Team:Paris/10 August 2009

From 2009.igem.org

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*For [https://2009.igem.org/Team:Paris/Freezer_PCR_products#A8 A8]OmpA-Linker and [https://2009.igem.org/Team:Paris/Freezer_PCR_products#A9 A9]pFecA
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*For [https://2009.igem.org/Team:Paris/Freezer_PCR_products#A8 A8] OmpA-Linker and [https://2009.igem.org/Team:Paris/Freezer_PCR_products#A9 A9] pFecA
*Duplicate with and without DMSO
*Duplicate with and without DMSO
**1:98°C 1min
**1:98°C 1min
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<br>
*Ligation 1
*Ligation 1
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**10µl RBS-tet XbaI/PstI
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**10µl RBS-tetR XbaI/PstI
**1µl pSB2K3(pLac) SpeI/PstI
**1µl pSB2K3(pLac) SpeI/PstI
**2µl Buffer T4 DNA Lygase 10x
**2µl Buffer T4 DNA Lygase 10x
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*10min at room temperature (~25?)
*10min at room temperature (~25?)
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*20min at 80°C
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*As usual, but I forget to done transformation with vector only...so I haven't any control... --!
*As usual, but I forget to done transformation with vector only...so I haven't any control... --!
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PCR
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[https://2009.igem.org/Team:Paris/Freezer_PCR_products#A11 A11] (OmpAsignal) [https://2009.igem.org/Team:Paris/Freezer_PCR_products#A12 A12] (Tg3p) [https://2009.igem.org/Team:Paris/Freezer_PCR_products#A13 A13] (TolRII) without (1,2,3) and with DMSO (4,5,6)
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temperature gradient
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tube n°1/4 : 2/5  : 3/6
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A11 : 68,6 : 70,2 : 71,8
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A12 : 62,2 : 62,9 : 64,0
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A13 : 71,8 : 73,1 : 74,0
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Waiting Heigh = A11: 135pb, A12: 274pb, A13: 279pb
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->gel
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[[Image:OmpAsignal_fusion_Nterm.JPG‎]]
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[[Image:Tg3p_fusion_N_term.JPG‎]]
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[[Image:TolRII fusion N term.JPG‎]]
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'''A11(OmpAsignal) and A13(TolRII) good and nothing for A12(Tg3p)'''
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purification with promega kits
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purification on tube n°5 (A11.5 : T°: 70,2 with DMSO and A13.5 : T°73,1 with DMSO)with promega kits
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gel purification -> Very good
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50µl final
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gel purification -> '''Very good'''
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[[Image:purif OmpA signal fusion & tolRII fusion N term.JPG‎]]
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Next : Digestion tomorrow
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Latest revision as of 11:42, 11 August 2009

Contents

NoteBook

June
MTWTFSS
1 2 3 4 5 6 7
8 9 10 11 12 13 14
15 16 17 18 19 20 21
22 23 24 25 26 27 28
29 30
July
MTWTFSS
    1 2 3 4 5
6 7 8 9 10 11 12
13 14 15 16 17 18 19
20 21 22 23 24 25 26
27 28 29 30 31
August
MTWTFSS
          1 2
3 4 5 6 7 8 9
10 11 12 13 14 15 16
17 18 19 20 21 22 23
24 25 26 27 28 29 30
31
September
MTWTFSS
  1 2 3 4 5 6
7 8 9 10 11 12 13
14 15 16 17 18 19 20
21 22 23 24 25 26 27
28 29 30
October
MTWTFSS
      1 2 3 4
5 6 7 8 9 10 11
12 13 14 15 16 17 18
19 20 21 22 23 24 25
26 27 28 29 30 31

← Yesterday - Tomorrow →

August 10th

Brain work

edit please ^^


Lab work

PCR

  • For A8 OmpA-Linker and A9 pFecA
  • Duplicate with and without DMSO
    • 1:98°C 1min
    • 2:98°C 10s
    • 3:59°C for A8) / 65°C for A9 30s
    • 4:72°C 8s
    • 5:72°C 10min
    • 6: 4°C ~

Mini-Prep for Plac

Same Protocol as usual ...

Do for sequencing

Dilution for Plasmids 1,2&3
Plasmid D0(000) D0(266/280) D0(320) Dilution Rule Primer Addition Water Addition
P1 3.10 1.72 0.004 600/310 = 1.93 ~ 2.0 µL 2.45 µL 10.55 µL
P2 1.34 1.34 0.000 600/134 = 4.48 (~ 4.5 µL) 2.45 µL 8.05 µL
P3 0.70 3.39 0.000 600/70 = 8.57 ~ 8.6 µL 2.45µL 3.95µL

Gel Migration

GEL!!!

  • Remigrate to be sure... pFecA seem to be good but not Ompa-Linker

Digestion

  • Digestion of P21 (pLac in pSB2K3) with SpeI/PstI (D12) in order to insert D11 RBS-tet (XbaI/PstI)
    • 20µl of P21
    • Vfinal=50µl
    • 2h at 37°C

Purification

  • Promega kit
    • 50µl final

GEL!!!(strange! none solution fall as quickly in the wholes)

DO260

  • D11: RBS-tet : 0,10µg/ml ~730bp
  • D12: pSB2K3(pLac) : 0,96µl/ml ~4400bp

Try for ligation

  • Ligation between [D12] pSB2K3(pLac) SpeI/PstI and [D11] RBS-tet XbaI/PstI. 20µl final
  • Ligation 1
    • 4,5µl RBS-tet XbaI/PstI
    • 1µl pSB2K3(pLac) SpeI/PstI
    • 2µl Buffer T4 DNA Lygase 10x
    • 1µl T4 DNA Lygase
    • 11,5µl H20


  • Ligation 1
    • 10µl RBS-tetR XbaI/PstI
    • 1µl pSB2K3(pLac) SpeI/PstI
    • 2µl Buffer T4 DNA Lygase 10x
    • 1µl T4 DNA Lygase
    • 6µl H20


  • 10min at room temperature (~25?)
  • 20min at 80°C

Transformation of the ligation

  • As usual, but I forget to done transformation with vector only...so I haven't any control... --!

PCR

A11 (OmpAsignal) A12 (Tg3p) A13 (TolRII) without (1,2,3) and with DMSO (4,5,6)

temperature gradient

tube n°1/4 : 2/5  : 3/6

A11 : 68,6 : 70,2 : 71,8

A12 : 62,2 : 62,9 : 64,0

A13 : 71,8 : 73,1 : 74,0

Waiting Heigh = A11: 135pb, A12: 274pb, A13: 279pb

->gel

OmpAsignal fusion Nterm.JPG


Tg3p fusion N term.JPG


TolRII fusion N term.JPG

A11(OmpAsignal) and A13(TolRII) good and nothing for A12(Tg3p)

Purification

purification on tube n°5 (A11.5 : T°: 70,2 with DMSO and A13.5 : T°73,1 with DMSO)with promega kits

50µl final

gel purification -> Very good

Purif OmpA signal fusion & tolRII fusion N term.JPG

Next : Digestion tomorrow

To do list

Matricule TODO
Luc
Romain
Charlotte
Stoff
Chris
Lisa
Caroline
Souf
Vicard
Pierre modelisation & Algorithmic (a bit...)
Sylvain
Guillaume


← Yesterday - Tomorrow →

Retrieved from "http://2009.igem.org/Team:Paris/10_August_2009"