Team:Kyoto/Florigen/Notebook
From 2012.igem.org
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==August 21== | ==August 21== |
Revision as of 08:06, 24 September 2012
Florigen Notebook
August 2
Mutation of FT
by Sato
FT gene has two BioBrick restriction enzyme sites, EcoR1 and Pst1 which is next to each other.
So we tried to delete both at once by using two primers with mutation.
10xBufer | 2mM dNTPs | primer fwd | primer rev | template | polymerase | MilliQ | Total |
---|---|---|---|---|---|---|---|
5 | 5 | 1.5 | 1.5 | 0.5 | 1 | 35.5 | 50 |
94℃ 2min, (98℃ 10sec, 68℃ 4min)x4cycles, 4℃ Hold
PCR product | Dpn1 |
---|---|
50 | 2 |
product | MilliQ | Ligase | T4 Kinase | Total |
---|---|---|---|---|
2 | 7 | 5 | 1 | 15 |
16℃, 1h incubate
competent cell | DNA |
---|---|
20 | 2 |
Cells were stored on ice for 30min.
After 42℃ 60sec heat shock, cells were stored on ice for 2min.
Then cells were precultureed at 37℃ for 1hr, plated to Kanamycin plate.
August 13
Liquid culture
FT at 37°C, for overnight.
August 14
Miniprep of FT
by Sato, Takeuchi
The concentration was 81.5ng/uL
Restriction digestion and Electrophoresis
by Sato
To check wheter mutation was succeed, we did restriction enzyme digestion.
DNA(FT,80ng/uL) | 10xBuferH | EcoR1 | Pst1 | MilliQ | Total |
---|---|---|---|---|---|
5 | 2 | 1 | - | 12 | 20 |
5 | 2 | - | 1 | 12 | 20 |
37°C 2h incubate
We did electrophoresis of three FT plasmids, non-cutted, EcoR1 cutted, Pst1 cutted.
However, we couldn't get any bands (data not shown.)
Liquid culture
FT (4mL)
August 15
Miniprep of FT
by Sato, Takeuchi, Hyungcheol
We couldn't get enough concentration of plasmids.
Electrophoresis
by Sato
We retried electrophoresis of three samples same as yesterday.
However, we couldn't get any bands as well.
August 16
Transformation
by Takeuchi, Ota
Name | Well | Sample | Competent Cells | Total | Plate | Colony |
---|---|---|---|---|---|---|
FT | - | 1 µL | 10 | 11 | LB (Kan+) | × |
pSB1C3 | 1-3-A | 1 | 10 | 11 | LB (CP+) | ○ |
I719005 | 1-15-N | 1 | 10 | 11 | LB (Amp+) | ○ |
August 17
Transformation
by Takeuchi
Name | Well | Sample | Competent Cells | MilliQ | Total | Plate | Colony |
---|---|---|---|---|---|---|---|
FT | - | 2 | 2 | 18 | 22 | LB (Kan+) | × |
We found that mutation of FT was not successful.
August 20
We decided to do PCR using FT specific primers before mutation.
PCR of FT
by Sato
10xBufer | dNTPs | MgSO4 | primer fwd | primer rev | template | polymerase | MilliQ | Total |
---|---|---|---|---|---|---|---|---|
5 | 5 | 3 | 1 | 1 | 1(130ng/µL) | 1(KOD plus neo) | 33 | 50 |
94°C 2min, (98°C 10sec, 68°C 15sec)x30cycles, 4°C Hold
After the ethanol precipitation, we diluted in 30µL of MilliQ.
The concentration was 203ng/µL.
Electrophoresis
Lane | Name | length(bp) |
---|---|---|
1 | 1kb ladder | - |
2 | FT | 600 |
August 21
Restriction digestion
by Sato
DNA(FT,203ng/µL) | 10xBuferM | Xba11 | Pst1 | MilliQ | Total |
---|---|---|---|---|---|
10 | 4 | 1 | 1 | 24 | 40 |
37°C, 5h incubate
After the ethanol precipitation, we diluted in 30µL of MilliQ.
The concentration was 54,9ng/µL.
Ligation
by Sato
Vector | Insert | Ligation High Ver.2 | ||
---|---|---|---|---|
pSB1C3 | 1 | FT | 10 | 5.5 |
Liquid culture
T7 promoter, pSB1C3 (4mL)
August 22
Miniprep
by Sato
T7 promoter | pSB1C3 |
---|---|
85.3ng/µL | 82.93ng/µL |
August 23
Ethanol Precipitation
diluted in 20µL 79.3ng/µL
mada dekite nai
August 24
Restriction enzyme processing
T7 promoter(85.3ng/µL) | Spel | Pstl | buffer M | MiliQ | Total |
---|---|---|---|---|---|
10 | 1 | 1 | 2 | 6 | 20 |
->purifying column 33.4ng/µL(dissolution 40µL)
pSB1C3(82.9ng/µL) | Xbal | Spel | buffer M | MiliQ | Total |
---|---|---|---|---|---|
20 | 1 | 1 | 4 | 14 | 40 |
->gene clean2 39.9ng/µL(dissolution 40µL)
<<picture1,2>>
Ligation
FT(600bp, 79.3ng/µL) | pSB1C3(2000bp,39.9ng/µL) | Ligation High Ver.2 |
---|---|---|
3µL => 597fmol | 2µL => 60fmol | 2.5µL |
FT(600bp, 79.3ng/µL) | T7(2100bp,33.4ng/µL) | Ligation High Ver.2 |
---|---|---|
2.4µL => 478fmol | 2µL => 48fmol | 2.2µL |
=> 16℃,1hr incubate
August 27
Colony PCR
2X Quick Tag | VF2 | VR | MiliQ | Total |
---|---|---|---|---|
25 | 1 | 1 | 23 | 50 |
Lane1: 1kb ladder
Lane2~16: FT(pSB1C3) about 800bp
FT(TOPO) PCR(re)
buffer | dNTPs | MgSO4 | primer f | primer r | Template(130ng/µL) | KODplus neo | MilliQ | Total |
---|---|---|---|---|---|---|---|---|
5 | 5 | 3 | 1 | 1 | 1 | 1 | 33 | 50 |
94℃ | 98℃ | 68℃ | cycles |
---|---|---|---|
2min | 10sec | 15sec | 30 |
Liquid culture
by Nobeyama
FT 4ml
August 28
Mutation of FT (re)
inverse PCR
MilliQ | buffer | dNTP | primer f | primer r | FT(130ng/µL) | KODplus | Total |
---|---|---|---|---|---|---|---|
35.5 | 5 | 5 | 1.5 | 1.5 | 0.5 | 1 | 50 |
94℃ | 98℃ | 68℃ | cycles |
---|---|---|---|
2min | 10sec | 4min | 18 |
Lane1: 1kb ladder
Lane2: FT
====Miniprep FT(TOPO====)
158ng/µL
Tranformation
competent cell: 20
BBa.I746902 : 2
(plate 316f)
(GFP generator of pBAD/araC-mut3 GFP:6His-DT)
August 29
Mutaion of FT(re;re)
Inverse PCR
first
MilliQ | buffer | dNTP | primer f | primer r | FT(130ng/µL) | KODplus | Total |
---|---|---|---|---|---|---|---|
35.5 | 5 | 5 | 1.5 | 1.5 | 0.5 | 1 | 50 |
second
MilliQ | buffer | dNTP | primer f | primer r | FT(52ng/µL) | KODplus | Total |
---|---|---|---|---|---|---|---|
35 | 5 | 5 | 1.5 | 1.5 | 1 | 1 | 50 |
94℃ | 98℃ | 68℃ | cycles |
---|---|---|---|
2min | 10sec | 4min | 30 |
Lane1: 1kb ladder
Lane2: first Template 130ng/µL
Lane3: second Template 53ng/µL
first sample | Dpnl | total |
---|---|---|
45µL | 2µL | 47µL |
in 37℃, 1 hour
Self-Ligation
PCR products | MilliQ | Ligation High | T4 kinase | total |
---|---|---|---|---|
2µL | 7µL | 5µL | 1µL | 15µL |
in 16℃, 1.5hour incubate
Transformation
competent cell: 20
DNA : 2
Liquid culture(I746902): 3mL
August 30
Liquid culture(FT) 4mL x2
August 31
Miniprep(FT)
(1) 64.9ng/µL
(2) 52.6ng/µL
Restriction enzyme processing (Mutation checking)
FT(52.6ng/µL) | bufferH | E.coli | Pst1 | MilliQ | total |
---|---|---|---|---|---|
1µL | 5µL | 0.5µL | 0.5µL | 3.5µL | 10µL |
in 37℃,1.5hour
PCR(RBS primer)
buffer for KODplus neo | dNTPs | MgSO4 | primer f | primer r | Template(52.6ng/µL) | KODplus neo | MilliQ | Total |
---|---|---|---|---|---|---|---|---|
5 | 5 | 3 | 1 | 1 | 1 | 1 | 33 | 50 |
94℃ | 98℃ | 68℃ | cycles |
---|---|---|---|
2min | 10sec | 15sec | 30 |
Lane1: 1kb ladder
Lane2: FT
Lane3: FT(E.coli)
Lane4: FT(Pst1)
Lane5: FT PCR
PCR(re)
buffer | dNTPs | MgSO4 | primer f | primer r | Template | KOD neo | MilliQ | Total |
---|---|---|---|---|---|---|---|---|
5 | 5 | 3 | 1 | 1 | 1 | 1 | 33 | 50 |
94℃ | 98℃ | 68℃ | cycles |
---|---|---|---|
2min | 10sec | 15sec | 35 |
Lane1: 1kb ladder
Lane2: FT
PCR(re)
buffer | dNTPs | MgSO4 | primer f | primer r | Template | KOD neo | MilliQ | Total |
---|---|---|---|---|---|---|---|---|
5 | 5 | 2 | 1 | 1 | 1 | 1 | 34 | 50 |
94℃ | 98℃ | 68℃ | cycles |
---|---|---|---|
2min | 10sec | 10sec | 30 |
September 2
PCR(re;re)
first
buffer | dNTPs | MgSO4 | primer f | primer r | Template(1ng/µL) | KODplus neo | MilliQ | Total |
---|---|---|---|---|---|---|---|---|
5 | 5 | 3 | 1 | 1 | 1 | 1 | 33 | 50 |
second
buffer | dNTPs | MgSO4 | primer f | primer r | Template(10ng/µL) | KODplus neo | MilliQ | Total |
---|---|---|---|---|---|---|---|---|
5 | 5 | 3 | 1 | 1 | 1 | 1 | 33 | 50 |
94℃ | 98℃ | 68℃ | cycles |
---|---|---|---|
2min | 10sec | 10sec | 25 |
Lane1: first Template 1ng
Lane2: second Template 10ng
Lane3: 1kb ladder
refine first Template => 132ng/µL
September 3
Restriction enzyme processing
FT(132ng/µL) | bufferM | EcoRI | SpeI | MilliQ | Total |
---|---|---|---|---|---|
10 | 2 | 1 | 1 | 6 | 20 |
37℃,overnight => refinement 31.6ng/µL (Elution 40µL)
Ligation
Insert(FT: 31.6ng/µL, 600bp ): 2µL = 26fmol
Vector(DT: 28.0ng/µL, 3300bp): 3µL = 240fmol
Ligation High ver.2 :2.5µL
=> 16℃, 2 hours
Transformation
competent cell | DNA | plate | colony |
---|---|---|---|
20µL | FT-DT 2µL | Amp | o |
20µL | pT7-6His:R9 2µL | Amp | o |
10µL | GFP generator 1µL | Amp | o |
September 4
Colony PCR
Quick Tag | VF2 | VR | MilliQ | Total |
---|---|---|---|---|
25 | 1 | 1 | 23 | 50 |
94℃ | 98℃ | 55℃ | 68℃ | cycles |
---|---|---|---|---|
2min | 30sec | 30sec | 1min | 25 |
Lane1: 1kb ladder
Lane2: FT-DT(about 700bp)
Liquid culture(4ml) 23:30 ~
GFP generator, FT-DT
September 5
Miniprep(FT-DT) by Sato
88.8ng/µL
Restriction enzyme processing
FT-DT(88.8ng/µL) | XbaI | PstI | bufferM | MiliiQ | total |
---|---|---|---|---|---|
20 | 1 | 1 | 4 | 14 | 40 |
at 37℃, 2 hours
Electrophoresis by Takeuchi
Restriction enzyme processingby Takeuchi
FT-DT(88.8ng/µL) | bufferM | XbaI/Spe | MiliiQ | total |
---|---|---|---|---|
4 | 1 | 0.5 | 4.5 | 10 |
FT-DT | bufferH | Pst/Eco | MiliiQ | total |
---|---|---|---|---|
4 | 1 | 0.5 | 4.5 | 10 |
at 37℃,1hour 10min
September 6
Western blotting(BBa,I746915)
Sample making
SOC(ampt) 50ml + pre culture 1ml x2
OD600 = 0.5~0.7 incubate at 37℃ (OD 0.642)
add IPTG final concentration is 1mM (negative control)
incubate at 37℃,4 hours
SDS-PAGE
Do spin down E.coli and make suspension put E.coli into 1mL 1x sample buffer
95℃,10min
electrophoresis at 500V, 30mA, 50min
Lane1: 10µL (IPTG -)
Lane2: 10µL (IPTG -)
Lane3: 10µL (IPTG +)
Lane4: 5µL (IPTG -)
Lane5: 5µL (IPTG +)
Lane6: 2µL (IPTG -)
Lane7: 2µL (IPTG +)
Blotting at 50V,100mA,30min
Put into blocking buffer and vibrating 30min
Incubate with Anti GFP(1/1000) 10mL at RT,1h
Washing with 10mL TBST (vibrating 10min x2)
Incubate with Anti-mouseAP(1/1000) 10mL at RT, 30min
Washing with 10mL TBST (vibrating 10min x3)
Put NBT,BCIP into dye buffer
September 9
Mutaion of FT
MilliQ | buffer | dNTP | primer f | primer r | FT(52ng/µL) | KODplus | Total |
---|---|---|---|---|---|---|---|
35 | 5 | 5 | 1.5 | 1.5 | 1 | 1 | 50 |
94℃ | 98℃ | 68℃ | cycles |
---|---|---|---|
2min | 10sec | 4min | 20 |
→ GeneClean II 32.6ng/µL
Dpn1 processing
TA buffer | DNA | Dpn1 | Total |
---|---|---|---|
3.3 | 31 | 2 | 36.3 |
Ligation
DNA | MiliiQ | Ligation high Ver.2 | T4 kinase | Total |
---|---|---|---|---|
2 | 7 | 5 | 1 | 15 |
Transformation
competent cell: 10
DNA : 1
September 10
Miniprep of FT
①116.9ng/µL
② 34.5ng/µL
Restriction enzyme processing(Mutation checking)
FT①/② | bufferHl | EcoRI | PstI | MiliQ | Total |
---|---|---|---|---|---|
4 | 1 | 0.5 | 0 | 4 | 10 |
4 | 1 | 0 | 0.5 | 4 | 10 |
PCR
Bufer | dNTPs | MgSO4 | primer(+/-RBS)fwd | primer(+/-RBS)rev | template①/② | KOD plus neo | MilliQ | Total |
---|---|---|---|---|---|---|---|---|
5 | 5 | 3 | 1 | 1 | 1 | 1 | 33 | 50 |
94℃ | 98℃ | 68℃ | cycles |
---|---|---|---|
2min | 10sec | 10sec | 25 |
->purifying column 17.4ng/µL
Restriction enzyme processing
FT(RBS+)32.6ng/µL | Xbal | Pstl | buffer M | BSA | Total |
---|---|---|---|---|---|
30 | 1 | 1 | 4 | 4 | 40 |
T7-His:R9(62.6ng/µL) | SpeI | Pstl | MilliQ | buffer M | Total |
---|---|---|---|---|---|
15 | 0.5 | 0.5 | 2 | 2 | 20 |
incubate at 37℃, 3hours
->purifying column 17.4ng/µL
September 11
Ligation
Vector(T7: 33.4ng/µL, 2100bp): 1µL = 24fmol
Insert(FT: 17.4ng/µL, 600bp ): 5µL = 217fmol
Ligation High ver.2 : 3µL
=> 16℃, 1 hours
Transformation
competent cell | DNA |
---|---|
20µL | T7-FT 2µL |
PCR(FT without RBS retry)
Bufer | dNTPs | MgSO4 | primer(-RBS)fwd | primer(-RBS)rev | template | KOD plus | MilliQ | Total |
---|---|---|---|---|---|---|---|---|
5 | 5 | 3 | 1 | 1 | 1 | 1 | 33 | 50 |
94℃ | 98℃ | 65℃ | 68℃ | cycles |
---|---|---|---|---|
2min | 15sec | 30sec | 30sec | 25 |
Lane1:FT(RBS-) 600bp
Lane2:Ladder 100bp
えいどうしゃしん
=>purifying column 34.6ng/µL
Restriction enzyme processing
FT(RBS-) | XbaI | PstI | bufferM | BSA | total |
---|---|---|---|---|---|
30 | 1 | 1 | 4 | 4 | 40 |
at 37℃, 2 hours
=> 6.2ng/μL
GFP-DT | XbaI | PstI | bufferM | BSA | MilliQ | total |
---|---|---|---|---|---|---|
15 | 1 | 1 | 3 | 3 | 7 | 30 |
at 37℃, 2 hours
=> 7.0ng/μL
Ligation
Vector(T7-6His-R9: 11.6ng/µL, 2100bp): 1µL = 9fmol
Insert(FT: 6.2ng/µL, 600bp ): 5µL = 79fmol
Ligation High ver.2 : 3µL
=> 16℃, 1 hours
Vector(T7-6His-R9: 11.6ng/µL, 2100bp): 1µL = 9fmol
Insert(GFP-DT: 7.0ng/µL, 1000bp ): 9µL = 95fmol
Ligation High ver.2 : 4µL
=> 16℃, 1 hours
September 12
Transformation
competent cell | DNA | plate | |
---|---|---|---|
20µL | T7-R9-GFP-DT 2µL | Amp | |
20µL | T7-R9-FT 2µL | Amp | |
BL21CDE3 10µL | T7-FT 1µL | Amp |
Miniprep (T7-FT)
37.1ng/µL
September 13
Miniprep
①T7-R9-GFP-DT 90ng/µL
②T7-R9-FT 160ng/μL
Restriction enzyme processing
T7-R9-GFP-DT (90ng/µL) | EcoRI | PstI | buffer H | MilliQ | total |
---|---|---|---|---|---|
20 | 1 | 1 | 3 | 5 | 30 |
at 37℃, 2 hours
=> 20.7ng/μL
T7-R9-FT (160ng/µL) | EcoRI | SpeI | buffer M | MilliQ | total |
---|---|---|---|---|---|
20 | 1 | 1 | 3 | 5 | 30 |
at 37℃, 2 hours
=> 20.1ng/μL
Transformation
competent cell BL21(DE3) | DNA | plate | |
---|---|---|---|
10µL | T7-R9-GFP-DT 1µL | Amp | |
10µL | T7-R9-FT 1µL | Amp |
Restriction enzyme processing
Buffer H | BSA | EcoRI | PstI | DpnⅠ | MilliQ | total |
---|---|---|---|---|---|---|
5 | 5 | 0.5 | 0.5 | 0.5 | 13.5 | 25 |
=>We define this solution "2× Master Mix"
2× Master Mix | pSB1C3(Linerarized Plasmid Backbone) |
---|---|
4 | 4 |
at 37℃, 30 minutes
80℃, 30 minutes
PCR(Insert His-tag)
MilliQ | Buffer for iPCR | dNTPs | primer fwd | primer rev | template(T7-FT 37.1ng/μL) | KOD plus | Total |
---|---|---|---|---|---|---|---|
35 | 5 | 5 | 1.5 | 1.5 | 1 | 1 | 50 |
94℃ | 94℃ | 56℃ | 68℃ | cycles |
---|---|---|---|---|
2min | 15sec | 30sec | 2.5min | 15 |
Lane1:Ladder 1kb
Lane2:T7-6His:FT about 2700bp
えいどうしゃしん
September 14
Ligation
Vector(pSB1C3: 12.5/µL, 2000bp) : 2µL = 19fmol
Insert(T7-R9-GFP-DT: 20.7ng/µL, 700bp ): 4µL = 180fmol
Ligation High ver.2 : 3µL
=> 16℃, 1 hours
Dpn1 processing
PCR products(9/13) | Dpn1 | Total |
---|---|---|
45 | 2 | 47 |
=>37℃, 1 hour
Self Ligation
PCR products | Ligation High | T4 Kinase | MilliQ | Total |
---|---|---|---|---|
2 | 5 | 1 | 7 | 15 |
=>16℃, 1 hour
Ligation
Vector(DT: 17.1/µL, 2100bp) : 2µL = 12fmol
Insert(T7-R9-FT: 20.1ng/µL, 650bp ): 5µL = 496fmol
Ligation High ver.2 : 3.5µL
=> 16℃, 1 hours
September 15
Restriction enzyme processing
FT without RBS (34.6ng/µL) | EcoRI | PstI | 10× buffer H | MilliQ | total |
---|---|---|---|---|---|
10 | 0.5 | 0.5 | 2 | 7 | 20 |
Colony PCR
Quick Tag | VF | VR | MilliQ | Total |
---|---|---|---|---|
25 | 1 | 1 | 23 | 50 |
94℃ | 94℃ | 55℃ | 68℃ | cycles |
---|---|---|---|---|
2min | 30sec | 30sec | 1min | 25 |
Electrophoresis
Lane1: ladder
Lane2: T7-R9-GFP-DT
Lane3: T7-R9-GFP-DT
Lane4: T7-R9-FT-DT
Lane5: T7-R9-FT-DT
Lane6: T7-R9-FT-DT
Lane7: T7-R9-FT-DT
Lane8: T7-R9-FT-DT
A member of secretion group electrophoresed DNA from Lane9 to Lane12.
Lane13: T7-His-FT
Lane14: T7-His-FT
Lane15: T7-His-FT
Lane16: T7-His-FT
Lane17: ladder
えいどうしゃしん
Liquid culture(3ml) 3:30~
T7-R9-FT-DT×2, T7-His-FT×2, T7-His-FT
September 16
Miniprep
①T7-R9-FT-DT 150ng/µL
②T7-R9-FT-DT 139ng/μL
③T7-R9-GFP-DT 67ng/µL
④T7-His-FT 153ng/μL
⑤T7-His-FT 73ng/μL
September 17
Purifying column
=>FT without RBS :36.4ng/µL
Ligation
Vector(PSB1C3: 12.5/µL, 2000bp) : 3µL = 9fmol
Insert(FT without RBS: 36.4ng/µL, 600bp ): 3µL = 92fmol
Ligation High ver.2 : 3µL
=> 16℃, 1 hours
September 18
Transformation by NAKAGAWA
competent cell | DNA | plate |
---|---|---|
20µL | PSB1C3 FT without RBS 1µL | CP+ |
Verification of R9 function by TAKEUCHI
R9(20µg/µL) | 0.9µL |
GFP(1.2mg/mL) | 2.23µL |
RBS | 16.85µL |
total | 20µL |
X5
Method:
1. Peel cuticles on parafilm by using the head of pencil.(Menasha,wI,54952)
2. Put plant cells into GFP&R9 or GFP for 5~30min.
3. Put plant cells into PBS.
4. Hoechst dyeing.
1 | 2 | 3 | 4 | 5 | 6 | |
R9 | o | o | o | x | o | o |
cuticle | o | o | o | o | x | x |
soak in GFP | 5min | 15min | 30min | 5min | 5min | 30min |
September 19
Transformation(re) by NAKAGAWA,TAKEUCHI
competent cell:20µL
DNA(No RBS FT):1µL
plate :CP+
Transformation(re;re) by NAKAGAWA,TAKEUCHI
competent cell:10µL
DNA(No RBS FT):1µL
LB :100µL
plate :CP+
Adjusted GM Agar Medium making by TAKEUCHI
Ingredient of MS medium(SIGMA M5519): 0.88g
MES : 0.1g
ion exchanged water : 200mL
NaOH : 26µL(adjust to pH5.6)
Agar medium : 1.6g
Autoclave 120℃
Colony PCR(re)
gelA
Lane1: 100bp Ladder
Lane2: No RBS FT colony number 9
Lane3: No RBS FT colony number 10
Lane4: No RBS FT colony number 11
Lane5: No RBS FT colony number 12
Lane6: No RBS FT colony number 13
Lane7: empty
Lane8: empty
gelB
Lane1: 100bp Ladder
Lane2: No RBS FT colony number 14
Lane3: No RBS FT colony number 15
Lane4: No RBS FT colony number 16
Lane5: No RBS FT colony number 17
Lane6: No RBS FT colony number 18
Lane7: No RBS FT colony number 19
Lane8: empty
gelA
Lane1: 100bp Ladder
Lane2: No RBS FT colony number 20
Lane3: No RBS FT colony number 21
Lane4: No RBS FT colony number 22
Lane5: No RBS FT colony number 23
Lane6: No RBS FT colony number 24
Lane7: empty
Lane8: empty
September 20
Liquid culture by NAKAGAWA
No RBS FT x8 (by using September 18)
Plate: CP+
Colony PCR
No RBS FT by using September19
Lane1 : 100bp ladder
Lane2 : colony number 1
Lane3 : colony number 2
Lane4 : colony number 3
Lane5 : colony number 4
Lane6 : colony number 5
Lane7 : colony number 6
Lane8 : colony number 7
Lane9 : colony number 8
Lane10: empty
Lane11: empty
Lane12: 100bp ladder
Liquid culture
A-11, A-12
Miniprep
No RBS FT(by using September20)
1.-10.4µg/mL
2.-4.7µg/mL
3.-3.6µg/mL
4.-7.6µg/mL
5.-4.5µg/mL
6.-8.4µg/mL
7. 1.8µg/mL(average)
8. 18.1µg/mL
Restriction enzyme processing
DNA(No RBS FT)x2 | E.coli | BufferH | MilliQ | total |
---|---|---|---|---|
30µL | 1µL | 4µL | 5µL | 40µL |
in 37℃,2hours
Electrophoresis
DNA(No RBS FT) sample7,8: 10µL
Loading Dye : 2µL
Lane1: 1kb ladder
Lane2: empty
Lane3: No RBS FT(E) sample7
Lane4: empty
Lane5: No RBS FT(E) sample8
Lane6: empty
Electrophoresis(re)
RNA Extraction
5 leaves: 100mg
ISOGEN : 1mL
Elution : 20µL
cDNA Synthesis(1/4)
gDNA wipeout buffer | template RNA | H2O | Total |
---|---|---|---|
1µL | 0.5µL | 5.5µL | 7µL |
Reverse Transcriptase | RT buffer | primer mix | template | Total |
---|---|---|---|---|
0.5µL | 2µL | 0.5µL | 7µL | 10µL |
RT PCR
buffer | dNTPs | MgSO4 | primer f | primer r | Template | KODplus | MilliQ | Total |
---|---|---|---|---|---|---|---|---|
5 | 5 | 2 | 1.5 | 1.5 | 1 | 1 | 34.5 | 50 |
94℃ | 94℃ | 54℃ | 68℃ | cycles |
---|---|---|---|---|
2min | 15sec | 30sec | 10sec | 30 |
1.TUBULIN
2.FUL
3.SEP3
4.AP1