Team:PKU Beijing/Notebook/AND Gate 1/Input/LuxR

From 2009.igem.org

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Revision as of 20:17, 26 September 2009

Notebook

Notes By Person (PDF)

2009.6.9 (with LinMin)

11:10
The e-coli cultivated yesterday did not grow
The material of the former culture medium went bad. Need renewing.

11:29
Practise minipreping the plasmids

12:58
Practise digesting the plasmids

2009.6.13 (with LinMin)

15:00
make the culture medium, repair computer, search Parts:

Parts Code	Location	Location	Plasmid	Containment	Description
BBa_E0240	Kit Plate 1	12M	Psb1A2	GFP rbs-repoter	Medium rbs
BBa_E0840	Kit Plate 1	12O	Psb1A2	GFP rbs-repoter	Strong rbs
BBa_R0080	Kit Plate 1	12E	Psb1A2	Ara Promoter
BBa_C0062	Kit Plate 1	4O	Psb1A2	Lux R gene	No LVA
BBa_C0051	Kit Plate 1	4E	Psb1A2	C1 repressor	With LVA
BBa_C0179	Kit Plate 2	8M	Psb1A2	lasR activator	No LVA
BBa_C0079	Kit Plate 1	14J	Psb1A2	lasR activator	With LVA
BBa_R0079	Kit Plate 1	12A	Psb1A2	LasR/Pal promoter

16:55
dissolve the plasmids, prepare to transform
add 15uL ddH2O

21:20
Transform plasmids above

2009.6.14

13:10
repair the computer

14:08
make the LB culture medium

21:00
search the rbs parts:

Parts Code	Location	Location	Plasmid	Containment	Description
BBa_B0030	Kit Plate 1	1H	Psb1A2	RBS	strong rbs
BBa_B0031	Kit Plate 1	2G	Psb1A2	RBS	Weak
BBa_B0032	Kit Plate 1	2I	Psb1A2	RBS	Medium
BBa_B0033	Kit Plate 1	2K	Psb1A2	RBS	Weaker
BBa_B0034	Kit Plate 1	2M	Psb1A2	RBS
BBa_J44001	Kit Plate 1	1J	Psb1A2	RBS
BBa_J61100	Kit Plate 1	5J	Psb1A2	RBS
BBa_J61101	Kit Plate 1	5L	Psb1A2	RBS
BBa_J61107	Kit Plate 1	5N	Psb1A2	RBS
BBa_J61117	Kit Plate 1	11L	Psb1A2	RBS
BBa_J61127	Kit Plate 1	11N	Psb1A2	RBS

2009.6.15

21:07
Transform plasmids above (2009/06/14)

21:48
begin to transforming

2009.6.16

11:50
cultivation is finished The results come out well

2009.6.19 (with Wu Shuke)

21:11
Select clones from the plate

2009.6.20

23:00
transform 1-12L

2009.6.21

9:50
Transform the 2008 Parts’ RBS

11:54
finish transformaion

2009.6.22

9:14
Transformation is failed, redoing

22:30
re-transformation

2009.6.23

1:00
start the cultivation

13:00
the second transformation is failed

2009.6.24

14:59
Prepare to make TOP10 Sensitive Cells

16:00
Begin to make LB, etc

17:30
Search for LuxR s

BBa_R0062	09 Kit1	6O	pSB1A2	Promoter
BBa_R0065	09 Kit1	8C	pSB1A2	Promoter
BBa_R1062	09 Kit1	8G	pSB1A2	Promoter

23:38
Cultivate TOP10 Cells

2009.6.25

21:44
Transform the rbs:
1003-12C; 1003-12G; 1004-2A; 1004-2C; 1004-3G

2009.6.26

22:36
Cultivate:
1004-1C; 1004-3C; 1004-4C; 1004-2G

23:07
Prepare to make 1-2I Sensitive Cells

23:15
Cultivate 1-2I Cells

2009.6.27

15:58
Miniprep the plasmids:
1004-1C; 1004-3C; 1004-4C; 1004-2G Failed

16:09
Make the 1-2I Sensitive Cells Failed

2009.6.28

20:18
Miniprep the plasmids:
1004-1C; 1004-2C; 1004-3C; 1004-4C; 1004-2G

21:37
Make the 1-2I Sensitive Cells

2009.6.29

17:40
Check the 1-2I Sensitive Cells Huge Success! The protocol is added to ftp

20:09
Prepare to make DH5A Sensitive Cells

2009.7.3

18:00
Search Parts:

BBa_J37032

1003

6C

pSB1A2

GFP controlled by LuxRP

22:44
Cultivate 1003-6C Failed. The plasmid is bad.

2009.7.3-2009.7.10

Searching for papers on T3P and T3Pol, which is basic for the second logic gate. Contact with the writer to get the plasmids.
During this time, a review on T7 and T3 systems is summarized, which has been sent to ftp.

2009.7.6

19:51
Miniprep the plasmids:

2-4O	LuxR+RBS	Amp+
1-18P	P(cat)	Kan+

21:08
Digest the plasmids of 2-4O and 1-18P:

Digestion System Insert	20μL
Plasmids	5μL
Pst1	1μL
Xbal1	1ul
Buffer 1*M	2μL
dd H2O	11μL

Digestion System Vector	20μL
Plasmids	5μL
Pst1	1μL
Spe1	1ul
Buffer 1*H	2μL
dd H2O	11μL

2009.7.7

0:34
The digestion reaction begins

7:46
add 0.4uL cip and 2ul buffer to the vector system

8:07
the result come out as follows:

18:03
Recycle the fragments.

19:40
Ligate the 2-4O insert to 1-18P vector:

Insert	3μL
Vector	1μL
Buffer 10*	1μL
Ligase	1uL
dd H2O	4μL

19:48
Ligation start

23:44
Begin the transformation of the ligation plasmid

2009.7.8

16:57
Cultivate the 2-4O->1-18P

2009.7.9

9:06
Miniprep the 2-4O->1-18P plasmids

11:52
Digest the plasmids of 2-4O->1-18P and 1-23L:

Digestion System Insert	20μL
Plasmids	5μL
EcoR1	1μL
Spe1	1ul
Buffer 1*H	2μL
dd H2O	11μL

Digestion System Vector	20μL
Plasmids	5μL
EcoR1	1μL
Xbal1	1ul
Buffer 1*M	2μL
dd H2O	11μL

12:13
Reaction Start

17:32
Stop the digestion

20:08
Prepare to Ligation

20:17
Ligation start

^Top

@@ Line 1: / Line 1: @@
-{{PKU_Beijing/New_Header}}
+{{PKU_Beijing/Header}}
-{{PKU_Beijing/New_Section_Notebook}}
+{{PKU_Beijing/Sidebar_Notebook}}
-{{PKU_Beijing/New_Nav}}
+{{PKU_Beijing/Header2}}
-{{PKU_Beijing/New_Sidebar_Notebook}}
+==='''2009.6.9 (with LinMin)'''===
-=='''2009.6.9 (with LinMin)'''==
 '''11:10'''<br>
@@ Line 15: / Line 14: @@
 Practise digesting the plasmids
-=='''2009.6.13 (with LinMin)'''==
+==='''2009.6.13 (with LinMin)'''===
 '''15:00'''<br>
 make the culture medium, repair computer, search Parts:<br>
-{|style="background:#DDDDDD" cellpadding=5
+{|cellpadding=5
 |Parts Code||Location||Location||Plasmid||Containment||Description
 |-
@@ Line 46: / Line 45: @@
 Transform plasmids above
-=='''2009.6.14'''==
+==='''2009.6.14'''===
 '''13:10'''<br>
@@ Line 56: / Line 55: @@
 '''21:00'''<br>
 search the rbs parts:<br>
-{|style="background:#DDDDDD" cellpadding=5
+{|cellpadding=5
 |Parts Code||Location||Location||Plasmid||Containment||Description
 |-
@@ Line 82: / Line 81: @@
 |}
-=='''2009.6.15'''==
+==='''2009.6.15'''===
 '''21:07'''<br>
@@ Line 90: / Line 89: @@
 begin to transforming
-=='''2009.6.16'''==
+==='''2009.6.16'''===
 '''11:50'''<br>
 cultivation is finished The results come out well
-=='''2009.6.19 (with Wu Shuke)'''==
+==='''2009.6.19 (with Wu Shuke)'''===
 '''21:11'''<br>
 Select clones from the plate
-=='''2009.6.20'''==
+==='''2009.6.20'''===
 '''23:00'''<br>
 transform 1-12L
-=='''2009.6.21'''==
+==='''2009.6.21'''===
 '''9:50'''<br>
@@ Line 113: / Line 112: @@
 finish transformaion
-=='''2009.6.22'''==
+==='''2009.6.22'''===
 '''9:14'''<br>
@@ Line 121: / Line 120: @@
 re-transformation
-=='''2009.6.23'''==
+==='''2009.6.23'''===
 '''1:00'''<br>
@@ Line 129: / Line 128: @@
 the second transformation is failed
-=='''2009.6.24'''==
+==='''2009.6.24'''===
 '''14:59'''<br>
@@ Line 139: / Line 138: @@
 '''17:30'''<br>
 Search for LuxR s<br>
-{|style="background:#DDDDDD" cellpadding=5
+{|cellpadding=5
 |BBa_R0062||09 Kit1||6O||pSB1A2||Promoter
 |-
@@ Line 150: / Line 149: @@
 Cultivate TOP10 Cells
-=='''2009.6.25'''==
+==='''2009.6.25'''===
 '''21:44'''<br>
@@ Line 156: / Line 155: @@
 -12C; 1003-12G; 1004-2A; 1004-2C; 1004-3G
-=='''2009.6.26'''==
+==='''2009.6.26'''===
 '''22:36'''<br>
@@ Line 168: / Line 167: @@
 Cultivate 1-2I Cells
-=='''2009.6.27'''==
+==='''2009.6.27'''===
 '''15:58'''<br>
@@ Line 177: / Line 176: @@
 Make the 1-2I Sensitive Cells Failed
-=='''2009.6.28'''==
+==='''2009.6.28'''===
 '''20:18'''<br>
@@ Line 186: / Line 185: @@
 Make the 1-2I Sensitive Cells
-=='''2009.6.29'''==
+==='''2009.6.29'''===
 '''17:40'''<br>
@@ Line 194: / Line 193: @@
 Prepare to make DH5A Sensitive Cells
-=='''2009.7.3'''==
+==='''2009.7.3'''===
 '''18:00'''<br>
 Search Parts:<br>
-{|style="background:#DDDDDD" cellpadding=5
+{|cellpadding=5
 |BBa_J37032||1003||6C||pSB1A2||GFP controlled by LuxRP
 |}
@@ Line 205: / Line 204: @@
 Cultivate 1003-6C Failed. The plasmid is bad.
-=='''2009.7.3-2009.7.10'''==
+==='''2009.7.3-2009.7.10'''===
 Searching for papers on T3P and T3Pol, which is basic for the second logic gate. Contact with the writer to get the plasmids.<br>
 During this time, a review on T7 and T3 systems is summarized, which has been sent to ftp.
-=='''2009.7.6'''==
+==='''2009.7.6'''===
 '''19:51'''<br>
 Miniprep the plasmids:<br>
-{|style="background:#DDDDDD" cellpadding=5
+{|cellpadding=5
 |2-4O||LuxR+RBS||Amp+
 |-
@@ Line 222: / Line 221: @@
 '''21:08'''<br>
 Digest the plasmids of 2-4O and 1-18P:<br>
-{|style="background:#DDDDDD" cellpadding=5
+{|cellpadding=5
 |Digestion System Insert||20μL
 |-
@@ Line 236: / Line 235: @@
 |}
-{|style="background:#DDDDDD" cellpadding=5
+{|cellpadding=5
 |Digestion System Vector||20μL
 |-
@@ Line 250: / Line 249: @@
 |}
-=='''2009.7.7'''==
+==='''2009.7.7'''===
 '''0:34'''<br>
@@ Line 267: / Line 266: @@
 '''19:40'''<br>
 Ligate the 2-4O insert to 1-18P vector:<br>
-{|style="background:#DDDDDD" cellpadding=5
+{|cellpadding=5
 |Insert||3μL
 |-
@@ Line 285: / Line 284: @@
 Begin the transformation of the ligation plasmid
-=='''2009.7.8'''==
+==='''2009.7.8'''===
 '''16:57'''<br>
 Cultivate the 2-4O->1-18P
-=='''2009.7.9'''==
+==='''2009.7.9'''===
 '''9:06'''<br>
@@ Line 297: / Line 296: @@
 '''11:52'''<br>
 Digest the plasmids of 2-4O->1-18P and 1-23L:<br>
-{|style="background:#DDDDDD" cellpadding=5
+{|cellpadding=5
 |Digestion System Insert||20μL
 |-
@@ Line 310: / Line 309: @@
 |dd H2O||11μL
 |}
-{|style="background:#DDDDDD" cellpadding=5
+{|cellpadding=5
 |Digestion System Vector||20μL
 |-
@@ Line 336: / Line 335: @@
 '''20:17'''<br>
 Ligation start
+{{PKU_Beijing/Foot}}
+__NOTOC__
-{{PKU_Beijing/New_End}}