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2010.08.17

PCR of primer&Digestion&Ligation

Descr	Win length	Fail length
1: marker 100bp
2: -	-	-
3: riboswitch	56 bp	none
4: riboswitch	56 bp	none
5: -	-	-
6: riboswitch	56 bp	none
7: riboswitch	56 bp	none
8: -	-	-
9: riboswitch	56 bp	none
10: riboswitch	56 bp	none
11: Positive Control	1100 bp	none
12: Negative Control		Contamination ~300bp

PCR mixfor 3 tubes(25+25+50)	total 50 μl	temp	time
template	1μl	94oC	120s
forward primer	1μ1	94oC	30s
reverse primer	1μ1	55oC	30s
dNTP	4μ1	72oC	40s
10x buffer	5μl	72oC	300s
ddH2O	39.75μl
pfu	0.5μ1

Plasmid extraction
Digestion
PCR purification(centrifuge)
Nanodrop
Ligation
Transform 20:00

2010.08.18

PCR mix
Run gel(2%argarose 100v)

Descr	Win length	Fail length
1: marker 100bp
2: th-ribo gene + vector	292bp	-
3: th-ribo gene + vector	292bp	-
4: -	-	-
5: Positive Control	1100 bp	none
6: Negative Control		Contamination ~3000bp

Total:(*2)	50μl
template	2μl
VF+VR	2μl
dNTP	2μl
Buffer	5μl
ddH2O	39.75μl
Enzyme tag	0.25μl

(negative contaminated and appeared three different bands)

3-in-1 11:30
Run PCR 12:00
put Liquid culture&plate at 17:00

2010.08.19

Because there are some mistake resulting from gel running, we decided to digest again.
- Digest 10:30
- Transformation 12:45

At the same time, we continued plasmid extraction of the result one of yesterday.
- plasmid extraction 10:30
- Digest 11:30
- run gel 13:00
- Ligation 14:00
- Transformation 14:30

2010.08.20

We decide to re-3-in-1 again.
PCR mix 10:30
3 in 1 11:30
Run PCR 01:00~02:30
Run gel 15:00(100v 20 mins)

Descr	Win length	Fail length
1: marker 100bp
2: ribo+vector	292bp
3: ribo+vector	292bp
4: -	-	-
5: Positive Control	1100 bp	none
6: Negative Control

Total:(*2)	50μl
template	2μl
VF+VR	2μl
dNTP	2μl
Buffer	5μl
ddH2O	39.75μl
Enzyme tag	0.25μl

Cut gel 16:30
Plasmid extraction 16:30

2010.08.23

the upper experiment are failed,so we restart the experiment.
- Run gel 11:00
- After nanodrop, we found that the concentration is too low(only 3.0), so we re-PCR-of-primer again.

PCR of primer 16:00
Transformation(GFP) 17:15

2010.08.24

Run gel 10:30am(5ul)

File:NYMU riboswitch .8.24.jpg

Descr	Win length	Fail length
1:
2: marker 100bp
3:
4: pcr riboswitch	56bp
5:
6: Positive Control		300bp
7: Negative Control

Total:(*2)	50μl
template	2μl
VF+VR	2μl
dNTP	2μl
Buffer	5μl
ddH2O	39.75μl
Enzyme tag	0.25μl

PCR Purify 10:45(45ul)
Digest 11:15

Total:	30μl
DNA	26μl
Digestion buffer	2μl
Enzyme 1(X)	1μl
Enzyme 2(P)	1μl

Digest purify 13:30
Nanodrop(19.8ng/ul)
Ligation 15:44
- Ligate riboswitch+pSB1A2(1:3) and ligate GFP+pSB1A2(1:2)(we use 2009's GFP+terminater so we have to ligate pSB1A2)

Total:	10μl
DNA of vector	1μl
DNA of insert	3μl
buffer	2μl
ligase	0.5μl
ddH2O	4.5μl

Total:	10μl
DNA of vector	1μl
DNA of insert	2μl
buffer	2μl
ligase	0.5μl
ddH2O	5.5μl

2010.08.25

3-in-1:GFP(1 colony),Riboswitch(2 colony) 17:00pm
Run PCR 17:20pm

2010.08.26

Run gel 10:30am
- Because we thought the result is unsure,we decide to digest to check.

File:NYMU P8290273riboswitch8.26.JPG

Descr	Win length	Fail length
1: GFP
2: (1)riboswitch+pSB1A2	292bp
3: (2)riboswitch+pSB1A2	292bp
4: Positive Control	1100bp
5: Negative Control	Contamination~1000 bp
6: Marker:100bp

Total:(*2)	50μl
template	2μl
VF+VR	2μl
dNTP	2μl
Buffer	5μl
ddH2O	39.25μl
Enzyme tag	0.25μl

Liquid culture 12:00
- the first step when we added MX1 we didn't resuspend,so we readded MX1~MX3.But the DNA may be less.
digest
- [GFP(XP),ribo1(SP,XP>>use 10 ul and 20ul protocal),ribo2(SP,XP>>use 10 ul and use 20ul protocal)]

Total:	10μl
DNA of vector(sp)	1μl
DNA of insert(xp)	3μl
buffer	2μl
ligase	0.5μl
ddH2O	4.5μl

run gel(xp)

File:NYMU P8290274ribo8.26-2.JPG

Descr	Win length	Fail length
1: ribo1	96bp
2:
3: ribo2	96bp
4:
5: Marker:100bp
6: GFP	854bp

Total:(*2)	50μl
template	2μl
VF+VR	2μl
dNTP	2μl
Buffer	5μl
ddH2O	39.75μl
Enzyme tag	0.25μl

purify(ribo-1(sp);ribo-2(sp);GFP(xp))
ligate
transform
liquid culture from the plate(8/24)

2010.08.27

PCR mix 10:30
- GFP+terminator+Riboswitch=1157bp
3 in 1 12:15
Run PCR 12:30~13:30
Run gel 13:45

Liquid culture again(use the plate 8/24) 10:30
- To check the wrong step of liquid culture
Digestion 13:40
Run gel 01:45pm[GFP(XP).Riboswitch-1(XP).Riboswitch-2(XP)]

File:NYMU P829027ribo.8.27.jpg

"

Descr	Win length	Fail length
1:	-	-
2: riboswitch+GFP	1167bp	292bp
3: riboswitch+GFP	1167bp	292bp
4:	-	-
5: Positive Control	1100 bp	none
6:	-	-
7: Negative Control		Contamination ~1000bp
8:	-	-
		n
10:	-	-
11: GFP(XP)	879bp	854bp
12:	-	-
13: ribo-1(xp)	292bp
14:	-	-
15: ribp-2(xp)	292bp

Total:(*2)	50μl
template	2μl
VF+VR	2μl
dNTP	2μl
Buffer	5μl
ddH2O	39.75μl
Enzyme tag	0.25μl

2010.08.28

3-IN-1 (another 3 colony from 08.26 Riboswitch+GFP-Terminator plate) 13:30
- PCR (Use new dNTP & Taq buffer & taq) 14:30
- Run Gel 16:20

Descr	Win length	Fail length
1: riboswitch+GFP	1167bp	292bp
2: riboswitch+GFP	1167bp	292bp
3: riboswitch+GFP	1167bp	292bp
4: positive control	1100bp	-
5: marker100 bp	-	-
6: negative control	-	-

Total:(*2)	50μl	temp	time
template	2μl	94^oC	60s
VF+VR	2μl	94^oC	15s
dNTP	2μl	55^oC	20s
Buffer	5μl	72^oC	100s
ddH2O	39.75μl	72^oC	300s
Enzyme tag	0.25μl

Transformation GFP+vector 17:00
3-IN-1 (2 Colony from the plate transformed on 08/27) 17:20
- PCR 18:25~19:40

2010.08.29

Run Gel (with green marker) at 11:00
- Ribo Vac1 and Ribo Vac2 from PCR on 8/28 at 18:25~19:40

Descr	Win length	Fail length
1: -	-	-
2: -	-	-
3: riboswitch1+vector	292bp	-
4: marker100 bp	-	-
5: riboswitch2+vector	292bp	-
6: positive control	1100bp	-
7: negative control	-	-

Total:(*2)	50μl
template	2μl
VF+VR
dNTP	2μl
Buffer	5μl
ddH2O	39.75μl
Enzyme tag	0.25μl

______________________________________________________________________________________________________________

3-in-1 (3 colonies of GFP+TERMINATOR and 1 of Riboswitch+PSB1A2 vector, both from plates transformed on 8/28)
- PCR 11:00~12:50
- Run Gel 15:30 (result shows no band!! but positive and negative controls are correct)

Descr	Win length	Fail length
1: GFP1	854bp
2: GFP2	854bp
3: GFP3	854bp
4: marker100 bp	-	-
5: riboswitch+vector	292bp	-
6: negative control	-	-
7: positive contril	1100bp	-

Total:(*2)	50μl
template	2μl
VF+VR	2μl
dNTP	2μl
Buffer	5μl
ddH2O	39.75μl
Enzyme tag	0.25μl

transform 16:30
- (1)the Ribo2 from 8.17 (2)the Ribo (check) from 08/19 (3)GFP+terminator from 08/27
  - put into incubator 17:30

2010.08.30

3-in-1: GFP,GFP+riboswitch,ribo-1,ribo-2 12:30pm
Run PCR 13:20
Run gel(2% argarose 100v)

Descr	Win length	Fail length
1: GFP1	854bp	-
2: GFP2	854bp	-
3: GFP3	854bp	-
4: riboswitch1+GFP	1167bp	-
5: riboswitch2+GFP	1167bp	-
6: riboswitch3+GFP	1167bp	-
7: marker100 bp	-	-
8: ribo1+vector	292bp	-
9: ribo1+vector	292bp	-
10: ribo2+vector	292bp	-
11: ribo2+vector	292bp	-
12: positive control	1100bp	-
13: negative control	-	-

Total:(*2)	50μl
template	2μl
VF+VR
dNTP	2μl
Buffer	5μl
ddH2O	39.75μl
Enzyme tag	0.25μl

Finally we Transform 19F(GFP+terminator), E0040 18:50

2010.08.31

3-in-1 (ribo(xp)+pSB1A2,E0040,J04630)11:00
Nanodrop
Ligation

Descr	Win length	Fail length
1: GFP1(J04630)	854bp	-
2: GFP2(J04630)	854bp	-
3: Riboswitch1+vector	292bp	-
4: Riboswitch+2vector	292bp	-
5: marker100 bp	-	-
6: GFP1(E0040)	720bp	-
7: GFP2(E0040)	720bp	-
8: ribo1+vector	292bp	-
9: ribo1+vector	292bp	-
10: ribo2+vector	292bp	-
11: ribo2+vector	292bp	-
12: positive control	1100bp	-
13: negative control	-	-

Total:(*2)	50μl
template	2μl
VF+VR
dNTP	2μl
Buffer	5μl
ddH2O	39.75μl
Enzyme tag	0.25μl

Descr	Win length	Fail length
1: GFP+terminator(19f)	854bp	-
2: GFP(E0040)	720bp	-
3: GFP(E0040)	720bp	-
4: marker 100bp	-	-
5: Positive Control	1100 bp
6: Negative Control

2010.09.01

GFP*3 Plasmid Extraction 10:30
Digestion　12:30 (13:20)
Run gel 15:30

Descr	Win length	Fail length
1: -	-	-
2: -	-	-
3: marker 100bp	-	-
4: -	-	-
5: (GFP)E0040-2	745bp
6: (GFP)E0040-1	745bp
7: (GFP)J04630	856bp

Total:(*2)	50μl
template	2μl
VF+VR	2μl
dNTP	2μl
Buffer	5μl
ddH2O	39.25μl
Enzyme tag	0.25μl

RG1,RG2,RG3,PR1,PR2,PR3 3-in-1 10:00
Colony PCR 11:00~13:00
Run Gel

"

Descr	Win length	Fail length
1: riboswitch+GFP(1-a)	1167bp	292bp
2: riboswitch+GFP(1-b)	1167bp	292bp
3: riboswitch+GFP(2-a)	1167bp	292bp
4: riboswitch+GFP(2-b)	1167bp	292bp
5: riboswitch+GFP(3-a)	1167bp	292bp
6: riboswitch+GFP(3-b)	1167bp	292bp
7: -	-	-
8: marker 100bp	-	-
9: promoter+ribo+GFP	bp	-
10: promoter+ribo+GFP	bp	-
11: promoter+ribo+GFP	bp	-
12: promoter+ribo+GFP	bp	-
13: promoter+ribo+GFP	bp	-
14: promoter+ribo+GFP	bp	-
15: positive control	1100bp	-
16: negative control	-	containment

Total:(*2)	50μl	temp	time
template	2μl	94	60s
VF+VR	2μl	94	15s
dNTP	2μl	55	20s
Buffer	5μl	72	90s
ddH2O	39.75μl	72	300s
Enzyme tag	0.25μl

2010.09.02

Liquid culture plasmid extraction 10:00
Nanodrop
Digestion 12:12
Purification
Nanodrop
Ligation
Transform 17:00

2010.09.03

3-in-1 chose 4 colony
PCR 11.20
run gel

Descr	Win length	Fail length
1: FRV1	1167bp	-
2: FRV2	1167bp	-
3: marker 100bp	-	-
4: FRV3	-	-
5: FRV4	745bp
6: positive control	1100bp
7: negative control		contamination~3000bp

Total:(*2)	50μl
template	2μl
VF+VR	2μl
dNTP	2μl
Buffer	5μl
ddH2O	39.75μl
Enzyme tag	0.25μl

(the marker takes the wrong one,1kb marker is correct)

- ligation failed
ligate again(insert+vector=8.5)
transform 16:40

2010.09.04

PCR 20:35pm (3 colony from 20100903 plate)
run gel(FRV1&2&3&+&-) 100V 35min

Descr	Win length	Fail length
1: FRV1	1167bp	-
2: FRV2	1167bp	-
3: marker 100bp	-	-
4: FRV3	-	-
5: FRV4	745bp
6: positive control	1100bp
7: negative control		contamination~3000bp

Total:(*2)	50μl
template	2μl
VF+VR	2μl
dNTP	2μl
Buffer	5μl
ddH2O	39.75μl
Enzyme tag	0.25μl

discuss

2010.09.05

digest again(because we used XP's protocol for SP)
purification at 14:25
nanodrop at 15:00
- we digest another tube (ribo2-2 SP) 15:50
ligation
transform 17:00

2010.09.06

Colony PCR 11:30
Run gel 14:30(2% argarose 100v 25 mins)

"

Descr	Win length	Fail length
1: riboswitch+GFP	1167bp	292bp
2: riboswitch+GFP	1167bp	292bp
3: riboswitch+GFP	1167bp	292bp
4: riboswitch+GFP	1167bp	292bp
5: riboswitch+GFP	1167bp	292bp
6: riboswitch+GFP	1167bp	292bp
7: marker 100bp	-	-
8: promoter+ribo+GFP	bp	-
9: ribo1+vector	292bp	-
10: ribo1+vector	292bp	-
11: ribo2+vector	292bp	-
12: ribo2+vector	292bp	-
13: ribo3+vector	292bp	-
14: positive control	1100bp	-
15: negative control	-	containment

Total:(*2)	50μl
template	2μl
VF+VR
dNTP	2μl
Buffer	5μl
ddH2O	39.75μl
Enzyme tag	0.25μl

Take out the digest(sp)yesterday 10:30
digest purify
nanodrop(13.2ng/nl)
ligate 11:40~14:30
transform 17:00

2010.09.07

3-in-1 10:30am
Run PCR 10:45am

"

Descr	Win length	Fail length
1: riboswitch+GFP	1167bp	292bp
2: riboswitch+GFP	1167bp	292bp
3: riboswitch+GFP	1167bp	292bp
4: riboswitch+GFP	1167bp	292bp
5: riboswitch+GFP	1167bp	292bp
6: riboswitch+GFP	1167bp	292bp
7: marker 100bp	-	-
8: promoter+ribo+GFP	bp	-
9: ribo1+vector	292bp	-
10: ribo1+vector	292bp	-
11: ribo2+vector	292bp	-
12: ribo2+vector	292bp	-
13: ribo3+vector	292bp	-
14: positive control	1100bp	-
15: negative control	-	containment

Total:(*2)	50μl
template	2μl
VF+VR
dNTP	2μl
Buffer	5μl
ddH2O	39.75μl
Enzyme tag	0.25μl

2010.09.08

plasmid extraction
digestion(FRV1(XP)) 11:10
- nanodrop 14μl
ligation 14:00
Transformation 17:00

2010.09.09

Because we didn't cut gel(Ribo+GFP:XP), we restart again.
Re-Digest

Real PCR

File:NYMU P9070327.JPG

Descr	Win length	Fail length
1: Real PCR :Riboswitch	56 bp	-
2: marker 100bp	-	-
3: positive control	200bp
4: negative control

Total:(*2)	50μl
template	2μl
VF+VR	2μl
dNTP	2μl
Buffer	5μl
ddH2O	39.75μl
Enzyme tag	0.25μl

2010.09.10

real PCR
run gel
cut gel
gel extraction
digest(xp)
nanodrop
ligate
transform

real pcr for 2 tubes

2010.09.11

3in1

two real tubes run gel and cut gel and gel extraction

2010.09.12

run gel(length isn't correct)
(real PCR) digestion 12:00
ligation 15:00
transform 19:40

2010.09.13

colony PCR 13:25 (3 in 1)

nanodrop
ligation 14:00
Colony PCR 15:00

2010.09.22

Real PCR

Total:	49μl	X1.7μl
FP	1μl	1.7μl	Theophylline Riboswitch Forward Primer
RP	1μl	1.7μl	Theophylline Riboswitch Reverse Primer
dNTP	2μl	3.4μl
10XBuff.	5μl	8.5μl
pfu	0.25μl	0.425μl
ddH2O	39.75μl	67.575μl

PCR Protocol
94	60s
94	15s
52	20s
68	30s	35 cycles
68	300s

Digest ribo(xp) overnight
Ligate ribo with vector(xp)
Transform:23:30

2010.09.23

Ligate ribo with vector again
Transform

2010.09.24

3-in-1 (ribo+vector)
colony PCR

Total:	49μl	X1.9μl
VR+VF	2μl	3.8μl
dNTP	2μl	3.8μl
10XBuff.	5μl	9.5μl
tag	0.25μl	0.475μl
ddH2O	39.75μl	75.525μl

PCR Protocol
94	60s
94	15s
55	20s
72	30s	30 cycles
72	300s

Cut gel(ribo&pSB1A2(xp) digested)

2010.09.26

3-in-1(0925 plate)
colony PCR

Total:	49μl	X2.5μl
VR+VF	2μl	5μl
dNTP	2μl	5μl
10XBuff.	5μl	12.5μl
tag	0.25μl	1.25mu;l
ddH2O	39.75μl	99.375μl

PCR Protocol
94	60s
94	15s
55	20s
72	30s	30 cycles
72	300s

2010.09.27

plasmid extraction(RV)
Digest RV 13:30
run gel

There is GFP on vector, so it's wrong.

Digest ribo again overnight

2010.09.28

cut gel(ribo& vector)

Ligate ribo with vector
Transform

According to 0927 gel pic, 30th colony may be correct RV, so we take out second plate and incubate in LB liguid.

plasmid extraction 21:30
Digest RV(SP) overnight

2010.09.29

Ligate RV(sp) with GFP(BBa_J04630 already have terminator)
Transform

2010.09.30

Transform BBa_J04630

2010.10.01

3-in-1
- colony PCR

Total:	49μl	X1.6μl
VR+VF	2μl	3.2μl
dNTP	2μl	3.2μl
10XBuff.	5μl	8μl
tag	0.25μl	0.4mu;l
ddH2O	39.75μl	63.6μl

PCR Protocol
94	60s
94	15s
55	20s
72	70s	30 cycles
72	300s

2010.10.02

BBa_J04630 plasmid extraction
Digest J04630(XP)
cut gel(GFP)

Ligate RV(SP) with GFP(XP)
Transform

2010.10.03

FRV(RV+GFP) 3-in-1

Total:	49μl	X1,9μl
VR+VF	2μl	3.8μl
dNTP	2μl	3.8μl
10XBuff.	5μl	9.5μl
tag	0.25μl	0.475mu;l
ddH2O	39.75μl	75.525μl

PCR Protocol
94	60s
94	15s
55	20s
72	100s	30 cycles
72	300s

2010.10.04

FRV plasmid extraction
Digest FRV (XP)
cut gel & purify(FRV)

Ligate FRV with pLac(from ssrA group)
Transform

pLac plasmid extraction
Digest pLac(SP) overnight

2010.10.05

pLac digest purify(run gel with 3-in-1)
PFRV, GFP, RV 3-in-1

Total: !! 49μl || X2.5μl

VR+VF	2μl	5μl
dNTP	2μl	5μl
10XBuff.	5μl	12.5μl
tag	0.25μl	0.625mu;l
ddH2O	39.75μl	99.375μl

PCR Protocol
94	60s
94	15s
55	20s
72	90s	30 cycles
72	300s

Digest pLac(SP) again overnight

2010.10.06

pLac cut gel

Ligate pLac(SP) with FRV(XP)
Transform 22:40

Digest FRV(XP) overnight

2010.10.07

FRV(XP) cut gel

Ligate FRV with pLac
Transform

2010.10.08

PFRV 3-in-1

Total:	49μl	3.8μl
VR+VF	2μl	μl
dNTP	2μl	3.8μl
10XBuff.	5μl	9.5μl
tag	0.25μl	0.475mu;l
ddH2O	39.75μl	75.525μl

PCR Protocol
94	60s
94	15s
55	20s
72	100s	30 cycles
72	300s

Ligate FRV with pLac
Transform 22:15

2010.10.09

PFRV 3-in-1

Total:	49μl	X3.8μl
VR+VF	2μl	7.6μl
dNTP	2μl	7.6μl
10XBuff.	5μl	17μl
tag	0.25μl	0.95mu;l
ddH2O	39.75μl	151.06μl

PCR Protocol
94	60s
94	15s
55	20s
72	90s	30 cycles
72	300s

colony PCR again

Total:	49μl	X3.8μl
VR+VF	2μl	7.6μl
dNTP	2μl	7.6μl
10XBuff.	5μl	17μl
tag	0.25μl	0.95mu;l
ddH2O	39.75μl	151.06μl

PCR Protocol
94	60s
94	15s
55	20s
72	180s	30 cycles
72	300s

Ligate FRV with pLac again
Transform

2010.10.10

PFRV 3-in-1

Total:	49μl	X3.2μl
VR+VF	2μl	6.4μl
dNTP	2μl	6.4μl
10XBuff.	5μl	15μl
tag	0.25μl	0.8mu;l
ddH2O	39.75μl	127.2μl

PCR Protocol
94	60s
94	15s
55	20s
72	180s	30 cycles
72	300s

length is correct!!!

F colony liquid culture
FRV liquid culture

Digest FRV(XP) again

2010.10.11

FRV&PFRV plasmid extraction
FRV cut gel

Digest PFRV(XP)&FRV&pSB1C3
Ligate PFRV with C3/ FRV with C3/ ribo with C3
Transform

2010.10.12

Ligate PFRV with C3/FRV with C3/ribo with C3 again
Transform 17:25

2010.10.13

PFRC&FRC&RC 3-in-1

Total:	49μl	X1.7μl
VR+VF	2μl	3.4μl
dNTP	2μl	3.4μl
10XBuff.	5μl	8μl
tag	0.25μl	0.425mu;l
ddH2O	39.75μl	67.575μl

PCR Protocol
94	60s
94	15s
55	20s
72	90s	30 cycles
72	300s

Ligate PFRV,FRV,ribo with C3
Transform 00:50

Digest PFRV(XP)&RV(XP) again overnight

2010.10.14

PFRV&RV run gel

Ligate RV,FRV,PFRV with C3 again
Transform

2010.10.15

FRC,RC 3-in-1

Total:	49μl	X2.5μl
VR+VF	2μl	5μl
dNTP	2μl	5μl
10XBuff.	5μl	12.5μl
tag	0.25μl	0.625mu;l
ddH2O	39.75μl	99.375μl

PCR Protocol
94	60s
94	15s
55	20s
72	90s	30 cycles
72	300s

3-in-1 again

Total:	49μl	X2.5μl
VR+VF	2μl	5μl
dNTP	2μl	5μl
10XBuff.	5μl	12.5μl
tag	0.25μl	0.625mu;l
ddH2O	39.75μl	99.375μl

PCR Protocol
94	60s
94	15s
55	20s
72	90s	30 cycles
72	300s

FRC and PFRC are correct, but RC is still incorrect

PFRC&FRC liquid culture

Ligate ribo with C3 again
Transform

2010.10.16

Theophylline solution
- Take 1.8012g Theophylline into 15ml DMSO;concentration is 0.67M
put 15 μl into LB liquid, concentration is 2.5mM;

put 30 μl into LB liquid, concentration is 5mM

Ligate ribo(xp) with C3 again
Transform

2010.10.17

transform second plate of PFRC into agar plate

positive:C3 30μl+theophylline 0.0027g

negative:C3

PFRC&FRC plasmid extraction

2010.10.18

PFRC PCR test

Total:	49μl	X1.3μl
VR+VF	2μl	2.6μl
dNTP	2μl	2.6μl
10XBuff.	5μl	6.5μl
tag	0.25μl	0.325mu;l
ddH2O	39.75μl	51.675μl

PCR Protocol
94	60s
94	15s
55	20s
72	90s	30 cycles
72	300s

Theophylline in DMSO
- add 1 ml DMSO + Theophylline into 4 ml LB

Ligate ribo with C3 again
Transform

Digest ribo(XP)& C3(XP)
ribo & C3 cut gel

2010.10.19

Assay Test

	O.D/2	O.D	add to liquid
PFRC	2.503	5.006	166.5
LB	0	0

- Because Theophylline entry into E. coli spend 6 hours at least, O.D= 0.0325
Assay:add 80 μl PFRC liquid into LB

	Theophylline concentration	Theophylline(0.67M)	PFRC liquid(μl)	Cm50(μl)
A	0 mM	0	80.4	4
B	0.5 mM	2.985 μl	80.4	4
C	1 mM	5.97 μl	80.4	4
D	2 mM	11.94 μl	80.4	4
E	4 mM	23.88 μl	80.4	4
F	5 mM	29.85 μpl	80,4	4

10/18 RC 3-in-1

Total:	49μl	X2.1μl
VR+VF	2μl	4.2μl
dNTP	2μl	4.2μl
10XBuff.	5μl	10.5μl
tag	0.25μl	0.525mu;l
ddH2O	39.75μl	83.475μl

PCR Protocol
94	60s
94	15s
55	20s
72	30s	30 cycles
72	300s

PFRC & C liquid culture

Ligate ribo with C3 again
Transform

2010.10.20

Assay

	Theophylline concentration	Theophylline(0.67M)	PFRC liquid(μl)	Cm50(μl)
O	0 mM	0	130	4
A	0.1 mM	0.597 μl	130	4
B	0.05 mM	1.4925 μl	130	4
C	0.5 mM	2.985 μl	130	4
D	1 mM	5.97 μl	130	4
E	2 mM	11.94 μl	130	4
F	4 mM	23.88 μpl	130	4
G	8 mM	47.76 μl	130	4

culture for 2 hours

Transform

2010.10.21

Assay

	Theophylline concentration	Theophylline(0.67M)	PFRC liquid(μl)	Cm50(μl)
O	0 μM	0	85.7	4
A	50 μM	0.2985 μl	85.7	4
B	100 μM	0.597 μl	85.7	4
C	200 μM	1.194 μl	85.7	4
D	500 μM	2.985 μl	85.7	4
E	1000 μM	5.97 μl	85.7	4
F	2000 μM	11.94 μl	85.7	4
G	4000 μM	23.88 μl	85.7	4
H	8000 μM	47.76 μl	85.7	4
I	10000 μM	59.7 μl	85.7	4
J	20000 μM	119.4 μl	85.7	4
K	40000 μM	238.8 μl	85.7	4

10/20 RC 3-in-1

Total:	49μl	X2.5μl
VR+VF	2μl	5μl
dNTP	2μl	5μl
10XBuff.	5μl	12.5μl
tag	0.25μl	1.25mu;l
ddH2O	39.75μl	99.375μl

PCR Protocol
94	60s
94	15s
55	20s
72	30s	30 cycles
72	300s

Digest ribo again

2010.10.22

Digest C3 from PFRC plasmid
Ligate ribo with C3
Transform

Theophylline solution; concentration is 0.1M
Assay

	Theophylline concentration	Theophylline(0.1M)	PFRC liquid(μl)	Cm50(μl)
O	0 μM	0	85.7	4
A	10 μM	0.4 μl	117.7	4
B	50 μM	2 μl	117.7	4
C	100 μM	4 μl	117.7	4
D	200 μM	8 μl	117.7	4
E	500 μM	20 μl	117.7	4
F	1000 μM	40 μl	117.7	4
G	2000 μM	80 μl	117.7	4
H	4000 μM	160 μl	117.7	4
I	8000 μM	320 μl	117.7	4
J	10000 μM	400 μl	117.7	4
K	20000 μM	800 μl	117.7	4

	Theophylline concentration	Theophylline(0.1M)	PFRC liquid(μl)	Cm50(μl)
O	0 μM	0	261	4
A	10 μM	0.4 μl	261	4
B	50 μM	2 μl	261	4
C	100 μM	4 μl	261	4
D	200 μM	8 μl	261	4
E	500 μM	20 μl	261	4
F	1000 μM	40 μpl	261	4
G	2000 μM	80 μl	261	4
H	4000 μM	160 μl	261	4
I	80000 μM	320 μl	261	4
J	10000 μM	400 μl	261	4
K	20000 μM	800 μl	261	4
NT	100 μM	4 μl	261	4
N	0 μM	0 μl	261	4

NT: FRC(without promoter)+Theophylline

N: FRC(without promoter)

2010.10.24

ribo 3-in-1

Total:	49μl	X0.9μl
VR+VF	2μl	1.8μl
dNTP	2μl	1.8μl
10XBuff.	5μl	4.5μl
tag	0.25μl	0.225mu;l
ddH2O	39.75μl	35.775μl

PCR Protocol
94	60s
94	15s
55	20s
72	30s	30 cycles
72	300s

ribo liquid culture
colony PCR

Total:	49μl	X1.6μl
VR+VF	2μl	3.2μl
dNTP	2μl	3.2μl
10XBuff.	5μl	8μl
tag	0.25μl	0.8mu;l
ddH2O	39.75μl	63μl

PCR Protocol
94	60s
94	15s
55	20s
72	30s	30 cycles
72	300s

Assay

	Theophylline concentration	Theophylline(0.1M)	LB(μl)	PFRC liquid(μl)	Cm50(μl)
O	0 μM	0	325	325	4
A	10 μM	0.4 μl	325	325	4
B	50 μM	2 μl	327	325	4
C	100 μM	4 μl	329	325	4
D	200 μM	8 μl	333	325	4
E	500 μM	20 μl	345	325	4
F	1000 μM	40 μpl	365	325	4
G	2000 μM	80 μl	405	325	4
H	4000 μM	160 μl	485	325	4
I	8000 μM	320 μl	645	325	4
J	10000 μM	400 μl	725	325	4
K	20000 μM	800 μl	1125	325	4
NT	100 μM	4 μl	504	500(FRC)	4
N	0 μM	0 μl	500	500(FRC)	4

Digest RV(XP)& FRC(XP)
Ligate ribo with C3
transform

PFRC&FRC liquid culture

2010.10.25

RC 3-in-1

Total:	49μl	X2.4μl
VR+VF	2μl	4.8μl
dNTP	2μl	4.8μl
10XBuff.	5μl	12μl
tag	0.25μl	0.6mu;l
ddH2O	39.75μl	95.4μl

PCR Protocol
94	60s
94	15s
55	20s
72	30s	30 cycles
72	300s

FRC&PFRC&RC liquid culture

Assay

	Theophylline concentration	Theophylline(0.1M)	LB(μl)	PFRC liquid(μl)	Cm50(μl)
O	0 μM	0	151	147	4
A	50 μM	2 μl	153	147	4
B	500 μM	20 μl	171	147	4
C	1000 μM	40 μl	191	147	4
D	4000 μM	160 μl	311	147	4
E	10000 μM	400 μl	551	147	4
NT	100 μM	4 μl	158	150(FRC)	4
N	0 μM	0 μl	154	150(FRC)	4

2010.10.26

Assay

	Theophylline concentration	Theophylline(0.1M)	LB(μl)	PFRC liquid(μl)	Cm50(μl)
O	0 μM	0	151	147	4
A	50 μM	2 μl	153	147	4
B	500 μM	20 μl	171	147	4
C	1000 μM	40 μl	191	147	4
D	4000 μM	160 μl	311	147	4
E	10000 μM	400 μl	551	147	4
NT	100 μM	4 μl	158	150(FRC)	4
N	0 μM	0 μl	154	150(FRC)	4

NYMU-Taipei iGEM 2010 Team

@@ Line 105: / Line 105: @@
 {| border=1|-
-![[Image:NYMU riboswitch.08.20.jpg]] !!
+![[Image:NYMU R20.JPG]] !!
 {{:Team:NYMU-Taipei/GELC|=
 |1: marker 100bp|||n|=

Team:NYMU-Taipei/Experiments/Riboswitch