Latest revision as of 17:04, 1 November 2017

Lab Notes

2016.12.06-2017.2.16

We attempted to be familiar with the rules of iGEM, and discussed our own project based on researches and the previous projects. We decided on our final project and initially designed the experimental plans.

2017.2.17-3.27

We screened some strains to obtain the phosphite dehydrogenase gene.

2017.3.28-5.28

We constructed the metabolic pathways of formamide and phosphite into the host to fit our special designed medium.

2017.5.29-6.14

We transformed an EGFP expressing vector into the host to verify effect of the construction.

2017.6.15-7.8

We cultivated the recombinant stains to test their normal growth situation.

2017.7.9-7.27

We verified the function of N&P pathways by using the unsterile cultivating medium and co-culturing the engineering strain with other microorganisms.

2017.7.28-8.12

We examined the enzymatic properties of the enzyme produced by recombinant strains.

2017.8.13-8.21

We selected and designed the target sequence from the genome of T7 phage.

2017.8.22-8.30

We constructed the pTarget-N₂₀, and confirmed its expression along with pCas.

2017.8.31-9.17

We began constructing Biobricks of pSB1C3 backbones.

2017.9.18-9.24

We verified the function of constructed CRISPR/Cas system in recombinant strain.

2017.9.25-10.9

We combined N&P pathways and CRISPR/Cas system together and confirmed the entire functions.

2017.10.10-10.30

We sent our BioBricks for this year. We worked on paperwork of our WIKI.

Lab of Applied Biocatalysis,
College of Food Sciences and Engineering,
South China University of Technology,
Guangzhou 510640,
Guangdong,
Peoples R China

PI. Dr.Lou wenyong
wylou@scut.edu.cn
Members. Email:
lihuixianscut@126.com
xjialiu5211@163.com

If you are interested in our project, welcome to contact us.

@@ Line 4: / Line 4: @@
      <h1><span>Lab Notes</span></h1>
      <h2>Lab Notes</h2>
-     <p>
+     <style>
-.12.06-2017.2.16<br>
+        .timeline {
-    We attempted to be familiar with the rules of iGEM, and discussed our own project based on researches and the previous projects. We decided on our final project and initially designed the experimental plans.<br>
+            position: relative;
-.2.17-3.27<br>
+            width: 100%;
-    We screened some strains to obtain the phosphite dehydrogenase gene.<br>
+        }
-.3.28-5.28<br>
+        .timeline::before {
-    We constructed the metabolic pathways of formamide and phosphite into the host to fit our special designed medium.<br>
+            content: '';
-.5.29-6.14<br>
+            height: 100%;
-    We transformed an EGFP expressing vector into the host to verify effect of the construction.<br>
+            width: 0px;
-.6.15-7.8<br>
+            left: 50%;
-    We cultivated the recombinant stains to test their normal growth situation.<br>
+            position: absolute;
-.7.9-7.27<br>
+            border: 2px solid #566474;
-    We verified the function of N&amp;P pathways by using the unsterile cultivating medium and co-culturing the engineering strain with other microorganisms.<br>
+        }
-.7.28-8.12<br>
+        .timeline-item {
-    We examined the enzymatic properties of the enzyme produced by recombinant strains.<br>
+            width: 45%;
-.8.13-8.21<br>
+            margin-left: 0;
-    We selected and designed the target sequence from the genome of T7 phage.<br>
+            margin-right: 0;
-.8.22-8.30<br>
+            margin-bottom: 35px;
-    We constructed the pTarget-N20, and confirmed its expression along with pCas.<br>
+        }
-.8.31-9.17<br>
+        .timeline-item::before {
-    We began constructing Biobricks of pSB1C3 backbones.<br>
+            content: '';
-.9.18-9.24<br>
+            position: absolute;
-    We verified the function of constructed CRISPR/Cas system in recombinant strain.<br>
+            left: 50%;
-.9.25-10.9<br>
+            margin-left: -12px;
-    We combined N&amp;P pathways and CRISPR/Cas system together and confirmed the entire functions.<br>
+            margin-top: 20px;
-.10.10-10.30<br>
+            border: 14px solid #566474;
-    We sent our BioBricks for this year. <br>
+            border-radius: 100%;
-    We worked on paperwork of our WIKI.
+        }
-     </p>
+        .timeline-item:nth-child(odd) {
+            margin-left: 1%;
+            text-align: right;
+        }
+        .timeline-item:nth-child(even) {
+            margin-left: 54%;
+            text-align: left;
+        }
+     </style>
+    <div class="timeline">
+        <div class="timeline-item">
+            <span class="bd">2016.12.06-2017.2.16</span>
+            <p>We attempted to be familiar with the rules of iGEM, and discussed our own project based on researches and the previous projects. We decided on our final project and initially designed the experimental plans.</p>
+        </div>
+        <div class="timeline-item">
+            <span class="bd">2017.2.17-3.27</span>
+            <p>We screened some strains to obtain the phosphite dehydrogenase gene.</p>
+        </div>
+        <div class="timeline-item">
+            <span class="bd">2017.3.28-5.28</span>
+            <p>We constructed the metabolic pathways of formamide and phosphite into the host to fit our special designed medium.</p>
+        </div>
+        <div class="timeline-item">
+            <span class="bd">2017.5.29-6.14</span>
+            <p>We transformed an EGFP expressing vector into the host to verify effect of the construction.</p>
+        </div>
+        <div class="timeline-item">
+            <span class="bd">2017.6.15-7.8</span>
+            <p>We cultivated the recombinant stains to test their normal growth situation.</p>
+        </div>
+        <div class="timeline-item">
+            <span class="bd">2017.7.9-7.27</span>
+            <p>We verified the function of N&amp;P pathways by using the unsterile cultivating medium and co-culturing the engineering strain with other microorganisms.</p>
+        </div>
+        <div class="timeline-item">
+            <span class="bd">2017.7.28-8.12</span>
+            <p>We examined the enzymatic properties of the enzyme produced by recombinant strains.</p>
+        </div>
+        <div class="timeline-item">
+            <span class="bd">2017.8.13-8.21</span>
+            <p>We selected and designed the target sequence from the genome of T7 phage.</p>
+        </div>
+        <div class="timeline-item">
+            <span class="bd">2017.8.22-8.30</span>
+            <p>We constructed the pTarget-N<sub>20</sub>, and confirmed its expression along with pCas.</p>
+        </div>
+        <div class="timeline-item">
+            <span class="bd">2017.8.31-9.17</span>
+            <p>We began constructing Biobricks of pSB1C3 backbones.</p>
+        </div>
+        <div class="timeline-item">
+            <span class="bd">2017.9.18-9.24</span>
+            <p>We verified the function of constructed CRISPR/Cas system in recombinant strain.</p>
+        </div>
+        <div class="timeline-item">
+            <span class="bd">2017.9.25-10.9</span>
+            <p>We combined N&amp;P pathways and CRISPR/Cas system together and confirmed the entire functions.</p>
+        </div>
+        <div class="timeline-item">
+            <span class="bd">2017.10.10-10.30</span>
+            <p>We sent our BioBricks for this year. We worked on paperwork of our WIKI.</p>
+        </div>
+     </div>
 </div>
 </html>
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Latest revision as of 17:04, 1 November 2017

Lab Notes

Lab Notes