Team:PKU Beijing/Notebook/AND Gate 1/Input/LacI TetR 4

From 2009.igem.org

(Difference between revisions)

Latest revision as of 18:38, 21 October 2009

Notebook

Notes By Person (PDF)

Notebook > AND Gate 1 > Input > Molecular cloning: Pcat-2M-lacI/tetR-term-lacP/tetP+GFP

Molecular cloning: Pcat-2M-lacI/tetR-term-lacP/tetP+GFP

Parts: K228817/18+E0840=K228819/20

Resource:
Pcat-2M-lacI/tetR-term-lacP/tetP (K228817/18): myself, colonies, renamed as L1, L2, L3, T1, T2 and T3.
GFP (E0840): from Lin Min, vector (has already digested by EcoR1 & Xba1)

2009.8.5

Plasmid mini prep:
L1, L2, L3

Double digest:
L1, L2 and L3:

EcoR1	1uL
Spe1	1uL
plasmid	10uL
Buffer	2uL
water	6uL

37 ℃ 4 hour

Gel electrophoresis:
Products of double digest of L1, L2 and L3,
marker: 100bp 250bp 500bp 750bp 1kb 2kb 3kb 5kb
loading buffer and DNA dye: 6×
voltage and time: 60V 5min; 120V 60min
lane1: Marker
lane2~4: L1~3;

The insert is about 1.4kb.

DNA Gel purification:
L1, L2 and L3

2009.8.6

DNA ligation:

System	10uL
Insert	6uL
vector	2uL
water	3uL
buffer	1uL
T4 DNA ligase	1uL

16℃ 4 hour
Insert: L1, L2;
Vertor: GFP

Transformation:
Products of ligation, competent cells 50uL each,
Smear to LB plate with Amp

Double digest:
T1, T2 and T3:

EcoR1	1uL
Spe1	1uL
plasmid	10uL
Buffer	2uL
water	6uL

37 ℃ 4 hour

Gel electrophoresis:
Products of double digest of T1, T2 and T3,
marker: 100bp 250bp 500bp 750bp 1kb 2kb 3kb 5kb
loading buffer and DNA dye: 6×
voltage and time: 60V 5min; 120V 15min

Lane 1, 2, 4: T1~3
Lane 3: Marker

DNA Gel purification:
T1, T2 and T3

2009.8.7

Every plate (L1,L2 +GFP) is very well: more than 100 clones
And many colonies are become green under the blue light, which means that the expression of LacI can not fully repressed the promoter lacP.

The second picture is for comparison with no GFP colonies.

PCR: (colony PCR)

Master mix	5ul
primer (standard primer)	0.5uL each
water	4uL
template	6 colonies of L+GFP

Gel electrophoresis:
Products of PCR
marker: 100bp 250bp 500bp 750bp 1kb 2kb 3kb 5kb
loading buffer and DNA dye: 6×
voltage and time: 60V 5min; 120V 15min

Lane 1: Marker;
Lane2~7: L1~6;
The correct insert is about 2.4kb, and we found that L1, L2, L3, L4, and L6 are all correct.

DNA ligation:

System	10uL
Insert	6uL
vector	2uL
water	3uL
buffer	1uL
T4 DNA ligase	1uL

16℃ 4 hour
Insert: T1, T2;
Vertor: GFP

2009.8.8

Transformation:
Products of ligation (T1+GFP, T2+GFP), competent cells 50uL each,
Smear to LB plate with Amp

2009.8.9

Every plate (T1,T2 +GFP) is very well: more than 100 clones
And many colonies are become green under the blue light, which means that the expression of tetR can not fully repressed the promoter tetP.

The second picture is for comparison with no GFP colonies.

2009.8.10

Plasmid mini prep:
T1+GFP, T2+GFP, T3+GFP;

Digest: (T1-G, T2-G)
Double:

EcoR1	1uL
Pst1	1uL
plasmid	4uL
Buffer	2uL
water	12uL

Single:

EcoR1	1uL
plasmid	4uL
Buffer	2uL
water	12uL

37 ℃ 4 hour

Gel electrophoresis: (to confirm the T1-G, T2-G)
Products of digest
marker: 100bp 250bp 500bp 750bp 1kb 2kb 3kb 5kb
loading buffer and DNA dye: 6×
voltage and time: 60V 5min; 120V 15min

Lane 1 & 5: plasmid, T1-G, T2-G
Lane 2 & 6: single digest T1-G, T2-G
Lane 3 & 7: double digest T1-G, T2-G
Lane 4: Marker

The insert is about 1.8kb, and the vector is about 2.1kb. It is very hard to separate them, yet from the gel, we know that the T1-G and T2-G are correct.

Result & Discussion

I successfully constructed the two clones: Pcat-2M-lacI/tetR-term-lacP/tetP-GFP (K228819/20). However, I disappointed to find that these clones are not work very well, because the GFP express significantly even on the plate (without induce)!!! That means the expression of lacI and tetR are not enough to repress the lacP and tetP. It is possible that the LVA tail of lacI and tetR make they degrade very soon. (for more information of LVA refer to parts C0012 and C0040). And other possibility is that the constitutive promoter Pcat is not strong enough.

^Top

@@ Line 2: / Line 2: @@
 {{PKU_Beijing/Sidebar_Notebook}}
 {{PKU_Beijing/Header2}}
+[[Team:PKU_Beijing/Notebook|Notebook]] > [[Team:PKU_Beijing/Notebook/AND_Gate_1|AND Gate 1]] > [[Team:PKU_Beijing/Notebook/AND_Gate_1/Input|Input]] > [[Team:PKU_Beijing/Notebook/AND_Gate_1/Input/LacI_TetR_4|Molecular cloning: Pcat-2M-lacI/tetR-term-lacP/tetP+GFP]]
 ==='''Molecular cloning: Pcat-2M-lacI/tetR-term-lacP/tetP+GFP'''===
 Parts: K228817/18+E0840=K228819/20
-==='''Resource'''===
+'''Resource:'''<br>
 Pcat-2M-lacI/tetR-term-lacP/tetP (K228817/18): myself, colonies, renamed as L1, L2, L3, T1, T2 and T3. <br>
 GFP (E0840): from Lin Min, vector (has already digested by EcoR1 & Xba1)
@@ Line 99: / Line 99: @@
 Every plate (L1,L2 +GFP) is very well: more than 100 clones <br>
 And many colonies are become green under the blue light, which means that the expression of LacI can not fully repressed the promoter lacP. <br>
-[[Image:PKU_20090807_Shuke_Wu_1.JPG|400px]]<br>
+[[Image:PKU_WSK0908051.png|400px]]<br>
-[[Image:PKU_20090807_Shuke_Wu_2.JPG|400px]]<br>
+[[Image:PKU_WSK0908052.png|400px]]<br>
 The second picture is for comparison with no GFP colonies.
@@ Line 112: / Line 112: @@
 |water||4uL
 |-
-|template||
+|template||6 colonies of L+GFP
 |}
-colonies of L+GFP
 '''Gel electrophoresis:'''<br>
@@ Line 142: / Line 141: @@
 ℃ 4 hour<br>
 Insert: T1, T2;<br>
 Vertor: GFP
 ==='''2009.8.8'''===
@@ Line 154: / Line 153: @@
 Every plate (T1,T2 +GFP) is very well: more than 100 clones <br>
 And many colonies are become green under the blue light, which means that the expression of tetR can not fully repressed the promoter tetP. <br>
-[[Image:PKU_20090809_Shuke_Wu_1.JPG|400px]]
+[[Image:PKU_WSK0908053.png|400px]]
-[[Image:PKU_20090809_Shuke_Wu_2.JPG|400px]]
+[[Image:PKU_WSK0908054.png|400px]]
 The second picture is for comparison with no GFP colonies.
 ==='''2009.8.10'''===