Team:NCTU Formosa/Notebook/Calendar

A group discussion. We discussed about the principle and some details of the project. We also designed the first step of the experimence and the protocols.

8/17

Today we devided our team into 5 subgroups and started the experimence. In each subgroup, we have to contribute a part of the whole project.

8/18

We transformed the bricks we need from the well.

8/21

we check DNA by agarose gel, SDS-PAGE.

8/22~23

To transfer E. coli to new LB broth, and incubate for 16hr, then Extract plasmid.

8/28

we design a logo of team NCTU_FORMOSA

September

9/1

The experiment is not so smoothly, we sink into infinite loop in the same experiments.

9/2

To digest the front part (8/23) and the behind part (8/26) of the biobrick, ligate, transform and run gel to check that if digestion is OK or not, then spread on the plate, and incubate for 20hr.

9/7

We use another enzyme to digest to double check if the plasmid is right or not

9/10

Today we have a meeting that we discuss how to solve the problems.

9/14~25

The plasmid's sequences are wrong and we repeat the digestion, ligation, and transform again.

9/16

BBa_K188343 is sequenced today.

9/28

Degenerated PCR, using BBa_K145279 as template

9/29

Degenerated PCR

October

10/2

Degenerated PCR. Restriction enzyme map.

10/7

Gel purification. To ligate gel purification products

10/11

to make restriction enzyme map. To select 14 plasmids

10/12

We had a team work to work on the wiki web. Flow cytometer.

10/14

Submitted the parts to be sequenced.

10/18

Updated the web of notebook and the project. We also had a group discussion about our results and the data.

10/21

To discuss our final result.

@@ Line 319: / Line 319: @@
 		<div class="select_sub">
 			<ul class="sub">
-				<li><a href="https://2009.igem.org/Team:NCTU_Formosa/WetLab/Mainworks" target="_self">Mainworks</a></li>
+				<li><a href="https://2009.igem.org/Team:NCTU_Formosa/WetLab/Labworks" target="_self">Lab works</a></li>
-				<li><a href="https://2009.igem.org/Team:NCTU_Formosa/WetLab/Groupworks" target="_self">Groupworks</a></li>
                  <li><a href="https://2009.igem.org/Team:NCTU_Formosa/WetLab/Timer" target="_self">Timer</a></li>
                  <li><a href="https://2009.igem.org/Team:NCTU_Formosa/WetLab/Counter" target="_self">Counter</a></li>
@@ Line 402: / Line 401: @@
 				<div class="events"><p>It is the beginning today!!!!!!!! </p></div>
 				<div class="date"><p><a name="0717" id="7/17"></a> 7/17 </p></div>
-				<div class="events">
+				<div class="events"><p>Lesson：Parts, Devices and Biobricks.&nbsp; In this lesson we learned about the principle of the construction of biobricks.</p></div>
-				  <p>Lesson：Parts, Devices and Biobricks.&nbsp; In this lesson we learned about the principle of the construction of biobricks.</p>
+				<div class="date"><p><a name="0720" id="7/20"></a> 7/20~22 </p></div>
-			  </div>
+				<div class="events"><p>To present 2008 IGEM projects.</p></div>
+				<div class="date"><p><a name="0727" id="7/27"></a> 7/27~29 </p></div>
+				<div class="events"><p>To present everyone’s primary idea.</p></div>
 			</div>
 		</div>
@@ Line 416: / Line 417: @@
              	<div class="date"><p><a name="0803" id="8/03"></a> 8/03 </p></div>
 				<div class="events"><p> A group duscussion of each one's personal idea.  </p></div>
+            	<div class="date"><p><a name="0805" id="8/05"></a> 8/05 </p></div>
+				<div class="events"><p> To collate everyone’s advantages.</p></div>
                  <div class="date"><p><a name="0807" id="8/07"></a> 8/07 </p></div>
 				<div class="events"><p> A group discussion.  &nbsp; We decided what kind of projects we're going to construct. </p></div>
@@ Line 428: / Line 431: @@
 				<div class="date"><p><a name="0821" id="8/21"></a> 8/21 </p></div>
 				<div class="events"><p>we check DNA by agarose gel, SDS-PAGE.</p></div>
+				<div class="date"><p><a name="0822" id="8/22"></a> 8/22~23 </p></div>
+				<div class="events"><p>To transfer E. coli to new LB broth, and incubate for 16hr, then Extract plasmid.</p></div>
 				<div class="date">
 				  <p><a name="0828" id="8/28"></a> 8/28 </p>
@@ Line 449: / Line 454: @@
 				<div class="date"><p><a name="0910" id="9/10"></a> 9/10 </p></div>
 				<div class="events"><p>Today we have a meeting that we discuss how to solve the problems.</p></div>
+				<div class="date"><p><a name="0914" id="9/14"></a> 9/14~25 </p></div>
+				<div class="events"><p> The plasmid's sequences are wrong and we repeat the digestion, ligation, and transform again.</p></div>
 				<div class="date"><p><a name="0916" id="9/16"></a> 9/16 </p></div>
 				<div class="events"><p>BBa_K188343 is sequenced today.</p></div>
 				<div class="date"><p><a name="0928" id="9/28"></a> 9/28 </p></div>
 				<div class="events"><p>Degenerated PCR, using BBa_K145279 as template</p></div>
+				<div class="date"><p><a name="0929" id="9/29"></a> 9/29 </p></div>
+				<div class="events"><p>Degenerated PCR</p></div>
 			</div>
 		</div>
@@ Line 466: / Line 475: @@
              <div class="date"><p><a name="1007" id="10/7"></a> 10/7 </p></div>
 			<div class="events"><p>Gel purification. To ligate gel purification products</p></div>
+            <div class="date"><p><a name="1011" id="10/11"></a> 10/11 </p></div>
+			<div class="events"><p>to make restriction enzyme map. To select 14 plasmids</p></div>
              <div class="date"><p><a name="1012" id="10/12"></a> 10/12 </p></div>
 			<div class="events"><p> We had a team work to work on the wiki web. Flow cytometer.  </p></div>