Team:Heidelberg/Notebook color output
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Revision as of 18:46, 18 October 2009
Multi-color OutputContents
8-3-2009
8-4-2009
8-5-2009
8-6-2009
8-7-2009
8-12-2009
8-14-2009
8-17-2009
8-18-2009
- Digested p31 and a Jet insert with NheI and SpeI. -Ligated both together for 3 hrs at RT. (insert:vector= 1:1, 3:1, 1:3) -Transformed bacteria with ligate and plated them on Amp plates. -Repeated mutagenesis PCR again for (p33, p35, p37, p37-Ras, p41, p43) 8-19-2009
8-20-2009
8-21-2009
8-22-2009
8-24-2009
8-26-2009BBBing of Insertsequences
8-27-2009
8-28-2009BBBing of Insertsequences2.0
8-29-2009BBBing of Insertsequences2.1
8-31-2009BBBing of Insertsequences2.1 (part 2)
9-01-2009BBBing of Insertsequences2.1 (part 3)
9-02-2009Mutagenesis PCR
BBBing of Insertsequences2.1 (part 3)
9-03-2009BBBing of Insertsequences2.1
9-04-2009Mutagenesis PCR of FP/LS
P41 (PstI, primers: 3,4) P37 (PstI, primers: 40,41) P35 (PstI, primers: 53,54) P33 (2nd site:primers 48/48')
9-07-2009Mutagenesis PCR of FP/LS
P41 (PstI, primers: 3,4) P37 (PstI, primers: 40,41) P35 (PstI, primers: 53,54) P33 (2nd site:primers 48/48') --> Seemed to have worked on the gel :) so bacteria were transformed. 9-08-09Mutagenesis PCR of FP/LS
P41 (PstI, primers: 3,4) P37 (PstI, primers: 40,41) P35 (PstI, primers: 53,54) P33 (2nd site:primers 48/48') -This time, ran it with a 1:10 dilution of primers, and in each with 3 different plasmid DNA concentrations (10, 20, 50 ng). Also, control plasmid was run with them and a volume of 15 microlitres was used for transformation, although in protocol provided it is mentioned that only 1micro is needed with supercompetent cells. --> 24hrs later, no colonies are yet present on any of the plates, including the control! *Picked a colony from each of p41, p49, p37 and p35 and grew in corresponding resistance LB. 9-09-2009BBBing 2nd gen. of GFP
Mutagenesis PCR -Plates from Monday's trials were picked. very few colonies for p33-mutax2, p37, p35 but none for p41. -Ran PCR for amplification of Ras and GPI-anchoring signal. 9-10-2009BBBing 2nd gen. of GFP
BBBing 2nd gen. mCherry
BBBing of PolyA
9-11-2009BBBing 2nd gen. of GFP
BBBing 2nd gen. mCherry
BBBing of PolyA
Mutagenesis PCR
--> colonies grew and were picked! 9-12-2009BBBing 2nd gen. of GFP
9-14-2009BBBing 2nd gen. of GFP
BBBing 2nd gen. mCherry
BBbing of inserts (into p49)
--> positive!!! Mutagenesis PCR
- p37 mutants worked but together with other mutations that seem to have arised. need for a test transfection! -p35 mutants worked but with a 2 base deletion. need for a test transfection! -p33 mutants worked but with funny point mutations. need for a test transfection!
-p37 (42/43) -p35 (51/52) -p33 (44/45) Sequencing primer addition to p31: -Ran a PCR using Highannealing program of p31 with 201, 202. -->PCR worked 9-15-2009BBBing 2nd gen. mCherry
Sequencing primer addition to p31 - Digested p31 with EcoRI and PstI. -Digest Purified PCR product with NsiI and Mhe-HF--> too little on gel for a second digest. Must redo with more amounts of PCR product tomorrow. Mutagenesis PCR -Transformed bacteria with 5 micro litre of mutagenesis mix-->nothing grew 9-16-2009Sequencing primer addition to p31 -Did a digest with Mfe-1. -Digest of P31-new looked funny. purified the plasmid and redigested it, because DNA seemed to be a lot and needed to make sure all was digested. 9-17-09-Digested PCR amplicon with Nsi1. -Redigested BB. --> Gel purified amplicon and BB and ligated at 16 degrees overnight. -Prepared Maxiprep cultures of submission plasmid 29-new. 9-18-09-Digested P31-new with EcoRI and PstI to isolate jet insert. -Digested submission plasmid with EcoRI and PstI. -->ligate intron into p29new and jet into p29new. CMV from p48 kept for later use. 9-21-09Biobricking
subm(er)izing:
-Intron -Jet (S1) -PolyA tail -->problem: No sequencing primers available for verification yet, so nothing is assured, but cloning will be resumed with available components. -Nevertheless, used one of the Jet submission plasmids (Jet1) to do the subcloning of a CMV core promoter with the Jet proximal. -->digested S1 with hindIII and NheI Cloning of sequencing primers into p31: -Ligation into p31 didn't work. No more PCR product is left, so ran PCR again.-->worked. -In the meantime, ligation was tried again with different molar ratios (1:1, 1:3, 3:1) --> no colonies grew. Mutagenesis PCR: -Didn't work :((( 9-22-09Biobricking Preps of the Ligations Subm(er)izing: -Ligated CMV-core (from p48) into digested S1. -->Problem: used the undigested plasmid instead of digested plasmid, so this failed. Cloning of sequencing primers into P31: -Transformed ligations from day before --> didn't work - Digested the new PCR product with NsiI and MfeI using two protocols for the sequential digest. I: Digest with Mfe-I HF in buffer 3 (low salt) then add NsiI in buffer 4. II: Digest with Mfe-I, PCR purify and then redigest in NsiI. -Ligated new PCR digest into the old p31. 9-23-09Biobricking Restriction, Purification, Ligation, Transformation of:
Subm(er)izing -Digest SI with HindIII and NheI. -Ligated CMV into SI. -Transformed and Plated BBBed Sar and GPI on Kana plates. (wrong selection, failed!!!) Mutagenesis PCR -One colony grew. Cloning sequencing primers into P31 -Ligated the new PCR product digest into the new p31 digest. 9-24-09Mutagenesis PCR Colonies grew on the 10ng plate of p41 Cloning of sequencing primers into p31 Transformed bacteria with the ligation from the day before. Subm(er)izing - Transformed the CMV/S1 ligation -Replated GPI and Sar BBBed plasmids on Amp. BioBricking Ligation
9-25-09BioBricking Transformation of yesterdays Ligation Ligation of:
Mutagenesis PCR Minipreped picked colonies for p41 (2x). Only one of which grew in LB. Sent for sequencing. Sequencing primers in p31: -minipreped picked colonies. -transformed new ligations. Subm(er)izing: -Minipreped picked clones for S21(Jet core and proximal) -Transformed S2 ligations (CMV core and Jet proximal) !!!Problem: Labels on samples got wiped off during minipreping. Digested all samples with 3 different protocols: 1) EcoRI and PstI: S1 should give an insert of ~200 bps. P41 muta shouldn't be cut. 2) Hind III and NotI: S1 should be digested and so should p41 muta (difference in lenght of backbone and p41 should have a ~500 bp insert) 3)Hind III (same for p31-neu): same as Hind III and NotI but no insert should be detectable. (only linearised fragments of different lenghts). --> Gel showed abnormal mixture of multiple fragments for all digests. Unassociatable with any of the expected plasmids. possible that plates were left too long in incubator and other bacteria grew on plates. 9-26-09Miniprep and testdigest of yesterdays Transformations Transformation of yesterdays Ligations Subm(er)izing: -Made minipreps of: -p37and p34 amplicons in p49 for minipreps of enough DNA to be digested and used for cloning into submission. --> test digest with EcoRI and PstI shows that the plasmids have not the expected insert. Possible that the plates were too overcrowded and the picked colonies were ones that were negative. -Made minipreps of: S2 bacterial suspensions. --> test digest with Hind and PstI shows that the colonies lack the correct insert. Sequencing primers for p31: -Made minipreps of picked colonies. --> Test digest with EcoRI and PstI shows that they have the correct insert. 4 samples were picked for sequencing. 9-27-09Miniprep and testdigest of yesterdays Transformations 28-09-09Transfektion of: * cmv-cherry + PolyA * cmv-myrcherry + PolyA * cmv-kzkcherry + PolyA * cmv-eGFP + PolyA * cmv-kzkeGFP + PolyA * cmv-myrpalm + cherry-PolyA * cmv-myrpalm + kzkcherry-PolyA * cmv-myrpalm + eGFP-PolyA * cmv-myrpalm + kzkeGFP-PolyA * cmv-myrpalm + myrcherry-PolyA Lokalisation of eGFP with myrpalm worked well, unfortunately cherry and kzkcherry did not work Biobricking of : * CMV-NLS-cherry-PolyA * CMV-NLS-kzkcherry-PolyA * CMV-NLS-myrcherry-PolyA * CMV-NLS-eGFP-PolyA * CMV-NLS-kzkeGFPPolyA 30-09-09Subm(er)izing: -Test digested S2 colonies minipreped before with NheI and Hind III to make sure that the digest was negative for reasons got to do with the unfamiliar digestion protocol used. --> Colonies were still negative. -Found BBBed inserts of P37 and P34 amplicons and ligated them into submission plasmid digested with SpeI and PstI. -Re-did the CMV/SI ligation. -Restreaked p29-neu. -Picked more S2 colonies. 01-10-09Transfection of * CMV-NLS-cherry-PolyA * CMV-NLS-kzkcherry-PolyA * CMV-NLS-myrcherry-PolyA * CMV-NLS-eGFP-PolyA * CMV-NLS-kzkeGFPPolyA 29-09-09Transformation of:
* CMV-NLS-cherry-PolyA * CMV-NLS-kzkcherry-PolyA * CMV-NLS-myrcherry-PolyA * CMV-NLS-eGFP-PolyA * CMV-NLS-kzkeGFP-PolyA 01-10-09Transfection of: * CMV-NLS-cherry-PolyA * CMV-NLS-kzkcherry-PolyA * CMV-NLS-myrcherry-PolyA * CMV-NLS-eGFP-PolyA * CMV-NLS-kzkeGFP-PolyA
-Transformed ligations of p37 and p34 amplicons and CMV/SI. -Minipreped the picked colonies of S2 and test digested them with HindIII and PstI and EcoRI and PstI. (negative for insert) -Digested Lars's L and S series of promoters with NheI and PstI. !!!Problem These were not BBBed parts, and needed to be cut with SpeI and HindIII. Needed to gel extract the uncut plasmids since they were the last available without need to plate out glycerol stocks. -Digested Corri's natural promoters with EcoRI and PstI. --> Gel extracted the parts. 02-10-09Transfection result: NLS does not work, as well as mCherry. plasma membrane localized mCherry works.
*cmv-flourophore-NLS Subm(er)izing: -Digested Lars's plasmids with SpeI and HindIII. -Picked colonies for P34 and P37 and CMV ligations in SI. 03-10-09Subemerizing -Minipreped:
-Ran digest of Lars's samples on gel for extraction. --> Gel broke with some of the S series some missing! 05-10-09NLS
06-10-09
07-10-09Time lapse fluorescence movie
*Jet-myrcherry-PolyA *NIIL10-eGFP-PolyA
11-10-09Time lapse fluorescence movie
12-10-09Time lapse fluorescence movie starting acquisition BioBricking of GPI Restriction, Extraction and Ligation to get the following constructs *cmv-GPI-eGFP-PolyA *cmv-eGFP-GPI-PolyA 12-10-09Time lapse fluorescence movie cells disattached after 4 h so there was no usable filmmaterial restart acquisition this evening --> less cells, therefore no acquisition |