@@ Line 1: / Line 1: @@
-{{EPF-Lausanne09}}
-<div CLASS="epfltrick">__TOC__
-</div><div CLASS="epfl09">
-=Wet Lab=
-==July==
-===06.07.09===
-LOVTAP plasmid AND TrpR plasmid were transformed in competent E. Coli following received protocol, and grown overnight (see Lab book for more details).
-<br>One problem: we actually don't know TrpR plasmid resistance, so we tried with three resistances available in the lab: Amp., Kana. and Chl.
-LOVTAP is in a plasmid called pCal-n (see picture below):
-[[Image: pCAL-n.jpg|500px|thumb|center|pCal-n plasmid]]
-<br>Some comments on the plasmid:
-<br>-CBP is a small peptide with which we could purify LOVTAP protein
-<br>-Thrombin target is a nucleotidic sequence that can be recognized by thrombin a peptidase. This peptidase will cut CBP once LOVTAP is purified
-===07.07.09===
-We have to grow the 3 strains generously sent by [mailto:j.beatty@ubc.ca Tom Beatty]
-The three strains are :
-:*''R.Palustris'' CEA001 (wild type) ; should be grown on LB medium only
-:*''R.Palustris'' BPHP1+ ; should be grown on LB with gentamycin (100 micrograms/ml)
-:*''E.Coli'' DH10B (pBPH/hmu0) ; should be grown on LB with gentamycin (20 micorgrams/ml)
-The transformed LOVTAP and TrpR worked well (N.B. the plasmid of TrpR is pUC19 so the antibiotic resistance is Amp -> see below)
-[[Image: RTEmagicC_puc19_2.gif.gif|500px|thumb|center|pUC19 plasmid]]
-We did the glycerol stock, located in the -80 fridge, first floor of the iGEM compartement.
-Then, a miniprep was done with both cultures.
-A LOVTAP plasmid aliquot was done, a TrpR plasmid aliquot was done, located in the -20 fridge, 2nd floor.
-===08.07.09===
-. R. Palustris culture grew. A glycerol stock has been done.
-A pellet is on the fridge level 2, waiting for a miniprep.
-. iGEM parts have been transformed:
-{| class="wikitable" width="80%"
-|+ <big> '''Parts&Characteristics''' </big>
-|-
-! scope=col | Part
-! scope=col | Characteristic
-! scope=col | Resistance
-! scope=col | Well (Kit Plate)
-|-
-| width="33%" |
-[http://partsregistry.org/Part:BBa_B0010 BBa_B0010]
-| width="33%" align="center"|
-Terminator
-| width="33%" align="center" |
-A
-| width="50%" align="center" |
-D (1)
-|-
-| width="33%" |
-[http://partsregistry.org/Part:BBa_R0010 BBa_R0010]
-| width="33%" align="center"|
-Promoter LacI
-| width="34%" align="center" |
-A
-| width="50%" align="center" |
-D (1)
-|-
-| width="33%" |
-[http://partsregistry.org/Part:BBa_B0030 BBa_B0030]
-| width="33%" align="center"|
-RBS
-| width="34%" align="center" |
-A
-| width="50%" align="center" |
-H (1)
-|-
-| width="33%" |
-[http://partsregistry.org/Part:BBa_E0240 BBa_E0240]
-| width="33%" align="center"|
-RBS-GFP-TER
-| width="34%" align="center" |
-A
-| width="50%" align="center" |
-M (1)
-|-
-| width="33%" |
-[http://partsregistry.org/Part:BBa_I13507 BBa_I13507]
-| width="33%" align="center"|
-RBS-mRFP-TER
-| width="34%" align="center" |
-A
-| width="50%" align="center" |
-O (1)
-|-
-| width="33%" |
-[http://partsregistry.org/Part:BBa_J13002 BBa_J13002]
-| width="33%" align="center"|
-pTetR-RBS
-| width="34%" align="center" |
-A
-| width="50%" align="center" |
-B (1)
-|-
-|}
-===09.07.09===
-. Miniprep and isolations of the yesterday transformed plasmids. (cf. [https://2009.igem.org/Team:EPF-Lausanne/Notebook/Wet_Lab#08.07.09 08.09.09 subpart])
-Concentrations of the plasmids: cf. lab notebook pp. 8-9
-. PCR of pCal-n to PCR up LOVTAP with the different primers designed the [https://2009.igem.org/Team:EPF-Lausanne/Notebook/Cloning_Strategy#06.07.09 06.09.09], the products are:
-<br>- Prom_T7-RBS-CBP-LOVTAP
-<br>- RBS-CBP-LOVTAP
-<br>- CBP-LOVTAP
-<br>- LOVTAP
-Result:  Prom_T7-RBS-CBP-LOVTAP didn't worked, the other were ok.
-. An agarose gel was runned to check PCR products
-. PCR products were digested with EcorI and SpeI and [http://partsregistry.org/Part:BBa_B0010 BBa_B0010] (plasmid chosen containing the terminator) was digested with EcorI and XbaI, the digestion products were treated with phosphatase. Then, PCR products were purified.
-Finally, LOVTAP (PCR products) were ligated on [http://partsregistry.org/Part:BBa_B0010 BBa_B0010] (plasmid chosen containing the terminator).
-. Two more iGEM parts have been transformed:
-{| class="wikitable" width="80%"
-|+ <big> '''Parts&Characteristics''' </big>
-|-
-! scope=col | Part
-! scope=col | Characteristic
-! scope=col | Resistance
-! scope=col | Well (Kit Plate)
-|-
-| width="33%" |
-[http://partsregistry.org/Part:BBa_I6007 BBa_I6007]
-| width="33%" align="center"|
-Double repressor: called Inverter TetR
-| width="33%" align="center" |
-A
-| width="50%" align="center" |
-C (2)
-|-
-| width="33%" |
-[http://partsregistry.org/Part:BBa_P1010 BBa_P1010]
-| width="33%" align="center"|
-Death Cassette
-| width="34%" align="center" |
-C
-| width="50%" align="center" |
-E (1)
-|-
-|}
-Remarks: [http://partsregistry.org/Part:BBa_P1010 BBa_P1010], the death gene has to be transformed in ccdB (death gene) resistant cells: One Shot ccdB survival 2T1 E. Coli
-===10.07.09===
-Miniprep of the yesterday transformations were done, glycerol stock of [http://partsregistry.org/Part:BBa_I6007 Inverter TetR (BBa_I6007)] and [http://partsregistry.org/Part:BBa_P1010 Death Cassette (BBa_P1010)] were done and finally they were put at -80°C.
-As Prom_T7-RBS-CBP-LOVTAP PCR product migration on the gel didn't worked (in fact there wasn't enough products) July the 9th, a second PCR was done with more cycles (40) to check wether the the primers were accurately designed.
-Results: The primers are correct -> Prom_T7-RBS-CBP-LOVTAP was correctly amplified.
-A digestion-ligation according iGEM special protocol [[Media:‎ BioBrick_Assembly_Manual.pdf|Biobrick_Assembly_Manual]] was done with LacI and RBS. And Term was digested (with E and X) to linearize the plasmid.
-As [http://partsregistry.org/Part:BBa_I6007 Inverter TetR (BBa_I6007)] and [http://partsregistry.org/Part:BBa_P1010 Death Gene (BBa_P1010)] were transformed with a contaminated SOC, we did a PCR with the isolated plasmids to check if the plasmids were correct.
-Results: [http://partsregistry.org/Part:BBa_P1010 Death Cassette (BBa_P1010)] sample contain the correct plasmid, [http://partsregistry.org/Part:BBa_I6007 Inverter TetR (BBa_I6007)] doesn't.
-Finally, a gel extraction was done to purify the digested [http://partsregistry.org/Part:BBa_B0010 Terminator (BBa_B0010)] (linearized plasmid)
-===13.07.09===
-[http://partsregistry.org/Part:BBa_I6007 Inverter TetR (BBa_I6007)]  was transformed again. And the new plasmid (created on July the 10th, [https://2009.igem.org/Team:EPF-Lausanne/Notebook/Wet_Lab#10.07.09 10.07.09]) LacI-RBS was transformed on DH5-alpha competent cells.
-We failed in purifing our [http://partsregistry.org/Part:BBa_B0010 Terminator (BBa_B0010)], do it again tomorrow, beginning with the digestion, etc.
-===14.07.09===
-The digestion of the [http://partsregistry.org/Part:BBa_B0010 Terminator (BBa_B0010)] was done, in order to purify it once more, using gel extraction.
-Miniprep of LacI-RBS and Inverter TetR, and PCR of the two of them.
-The linearized [http://partsregistry.org/Part:BBa_B0010 Terminator (BBa_B0010)] was runned on an agarose gel and purified with a gel extraction kit.
-Even though linearized [http://partsregistry.org/Part:BBa_B0010 Terminator (BBa_B0010)] concentration was very low, we tried to ligate the previously amplified LOVTAP [https://2009.igem.org/Team:EPF-Lausanne/Notebook/Wet_Lab#09.07.09 (08.07.09)] in linearized [http://partsregistry.org/Part:BBa_B0010 Terminator (BBa_B0010)]
-===15.07.09===
-Miniprep of LacI-RBS (again, because we had a very low concentration yesterday). We obtained a better concentration.
-Transformation of LovTAP-Term (LB + plates).
-LB-Agar plates without antibiotic and with chlorophenicol & Ampicilin have been made.
-===16.07.09===
-Our plates and tubes from yesterday transformation are the same for the negative control and the LovTAP-Term. So either the ligation or the transformation didn't work. Actually we think that it is the transformation, because we put the wrong antibiotics : Chl instead of Amp. As we don't have any ligation products any more, we did the digestion, gel extraction and ligation again.
-We also did a PCR of LacI-RBS product of the second transformation (of 15.07.09), as the concentration for the transformation of 14.07.09 was too low. We then ran the gel.
-===17.07.09===
-===20.07.09===
-==August==
-</div><div CLASS="epfl09bouchon"></div>

Team:EPF-Lausanne/Notebook/Wet Lab

From 2009.igem.org

Latest revision as of 08:05, 28 July 2009