Team:Osaka/Meeting

From 2009.igem.org

(Difference between revisions)
(Lab protocol)
 
(41 intermediate revisions not shown)
Line 1: Line 1:
-
<div style="width: 120px; margin-left: 30px; float:left;">
+
{{Template:Osaka1}}
-
{|align="center"
+
<div style="width: 700px; margin-left: 200px; float:center;">
-
|[[Image:iGEMOSAKALogo.png|100px|center]]
+
-
|}
+
-
'''References for wiki'''
+
From [[Team:Osaka/Notebook|Notebook]]
-
*[https://2008.igem.org/Team:Chiba/Internal/foredit iGEM2008 Chiba]
+
-
*[https://2009.igem.org/Help:Editing iGEM2009 Help]
+
 +
=Material and Methods=
-
</div>
+
==Preparing CaCl<sub>2</sub>competent cell==
-
 
+
;#Pick a single colony (strain -> Nova Blue) and inoculate 5 ml LB
-
<div style="width: 700px; margin-left: 200px; float:center;">  
+
;#Incubate overnight at 37°C
-
 
+
;#Inoculate 30 ml LB with 1ml of o/n preculture in sterile 100 ml erlenmeyer
-
{| style="color:#000000;background-color:#fff;" cellpadding="3" cellspacing="1" border="1" bordercolor="#fff" width="100%" align="center"
+
;#Incubate culture at 37°C on a shaker up to OD<sub>600</sub>=0.3~0.5 (Measure OD value first 1hr and each 30min)
-
!align="center"|[[Team:Osaka|Home]]
+
;#When the culture reaches an OD<sub>600</sub> between 0.3 and 0.5, transfer the culture into 50 centrifugation tube(sterile)
-
!align="center"|[[Team:Osaka/Team|Team]]
+
;#On ice for 10min
-
!align="center"|[[Team:Osaka/Project|Project]]
+
;#Centrifuge:8krpm,5min,4°C
-
!align="center"|[[Team:Osaka/Parts & Devices|Parts & Devices]]
+
;#Discard supernatant
-
!align="center"|[[Team:Osaka/Notebook|Notebook]]
+
;#Resuspend each pellet in 20 ml chilled '''0.1 M MgCl<sub>2</sub>''' and add further 15 ml 0.1 M MgCl (total 45 ml)
-
<!-- !align="center"|[[Team:Osaka/Deliverable|Deliverable]] -->
+
;#On ice for 10min
-
<!-- !align="center"|[[Team:Osaka/Future Work|Future Work]] -->
+
;#Centrifuge:8krpm,5min,4℃
-
<!-- !align="center"|[[Team:Osaka/Atelier|Atelier]] -->
+
;#Discard supernatant
-
!align="center"|[[Team:Osaka/Links|Links]]
+
;#Resuspend each pellet in 20 ml chilled '''0.1 M CaCl<sub>2</sub>''' and add further 15 ml 0.1 M MgCl (total 45 ml)
-
|}
+
;#On ice 30min
 +
;#Centrifuge:8krpm,5min,4℃
 +
;#Discard supernatant carefuly
 +
;#Resuspend each pellet in 750 µl pre-chilled 0.1 M CaCl<sub>2</sub> and 750 µl pre-chilled 50%(v/v) Glycerol
 +
;#Aliquot 500~100 ul of the mix into sterile microfuge tubes that are pre-chiled at -80℃
 +
;#stock at -80℃
 +
==Transformation of chemical competent cell==
 +
;#Thaw competent cells on ice
 +
;#Mix 2~5 ul pDNA and 100 ul competent cells in 1.5 ml pre-chiled sterile tube
 +
;#On ice for 30min
 +
;#Heat shock 42℃ for 2~1min
 +
;#On ice for 5min
 +
;#Add 900 ul LB
 +
;#Incubate at 37℃ for 1hour (During this, warm plates at 42℃)
 +
;#Harvest cells by centrifuge (14krpm, 1min, r.t.)
 +
;#Discard 900~800 ul of supernatant
 +
;#Resuspend pellet by pipetting
 +
;#Plating all cells on the plate with appropriate antibiotics by glass beads
 +
;#Incubate overnight at 37°C
 +
;#Watch the plate and find colony
-
=2009/04/01=
+
==Plasmid mini prep (QIAprep Spin Miniprep kit)==
 +
;#Pick a single colony from transformed cells and inoculate 5 ml LB with the appropriate selective antibiotics (Amp->5 ul, Kan->25 ul)
 +
;#Incubate overnight at 37°C
 +
;#Harvest the cells by centrifugation 13krpm, 1min, r.t.
 +
;#Resuspend pelleted cells in '''250 ul Buffer P1'''. No cell clumps should be visible after resuspension of the pellet. So, pipetting an vortex well!.P1 buffer must be stocked at 4°C
 +
;#Add '''250 ul Buffer P2''' and inventing the tubes 4-6times
 +
;#Add '''350 ul Buffer N3''' and inventing the tubes 4-6times soon after step 5
 +
;#Centrifuge:15krpm, 10min, 4°C
 +
;#Transfer the supernatants to the Ecospin column (economical..) or QlAprep spin column by pipetting
 +
;#Centrifuge: 13krpm, 1min, r.t.
 +
;#Reapply the flow-through to column for improving yield
 +
;#Centrifuge: 13krpm, 1min, r.t. and discard the flow-through
 +
;#Add '''500 ul Buffer PB''' in column
 +
;#Centrifuge: 13krpm, 1min, r.t. and discard the flow-through
 +
;#Add '''750 ul Buffer PE''' in column
 +
;#Centrifuge: 13krpm, 1min, r.t. and discard the flow-through
 +
;#Centrifuge: 14krpm, 3min, r.t. to remove residual wash buffer. And then, discard the flow-through
 +
;#Place the column in a clean 1.5 ml tube. Add 100~50 ul Buffer EB or sterile water to the center of each column
 +
;#Keep at r.t. for 3~5min
 +
;#Centrifuge:15krpm, 1min
 +
;#stock -30°C
 +
==Restriction Digestion==
 +
For cloning experiments, the final volume should be 20 or 50
</div>
</div>

Latest revision as of 08:02, 11 August 2009

IGEMOSAKALogo.png
References for wiki
iGEM2009 Home
iGEM2008 Chiba
iGEM2009 Help



Home Team Project Parts & Devices Notebook Links


From Notebook

Contents

Material and Methods

Preparing CaCl2competent cell

  1. Pick a single colony (strain -> Nova Blue) and inoculate 5 ml LB
  2. Incubate overnight at 37°C
  3. Inoculate 30 ml LB with 1ml of o/n preculture in sterile 100 ml erlenmeyer
  4. Incubate culture at 37°C on a shaker up to OD600=0.3~0.5 (Measure OD value first 1hr and each 30min)
  5. When the culture reaches an OD600 between 0.3 and 0.5, transfer the culture into 50 centrifugation tube(sterile)
  6. On ice for 10min
  7. Centrifuge:8krpm,5min,4°C
  8. Discard supernatant
  9. Resuspend each pellet in 20 ml chilled 0.1 M MgCl2 and add further 15 ml 0.1 M MgCl (total 45 ml)
  10. On ice for 10min
  11. Centrifuge:8krpm,5min,4℃
  12. Discard supernatant
  13. Resuspend each pellet in 20 ml chilled 0.1 M CaCl2 and add further 15 ml 0.1 M MgCl (total 45 ml)
  14. On ice 30min
  15. Centrifuge:8krpm,5min,4℃
  16. Discard supernatant carefuly
  17. Resuspend each pellet in 750 µl pre-chilled 0.1 M CaCl2 and 750 µl pre-chilled 50%(v/v) Glycerol
  18. Aliquot 500~100 ul of the mix into sterile microfuge tubes that are pre-chiled at -80℃
  19. stock at -80℃

Transformation of chemical competent cell

  1. Thaw competent cells on ice
  2. Mix 2~5 ul pDNA and 100 ul competent cells in 1.5 ml pre-chiled sterile tube
  3. On ice for 30min
  4. Heat shock 42℃ for 2~1min
  5. On ice for 5min
  6. Add 900 ul LB
  7. Incubate at 37℃ for 1hour (During this, warm plates at 42℃)
  8. Harvest cells by centrifuge (14krpm, 1min, r.t.)
  9. Discard 900~800 ul of supernatant
  10. Resuspend pellet by pipetting
  11. Plating all cells on the plate with appropriate antibiotics by glass beads
  12. Incubate overnight at 37°C
  13. Watch the plate and find colony

Plasmid mini prep (QIAprep Spin Miniprep kit)

  1. Pick a single colony from transformed cells and inoculate 5 ml LB with the appropriate selective antibiotics (Amp->5 ul, Kan->25 ul)
  2. Incubate overnight at 37°C
  3. Harvest the cells by centrifugation 13krpm, 1min, r.t.
  4. Resuspend pelleted cells in 250 ul Buffer P1. No cell clumps should be visible after resuspension of the pellet. So, pipetting an vortex well!.P1 buffer must be stocked at 4°C
  5. Add 250 ul Buffer P2 and inventing the tubes 4-6times
  6. Add 350 ul Buffer N3 and inventing the tubes 4-6times soon after step 5
  7. Centrifuge:15krpm, 10min, 4°C
  8. Transfer the supernatants to the Ecospin column (economical..) or QlAprep spin column by pipetting
  9. Centrifuge: 13krpm, 1min, r.t.
  10. Reapply the flow-through to column for improving yield
  11. Centrifuge: 13krpm, 1min, r.t. and discard the flow-through
  12. Add 500 ul Buffer PB in column
  13. Centrifuge: 13krpm, 1min, r.t. and discard the flow-through
  14. Add 750 ul Buffer PE in column
  15. Centrifuge: 13krpm, 1min, r.t. and discard the flow-through
  16. Centrifuge: 14krpm, 3min, r.t. to remove residual wash buffer. And then, discard the flow-through
  17. Place the column in a clean 1.5 ml tube. Add 100~50 ul Buffer EB or sterile water to the center of each column
  18. Keep at r.t. for 3~5min
  19. Centrifuge:15krpm, 1min
  20. stock -30°C

Restriction Digestion

For cloning experiments, the final volume should be 20 or 50

Retrieved from "http://2009.igem.org/Team:Osaka/Meeting"