Difference between revisions of "Team:TJU China/Notebook/Group1"

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-     <div class="notebook_month"> class="notebook_month_p"
+     <div class="notebook_month">
-         <div class="notebook_month_p">March</div>
+         <div class="notebook_month_p">Mar.</div>
-         <div class="notebook_month_p">April</div>
+         <div class="notebook_month_p">Apr.</div>
          <div class="notebook_month_p">May</div>
-         <div class="notebook_month_p">June</div>
+         <div class="notebook_month_p">Jun.</div>
-         <div class="notebook_month_p">July</div>
+         <div class="notebook_month_p">Jul.</div>
-         <div class="notebook_month_p">August</div>
+         <div class="notebook_month_p">Aug.</div>
-         <div class="notebook_month_p">September</div>
+         <div class="notebook_month_p">Sep.</div>
-         <div class="notebook_month_p">October</div>
+         <div class="notebook_month_p">Oct.</div>
      </div>
      <div class="notebook_timeline">
@@ Line 388: / Line 389: @@
          <div id="notebook_March">
              <div class="notebook_Month_head">March</div>
-             <div class="notebook_week">
+             <div class="notebook_week_p">Group1 get started at July.</div>
-                <div>
-                    <button id="3week1" class="notebook_information_button1">week1</button>
-                </div>
-                <div id="3notebook_week1" class="notebook_information_word1" style="display:none;">
-                    <div class="notebook_week_p">After a lot of document viewing and brainstorms, we finally came up with a clear idea about how we were
-                        going to carry out our part of project. We decided to construct the RNPs (complex of sgRNA and Cas9
-                        protein) and to wrap them with delivery vector in order to improve the gene-editing efficiency of
-                        the system into the cells.</div>
-                </div>
-                <div>
-                    <button id="3week2" class="notebook_information_button2">week2</button>
-                </div>
-                <div id="3notebook_week2" class="notebook_information_word2" style="display:none;">
-                    <div class="notebook_week_p">After daily meetings and discussions, we exchanged knowledge and ideas from the literatures we read.
-                        Comparing different transportation methods, including physical electroporation, chemical nanoparticles,
-                        and even virus methods, we decided to improve the transport efficiency of the system by using two-dimensional
-                        nanomaterials to encapsulate the cas9/sgRNA complex assembled in vitro to transport into the cells.</div>
-                </div>
-                <div>
-                    <button id="3week3" class="notebook_information_button3">week3</button>
-                </div>
-                <div id="3notebook_week3" class="notebook_information_word3" style="display:none;">
-                    <div class="notebook_week_p">We began to delve into more detailed and specific knowledge, such as the structure of cas9 protein and
-                        how it works, the structure and composition of sgRNA and how it is assembled with cas9 protein, the
-                        method of primer design, learning how to design sgRNA, and so on.</div>
-                </div>
-                <div>
-                    <button id="3week4" class="notebook_information_button4">week4</button>
-                </div>
-                <div id="3notebook_week4" class="notebook_information_word4" style="display:none;">
-                    <div class="notebook_week_p">After confirming the type of cas9 protein, we started buying and asking other labs if they had the same
-                        cas9 protein. While waiting for an answer, we are continuing to refine the questions left over from
-                        last week's knowledge and begin to learn the experimental procedures and necessary knowledge related
-                        to protein expression purification.</div>
-                </div>
-             </div>
          </div>
          <div id="notebook_April">
              <div class="notebook_Month_head">April</div>
-             <div class="notebook_week">
+             <div class="notebook_week_p">Group1 get started at July.</div>
-                <div>
-                    <button id="4week1" class="notebook_information_button1">week1</button>
-                </div>
-                <div id="4notebook_week1" class="notebook_information_word1" style="display:none;">
-                    <div class="notebook_week_p"> We continued to search for related documents in order to choose the appropriate target sequences of gene
-                        for our project. After the final decision of making eGFP as our interested sequence of gene, we immediately
-                        sent out the primers of sgRNA we designed to GENEWIZ, and we also sent lots of emails to different
-                        labs to see if they can offer us a stable cell strain expressing eGFP protein.</div>
-                </div>
-                <div>
-                    <button id="4week2" class="notebook_information_button2">week2</button>
-                </div>
-                <div id="4notebook_week2" class="notebook_information_word2" style="display:none;">
-                    <div class="notebook_week_p">Meanwhile, we successfully transformed the plasmid pET-NLS-Cas9-6xHis (purchased from Addgene) into E.coli
-                        (BL21), then we tried to express and purify the cas9 protein according to the protocol[1]. But the
-                        results were not so ideal.
-                        <br> 【1】Ha J S, Lee J S, Jeong J, et al. Poly-sgRNA/siRNA ribonucleoprotein nanoparticles for targeted
-                        gene disruption[J]. Journal of Controlled Release, 2017, 250:27-35.</div>
-                </div>
-             </div>
          </div>
          <div id="notebook_May">
              <div class="notebook_Month_head">May</div>
+            <div class="notebook_week_p">Group1 get started at July.</div>
+        </div>
+        <div id="notebook_June">
+            <div class="notebook_Month_head">June</div>
+            <div class="notebook_week_p">Group1 get started at July.</div>
+        </div>
+        <div id="notebook_July">
+            <div class="notebook_Month_head">July</div>
              <div class="notebook_week">
                  <div>
-                     <button id="5week1" class="notebook_information_button1">week1</button>
+                     <button id="7week2" class="notebook_information_button2">week2</button>
                  </div>
-                 <div id="5notebook_week1" class="notebook_information_word1" style="display:none;">
+                 <div id="7notebook_week2" class="notebook_information_word2" style="display:none;">
-                     <div class="notebook_week_p">PCR and Gel Purification (TIANgel Midi Purification Kit) of the template of sgRNA, we tried different
+                     <div class="notebook_week_p">Activate smURFP glycerol.</div>
-                        Tm temperatures.</div>
+                     <img src="https://static.igem.org/mediawiki/2018/8/88/T--TJU_China--g1.1.png">
-                     <img src="./img/group3May1pic1.PNG">
+                    <div class="notebook_week_p">
-                     <img src="./img/group3May1pic2.PNG">
+                        <b>Figure 1.</b> Incubate to activate the smURFP plasmid PCR amplification of smURFP fragments.</div>
+                     <img src="https://static.igem.org/mediawiki/2018/6/67/T--TJU_China--g1.2.png">
+                    <div class="notebook_week_p">
+                        <b>Figure 2.</b> The result of nucleic acid gel electrophoresis of smURFP after PCR. Lane M, Marker.
+                        Lane1-8，smURFP.
+                        <br>Gel Extraction purification of the PCR product.
+                        <br>Find the arsenic ion plasmid inside the box and transform the plasmid into E.coli DH5α.</div>
                  </div>
                  <div>
-                     <button id="5week2" class="notebook_information_button2">week2</button>
+                     <button id="7week3" class="notebook_information_button3">week3</button>
                  </div>
-                 <div id="5notebook_week2" class="notebook_information_word2" style="display:none;">
+                 <div id="7notebook_week3" class="notebook_information_word3" style="display:none;">
-                     <div class="notebook_week_p">After two weeks of hard working, we got our first batch of Cas9 protein.
+                     <div class="notebook_week_p">Transform the plasmid（Bba-J33201） inside the box.
-                         <br> At the same time, we tried our first transcription and preparation of sgRNA using T7 High Efficiency
+                        <br>Amplification of PCR fragments.
-                         Transcription Kit and EasyPure RNA Purification Kit (TransGene Biotech) but failed. We supposed that
+                         <br>PCR amplification of arsenic ion loop.</div>
-                         the template might be polluted by RNase during the process.</div>
+                    <img src="https://static.igem.org/mediawiki/2018/2/2b/T--TJU_China--g1.3.png">
+                    <div class="notebook_week_p">
+                         <b>Figure 3.</b> The result of nucleic acid gel electrophoresis of Bba-J33201 after PCR. Lane M, Marker.
+                        Lane 1-6，BBa-J33201.</div>
+                    <div class="notebook_week_p">PCR amplification of ArsR promoter and ArsR protein fragment.
+                         <br>Transform plasmid pKM586 into E.coli BL21.
+                        <br>Activate and extract pKM586 plasmid.</div>
                  </div>
                  <div>
-                     <button id="5week3" class="notebook_information_button3">week3</button>
+                     <button id="7week4" class="notebook_information_button4">week4</button>
                  </div>
-                 <div id="5notebook_week3" class="notebook_information_word3" style="display:none;">
+                 <div id="7notebook_week4" class="notebook_information_word4" style="display:none;">
-                     <div class="notebook_week_p">We searched for information and knowledge of experiments dealing with RNA and then retried the PCR and
+                     <div class="notebook_week_p">Activate smURFP glycerol.</div>
-                        Gel Purification of the template according strictly to the RNA principles. However, we failed again.
+                     <img src="https://static.igem.org/mediawiki/2018/7/74/T--TJU_China--g1.4.png">
-                        <br> On the other hand, we managed to get plasmid encoding AcGFP by using TIANprep Mini Plasmid Kit (TIANGEN).</div>
+                    <div class="notebook_week_p">
-                     <img src="./img/group3May3pic1.png">
+                        <b>Figure 4.</b> The result of nucleic acid gel electrophoresis after overlapping of ArsR Promoter and
-                </div>
+                         smURFP. Lane M, Marker. Lane 1-10, ArsR Promoter＋smURFP</div>
-                <div>
-                    <button id="5week4" class="notebook_information_button4">week4</button>
-                </div>
-                <div id="5notebook_week4" class="notebook_information_word4" style="display:none;">
-                    <div class="notebook_week_p">We confirmed the best Tm temperature of PCR was 67.2℃ after several preliminary experiments. And this
-                         time, there were lines shown on the RNA gel, but they were not clear. And the RNA marker (TAKARA)
-                        didn’t appear exactly as the instruction. Then we moved forward to the In vitro digestion of DNA
-                        but failed. Since that the result of the SDS-PAGE of Cas9 protein showed no problem, we considered
-                        that the sgRNA might degraded.</div>
-                    <img src="./img/group3May4pic1.png">
-                    <img src="./img/group3May4pic2.png">
-                    <div class="notebook_week_p">Line1，plasmid；2，cleavage result</div>
                  </div>
              </div>
-        </div>
-        <div id="notebook_June">
-            <div class="notebook_Month_head">June</div>
-            <div class="notebook_week">
-                <div style="text-align: left;font-size: 20px;text-indent: 2em;">Preparation for the final-term exams. </div>
-            </div>
          </div>
-        <div id="notebook_July">
-            <div class="notebook_Month_head">July</div>
-            <div class="notebook_week">
-                <div style="text-align: left;font-size: 20px;text-indent: 0;">week1-3
-                    <br> Most members joined a summer camp as a part of school lessons.
-                    <br> week4
-                    <br> In order to reduce the influence of RNase on the subsequent experiment, the phenol-chloroform method
-                    was used to remove RNase. But it turned out that quantity of DNA was not sufficient enough to be extracted.
-                    We tried for several times but the results of the nucleic acid gel electrophoresis showed that we got
-                    nothing after the purification.</div>
-            </div>
-        </div>
          <div id="notebook_August">
              <div class="notebook_Month_head">August</div>
@@ Line 526: / Line 465: @@
                  </div>
                  <div id="8notebook_week1" class="notebook_information_word1" style="display:none;">
+                     <div class="notebook_week_p">Double digestion of pKM586 plasmid.</div>
+                    <img src="https://static.igem.org/mediawiki/2018/7/74/T--TJU_China--g1.5.png">
+                    <div class="notebook_week_p">
+                        <b>Figure 5.</b> Double digestion of pKM586 with AatII and BamHI. Lane M, Marker. Lane 1，pKM586; Lane
+-3, plasmid pKM586 after double enzyme digestion
+                        <br>Overlap ArsR + Arsr Promoter,but failed.
+                        <br>Overlap ArsR Promoter + smURFP, failed.
+                        <br>Enzyme digestion of pwj66.</div>
                  </div>
                  <div>
                      <button id="8week2" class="notebook_information_button2">week2</button>
                  </div>
                  <div id="8notebook_week2" class="notebook_information_word2" style="display:none;">
+                     <div class="notebook_week_p">Enzyme digestion of pwj66.
+                        <br>Connect pwj66+ TARGETDNA.
+                        <br>Double digestion of pKM586.
+                        <br>Overlap ArsR + Arsr Promoter.
+                        <br>Overlap ArsR Promoter + smURFP.
+                        <br>PCR of ParsR promoter ArsR protein fragment.</div>
+                    <img src="https://static.igem.org/mediawiki/2018/1/13/T--TJU_China--g1.6.png">
+                    <div class="notebook_week_p">
+                        <b>Figure 6.</b>LB media of pKM586 after transformed</div>
                  </div>
                  <div>
                      <button id="8week3" class="notebook_information_button3">week3</button>
                  </div>
                  <div id="8notebook_week3" class="notebook_information_word3" style="display:none;">
+                     <div class="notebook_week_p">Enzyme digestion of pwj66.
+                        <br>Connect pwj66+ spacer.
+                        <br>Double digestion pkm586.
+                        <br>Overlap ArsR + Arsr Promoter.
+                        <br>Overlap ArsR Promoter + smURFP.</div>
+                    <img src="https://static.igem.org/mediawiki/2018/6/64/T--TJU_China--g1.7.png">
+                    <div class="notebook_week_p">
+                        <b>Figure 7.</b>The result of nucleic acid gel electrophoresis after overlapping of ArsR Promoter and
+                        smURFP. Lane M, Marker. Lane 1-7, ArsR Promoter＋smURFP. PCR of ParsR promoter ArsR protein fragment.</div>
                  </div>
                  <div>
@@ Line 544: / Line 512: @@
                  </div>
                  <div id="8notebook_week4" class="notebook_information_word4" style="display:none;">
+                     <div class="notebook_week_p">Anneal two J23104 oligo chains.
+                        <br>PCR amplification of Bba-J23104 fragments. .
+                        <br>Overlap J23104 + ArsR protein fragment.
+                        <br>Overlap smURFP + ArsR promoter.</div>
+                    <img src="https://static.igem.org/mediawiki/2018/9/92/T--TJU_China--g1.8.png">
+                    <div class="notebook_week_p">
+                        <b>Figure 8.</b> The result of nucleic acid gel electrophoresis after overlapping of ArsR Promoter and
+                        smURFP. Lane M, Marker. Lane 1, smURFP. Lane 2-4, ArsR Promoter＋smURFP.</div>
+                    <div class="notebook_week_p">Overlapping the two overlapped fragments.
+                        <br>Gel Extraction purification.
+                        <br>Double enzyme digestion of the entire arsenic loop.
+                        <br>Double digestion of pKM586.</div>
+                    <img src="https://static.igem.org/mediawiki/2018/4/47/T--TJU_China--g1.9.png">
+                    <div class="notebook_week_p">
+                        <b>Figure 9.</b>Double digestion of pKM586 with AatII and BamHI. Lane M, Marker. Lane 1,Plasmid pKM586.
+                        Lane 2, Plasmid pKM586 after double enzyme digestion
+                        <br>Connection the two fragments after enzyme digestion
+                        <br>Transform the product into E.coli DH5α</div>
                  </div>
@@ Line 556: / Line 541: @@
                  </div>
                  <div id="9notebook_week1" class="notebook_information_word1" style="display:none;">
+                     <div class="notebook_week_p">We did a full fragment overlap of the arsenic loop and the result failed. Double digestion of pKM586
+                        vector, plasmid extraction results and double enzyme digestion results are not ideal</div>
+                    <img src="https://static.igem.org/mediawiki/2018/3/3e/T--TJU_China--g1.10.png">
+                    <div class="notebook_week_p">
+                        <b>Figure 10.</b>Double digestion of pKM586 with AatII and BamHI. Lane M, Marker. Lane 1, pKM586; Lane
+-3, plasmid pKM586 after double enzyme digestion</div>
                  </div>
                  <div>
@@ Line 562: / Line 552: @@
                  </div>
                  <div id="9notebook_week2" class="notebook_information_word2" style="display:none;">
+                    <div class="notebook_week_p">We modified the arsenic loop full-segment overlap system and the PCR program, and the results were successful.</div>
+                    <img src="https://static.igem.org/mediawiki/2018/7/79/T--TJU_China--g1.11.png">
+                    <div class="notebook_week_p">
+                        <b>Figure 11.</b>The result of nucleic acid gel electrophoresis after overlapping the whole arsenic
+                        loop. Lane M, Marker. Lane1-7 the whole arsenic loop.</div>
+                    <div class="notebook_week_p">Reconstruction of pKM586 original plasmid, the quality of plasmid extraction is not high</div>
                  </div>
                  <div>
@@ Line 568: / Line 563: @@
                  </div>
                  <div id="9notebook_week3" class="notebook_information_word3" style="display:none;">
+                     <div class="notebook_week_p">Try pKM586 step-by-step double enzyme digestion pre-experiment, resulting in significant improvement
+                        in cutting efficiency. The arsenic loop complete fragment double digestion and pKM586 double digestion
+                        product gel recovery, as well as ligation transformation.</div>
+                    <img src="https://static.igem.org/mediawiki/2018/8/83/T--TJU_China--g1.12.png">
+                    <div class="notebook_week_p">
+                        <b>Figure 12.</b>the arsenic loop after transformed into DH5α</div>
                  </div>
                  <div>
@@ Line 574: / Line 574: @@
                  </div>
                  <div id="9notebook_week4" class="notebook_information_word4" style="display:none;">
+                     <div class="notebook_week_p">The plasmid was extracted and verified by double enzyme digestion. The result was successful.</div>
+                    <img src="https://static.igem.org/mediawiki/2018/f/f0/T--TJU_China--g1.13.png">
+                    <div class="notebook_week_p">
+                        <b>Figure 13.</b>Double digestion to verify the ligation product. Lane M, Marker. Lane 1, Plasmid pKM586.
+                        Lane 2, Plasmid pKM586 single digestion with BamHI. Lane 3, Plasmid pKM586 double digestion with
+                        AatII and BamHI. Lane 4, Plasmid ArS. Lane 5, Plasmid ArS single digestion with BamHI. Lane 6, Plasmid
+                        ArS double gigestion with AatII and BamHI. Lane 7, Plasmid ArS. Lane 8, Plasmid ArS single digestion
+                        with BamHI. Lane 9, Plasmid ArS double digestion with AatII and BamHI.</div>
                  </div>
@@ Line 586: / Line 593: @@
                  </div>
                  <div id="10notebook_week1" class="notebook_information_word1" style="display:none;">
+                     <div class="notebook_week_p">Transform the successfully constructed plasmid into E. coli BL21, pick a single colony, incubate the
+                        tube for the first arsenic ion delivery experiment, but the result shows no fluorescence.</div>
+                    <img src="https://static.igem.org/mediawiki/2018/9/94/T--TJU_China--g1.14.png">
+                    <div class="notebook_week_p">
+                        <b>Figure 14.</b>the arsenic loop after transformed into BL21</div>
                  </div>
                  <div>
@@ Line 592: / Line 603: @@
                  </div>
                  <div id="10notebook_week2" class="notebook_information_word2" style="display:none;">
+                     <div class="notebook_week_p">After the successful construction of the plasmid, we began to try to test whether the transformed E.
-                </div>
+                        coli can express fluorescence after adding arsenic ions. We chose to culture the tube for 6 hours
-                <div>
+                        and then add different concentrations of arsenic ions for detection. For the second time, we failed
-                    <button id="10week3" class="notebook_information_button3">week3</button>
+                        again.
-                </div>
+                        <br>And we continue to try to change the condition to make it express fluorescence.</div>
-                <div id="10notebook_week3" class="notebook_information_word3" style="display:none;">
-                </div>
-                <div>
-                    <button id="10week4" class="notebook_information_button4">week4</button>
-                </div>
-                <div id="10notebook_week4" class="notebook_information_word4" style="display:none;">
                  </div>
@@ Line 658: / Line 661: @@
              }
-            notebook_display('3week1', '3notebook_week1');
-            notebook_display('3week2', '3notebook_week2');
-            notebook_display('3week3', '3notebook_week3');
-            notebook_display('3week4', '3notebook_week4');
-            notebook_display('4week1', '4notebook_week1');
-            notebook_display('4week2', '4notebook_week2');
-            notebook_display('5week1', '5notebook_week1');
-            notebook_display('5week2', '5notebook_week2');
-            notebook_display('5week3', '5notebook_week3');
-            notebook_display('5week4', '5notebook_week4');
-            notebook_display('7week1', '7notebook_week1');
              notebook_display('7week2', '7notebook_week2');
              notebook_display('7week3', '7notebook_week3');
@@ Line 700: / Line 690: @@
      </script>
 </body>
+<!--
+                    <div class="notebook_week_p"></div>
+                    <img src="">
+                    <div class="notebook_week_p"><b>Figure .</b></div>
+-->
 </html>

Latest revision as of 12:11, 17 October 2018

<!DOCTYPE >

Home
Project
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Model
HP
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- Public Engagement
Team

Mar.

Apr.

May

Jun.

Jul.

Aug.

Sep.

Oct.

class="notebook_week_p"

March

Group1 get started at July.

April

Group1 get started at July.

May

Group1 get started at July.

June

Group1 get started at July.

July

Activate smURFP glycerol.

Figure 1. Incubate to activate the smURFP plasmid PCR amplification of smURFP fragments.

Figure 2. The result of nucleic acid gel electrophoresis of smURFP after PCR. Lane M, Marker. Lane1-8，smURFP.
Gel Extraction purification of the PCR product.
Find the arsenic ion plasmid inside the box and transform the plasmid into E.coli DH5α.

Transform the plasmid（Bba-J33201） inside the box.
Amplification of PCR fragments.
PCR amplification of arsenic ion loop.

Figure 3. The result of nucleic acid gel electrophoresis of Bba-J33201 after PCR. Lane M, Marker. Lane 1-6，BBa-J33201.

PCR amplification of ArsR promoter and ArsR protein fragment.
Transform plasmid pKM586 into E.coli BL21.
Activate and extract pKM586 plasmid.

Activate smURFP glycerol.

Figure 4. The result of nucleic acid gel electrophoresis after overlapping of ArsR Promoter and smURFP. Lane M, Marker. Lane 1-10, ArsR Promoter＋smURFP

August

Double digestion of pKM586 plasmid.

Figure 5. Double digestion of pKM586 with AatII and BamHI. Lane M, Marker. Lane 1，pKM586; Lane 2-3, plasmid pKM586 after double enzyme digestion
Overlap ArsR + Arsr Promoter,but failed.
Overlap ArsR Promoter + smURFP, failed.
Enzyme digestion of pwj66.

Enzyme digestion of pwj66.
Connect pwj66+ TARGETDNA.
Double digestion of pKM586.
Overlap ArsR + Arsr Promoter.
Overlap ArsR Promoter + smURFP.
PCR of ParsR promoter ArsR protein fragment.

Figure 6.LB media of pKM586 after transformed

Enzyme digestion of pwj66.
Connect pwj66+ spacer.
Double digestion pkm586.
Overlap ArsR + Arsr Promoter.
Overlap ArsR Promoter + smURFP.

Figure 7.The result of nucleic acid gel electrophoresis after overlapping of ArsR Promoter and smURFP. Lane M, Marker. Lane 1-7, ArsR Promoter＋smURFP. PCR of ParsR promoter ArsR protein fragment.

Anneal two J23104 oligo chains.
PCR amplification of Bba-J23104 fragments. .
Overlap J23104 + ArsR protein fragment.
Overlap smURFP + ArsR promoter.

Figure 8. The result of nucleic acid gel electrophoresis after overlapping of ArsR Promoter and smURFP. Lane M, Marker. Lane 1, smURFP. Lane 2-4, ArsR Promoter＋smURFP.

Overlapping the two overlapped fragments.
Gel Extraction purification.
Double enzyme digestion of the entire arsenic loop.
Double digestion of pKM586.

Figure 9.Double digestion of pKM586 with AatII and BamHI. Lane M, Marker. Lane 1,Plasmid pKM586. Lane 2, Plasmid pKM586 after double enzyme digestion
Connection the two fragments after enzyme digestion
Transform the product into E.coli DH5α

September

We did a full fragment overlap of the arsenic loop and the result failed. Double digestion of pKM586 vector, plasmid extraction results and double enzyme digestion results are not ideal

Figure 10.Double digestion of pKM586 with AatII and BamHI. Lane M, Marker. Lane 1, pKM586; Lane 2-3, plasmid pKM586 after double enzyme digestion

We modified the arsenic loop full-segment overlap system and the PCR program, and the results were successful.

Figure 11.The result of nucleic acid gel electrophoresis after overlapping the whole arsenic loop. Lane M, Marker. Lane1-7 the whole arsenic loop.

Reconstruction of pKM586 original plasmid, the quality of plasmid extraction is not high

Try pKM586 step-by-step double enzyme digestion pre-experiment, resulting in significant improvement in cutting efficiency. The arsenic loop complete fragment double digestion and pKM586 double digestion product gel recovery, as well as ligation transformation.

Figure 12.the arsenic loop after transformed into DH5α

The plasmid was extracted and verified by double enzyme digestion. The result was successful.

Figure 13.Double digestion to verify the ligation product. Lane M, Marker. Lane 1, Plasmid pKM586. Lane 2, Plasmid pKM586 single digestion with BamHI. Lane 3, Plasmid pKM586 double digestion with AatII and BamHI. Lane 4, Plasmid ArS. Lane 5, Plasmid ArS single digestion with BamHI. Lane 6, Plasmid ArS double gigestion with AatII and BamHI. Lane 7, Plasmid ArS. Lane 8, Plasmid ArS single digestion with BamHI. Lane 9, Plasmid ArS double digestion with AatII and BamHI.

October

Transform the successfully constructed plasmid into E. coli BL21, pick a single colony, incubate the tube for the first arsenic ion delivery experiment, but the result shows no fluorescence.

Figure 14.the arsenic loop after transformed into BL21

After the successful construction of the plasmid, we began to try to test whether the transformed E. coli can express fluorescence after adding arsenic ions. We chose to culture the tube for 6 hours and then add different concentrations of arsenic ions for detection. For the second time, we failed again.
And we continue to try to change the condition to make it express fluorescence.