Difference between revisions of "Team:Paris Saclay/Notebook/August/26"

(Friday 26th August)
(Lab work)
 
(3 intermediate revisions by one other user not shown)
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= Friday 26<sup>th</sup> August=
 
= Friday 26<sup>th</sup> August=
==Lab work==
+
 
 
===Visualization===
 
===Visualization===
 
====Purification of pPS16-003 and pPS16_004 ligation products====
 
====Purification of pPS16-003 and pPS16_004 ligation products====
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Ligation products pPS16-003 and pPS16_004 frome the [[Team:Paris_Saclay/Notebook/August/25#Visualization|day before]] were purificated according to the usual [[Team:Paris_Saclay/Experiments#Purification_:_PCR_clean-up_with_NucleoSpin_Gel_and_PCR_Clean-up|protocol]]
 
Ligation products pPS16-003 and pPS16_004 frome the [[Team:Paris_Saclay/Notebook/August/25#Visualization|day before]] were purificated according to the usual [[Team:Paris_Saclay/Experiments#Purification_:_PCR_clean-up_with_NucleoSpin_Gel_and_PCR_Clean-up|protocol]]
  
 
 
====Q5 high fidelity PCR of pPS16_003 - pPS16_004 ligation product====
 
====Q5 high fidelity PCR of pPS16_003 - pPS16_004 ligation product====
 
'' By Mathilde ''
 
'' By Mathilde ''
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'' By Mathilde''
 
'' By Mathilde''
  
The purification was made following the usual [[https://2016.igem.org/Team:Paris_Saclay/Experiments#Purification_:_PCR_clean-up_with_NucleoSpin_Gel_and_PCR_Clean-up|protocol]].
+
The purification was made following the usual [[Team:Paris_Saclay/Experiments#Purification_:_PCR_clean-up_with_NucleoSpin_Gel_and_PCR_Clean-up|protocol]].
 
Each of those purification products were quantified on nanodrop.  
 
Each of those purification products were quantified on nanodrop.  
  
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|-
 
|-
 
|1
 
|1
|2
 
|-
 
 
|84,20
 
|84,20
 
|1,25
 
|1,25
 
|1,84
 
|1,84
 
|-
 
|-
 +
|2
 
|169,88
 
|169,88
 
|1,29
 
|1,29
 
|1,83
 
|1,83
 
|}
 
|}
 +
 +
Enough DNA quantity was obtained to perform a Gibson assembly on segments 1 and 2.
 +
 +
====Gibson Assembly of segments 1 and 2====
 +
''By mathilde''
 +
 +
Two preparations were made :
 +
* the 1-2 Gibson assembly product tube : 1,12µL of purified segment 1 and 0,56µL of purified segment 2 +  0,85µL of digested pSB1C3 + 7,47 µL of sterile water + 10µL of NEB Builder Hifi DNA Assembler Master Mix
 +
* the control tube : 0,85µL of digested pSB1C3 + 17,47 µL of sterile water
 +
 +
Gibson products were incubated 1h at 52°c.
 +
 +
====Transformation in DH5α with the 1-2 Gibson assembly product====
 +
''By Mathilde''
 +
 +
The transformation was performed following the usual [[Team:Paris_Saclay/Experiments#Heat_shock_competent_cells|protocol]] with 2µL of plasmid.
 +
* 50, 150 and 350µL of the transformed DH5α with the 1-2 Gibson assembly product were plated on 3 plates of LB + chloramphenicol (30µg/mL)
 +
* 350 µL of each Gibson assembly control and transformation control were plated on 2 plates of B + chloramphenicol (30µg/mL)
 +
 +
Petri cultures were incubated at 37°c overnight.
  
  
 
{{Team:Paris_Saclay/notebook_footer}}
 
{{Team:Paris_Saclay/notebook_footer}}

Latest revision as of 17:00, 9 October 2016


Friday 26th August

Visualization

Purification of pPS16-003 and pPS16_004 ligation products

By Mathilde

Ligation products pPS16-003 and pPS16_004 frome the day before were purificated according to the usual protocol

Q5 high fidelity PCR of pPS16_003 - pPS16_004 ligation product

By Mathilde

The Q5 PCR was conducted following the exact same protocol than the 25/08/2016 on the ligation product from the day before.

Migration Results

The two bands are at the expected size (1860 pb), so the fragment 2 (16-003 and pPS16_004 ligation product) is purified.

Purification of fragments 1(16-001 + pPS16_002) and 2 (16-003 + pPS16_004)

By Mathilde

The purification was made following the usual protocol. Each of those purification products were quantified on nanodrop.

Segment DNA quantity (ng/µL) 260/230 260/280
1 84,20 1,25 1,84
2 169,88 1,29 1,83

Enough DNA quantity was obtained to perform a Gibson assembly on segments 1 and 2.

Gibson Assembly of segments 1 and 2

By mathilde

Two preparations were made :

  • the 1-2 Gibson assembly product tube : 1,12µL of purified segment 1 and 0,56µL of purified segment 2 + 0,85µL of digested pSB1C3 + 7,47 µL of sterile water + 10µL of NEB Builder Hifi DNA Assembler Master Mix
  • the control tube : 0,85µL of digested pSB1C3 + 17,47 µL of sterile water

Gibson products were incubated 1h at 52°c.

Transformation in DH5α with the 1-2 Gibson assembly product

By Mathilde

The transformation was performed following the usual protocol with 2µL of plasmid.

  • 50, 150 and 350µL of the transformed DH5α with the 1-2 Gibson assembly product were plated on 3 plates of LB + chloramphenicol (30µg/mL)
  • 350 µL of each Gibson assembly control and transformation control were plated on 2 plates of B + chloramphenicol (30µg/mL)

Petri cultures were incubated at 37°c overnight.