b><li>NaNO<sub>3</sub>: 1.5 g/L</li> |
| + | <li>K<sub>2</sub>HPO<sub>4</sub>·3H<sub>2</sub>O: 0.04 g/L</li> |
| + | <li>MgSO<sub>4</sub>·7H<sub>2</sub>O: 0.075 g/L</li> |
| + | <li>CaCl<sub>2</sub>·2H<sub>2</sub>O: 0.036 g/L</li> |
| + | <li>Citric acid: 0.006 g/L</li> |
| + | <li>Ferric ammonium citrate: 0.006 g/L</li> |
| + | <li>EDTA(disodium magnesium salt): 0.001 g/L</li> |
| + | <li>Na<sub>2</sub>CO<sub>3</sub>: 0.02 g/L</li> |
| + | <li>Trace metal mix A5+Co: 1 mL/L</li> |
| + | <li>Deionized water: 1000 mL</li> |
| + | <li>pH after autoclaving and cooling: 7.4 </li></b> |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | |
| + | </div> |
| + | <a class="expand-btn22">Show More</a> |
| + | |
| + | </div><!-- .entry-content --> |
| | | |
| </div><!-- #content --> | | </div><!-- #content --> |
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