Team:Slovenia/Notebook.html

From 2009.igem.org

(Difference between revisions)

Revision as of 02:42, 22 October 2009

{{SLOtemp| Content=

@@ Line 2: / Line 2: @@
 Content=
 __NOTOC__
-===June 16th, 2009===
-We prepared competent DH5α cells and tested competence of DH5α and DB3.1 cells as follows:
-- DB3.1 with ccdB (incubation on Amp plate)
-- DH5α with p53 (incubation on Kan plate)
-- DH5α with PSBA (incubation on Amp plate)
-- DH5α with PSBK (incubation on Kan plate)
-<br>
-<br>
-We prepared 50 LB mini-prep flasks (10ml),  LB plates with Kan, LB plates with Amp and 4×100ml LB media.
-<br>
-<br>
-===June 17th, 2009===
-We prepared our own competent  DH5α cells.
-We inoculated transformed cells (from the previous day) into 10 mL of LB with antibiotic.
-<br>
-<br>
-===June 18th, 2009===
-We transformed competent cells DH5α with pLUC in order to test the competence.
-We isolated following vectors:
-PSBK_1, PSBK_2, p53_1, p53_2, PSBA_2, ccdB_1 and ccdB_2 and ran them (except vectors with ccdB domain) on agarose gel electrophoresis. Only p53_1 isolation was successful.
-<br>
-<br>
-===June 19th, 2009===
-pET3a and p53 vectors were cut using NdeI/BamHI.
-Three groups of competent DH5α cells were transformed with plasmids M13, pET3 and 7G and then incubated on LB Amp (M13) ad LB Kan plates (pET2 and 7G).
-<br>
-<br>
-===June 22nd, 2009===
-We separated the restriction products (pET3a and p53 vectors, that were cut with NdeI/BamHI) on gel electrophoresis, isolated them from gel using MINElute Extraction Kit and measured their concentrations.
-p53 had not been cut with both mentioned enzymes at the same time, but in a way that we got fragments d53 and dimtetra.
-We inoculated mini-prep flasks with colonies that had grown on Amp and Kan plates from 19th July.
-<br>
-<br>
-===June 23rd, 2009===
-We isolated M13, pET3 and 7G plasmids from over-night culture.
-We purified restriction products d53 and Dimtetra and ligated them into pETa (+ backligation).
-<br>
-<br>
-===June 24th, 2009===
-We transformed DH5α cells with the ligation products made on 23th June.
-<br>
-<br>
-===June 25th, 2009===
-Transformed DH5α cells were inoculated into mini-prep flasks.
-<br>
-<br>
-===June 26th, 2009===
-From transformed DH5α cells we isolated:
-- pET3a containing d53
-- pET3a containing Dimtetra
-and performed control restriction.
-Gel electrophoresis of restriction products revealed that either restriction or ligation was not successful.
-Control restriction was done again, this time successfully. Therefore appropriate d53 and Dimtetra colonies were inoculated into 10 mL of LB+antibiotic in mini-prep flasks.
-<br>
-<br>
-Following primers were ordered:
-T7p-f
-ccdB-MCS-I-T7-p-r
-T7p-MCS-ccdB-f
-His-MCS-II-ccdB-reverse
-His-MCS-II-ccdB-r
-nYFP-r
-nYFP-f
-foldon-f
-foldon-r
-KSI-DP-f
-KSI-DP-r
-YFPc-f
-YFPc-r
-YFPn-mut-f
-YFPn-mut-r
-gyrB-f
-gyrB-r
-LL-37-f
-LL-37-r
-CutA1-f
-CutA1-r
-<br>
-<br>
-===June 29th, 2009===
-We isolated vectors containing d53 and Dimtetra. Gel electrophoresis showed that isolation was successful.
-BL21DE3 pLysS cells (for protein production) were transformed with the isolated vectors.<br>
-Other group of BL21DE3 pLysS cells was inoculated on LB plates with chloramphenicol.
-<br>
-<br>
-We multiplied ccdB domain and p53 monomer with PCR using ccdB-f, ccdB-r, p53-f and p53-r primers.
-<br>
-<br>
-===June 30th, 2009===
-Gel electrophoresis of PCR products (see June 29th).<br>
-BL21DE3 pLysS cells transformed with vectors, containing d53 and Dimtetra, were inoculated.
-}}