Team:Tsinghua-A/Parts

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Parts List

Name	Type	Description	Length
BBa_K574000	Composite	pLux + TetR	903
BBa_K574001	Composite	TetR regulated by 3OC6HSL	1890
BBa_K574002	Composite	pluxR + CFP	941
BBa_K574003	Device	3OC6HSL -> TetR && reporter	2839
BBa_K574004	Composite	3OC12HSL regulated by TetR	797
BBa_K574005	Composite	3OC12HSL and YFP regulated by pBad	1712
BBa_K574006	Device	3OC12HSL regulated by pTet and pBad	2517
BBa_K574007	Composite	lasR + TT	918
BBa_K574008	Composite	a constitutive LasR producer	982
BBa_K574009	Composite	3OC12HSL -> PoPS Receiver	1147

Parts Data

Description:

We assembled BBa_E0840 under the pLas promoter BBa_R0079 that was contained into K574009. We kept pSB1A2 as the scaffold vector.

Methods:
1. Ligate BBa_E0840 downstream of BBa_K574009, which acts as a reporter.
2. Culture the positive colony at 37°C, 220 rpm for 12 hours, as well as the DH5alpha.
3. Dilute 1:25 the former in 12 falcon tubes (4 ml cultures), each 3 tubes as a group. The later is also diluted in 3 tubes as the negative control.
4. After culturing for another 2 hours, as their OD600 reach 0.2, induce with 3OC12HSL 0, 1e-6 M, 1e-5 M and 1e-4 M respectively.
5. Take samples after 1 hour, 4 hours, 8 hours and 24 hours, that is, centrifugalizate 0.5 mL of each culture and suspend them by 1 mL of PBS (phosphate-buffered saline).
6. Measure the fluorescence of the samples with the flow cytometer.

Results:

From the chart, we can see that cells were hardly induced in the control group, and with the concentration of inducer growing, the intensity of GFP increased by groups. The most efficient concentration of inducer was around 10^-6M, and to most groups, the intensity of GFP reached its maxium after 4 hours.

@@ Line 277: / Line 277: @@
 <P><Br></P>
-<P ALIGN=LEFT STYLE="line-height: 0.58cm; widows: 2; orphans: 2"><FONT COLOR="#000000"><FONT FACE="Arial Unicode MS, sans-serif"><FONT SIZE=3 STYLE="font-size: 11pt"><SPAN LANG="en-US">Description:
+<P ALIGN=LEFT STYLE="line-height: 0.58cm; widows: 2; orphans: 2"><FONT COLOR="#000000"><FONT FACE="Arial Unicode MS, sans-serif"><FONT SIZE=4><SPAN LANG="en-US">Description:
 </SPAN></FONT></FONT></FONT>
 </P>
-<P ALIGN=LEFT STYLE="line-height: 0.58cm; widows: 2; orphans: 2"><FONT COLOR="#000000"><FONT FACE="Arial Unicode MS, sans-serif"><FONT SIZE=3 STYLE="font-size: 11pt"><SPAN LANG="en-US">We
+<P ALIGN=LEFT STYLE="line-height: 0.58cm; widows: 2; orphans: 2"><FONT COLOR="#000000"><FONT FACE="Arial Unicode MS, sans-serif"><FONT SIZE=3 STYLE="font-size: 11pt"><SPAN LANG="en-US"><FONT SIZE=4>We
 assembled <A HREF="http://partsregistry.org/wiki/index.php/Part:BBa_E0840">BBa_E0840</A>
 under the pLas promoter <A HREF="http://partsregistry.org/wiki/index.php/Part:BBa_R0079">BBa_R0079</A>
 that was contained into K574009. We kept pSB1A2 as the scaffold
-vector.<BR></SPAN></FONT></FONT></FONT><BR><BR>
+vector.<BR></FONT></SPAN></FONT></FONT></FONT><BR><BR>
 </P>
-<P ALIGN=LEFT STYLE="line-height: 0.58cm; widows: 2; orphans: 2"><FONT COLOR="#000000"><FONT FACE="Arial Unicode MS, sans-serif"><FONT SIZE=3 STYLE="font-size: 11pt"><SPAN LANG="en-US">Methods:<BR>1.
+<P ALIGN=LEFT STYLE="line-height: 0.58cm; widows: 2; orphans: 2"><FONT COLOR="#000000"><FONT FACE="Arial Unicode MS, sans-serif"><FONT SIZE=3 STYLE="font-size: 11pt"><SPAN LANG="en-US"><FONT SIZE=4>Methods:<BR>1.
 Ligate <A HREF="http://partsregistry.org/wiki/index.php/Part:BBa_E0840">BBa_E0840</A>
 downstream of <A HREF="http://partsregistry.org/wiki/index.php/Part:BBa_K574009">BBa_K574009</A>,
@@ Line 298: / Line 298: @@
 centrifugalizate 0.5 mL of each culture and suspend them by 1 mL of
 PBS (phosphate-buffered saline).<BR>6. Measure the fluorescence of
-the samples with the flow cytometer.</SPAN></FONT></FONT></FONT></P>
+the samples with the flow cytometer.</FONT></SPAN></FONT></FONT></FONT></P>
-<P STYLE="line-height: 0.58cm; widows: 2; orphans: 2"><FONT FACE="Times New Roman, serif"><SPAN LANG="en-US"><FONT COLOR="#000000"><FONT FACE="Arial, Helvetica, sans-serif"><FONT SIZE=3 STYLE="font-size: 11pt"><SPAN STYLE="font-style: normal"><SPAN STYLE="font-weight: normal"><BR><BR><BR>Results:</SPAN></SPAN></FONT></FONT></FONT></SPAN></FONT></P>
+<P STYLE="line-height: 0.58cm; widows: 2; orphans: 2"><FONT FACE="Times New Roman, serif"><FONT SIZE=4><SPAN LANG="en-US"><FONT COLOR="#000000"><FONT FACE="Arial, Helvetica, sans-serif"><SPAN STYLE="font-style: normal"><SPAN STYLE="font-weight: normal"><BR><BR><BR>Results:</SPAN></SPAN></FONT></FONT></SPAN></FONT></FONT></P>
-<P STYLE="line-height: 0.58cm; widows: 2; orphans: 2"><FONT FACE="Times New Roman, serif"><SPAN LANG="en-US"><FONT COLOR="#000000"><FONT FACE="Arial, Helvetica, sans-serif"><FONT SIZE=3 STYLE="font-size: 11pt"><SPAN STYLE="font-style: normal"><SPAN STYLE="font-weight: normal">From
+<P STYLE="line-height: 0.58cm; widows: 2; orphans: 2"><FONT FACE="Times New Roman, serif"><FONT SIZE=4><SPAN LANG="en-US"><FONT COLOR="#000000"><FONT FACE="Arial, Helvetica, sans-serif"><SPAN STYLE="font-style: normal"><SPAN STYLE="font-weight: normal">From
 the chart, we can see that cells were hardly induced in the control
 group, and with the concentration of inducer growing, the intensity
 of GFP increased by groups. The most efficient concentration of
 inducer was around 10^-6M, and to most groups, the intensity of GFP
-reached its maxium after 4 hours.</SPAN></SPAN></FONT></FONT></FONT></SPAN></FONT></P>
+reached its maxium after 4 hours.</SPAN></SPAN></FONT></FONT></SPAN></FONT></FONT></P>