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Material & Method

General protocol

CelC

Agro Notebook

5/31 Cloning of CelC and Restriction Enzyme

By Koki Tsutsumi

CelC gene had produced clone from Agrobacterium tumefaciens C58, but I confirmed whether it’s true or not. CelC gene has restriction enzyme sites,EcoRI and BamHI.

No	Name	volume
1	500bp DNA ladder	10μL
2	λ-HindⅢ	10μL
3	CelC_nonRE	12μL
4	CelC/BamHI	12μL
5	CelC/EcoRI	12μL
6	λ-HindⅢ	10μL
7	500bp DNA ladder	10μL
8	-	-

Inverse PCR

※Restriction Enzyme sol.(line No.5 CelC_EcoRI)which has 1M NaCl dissolved in it, so, the band in lane no.5 appeared as upper-side.

CelC_Fw: TGACGAAAGCACTGATCTGC

CelC_Rv: GAAAAGATCGAAACGGTGG

TA cloning of CelC

16℃ 30min incubate

Ligation of CelC/pMD20 and Transformation in JM109.

Cells were stored on ice for 30min.

After 42℃ 30sec heat shock, cells were stored on ice for 2min.

Then cells were pre-cultured at 37℃ for 1hr, plated to Ampicillin plate.

6/1 Liquid clluture

CelC/pMD20 22 samples at 37°C, for overnight.

6/2 MiniPrep of CelC

Linear CelC/pMD20 DNA :2736bp. This CelC/pMD20 sample is cccDNA. So,white 6,white 7,white 8,white 9,white 14 probably picked up CelC/pMD20.

6/3 Restriction Enzyme of CelC/pMD20

CelC gene had produced clone from Agrobacterium tumefaciens C58, I confirmed whether it’s true or not. CelC/pMD20 gene has 2 restriction enzyme sites,BamHI

I confirmed the direction of CelC gene.

6/ Sequence of CelC/pMD20

7/18 PointMutation of CelC

CelC gene had Restriction Enzyme Site,EcoRI. We directed the EcoRI site.

Front

Fw1 Primer:

TATATATTCTAGATGAAGAGCGGGATTTCG

Rv2 Primer:

CATTATATCCGAACTCCGGCTG

Rear

Fw2 Primer:

AGCCGGAGTTCGGATATAATGC

Rv1 Primer:

CAGCACGAACTAGTATTATTATCATCGGC

7/19 Gel Purification of CelC gene’s Front Fragment and Rear Fragment

Front Fragment DNA and Rear Fragment DNA that 765bp and 347bp band performed Gel Purification by illustra GFX PCR Purification Kit.

7/21 CelC gene’s Front Fragment and Rear Fragment Overlap PCR

No.6,7,8,9,14 each fragment Overlap PCR completed.

I selected No.8.

7/22 Gel Purification of CelC gene No.8

No.8 DNA that about 1ooo bp band performed Gel Purification by illustra GFX PCR Purification Kit.

8/1 Adapter PCR of CelC gene No.8 (BioBrick Part)

Fw Primer:

GTTTCTTCGAATTCGCGGCCGCTTCTAGATG

Rv Primer:

GTTTCTTCCTGCAGCGGCCGCTACTAGTATTATTATC

8/11 BioBrick of CelC Restrict Enzyme ,EcoRI.

No	Name	volume
1	500bp DNA ladder	10μL
2	λ-HindⅢ	10μL
3	PCR sample A non RE	12μL
4	PCR sample A EcoRⅠ RE	12μL
5	PCR sample B non RE	12μL
6	PCR sample B EcoRⅠ RE	12μL
7	λ-HindⅢ	10μL
8	500bp DNA ladder	10μL

I confirmed BioBrick of CelC non-Restriction Enzyme ,EcoRI.

9/5 Brick Part of CelC and pSB1C3 Restrict Enzyme,EcoRI and PstI.

・CelC
S.D.W	10μL
EcoRⅠ	1μL
PstⅠ	1μL
PCR sample	6μL
10×H buffer	2μL
Total	20μL

・pSB1C3
S.D.W	10μL
EcoRⅠ	1μL
PstⅠ	1μL
pSB1C3	6μL
10×H buffer	2μL
Total	20μL

9/5 Ligation of CelC/pSB1C3 and Transformation in JM109.

CelC/EcoRⅠ,PstⅠ(100ng)	1μL
pSB1C3/EcoRⅠ,PstⅠ(50ng)	2μL
Ligation kit ver.2	3μL
Total	6μL

9/7 Colony PCR of CelC/pSB1C3

No	Name	volume
1	500bp DNA ladder	10μL
2	λ-HindⅢ	10μL
3	No.1	12μL
4	No.2	12μL
5	No.3	12μL
6	No.4	12μL
7	No.5	12μL
8	No.6	12μL
9	No.7	12μL
10	No.8	12μL
11	No.9	12μL
12	No.10	12μL
13	No.11	12μL
14	No.12	12μL
15	No.13	12μL
16	No.14	12μL
17	No.15	12μL
18	-	-

CelC/pSB1C3 DNA(VR-VF2) :1370bp. So,No.5 and No.12 probably picked up CelC/pSB1C3

9/8 Miniprep of CelC/pSB1C3

No	Name	volume
1	500bp DNA ladder	10μL
2	λ-HindⅢ	10μL
3	No.1	12μL
4	No.2	12μL
5	No.3	12μL
6	No.4	12μL
7	No.5	12μL
8	No.6	12μL
9	No.7	12μL
10	No.8	12μL
11	No.9	12μL
12	No.10	12μL
13	No.11	12μL
14	No.12	12μL
15	No.13	12μL
16	No.14	12μL
17	No.15	12μL
18	-	-

Linear CelC/pSB1C3 DNA :3126bp. This CelC/pSB1C3 sample is cccDNA. So,No.5 and No.12 probably picked up CelC/pSB1C3.

9/15. Sequence of CelC Brick Part sequence.

Result of NCBI BLAST

CrdS

Cloning of CrdS and Restriction Enzyme

By Koki Tsutsumi

CrdS gene had produced clone from Agrobacterium tumefaciens C58, but I confirmed whether it’s true or not. CrdS gene has restriction enzyme sites,EcoRI and PstI.

No	Name	volume
1	500bp DNA ladder	10μL
2	λ-HindⅢ	10μL
3	CrdS	12μL
4	-	-
5	-	-
6	-	-
7	-	-
8	-	-

No	Name	volume
1	500bp DNA ladder	10μL
2	λ-HindⅢ	10μL
3	CrdS_nonRE	12μL
4	CrdS/EcoRⅠ	12μL
5	CrdS/PstⅠ	12μL
6	λ-HindⅢ	10μL
7	500bp DNA ladder	10μL
8	-	-

Inverse PCR

Prime STAR MAX	25μL
10pmol/μL Primer F	1μL
10pmol/μL Primer R	1μL
PCR反応液(2ng)	1μL
dH2O	22μL
Total	22μL

CrdS_Fw: AGTACGATCCGCTATTTTCCCG

CrdS_Rv: CAGACCAAGATTTCGCGAACTC

94℃ 2min

↓

98℃ 10sec

48℃ 30sec 35cycles

72℃ 2min

↓

72℃ 2min

TA cloning of CrdS

PCR product	1μL
pMD20	2μL
Ligation kit ver.2	3μL

16℃ 30min incubate

Ligation of CrdS/pMD20 and Transformation in JM109

Competent cell	100μL
DNA	6μL

↓Cells were stored on ice for 30min.

↓After 42℃ 30sec heat shock, cells were stored on ice for 2min.

↓Then cells were pre-cultured at 37℃ for 1hr, plated to Ampicillin plate.

Liquid culluture

CrdS/pMD20 21 samples at 37℃,for overnight

MiniPrep of CrdS/pMD20

Linear CrdS/pMD20 DNA :4995bp. This CrdS/pMD20 sample is cccDNA. So, probably picked up CrdS/pMD20.

No	Name	volume
1	500bp DNA ladder	10μL
2	λ-HindⅢ	10μL
3	CrdS No.5	12μL
4	CrdS No.6	12μL
5	CrdS No.8	12μL
6	CrdS No.15	12μL
7	CrdS No.17	12μL
8	-	-

Restriction Enzyme of CrdS/pMD20

CrdS gene had produced clone from Agrobacterium tumefaciens C58, I confirmed whether it’s true or not. CrdS/pMD20 gene has 2 restriction enzyme sites,EcoRI.

No	Name	volume
1	500bp DNA ladder	10μL
2	λ-HindⅢ	10μL
3	CrdS No.5	12μL
4	CrdS No.6	12μL
5	CrdS No.2	12μL
6	CrdS No.15	12μL
7	CrdS No.17	12μL
8	-	-

I comfirmed the direction of CrdS gene.

Sequence of CrdS/pMD20

PointMutation of CrdS

CrdS gene had Restriction Enzyme Site,EcoRI. We removed the EcoRI site.

No	Name	volume
1	500bp DNA ladder	10μL
2	λ-HindⅢ	10μL
3	CrdS Negative Front Fragment	12μL
4	CrdS Negative Rear Fragment	12μL
5	CrdS No.6 Front Fragment	12μL
6	CrdS No.6 Middle Fragment	12μL
7	CrdS No.6 Rear Fragment	12μL
8	CrdS No.15 Front Fragment	12μL
9	CrdS No.15 Middle Fragment	12μL
10	CrdS No.15 Rear Fragment	12μL
11	-	-
12	-	-
13	-	-
14	-	-
15	λ-HindⅢ	10μL
16	500bp DNA ladder	10μL

Front

Fw0 Primer:GGCCGCTTCTAGATGTATTTCAGTGC

Rv1 Primer:CGTTTCGAGGGAGAACTCCAGCG

Middle

Fw1Primer:CGCTGGAGTTCTCCCTCGAAACG

Rv2Primer:CAGCTCATCGGCCTGAAGCGCC

Rear

Fw2 Primer:GGCGCTTCAGGCCGATGAGCTG

Rv0 Primer:GGCGCTACTAGTATTATTATCACCCGAATG

5xPS Buffer	10μL
dNTP Mixture	4μL
10pmol/µl Primer Fw1 or Fw2	1μL
10pmol/µl Primer Rv2 or Rv1	1μL
Templete	1μL
Prime STAR HS	0.5μL
dH2O	32.5μL
Total	50μL

94℃ 2min

↓

98℃ 10sec

55℃ 5sec 35cycles

72℃ 70sec

↓

4℃ ∞

Gel Purification of CrdS gene’s Front Fragment and Rear Fragment

Front Fragment DNA and Rear Fragment DNA ,Middle Fragment DNA that 223 bp and 1037 bp ,782 bp band performed Gel Purification by illustra GFX PCR Purification Kit.

CrdS gene’s Front Fragment and Rear Fragment Overlap PCR

No	Name	volume
1	500bp DNA ladder	10μL
2	λ-HindⅢ	10μL
3	CrdS N Front+Middle DNA	12μL
4	CrdS No.6 Front+Middle DNA	12μL
5	CrdS No.15 Front+Middle DNA	12μL
6	λ-HindⅢ	10μL
7	500bp DNA ladder	10μL
8	-	-

No	Name	volume
1	500bp DNA ladder	10μL
2	λ-HindⅢ	10μL
3	CrdS N Front+Rear DNA	12μL
4	CrdS No.6 Front+Rear DNA	12μL
5	CrdS No.15 Front+Rear DNA	12μL
6	λ-HindⅢ	10μL
7	500bp DNA ladder	10μL
8	-	-

N, No.6, No.15 each fragment Overlap PCR completed.

Gel Purification of CrdS

No.8 DNA that about 2ooo bp band performed Gel Purification by illustra GFX PCR Purification Kit.

Adapter PCR of CrdS gene (BioBrick Part)

No	Name	volume
1	2-log DNA ladder	5μL
2	λ-HindⅢ	6μL
3	PCR saample	18μL
4	-	-
5	-	-
6	-	-
7	-	-
8	-	-

Fw Primer: GTTTCTTCGAATTCGCGGCCGCTTCTAGATG

Rv Primer: GTTTCTTCCTGCAGCGGCCGCTACTAGTATTATTATC

Brick Part of CrdS Restrict Enzyme,EcoRI and PstI.

No	Name	volume
1	500bp DNA ladder	10μL
2	λ-HindⅢ	10μL
3	CrdS N F+M non-RE	12μL
4	CrdS N F+M EcoRⅠ-RE	12μL
5	CrdS No.6 F+M non-RE	12μL
6	CrdS No.6 F+M EcoRⅠ-RE	12μL
7	CrdS No.15 F+M non-RE	12μL
8	CrdS No.15 F+M EcoRⅠ	12μL
9	CrdS N F+M+R non-RE	12μL
10	CrdS N F+M+R PstⅠ-RE	12μL
11	CrdS No.6 F+M+R non-RE	12μL
12	Crds No.6 F+M+R PstI RE	12μL
13	CrdS No.15 F+M+R non-RE	12μL
14	CrdS No.15 F+M+R PstI RE	12μL
15	λ-HindⅢ	10μL
16	500bp DNA ladder	10μL
17	-	-
18	-	-

N,No.6,No.15 of CrdS was cut on EcoRI site. Point Mutation of CrdS is unsuccessful.

Team:Biwako Nagahama/Material & Method

From 2013.igem.org

Contents

Material & Method

Material & Method

General protocol

General protocol

CelC

CelC

Inverse PCR

CrdS

CrdS

Cloning of CrdS and Restriction Enzyme

By Koki Tsutsumi

Inverse PCR

TA cloning of CrdS

Ligation of CrdS/pMD20 and Transformation in JM109

Liquid culluture

MiniPrep of CrdS/pMD20

Restriction Enzyme of CrdS/pMD20

Sequence of CrdS/pMD20

PointMutation of CrdS

Gel Purification of CrdS gene’s Front Fragment and Rear Fragment

CrdS gene’s Front Fragment and Rear Fragment Overlap PCR

Gel Purification of CrdS

Adapter PCR of CrdS gene (BioBrick Part)

Brick Part of CrdS Restrict Enzyme,EcoRI and PstI.

Team:Biwako Nagahama/Material &amp; Method

From 2013.igem.org

Contents

Material & Method

Material & Method

General protocol

General protocol

CelC

CelC

Inverse PCR

CrdS

CrdS

Cloning of CrdS and Restriction Enzyme

By Koki Tsutsumi

Inverse PCR

TA cloning of CrdS

Ligation of CrdS/pMD20 and Transformation in JM109

Liquid culluture

MiniPrep of CrdS/pMD20

Restriction Enzyme of CrdS/pMD20

Sequence of CrdS/pMD20

PointMutation of CrdS

Gel Purification of CrdS gene’s Front Fragment and Rear Fragment

CrdS gene’s Front Fragment and Rear Fragment Overlap PCR

Gel Purification of CrdS

Adapter PCR of CrdS gene (BioBrick Part)

Brick Part of CrdS Restrict Enzyme,EcoRI and PstI.

Team:Biwako Nagahama/Material & Method