"

 

From 2008.igem.org

5^th week

go back to 4^th week

go back to the overview

Contents 1 Monday 09/01/2008 1.1 Colicin Receiver 1.1.1 pSB1A3-Receiver-Colicin-Cloning 1.1.2 Activity Test 1.2 Sender part 1.2.1 pBAD-Sender Cloning 1.3 General 2 Tuesday 09/02/2008 2.1 Colicin Receiver 2.1.1 pSB1A3-Receiver-Colicin-Cloning 2.1.2 Activity Test 2.2 Sender part 2.2.1 pBAD-Sender Cloning 2.2.2 Activity Test 3 Wednesday 09/03/2008 3.1 Colicin Receiver 3.1.1 pSB1A3-Receiver-Colicin-Cloning 3.1.2 Activity Test 3.2 Sender part 3.2.1 pBAD-Sender Cloning 4 Thursday 09/04/2008 4.1 Colicin Receiver 4.1.1 pSB1A3-Receiver-Colicin-Cloning 4.1.2 Activity Test 4.2 Sender part 4.2.1 pBAD-Sender Cloning 5 Friday 09/05/2008 5.1 Colicin Receiver 5.1.1 pSB1A3-Receiver-Colicin-Cloning 5.2 Sender part 5.2.1 Activity Test

Monday 09/01/2008

Colicin Receiver

pSB1A3-Receiver-Colicin-Cloning

• Transformationresults of ligation pSB1A3-RecluxpR no colonies
• Retransformation of ligation into TOP 10 -> standard protocoll

Activity Test

• Inoculation of TOP10 ONC for colicin-test next day:
  • +2 ml MG1655
  • +0.002 µg/ml Mytomycin C
  • 2 ml ColE1 unstressed
  • 2 ml ColE1 stressed
  • 2 ml ColE9 unstressed
  • 2 ml ColE9 stressed
• Inoculation for growthcurve measurement over the day (tomorrow):
  • ColE1 unstressed
  • ColE1 stressed
  • ColE9 unstressed
  • ColE9 stressed
  • DH5alpha
  • TOP10
  • MG1655

Sender part

pBAD-Sender Cloning

• Double transformation of pBAD-F1610-9 and AI-2-Sender int TOP 10 and DH5 alphha
• Inoculation of ONC with pBAD-F1610 colony 9 (from glycerolstock)

General

• Preparation of M9 media

[back]

Tuesday 09/02/2008

Colicin Receiver

pSB1A3-Receiver-Colicin-Cloning

• Inoculation of liquid cultures from Transformation of ligation: pSB1A3-RecluxpR.

Activity Test

Sender part

pBAD-Sender Cloning

• Miniprep of pBAD-F1610,9: 179,6 ng/ul; Qiagen Miniprepkit
• Inoculation of liquid cultures from Transformation of double-transformation.

Activity Test

• Results of Colicintest: You can see that stressed Colicin E1 cells are able to kill TOP 10. But this could also be caused by Mytomycin C.
  
• Growthcurve:
  • Inoculation of TOP10s with 1ml/2ml supernatant of:
    • MG1655
    • ColicinE1 unstressed
    • ColicinE1 stressed
    • ColicinE9 unstressed
    • ColicinE9 stressed
  • OD was measured hourly in tecan plate reader
  • New inoculation of same cultures in LB media.

[back]

Wednesday 09/03/2008

Colicin Receiver

pSB1A3-Receiver-Colicin-Cloning

• Minipreps of the ligation ONCsvfrom 02.09.:

concentrations:
  R1: 152,3 ng/ul
  R2: 150,4 ng/ul
  R3: 76,7 ng/ul
  R4: 132,8 ng/ul
  R5: 142,1 ng/ul 
  R6: 138,4 ng/ul
  R7: 136,8 ng/ul
  R8: 187,7 ng/ul

• Controldigestions of ligation with XbaI and SpeI

10.0 µl DNA
 2.0 µl NEBuffer 2
 2.0 µl BamHI
 2.0 µl XbaI
 2.0 µl BSA 10x
 2.0 µl H2o
-------
20.0 µl

• Gel of digestion:
  
• Gelresults: Expected fragments 2150 bp and 1088 bp. The 2150 bp fragments are there but there is a 1500 bp fragment instead of the 1088 bp fragment. Despite this we made some new glycerolstocks.

Activity Test

• Results of growth curve test from yesterday: The results were very diffusing so that we perform this test again.
  
• New hourly growth curve measurement (see Tuesdaysday for details). No significant effect of colicins can be seen. Only Mytomycin C kills the TOP 10 cells very effectively
  

Sender part

pBAD-Sender Cloning

• Minipreps of doubletransformations:

concentrations
  prey_Top10,1: 123,6 ng/ul
  prey_Top10,2: 157,4 ng/ul
  prey_DH5-a,1: 202,0 ng/ul
  prey_DH5-a,2: 174,2 ng/ul

[back]

Thursday 09/04/2008

Colicin Receiver

pSB1A3-Receiver-Colicin-Cloning

• Despite of the strange digestion pattern we try the next step of the cloning.
• PCR of colicins:

25.0 µl Phusion MasterMix
 2.5 µl colE1prot/colE9prot_fw_BamHI
 2.5 µl colE1prot/colE9prot_rv_SpeI
18.0 µl H2O
 2.0 µl DNA templates
-------
50.0 µl

program:
98 °C  30 sec
98 °C  10 sec
59 °C  20 sec
72 °C  45 sec
72 °C   8 min
 4 °C  constant

• PCR purification and analytic gel: Expected fragments are there
  
• Digestion of purified PCR products with BamHI and SpeI: 1h -> 37 °C

Vector:
 6.0 µl DNA
 2.0 µl NEBuffer 2
 2.0 µl SpeI
 2.0 µl BamHI
 2.0 µl BSA10x
 6.0 µl H2O
-------
20.0 µl

Insert:
10.0 µl DNA
 2.0 µl NEBuffer 2
 2.0 µl SpeI
 2.0 µl BamHI
 2.0 µl BSA10x
 2.0 µl H2O
-------
20.0 µl

• Gel & Gelextraction: The expected bands were visible. After cutting we purified them using the Qiagen Gel Extraction Kit.
• Sequencing: Send R1 (LuxR-Receiver) to GATC.
• Inoculation of 4 receiver colonies

Activity Test

• New plans for characterization:
  • Cloning of Colicin proteins into pQE-30 vector for His-Tag purification of colicins. Therefore we designed reverse primers with HindIII (ColE1) and XmaI(ColE9) sites.

Sender part

pBAD-Sender Cloning

• Inoculation of 4 cotransformations for activity tests

Friday 09/05/2008

Colicin Receiver

pSB1A3-Receiver-Colicin-Cloning

• Ligation and Transformation of pRecluxpR with ColE1/ColE9: no results

Sender part

Activity Test

• Activity test over the day: no results

go to 6^th week

• Recent changes
• What links here
• Related changes
• Special pages
• My preferences

• Printable version
• Permanent link
• Privacy policy
• Disclaimers