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| Line 125: |
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| | <p class="article-p">▲Fig1-2:Circuit design of detecting Copper ion.</p> | | <p class="article-p">▲Fig1-2:Circuit design of detecting Copper ion.</p> |
| | </article> | | </article> |
| − | <article class="article">
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| − | <h3 class="article-title">Result</h3>
| |
| − | <ol class="article-ol">
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| − | <li>
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| − | <span>Whether Mercury can enter e.coli or not</span>
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| − | <ol class="article-ol" type="A">
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| − | <li><span>Method</span>
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| − | <h4 class="article-h4">Detection of the amount of toxins in the e.coli.</h4>
| |
| − | <ol class="article-ol" type="I">
| |
| − | <li>Add 100μl of DH5α and 900μl of LB broth into the tube and incubate for 1hr.</li>
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| − | <li>Centrifuge at 4000rpm for 3min and clicard 800μl of the supernatant</li>
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| − | <li>
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| − | <p class="article-p">Plate each 100μl of the bacteria onto the dishes and spread.</p>
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| − | <p class="article-p">Incubate the plates at 37℃ overnight</p>
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| − | </li>
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| − | <li>
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| − | <p class="article-p">Prepare each concentration of the toxin.</p>
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| − | <p class="article-p">Statutory standards *100 / *10 / *1 / *0.1 / *0.01</p>
| |
| − | </li>
| |
| − | </ol>
| |
| − | <h4 class="article-h4">Next day</h4>
| |
| − | <ol class="article-ol" type="I">
| |
| − | <li>
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| − | <p class="article-p">Prepare 16 microcentrifuge tubes.(5 kinds of concentration *3 timings+control)</p>
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| − | <p class="article-p">Add 500μl of DH5α to each tube.</p>
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| − | <p class="article-p">Centrifuge all tubes at 4000rpm for 3min.</p>
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| − | <p class="article-p">Remove the supernatent.</p>
| |
| − | </li>
| |
| − | <li>
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| − | <p class="article-p">Add 1000μl of the toxic solution each time.</p>
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| − | <p class="article-p">Follow the concentration and 3 timings(0.5hr / 1hr / 1.5hr).</p>
| |
| − | </li>
| |
| − | <li>
| |
| − | <ol class="article-ol" type="i">
| |
| − | <li>Add 0.5cc of ddH<sub>2</sub>O and mix with the bacterias</li>
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| − | <li>Centrifuge at 13000rpm for 30 sec</li>
| |
| − | <li>Remove the water</li>
| |
| − | <li>Repeat step1~step3 for three times</li>
| |
| − | </ol>
| |
| − | </li>
| |
| − | <li>
| |
| − | <p class="article-p">Add 1cc of ddH<sub>2</sub>O and mix with the bacterias</p>
| |
| − | <p class="article-p">Centrifuge at 13000rpm for 30sec.</p>
| |
| − | <p class="article-p">Remove 700μl of the supernatant</p>
| |
| − | </li>
| |
| − | <li>
| |
| − | <p class="article-p">Kill the bacteria:</p>
| |
| − | <ol class="article-ol" type="i">
| |
| − | <li>Put all the tubes in the Liquid nitrogen</li>
| |
| − | <li>When they freeze,heat them at 100℃</li>
| |
| − | <li>Repeat step1~step2 for 3 times</li>
| |
| − | </ol>
| |
| − | </li>
| |
| − | </ol>
| |
| | | | |
| − | </li>
| |
| − | <li><span>Result</span></li>
| |
| − | <img src="https://static.igem.org/mediawiki/2015/d/dc/2015_hsnu_hg_1111111.jpg" width="70%">
| |
| − | <p class="article-p">▲Fig3:The absorption by using gold nanoparticles in different Hg<sup>+</sup> concentration.</p>
| |
| − | <p class="article-p">With this figure, we can know that the higher Hg<sup>2+</sup> concentration, the lower fluorescence intensity it showed.</p>
| |
| − |
| |
| − |
| |
| − | </ol>
| |
| − | </li>
| |
| − | <li>
| |
| − | <span>Whether e.coli is alive in the poisons, condition or not</span>
| |
| − | <ol class="article-ol" type="A">
| |
| − | <li><span>Method</span>
| |
| − | <div class="section note">
| |
| − | <h2 class="note-title">DH5α-Pretest</h2>
| |
| − | <div class="note-content">
| |
| − | <h3 class="note-subtitle">Procedure</h3>
| |
| − | <p class="note-caption">Because we must test E.coli’s Survival in the environment there is Mercury by counting the colonies,First we test how much concentration is the best.</p>
| |
| − | <ol class="note-ordered-list" type="I">
| |
| − | <li>
| |
| − | <p class="note-caption">culture</p>
| |
| − | <p class="note-caption">STEP1:take 1μL DH5α to spread the plate(no Antibiotic)</p>
| |
| − | <p class="note-caption">STEP2:put in 37 degree Celsius 12~16hr</p>
| |
| − | </li>
| |
| − | <li>
| |
| − | <p class="note-caption">liquid culture</p>
| |
| − | </li>
| |
| − | <li>
| |
| − | <p class="note-caption">STEP1:put 80μL into 2ml LB broth </p>
| |
| − | <p class="note-caption">STEP2:recovering</p>
| |
| − | <p class="note-caption">STEP3: After 2hr,dilute it to 10<sup>-4</sup>,10<sup>-5</sup>,10<sup>-6</sup>,10<sup>-7</sup>,and then go to spread the plate (no Antibiotic)</p>
| |
| − | <p class="note-caption">STEP4: After 4hr dilute it to 10<sup>-4</sup>, 10<sup>-5</sup> ,10<sup>-6</sup> ,10<sup>-7</sup> ,and then go to spread the plate (no Antibiotic), 6hr and 8hr Similarly</p>
| |
| − | <p class="note-caption">STEP5:Take 200μL out from the tube and spread the plate(AMP+)</p>
| |
| − | <p class="note-caption">STEP6: put in 37 degree Celsius 12~16hr</p>
| |
| − | </li>
| |
| − | </ol>
| |
| − |
| |
| − | </div>
| |
| − | </div>
| |
| − |
| |
| − | <div class="section note">
| |
| − | <h2 class="note-title">Survival</h2>
| |
| − | <div class="note-content">
| |
| − | <h3 class="note-subtitle">Procedure</h3>
| |
| − | <p class="note-caption">First we culture DH5α with LB only plate for 15hr. Then,pick one colony in the LB broth,and liquid culture for 15hr.</p>
| |
| − | <p class="note-caption">We divided two categories A and B.</p>
| |
| − | <h3 class="note-subtitle">A:</h3>
| |
| − | <p class="note-caption">Take 80μL into 2ml LB broth × 6 tubes and then culture 1 hr.</p>
| |
| − | <p class="note-caption">After 1hr,add 20μL Mercury into three tubes(conc. Is 2000ppb(A thousand times the standard value))</p>
| |
| − | <p class="note-caption">And add 20μL DMSO into the other tubes.Then,culture for 3hr.</p>
| |
| − | <p class="note-caption">After 3hr,dilute the broth to 10<sup>-6</sup></p>
| |
| − | <p class="note-caption">And take 200μL to spread the plate.</p>
| |
| − | <h3 class="note-subtitle">B:</h3>
| |
| − | <p class="note-caption">Take 80μL into 2ml LB broth in a tube And then culture 1 hr.</p>
| |
| − | <p class="note-caption">After 1hr, put them into 6 tubes equally.</p>
| |
| − | <p class="note-caption">Dilute the broth to 5×10<sup>-4</sup></p>
| |
| − | <p class="note-caption">Add 0.4μL Mercury(2×10<sup>-4</sup>) in three tubes.</p>
| |
| − | <p class="note-caption">Add 0.4μL DMSO in the other three tubes.</p>
| |
| − | <p class="note-caption">Go to 37 degree Celsius shaking for 10min.</p>
| |
| − | <p class="note-caption">Take 200μL to spread the plate.</p>
| |
| − | <p class="article-p">▼Table1: E. coli on the agar plate.</p>
| |
| − | <img src="https://static.igem.org/mediawiki/2015/b/b0/HSNU-TAIPEI-reasult-mercury.jpg" width="70%">
| |
| − |
| |
| − | </div>
| |
| − | </div>
| |
| − | </li>
| |
| − | </ol>
| |
| − | </li>
| |
| − | <ol>
| |
| − | </article>
| |
| | <article class="article"> | | <article class="article"> |
| | <h3 class="article-title">Reference</h3> | | <h3 class="article-title">Reference</h3> |
