From 2013.igem.org

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Revision as of 02:59, 28 September 2013

导航栏

Biobrick Transformation (6.24-6.30)

2013/9/26 20:16:17--Chun Tang

2013/9/26 20:16:39

2013/9/26 20:17:26

Plasmids Construction (7.1-7.28, 8.15-9.16)

2013/9/26 20:36:39--Chun Tang

2013/9/26 20:36:58

2013/9/28 01:03:53

2013/9/26 20:37:51--Chun Tang

2013/9/26 20:38:17

2013/9/28 01:05:10

2013/9/28 01:05:15

2013/9/26 20:40:10--Chun Tang

2013/9/26 20:40:27

2013/9/28 01:06:41

2013/9/28 01:06:51

2013/9/26 20:43:04--Chun Tang

2013/9/26 20:43:20

2013/9/28 01:10:10

2013/9/28 01:10:38

2013/9/26 20:44:56--Chun Tang

2013/9/26 20:45:14

2013/9/28 01:11:54

2013/9/28 01:12:42

2013/9/26 20:47:01--Chun Tang

2013/9/26 20:47:15

2013/9/28 01:16:48

2013/9/28 01:17:27

2013/9/26 20:48:37--Chun Tang

2013/9/26 20:48:50

2013/9/28 01:19:02

Transformation (7.29-9.20)

2013/9/26 20:49:56--Chun Tang

2013/9/26 20:50:04

2013/9/28 01:21:56

2013/9/28 01:22:37

2013/9/26 20:51:34--Chun Tang

2013/9/26 20:51:47

2013/9/28 01:23:53

2013/9/26 20:52:47--Chun Tang

2013/9/26 20:53:01

2013/9/28 01:24:59

2013/9/26 20:55:54--Chun Tang

2013/9/26 20:56:19

SDS-PAGE

2013/9/26 21:48:57--Tang Chun

2013/9/26 21:49:44

2013/9/26 21:50:08--Tang Chun

2013/9/26 21:51:07

2013/9/26 21:53:17--Tang Chun

2013/9/26 21:55:45

2013/9/26 22:02:08--Tang Chun

2013/9/26 22:03:34

2013/9/26 22:04:18--Tang Chun

2013/9/26 22:07:07

2013/9/26 22:07:33--Tang Chun

2013/9/26 22:08:04

2013/9/26 22:07:46

2013/9/26 22:08:31--Tang Chun

2013/9/26 22:08:47

2013/9/26 22:09:10--Tang Chun

2013/9/26 22:09:28

2013/9/26 22:09:40

2013/9/26 22:10:13--Tang Chun

2013/9/26 22:10:54

2013/9/26 22:11:28

2013/9/26 22:12:08--Tang Chun

2013/9/26 22:12:23

2013/9/26 22:12:32

2013/9/26 22:13:05--Tang Chun

2013/9/26 22:13:16

2013/9/28 07:03:20--Chun Tang

2013/9/28 07:03:54

2013/9/28 08:44:02--Chun Tang

2013/9/28 08:44:22

2013/9/28 08:47:11

2013/9/28 08:44:24

2013/9/28 08:44:28

Microfluidic Experiment Record

2013/9/18 10:50:50--Chun Tang

2013/9/25 20:38:47

2013/9/18 10:51:01--Chun Tang

2013/9/25 20:42:38

2013/9/18 10:51:41--Chun Tang

2013/9/25 20:45:15

2013/9/18 10:52:00--Chun Tang

2013/9/25 20:46:04

2013/9/18 10:52:31--Chun Tang

2013/9/25 20:47:42

2013/9/18 10:53:02--Chun Tang

2013/9/25 20:50:35

2013/9/18 10:53:24--Chun Tang

2013/9/25 20:52:02

2013/9/25 21:10:34--Chun Tang

2013/9/25 21:11:06

2013/9/25 21:12:48--Chun Tang

2013/9/25 21:13:01

2013/9/28 07:14:25

2013/9/28 07:14:27

2013/9/28 07:14:28

2013/9/25 21:15:00--Chun Tang

2013/9/25 21:15:47

2013/9/25 21:16:23

2013/9/25 21:16:51

RFU (9.24-9.27)

2013/9/27 21:59:07--Chun Tang

2013/9/27 21:59:17

2013/9/28 03:11:44

2013/9/28 03:30:57

2013/9/28 03:31:38

2013/9/28 03:34:06

@@ Line 172: / Line 172: @@
 Data analysis:
    The band marked in red disappeared is pSB1C3-gfp-luxI/BL21.The LuxR, GFP and AiiA  are the same of size (marked in yellow). However the band of AiiA was not clear. Many target proteins were misfolded. Therefore the culture condition should be optimized.
-</textarea>				<br>			</td>		</tr>	</tbody></table>	</td>		</tr>		</tbody></table>				<div class="M1_exp_stepInfo" title="3. (8.12)" id="sb7s5" >			<button class="M1_exp_step_name_button" ><input value="3. (8.12)" class="M1_exp_step_name"></button>			<span class="M1_exp_step_time">2013/9/26 22:07:33--Tang Chun</span>		</div>		<table class="M1_exp_stepBoard">		<tbody><tr class="M1_exp_stepItem">			<td class="M1_exp_item_time" id="ib7s5i0">2013/9/26 22:08:04</td>			<td class="M1_exp_item_content"><textarea id="i7s5i0" class="C0" rows="1" disabled="" style="background-color: white;"> Characterization of expression of E.coli transformed into triple plasmids and testing if our target proteins expressed by our constructed gene circuits were concentrated in precipitation or supernatant  (8.12)</textarea></td>		</tr>				<tr class="M1_exp_stepItem">			<td class="M1_exp_item_time" id="ib7s5i1">2013/9/26 22:07:46</td>			<td class="M1_exp_item_content">	<table id="i7s5i1" class="C1">		<tbody><tr>			<td class="C1_td">				<img id="i7s5i10" width="" src="http://trysomething-block.stor.sinaapp.com/t14i9s5i03.png"><br>				<form id="i7s5i14" target="M7" action="img.php" method="post" enctype="multipart/form-data"></form>				<input name="img" type="file" id="i7s5i12" form="i7s5i14" class="C1_button1" required="required" disabled="" style="background-color: white;">				<input name="pname" type="hidden" value="t14" form="i7s5i14">				<input name="id" type="hidden" value="i7s5i1" form="i7s5i14">				<input name="oldgraph" type="hidden" id="i7s5i15" form="i7s5i14" value="t14i9s5i03.png">				<input id="i7s5i16" type="submit" value="submit" form="i7s5i14" class="C1_button2" disabled="" style="background-color: white;">				<div id="i7s5i13" class="M1_exp_img"></div>				</td>			<td class="C1_td_text">				<textarea id="i7s5i11" class="C1_text" disabled="" style="background-color: white;">Description :
+</textarea>				<br>			</td>		</tr>	</tbody></table>	</td>		</tr>		</tbody></table>				<div class="M1_exp_stepInfo" title="3. (8.12)" id="sb7s5" >			<button class="M1_exp_step_name_button" ><input value="3. (8.12)" class="M1_exp_step_name"></button>			<span class="M1_exp_step_time">2013/9/26 22:07:33--Tang Chun</span>		</div>		<table class="M1_exp_stepBoard">		<tbody><tr class="M1_exp_stepItem">			<td class="M1_exp_item_time" id="ib7s5i0">2013/9/26 22:08:04</td>			<td class="M1_exp_item_content"><textarea id="i7s5i0" class="C0" rows="1" disabled="" style="background-color: white;"> Characterization of expression of E.coli transformed into triple plasmids and testing if our target proteins expressed by our constructed gene circuits were concentrated in precipitation or supernatant  (8.12)</textarea></td>		</tr>				<tr class="M1_exp_stepItem">			<td class="M1_exp_item_time" id="ib7s5i1">2013/9/26 22:07:46</td>			<td class="M1_exp_item_content">	<table id="i7s5i1" class="C1">		<tbody><tr>			<td class="C1_td">				<img id="i7s5i10" width="600" src="http://trysomething-block.stor.sinaapp.com/t14i9s5i03.png"><br>				<form id="i7s5i14" target="M7" action="img.php" method="post" enctype="multipart/form-data"></form>				<input name="img" type="file" id="i7s5i12" form="i7s5i14" class="C1_button1" required="required" disabled="" style="background-color: white;">				<input name="pname" type="hidden" value="t14" form="i7s5i14">				<input name="id" type="hidden" value="i7s5i1" form="i7s5i14">				<input name="oldgraph" type="hidden" id="i7s5i15" form="i7s5i14" value="t14i9s5i03.png">				<input id="i7s5i16" type="submit" value="submit" form="i7s5i14" class="C1_button2" disabled="" style="background-color: white;">				<div id="i7s5i13" class="M1_exp_img"></div>				</td>			<td class="C1_td_text">				<textarea id="i7s5i11" class="C1_text" disabled="" style="background-color: white;">Description :
   We had transformed triple plasmids into one E.coli and the DNA gel picture indicated it was ligated successfully. So now we were very eager to know if our circuits could work well in E.coli.
 Furthermore, we wanted to know that if our target proteins expressed by our constructed gene circuits, in other words, pSB1C3-gfp-luxI and pSB13T5-aiiA were aggregated in precipitation or supernatant. So we run SDS-PAGE using BL21(blank control), three cells transformed into different single plasmids(aiiA, ndh and gfp), one cell transformed into double plasmids(aiiA and gfp) and our E.coli transformed into triple plasmids in three forms respectively, whole cell, precipitation and supernatant.

Team:XMU-China/wetlab journal