Difference between revisions of "Part:BBa K1096002:Design"

 
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Sequence obtained from E.coli K-12 genome
 
Sequence obtained from E.coli K-12 genome
 +
 +
==2016 iGEM Tokyo_Tech
 +
===Materials and Methods===
 +
 +
====Construction====
 +
-Strain
 +
 +
All the plasmids were prepared in XL1-Blue strain.
 +
 +
=====Ⅰ.Adjustment of MazF Expression=====
 +
 +
-Plasmids
 +
 +
GFP :  Pcon - <i>rbs</i> - <i>gfp</i> (pSB6A1), Plac - <i>rbs</i> (pSB3K3)<br>
 +
 +
MazF : PBAD - <i>rbs - mazF - tt</i> - Pcon - <i>rbs - gfp</i> (pSB6A1), Plac - <i>rbs</i> (pSB3K3)
 +
 +
=====Ⅱ.<i>mazEF</i> System Assay ~Stop & GO~=====
 +
 +
-Plasmids
 +
 +
vector : PBAD - <i>rbs</i> (pSB6A1), Plac - <i>rbs</i> (pSB3K3)
 +
 +
GFP : Pcon - <i>rbs - gfp</i> (pSB6A1), Plac - <i>rbs</i> (pSB3K3)
 +
 +
MazF + MazE : PBAD - <i>rbs - mazF - tt</i> - Pcon - <i>rbs - gfp</i> (pSB6A1), Plac - <i>rbs - mazE</i> (pSB3K3)
 +
 +
MazF : PBAD - <i>rbs - mazF - tt</i> - Pcon - <i>rbs - gfp</i> (pSB6A1), Plac - <i>rbs</i> (pSB3K3)
 +
 +
=====Ⅲ.<i>mazEF</i> System Assay ~Go & Stop~=====
 +
 +
-Plasmids
 +
 +
vector : PBAD - <i>rbs</i>(pSB6A1), Plac - <i>rbs</i> (pSB3K3)
 +
 +
GFP : Pcon - <i>rbs - gfp</i> (pSB6A1), Plac - <i>rbs</i>(pSB3K3)
 +
 +
MazF + MazE(weak) : PBAD - <i>rbs - mazF - tt</i> - Pcon - <i>rbs - gfp</i> (pSB6A1), Pcon - <i>rbs</i>(weak) - <i>mazE</i> (pSB3K3)
 +
 +
MazF + MazE : PBAD - <i>rbs - mazF - tt</i> - Pcon - <i>rbs - gfp</i> (pSB6A1), Pcon - <i>rbs - mazE</i> (pSB3K3)
 +
 +
MazF : PBAD - <i>rbs - mazF - tt</i> - Pcon - <i>rbs - gfp</i> (pSB6A1), vector (pSB3K3)
 +
 +
=====Ⅳ.Control of Cell Growth=====
 +
 +
-Plasmid
 +
 +
vector : PBAD - <i>rbs</i> (pSB6A1), Plac - <i>rbs</i> (pSB3K3)
 +
 +
MazF + MazE : PBAD - <i>rbs - mazF</i> (pSB6A1), Plac - <i>rbs - mazE</i> (pSB3K3)
 +
 +
MazF : PBAD - <i>rbs - mazF</i>(pSB6A1), Plac - <i>rbs</i> (pSB3K3)
 +
 +
====Assay protocol====
 +
=====Ⅰ.Adjustment of MazF Expression=====
 +
 +
 +
======Pre-culture======
 +
1)Suspend colonies on a master plate into LB medium containing ampicillin (50 microg / mL) and kanamycin (50 microg / mL).
 +
 +
2)Incubate with vigorous shaking for 12 h.
 +
 +
======Incubation and Assay======
 +
1)Measure the turbidity of the pre-cultures.
 +
 +
2)Dilute the pre- cultures to 1 / 30 into LB medium containing 4 mL ampicillin and kanamycin.
 +
 +
3)Incubate with vigorous shaking so that the turbidity becomes 0.03.
 +
 +
4)Add arabinose so that the final concentration becomes 0.2%, 0.02%, 0.002% 0.0002% and 0%.
 +
 +
5)Incubate with vigorous shaking for 24 h, and measure the turbidity and the RFU of GFP.
 +
 +
=====Ⅱ.<i>mazEF</i> System Assay ~Stop & GO~=====
 +
======Pre-culture======
 +
1)Suspend colonies on a master plate into LB medium containing ampicillin (50 microg / mL) and kanamycin (50 microg / mL).
 +
 +
2)Incubate with vigorous shaking for 12 h.
 +
 +
======Incubation and Assay======
 +
1)Measure the turbidity of the pre-cultures.
 +
 +
2)Dilute the pre- cultures to 1 / 30 into LB medium containing 4 mL ampicillin and kanamycin.
 +
 +
3)Incubate with vigorous shaking so that turbidity becomes 0.03.
 +
 +
4)Add arabinose so that the final concentration becomes 0.02%.
 +
 +
5)Add IPTG until the concentration becomes 2 mM after adding arabinose.
 +
 +
6)Incubate with vigorous shaking for 24 h, and measure turbidity and RFU of GFP at the proper time.
 +
 +
=====Ⅲ.<i>mazEF</i> System Assay ~Go & Stop~=====
 +
======Pre-culture======
 +
1)Suspend colonies on a master plate into LB medium containing ampicillin (50 microg / mL) and kanamycin (50 microg / mL).
 +
 +
2)Incubate with vigorous shaking for 12 h.
 +
 +
======Incubation and Assay======
 +
1)Measure the turbidity of the pre-cultures.
 +
 +
2)Dilute the pre- cultures to 1 / 30 into LB medium containing 4 mL ampicillin and kanamycin.
 +
 +
3)Incubate with vigorous shaking so that the turbidity becomes 0.03.
 +
 +
4)Add arabinose so that the final concentration becomes 0.02%.
 +
 +
5)Incubate with vigorous shaking for 24 h, and measure the turbidity and the RFU of GFP at proper times.
 +
 +
=====Ⅳ.Control of Cell Growth=====
 +
1)Making LB agar medium(see Table 1.).<br>
 +
[[Image:Agar medium.jpg|center|600px]]<br>
 +
[[Image:Tokyo Tech1.png|thumb|center|600px|Fig. 1. Procedure of experiment]]<br>
 +
2)<i>E. coli</i> are applied at 3 agar medium (in arabinose, in IPTG, in arabinose and IPTG)(Fig. 1.).
 +
 +
3)Overnight culture at 37°C for 24 h.
 +
 +
4)To confirm TA system, inoculate colonies of <i>E. coli</i> having plasmids at agar medium containing arabinose and IPTG.
 +
 +
5)Overnight culture at 37°C for 24 h.
 +
 +
6)Inoculate colonies of <i>E. coli</i> into agar medium containing arabinose.
 +
 +
7)Overnight culture at 37°C for 24 h.
 +
 +
8)Inoculate colonies of <i>E. coli</i> into agar medium in arabinose and IPTG.
 +
 +
9)Overnight culture at 37°C for 24 h.
  
 
===References===
 
===References===
 +
1)Hazan, R., B. Sat, and H. Engelberg-Kulka. <i>Escherichia coli mazEF</i> mediated cell death is triggered by various stressful conditions. J. Bacteriol.186:3663–3669.

Revision as of 15:05, 19 October 2016


MazF protein (E. coli)


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    COMPATIBLE WITH RFC[12]
  • 21
    COMPATIBLE WITH RFC[21]
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    COMPATIBLE WITH RFC[25]
  • 1000
    COMPATIBLE WITH RFC[1000]


Design Notes

-


Source

Sequence obtained from E.coli K-12 genome

==2016 iGEM Tokyo_Tech

Materials and Methods

Construction

-Strain

All the plasmids were prepared in XL1-Blue strain.

Ⅰ.Adjustment of MazF Expression

-Plasmids

GFP : Pcon - rbs - gfp (pSB6A1), Plac - rbs (pSB3K3)

MazF : PBAD - rbs - mazF - tt - Pcon - rbs - gfp (pSB6A1), Plac - rbs (pSB3K3)

Ⅱ.mazEF System Assay ~Stop & GO~

-Plasmids

vector : PBAD - rbs (pSB6A1), Plac - rbs (pSB3K3)

GFP : Pcon - rbs - gfp (pSB6A1), Plac - rbs (pSB3K3)

MazF + MazE : PBAD - rbs - mazF - tt - Pcon - rbs - gfp (pSB6A1), Plac - rbs - mazE (pSB3K3)

MazF : PBAD - rbs - mazF - tt - Pcon - rbs - gfp (pSB6A1), Plac - rbs (pSB3K3)

Ⅲ.mazEF System Assay ~Go & Stop~

-Plasmids

vector : PBAD - rbs(pSB6A1), Plac - rbs (pSB3K3)

GFP : Pcon - rbs - gfp (pSB6A1), Plac - rbs(pSB3K3)

MazF + MazE(weak) : PBAD - rbs - mazF - tt - Pcon - rbs - gfp (pSB6A1), Pcon - rbs(weak) - mazE (pSB3K3)

MazF + MazE : PBAD - rbs - mazF - tt - Pcon - rbs - gfp (pSB6A1), Pcon - rbs - mazE (pSB3K3)

MazF : PBAD - rbs - mazF - tt - Pcon - rbs - gfp (pSB6A1), vector (pSB3K3)

Ⅳ.Control of Cell Growth

-Plasmid

vector : PBAD - rbs (pSB6A1), Plac - rbs (pSB3K3)

MazF + MazE : PBAD - rbs - mazF (pSB6A1), Plac - rbs - mazE (pSB3K3)

MazF : PBAD - rbs - mazF(pSB6A1), Plac - rbs (pSB3K3)

Assay protocol

Ⅰ.Adjustment of MazF Expression
Pre-culture

1)Suspend colonies on a master plate into LB medium containing ampicillin (50 microg / mL) and kanamycin (50 microg / mL).

2)Incubate with vigorous shaking for 12 h.

Incubation and Assay

1)Measure the turbidity of the pre-cultures.

2)Dilute the pre- cultures to 1 / 30 into LB medium containing 4 mL ampicillin and kanamycin.

3)Incubate with vigorous shaking so that the turbidity becomes 0.03.

4)Add arabinose so that the final concentration becomes 0.2%, 0.02%, 0.002% 0.0002% and 0%.

5)Incubate with vigorous shaking for 24 h, and measure the turbidity and the RFU of GFP.

Ⅱ.mazEF System Assay ~Stop & GO~
Pre-culture

1)Suspend colonies on a master plate into LB medium containing ampicillin (50 microg / mL) and kanamycin (50 microg / mL).

2)Incubate with vigorous shaking for 12 h.

Incubation and Assay

1)Measure the turbidity of the pre-cultures.

2)Dilute the pre- cultures to 1 / 30 into LB medium containing 4 mL ampicillin and kanamycin.

3)Incubate with vigorous shaking so that turbidity becomes 0.03.

4)Add arabinose so that the final concentration becomes 0.02%.

5)Add IPTG until the concentration becomes 2 mM after adding arabinose.

6)Incubate with vigorous shaking for 24 h, and measure turbidity and RFU of GFP at the proper time.

Ⅲ.mazEF System Assay ~Go & Stop~
Pre-culture

1)Suspend colonies on a master plate into LB medium containing ampicillin (50 microg / mL) and kanamycin (50 microg / mL).

2)Incubate with vigorous shaking for 12 h.

Incubation and Assay

1)Measure the turbidity of the pre-cultures.

2)Dilute the pre- cultures to 1 / 30 into LB medium containing 4 mL ampicillin and kanamycin.

3)Incubate with vigorous shaking so that the turbidity becomes 0.03.

4)Add arabinose so that the final concentration becomes 0.02%.

5)Incubate with vigorous shaking for 24 h, and measure the turbidity and the RFU of GFP at proper times.

Ⅳ.Control of Cell Growth

1)Making LB agar medium(see Table 1.).

Agar medium.jpg

Fig. 1. Procedure of experiment

2)E. coli are applied at 3 agar medium (in arabinose, in IPTG, in arabinose and IPTG)(Fig. 1.).

3)Overnight culture at 37°C for 24 h.

4)To confirm TA system, inoculate colonies of E. coli having plasmids at agar medium containing arabinose and IPTG.

5)Overnight culture at 37°C for 24 h.

6)Inoculate colonies of E. coli into agar medium containing arabinose.

7)Overnight culture at 37°C for 24 h.

8)Inoculate colonies of E. coli into agar medium in arabinose and IPTG.

9)Overnight culture at 37°C for 24 h.

References

1)Hazan, R., B. Sat, and H. Engelberg-Kulka. Escherichia coli mazEF mediated cell death is triggered by various stressful conditions. J. Bacteriol.186:3663–3669.