Team:Chiba/Notebook 2

From 2010.igem.org

Revision as of 15:57, 26 October 2010 by Lhae23 (Talk | contribs)




 




2010-09-21

PCR 

Because it didn’t come out vector PCR(gel electrophoresis), 
we operated re-experiment to change template and template amounts.

Using template
 1. Biobrick 2010 1-3A(pSB1C3)
 2. Biobrick 2010 pSB1C3
 3. Biobrick 2010 2-9A(pSB1A3)
 4. control

Using primer
 Fwd : pSB1C3 FASTR-F
 Rev : pSB1C3 FASTR-R

 -------------------------
 template       5uL
 primer Fwd     5uL
 primer Rev     5uL
 dNTP           5uL
 10xbuffer      5uL
 NFW            24uL
 VentP          1uL
 -------------------------
                50uL

PCR(TAKARA)
 94°C – 5min
 94°C – 15sec    --
 51°C – 30sec      │- 25 cycles
 72°C – 1min     -- 
 72°C – 10min

Vector PCR 

Using template
 1. Biobrick 2010 1-3A(pSB1C3)
 2. Biobrick 2010 pSB1C3
 3. Biobrick 2010 2-9A(pSB1A3)
 4. control

 -------------------------
 template      3uL
 primer Fwd    5uL
 primer Rev    5uL
 dNTP          5uL
 10xbuffer     5uL
 NFW           26uL
 VentP         1uL
 -------------------------
               50uL

Using primer
 Fwd : pSB1C3 FASTR-F
 Rev : pSB1C3 FASTR-R

PCR Condition
 94°C – 5min
 94°C – 30sec      --
 51°C – 30sec        │-25 cycles
 72°C – 2min       --
 72°C – 10min

2010-09-22

Biobrick 2010 2-9A(pSB1A3) -> Gel extraction Gel Electrophoresis 

Biobrick 2010 2-9A(pSB1A3), Biobrick 2010 1-3A(pSB1C3), Biobrick 2010 pSB1C3, Biobrick 2010 2-9A(pSB1A3)
As a result, it didn’t come out band of 1-3A and pSB1C3. 
We concluded re-experiment from liquid incubation to mini-prep. Must check gel electrophoresis band after mini-prep.

FASTR Cloning (Plasmid1) 

Vector (about 2kbp)
-pSB1A3 (conservative solution 100ng/uL)

Insert (about 1kbp)
 1. Pet-LuxR-PT7/cI(OR2)-GFP (conservative solution 25ng/uL)
 2. Pet-LuxR-PT7/cI(OR1)-GFP (conservative solution 25ng/uL)
 3. Prom-LuxR-PT7/cI(OR2)-GFP (conservative solution 25ng/uL)
 4. Prom-LuxR-PT7/cI(OR1)-GFP (conservative solution 25ng/uL)

master mix
---------------------------------------------------------------------
Vector(50ng)         	0.5	2
Insert(75ng)	          3     -
Tango buffer	        0.5	2
T4 Ligase buffer	0.5	2
ATP	                  1	4
LguI	                0.5	2
Ligase           	0.5	2
DpnI	                0.5	2
NFW	                  3	12
-----------------------------------------------------------------------
Total           	10uL	28uL
Room temperature 2h

Transformation 

Using cell strain : BL21(DE3) 50uL
Using plasmid
 L1 : Pet-LuxR-PT7/cI(OR2)-GFP   5uL
 L2 : Pet-LuxR-PT7/cI(OR1)-GFP   5uL
 L3 : Prom-LuxR-PT7/cI(OR2)-GFP 5uL
 L4 : Prom-LuxR-PT7/cI(OR1)-GFP 5uL

After transformation 

We added IPTG(0μM / 100μM / 200μM) to each cell strain. It became 12 plates.
※A Reason of using DE3 cell strain
DE3 cell strain has T7 RNA Polymerase gene in genome, and under IPTG derivation T7RNAP is expressed.
Plasmid1 has  T7/cI hybrid promoter. 
So if this promoter is accelerated by T7RNAP, GFP is expressed and shines green. 
In other words, we used DE3 cell strain to check T7 accelerating function of PT7/cI.

2010-09-23

From yesterday, we did mini-prep liquid incubated sample 1-3A and pSB1C3. And then it is eluted by 50uL Elution Solution. ↓ Gel Electrophoresis(1uL) 

L1 : Pet-LuxR-PT7/cI(OR2)-GFP   5uL
L2 : Pet-LuxR-PT7/cI(OR1)-GFP   5uL
L3 : Prom-LuxR-PT7/cI(OR2)-GFP 5uL
L4 : Prom-LuxR-PT7/cI(OR1)-GFP 5uL
Remaining of above sample is transformed and incubated.
cell strain : XL10G(50uL/tube)
plasmid : L1~L4(total 4)

FASTR Cloning (Plasmid1) 

Vector (about 2kbp)
 -pSB1A3 (conservative solution 100ng/uL)
Insert (about 1kbp)
 1. Pet-LuxR-PT7/cI(OR2)-GFP (conservative solution 25ng/uL)
 2. Pet-LuxR-PT7/cI(OR1)-GFP (conservative solution 25ng/uL)
 3. Prom-LuxR-PT7/cI(OR2)-GFP (conservative solution 25ng/uL)
 4. Prom-LuxR-PT7/cI(OR1)-GFP (conservative solution 25ng/uL)
master mix
---------------------------------------------------------------------
Vector(50ng)         	0.5	2
Insert(75ng)	          3	-
Tango buffer	        0.5	2
T4 Ligase buffer	0.5	2
ATP	                  1	4
LguI	                0.5	2
Ligase	                0.5	2
DpnI	                0.5	2
NFW	                  3	12
-----------------------------------------------------------------------
Total	               10uL	28uL
Room temperature 2h

After ligation plasmid is transformed and incubated in LB broth. cell strain : BL21(DE3), XL10G(each 50uL/tube) plasmid : L1~L4

2010-09-24

At 23th September Remaining of above sample is transformed and incubated. cell strain : XL10G(50uL/tube) plasmid : L1~L4(total 4) We picked 4 colonies of each plate out from L1~L4 plates and operated colony PCR. Moreover, we did liquid incubation each colony.
Insert Check Colony PCR(Plasmid 1) 

master mix
--------------------------------------------------------------------------
Template(picked colonies)
Primer VF	         2uL	40uL
Primer VR	         2uL	40uL
10x Buffer	         2uL	40uL
dNTP	                 2uL	40uL
NFW	                10uL	200uL
Taq DNA Polymerase	0.5uL	5uL
--------------------------------------------------------------------------
Total	                20uL	400uL
↓
PCR
 94°C – 5min
 94°C – 30sec      --
 51°C – 30sec        │-20 cycles
 72°C – 1min       --
 72°C – 10min
↓
Gel Electrophoresis

2010-09-25

Mini-prep and gel electrophoresis of liquid culture medium at 24th September. 

Gel Electrophoresis picture
↓
Transformation to BL21(DE3) 
↓
Incubation in LB broth, IPTG(0, 10, 100 μM) 
↓37°C
About total sample, it is shown GFP ON/OFF switching on eyes.
↓
For the purpose of measuring fluorescence level, we did liquid incubation from each plate.
IPTG(0, 10, 100 μM) x 6 samples = 18 test tubes
↓37°C
∙ measuring fluorescence level(liquid incubation)
∙ pelletization of cell

Digestion and ligation of BBa-J01011(Ptet-cI) and pSB3C5 

(Digestion)
           Insert(J01011)	   Vector(pSB3C5)
DNA	       10uL	                10uL
NFW	       32.5uL	               32.5uL
NEB Buffer 2	5uL	                5uL
BSA	       0.5uL	               0.5uL
EcoRI	        1uL	               1uL
PstI	        1uL	               1uL
------------------------------------------------------------------------
total                      50uL                50uL
↓37°C 15min incubator
↓65°C 20min (sterilization dryer)
※After digestion, we did gel electrophoresis

(Ligation)
  13uL NFW
   2uL Insert(digested)
   2uL Vector(digested)                  total 20uL in 0.2mL PCR tube
   2uL 10x T4 DNA Ligase Buffer
   1uL T4 DNA Ligase

↓10min at room temperature
↓20min at 65°C (sterilization dryer)

(Transformation)
Transformation XL10G 50uL to 10uL of ligation product
↓37°C
Insert check of living colonies(colony PCR)     /     liquid incubation
↓total 7 colonies                               ↓37°C
Insert Check Colony PCR(Plasmid 1)	                    ↓We did mini-prep only No.4 sample checked insert.
--------------------------------------------
Template(picked colonies)                                  ↓
Primer VF	2uL	                                    Gel electrophoresis
Primer VR	2uL	
10x Buffer	2uL
dNTP	2uL
NFW	11.5uL
Taq DNA Polymerase	0.5uL
--------------------------------------------------------
Total	20uL
↓
PCR
 94°C 5min
 94°C 30sec   --
 51°C 30sec     │-30 cycle
 72°C 1min    --
 72°C 10min
↓
Gel electrophoresis
Retrieved from "http://2010.igem.org/Team:Chiba/Notebook_2"