Team:Potsdam Bioware/Lab/Labjournal/June

From 2012.igem.org

(Difference between revisions)
(2012-06-14)
 
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<p style="background-color: rgb(238, 221, 130); font-weight: bold;">Topic: Primer design - Cloning: Sortase-Tag an VP2 + PCR for VP2 with Kozak-sortase_tag-myc_tag </p>
<p style="background-color: rgb(238, 221, 130); font-weight: bold;">Topic: Primer design - Cloning: Sortase-Tag an VP2 + PCR for VP2 with Kozak-sortase_tag-myc_tag </p>
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<b>Investigators:</b> Kathi, Laura, Tobias, Xenia <br>
+
<b>Investigators:</b> Kathi, Laura, Tobias and Xenia <br>
<b>Aim:</b>
<b>Aim:</b>
-
Change primer of 2012-06-07, generate primers for the cmv region + cmv-suffix with SpeI restriction site, include XbalI restriction site in VP2-prefix include myc-tag<br>
+
Change primer of 2012-06-07, generate primers for the cmv region + cmv-suffix with SpeI restriction site, include XbaI restriction site in VP2-prefix include myc-tag<br>
<b>Materials:</b>
<b>Materials:</b>
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* Kozak-sequence: gccgcc
* Kozak-sequence: gccgcc
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* restriction sites: SpeI and XbalI <br>
+
* restriction sites: SpeI and XbaI <br>
<b>Method:</b> Geneious <br>
<b>Method:</b> Geneious <br>

Latest revision as of 19:10, 25 September 2012



Contents

AID-Group

1st Labday 2012-06-09

Topic: Planing the wildtype AID construct (BBa_K929000)

Investigators: Tom S., Chris, Basia, Rico, Mario, Kevin


Aim: planing the construction of the wildtype AID in pSB1C3


Material: Genious


Results:

  • pSB1C3 with CMV -> (cut with SpeI and PstI) 2715 bp (CMV insert+backbone) + 18 bp (rest)
  • pSB1A3 with AID -> (cut with XbaI and PstI) 626 bp (AID insert) + 2061 bp (backbone)
  • pSB1C3 with hGH -> (cut with XbaI and PstI) 505 bp (hGH insert) + 2053 bp (backbone)

AID_Wirkorte


Further tasks:

  • practice part

Topic: Planing the modified AID construct (BBa_K929002)

Investigators: Tom S., Chris, Basia, Rico, Mario, Kevin


Aim: planing the modified AID with Kozak sequence, NLS and without NES, Primer design


Material: Genious


Results:

UP12 superAID.JPG

  • reverse primer without NES


Further tasks:

  • design of the forward primer
  • design of the practice part

2012-06-24

Topic: Preparation of overnight culture of E. coli strain XL-1 Blue

Investigators:

Basia

Aim:

preparation of competent cells of E. coli strain XL-1 Blue


Materials:

LB Medium, Tetracycline, XL-1 Blue stock


Method:

Competent E. coli -> Standard protocols


Results:

culture grew


Further tasks:

further preparation of competent cells with MgCl2 and CaCl2.


2012-06-25

Topic: making competent XL1 Blue E. coli

Investigators:

Sascha, Maria, Tarek, Chris

Aim:

get competent E. coli Xl1 Blue


Materials:

CaCl2, Glycerol, overnight culture


Method:

Competent E. coli -> Standard protocols


Results:

  • ca. 80 (100 µL) Stocks frozen competent E. coli XL1 Blue
  • location: competent E. coli Xl1 Blue in -80°C Freezer

Further tasks:

  • testing ability for transformation of competent cells

2012-06-27

Topic: Picking clones/start overnight culture: AID(BBa_K103001); start overnight culture with pcdna5/ftr

Investigators:

Chris, Mario

Aim:

Picking clones/start 5 mL culture: 2 * 5 mL, 1*20 mL for Miniprep AID(BBa_K103001) & glycerolstock; 1 * 5 mL (Plasmid Sascha:pcdna5/frt) per competent cell line ("good", "bad" and "AG")


Materials:

E. coli colonies from agar-plates (antibiotic: Amp), test tubes+ 5 mL LB+1:1000 AMP, 37 °C shaker


Method:

picking clones, inoculate in 5 mL fresh LB-media with Ampicilin (1:1000), incubation over night


Results:

ready for Miniprep: 2*5 mL and 1*20 mL E. coli XL1 with AID(BBa_K103001); 1 * 5 mL (Plasmid Sascha:pcdna5/frt) per competent cell line ("good", "bad" and "AG")

  • location: incubator 37 °C

Further tasks:

  • Preparation of glycerol stocks (one of XL1 with AID (BBa_K103001), one of XL1 with pcdna5/frt)
  • Miniprep Thursday 28.06.2012

2012-06-28

Topic: MiniPrep of AID(BBa_K103001) and pcdna5/frt + preparation of cryostocks of the cells

Investigators:Basia


Aim:

Miniprep & glycerol stock AID(BBa_K103001); Miniprep and cryostock of pcdna5/frt per competent cell line ("good", "bad" and "AG")



Materials:

Cells grown in test tubes, Miniprep Kit, glycerin, centrifuge



Method:

Glycerol stock: 500 µL of 100 % Glycerin + 500 µL of the liquid overnight culture

MiniPrep: according to the manual



Results:

ready plasmids AID(BBa_K103001) and pcdna5/frt per competent cell line ("good", "bad" and "AG")

  • location: Plasmids: AID(BBa_K103001)- 4th drawer in the -20 °C freezer, pcdna5/frt per competent cell line ("good", "bad" and "AG")-2nd drawer in the -20 °C freezer

Glycerolstocks-box in -80 °C freezer marked with the green tape with a label(BM 28.6.2012, iGEM, AID, pcdna5/FRT)


Further tasks:

Gel electrophoresis for AID to check if it is intact.

Antikörper

2012-06-11

Topic: Culture of CHO-Flp-In Cells

Investigators: Stefan, Tarek


Aim: Thawing of CHO-Flp-In Cells


Date/Time: 2012-06-11,11-20:00


Materials:

  • Cryostock of CHO-Flp-In Cells
  • Complete Medium (Ham´s F12 + 10% FBS + 1% Pen/Strep + 2 mM L-Glutamin)
  • Zeocin
  • 75 cm² culture flask


Method:

Growth and Maintenance of Flp-In Cell Lines (Invtrogen):

  • incubation of thawed cells in 12 ml complete medium without Zeocin for 3h
  • change of medium (get rid of DMSO) and incubation overnight 37°C , 5% CO2


Results:

  • 1x 75cm² culture flask with attached cells


Further tasks:

  • change medium against medium with 100 µg/ml Zeocin (done on 2012-06-12)
  • change medium after 2-3 days (done on 2012-06-14)
  • get the cells to 80-90% confluence (daily check) for splitting

2012-06-13

Topic: Plasmid DNA Purification

Investigators: Kerstin, Maria


Aim: Purification of Plasmids pFRT/lacZeo,pcDNA5/FRT, pOG44


Date/Time: 2012-06-13,12:00-14.00


Materials: Macherey-Nagel Purification Kit

  • E.coli XL-1 blue culture transformed with pFRT/lacZeo, pcDNA5/FRT, pOG44
  • 2 clones of each plasmid
  • 2 ml of each culture taken


Method: Plasmid purification (Miniprep)

Protocol-at-a-glance (Macherey-Nagel)

  • pellet of 2 ml from each culture

variation: centrifugation steps 1 min instead of 30 sec



Results:

Plasmids pFRT/lacZeo, pcDNA5/FRT, pOG44

  • location: freezer -20°, Box2


Further tasks:

  • measurement of DNA concentration
  • control with restriction digest

2012-06-15

Topic: Culture of CHO-Flp-In Cells

Investigators: Tarek


Aim: Splitting of CHO-Flp-In Cells


Date/Time: 2012-06-15, 14-16:00


Materials:

  • 1 x 75 cm² flask with confluent CHO-Flp-In Cells
  • 8 x 75 cm² culture flasks
  • complete Medium with Zeocin
  • PBS
  • Trypsin/EDTA


Method:

Growth and Maintenance of Flp-In Cell Lines (Invitrogen):

  • remove medium and wash the cells with 10 ml PBS
  • Add 2 ml Trypsin/EDTA solution (ca. 3 min ´til the cells detached)
  • Add 8 ml of complete medium (+Zeocin), and briefly resuspend the cells
  • 1 x 2 ml of the cellsuspension in 13 ml complete medium (1:5 splitting)
  • 7 x 1 ml of the cellsuspension in 14 ml complete medium (1:10 splitting)
  • incubation 37°C, 5% CO2


Results:

  • 1 x 1:5 CHO-Flp-In Cells
  • 7 x 1:10 CHO-Flp-In Cells

Further tasks:

  • get the cells to 90% confluence
  • freezing cells

2012-06-19

Topic: Culture of CHO-Flp-In Cells

Investigators: Stefan, Tarek


Aim: Freezing and passaging cultured CHO-Flp-In Cells


Date/Time: 2012-06-19, 10-12:00


Materials:

  • confluent CHO-Flp-In Cells
  • Complete Medium
  • Freezing Medium (90% Complete Medium + 10% DMSO)
  • PBS
  • Trypsin/EDTA
  • Neubauerzählkammer
  • Falcon-tubes (15ml + 50ml)


Method:

Growth and Maintenance of Flp-In Cell Lines (Invitrogen);

Freezing Cells:

  • prepare 20 ml of Freezing medium; label cryovials
  • trypsinate the cells (like 2012-06-15); 5 x 75 cm² flasks
  • counting the cells in Neubauerzählkammer = 2,3 x 10e6/ml = 2,3 x 10e7/flask = 5 Cryostocks per flask á 4,6 x 10e6 cells (min 3 x 10e6 cells/ml)
  • centrifugate the cells in two 50 ml falcon tubes (á 25 ml) and aspirate off the medium
  • resuspend the cellpellets in 10 ml freezing medium
  • add 1 ml cell suspension into one cryovial (x20)
  • place the vials in a styroporbox and freeze them in -80°C Freezer
  • passaging cells (2 x 75 cm² flasks) was done like on 2012-06-15


Results:

  • 19 cryovials with CHO-Flp-In Cells
  • 2 x 1:10 CHO Flp-In Cells

Further tasks:

  • reactivate one cryostock

2012-06-20

Topic: Culture of CHO-Flp-In Cells

Investigators: Tarek


Aim: Reactivate/Thawing CHO-Flp-In Cryostock


Date/Time: 2012-06-20, 12-13


Materials:

  • Cryostock of CHO-Flp-In Cells
  • Complete Medium (Ham´s F12 + 10% FBS + 1% Pen/Strep + 2 mM L-Glutamin)
  • Zeocin
  • 75 cm² culture flask


Method:

Growth and Maintenance of Flp-In Cell Lines (Invitrogen):


changes to 2012-06-11:

  • resuspend the thawed cells in 12 ml complete medium and centrifugate (to save 3h), 250 g, 5 min, RT
  • aspirate off the medium
  • resuspend the cells in complete medium (5ml)
  • place the resuspended cells in a culture flasks with 10ml complete medium + 15 µl Zeocin


Results:

  • 1 x 75 cm² flasks with reactivated crystock of CHO-Flp-In Cells

Further tasks:

  • change medium
  • get reactivated cryostock to confluence
  • splitting cells
  • freeze second charge of cells

2012-06-22

Topic: Culture of CHO-Flp-In Cells

Investigators: Tarek


Aim: Splitting Cells for 2nd freezing charge


Date/Time: 2012-06-22, 15-16:00


Materials:

  • confluent CHO-Flp-In Cells (reactivated cryostock)
  • 5 x 75 cm² culture flasks
  • complete medium + Zeocin
  • PBS
  • Trypsin/EDTA


Method:

like 2012-06-15


Results:

  • 5 x 75 cm² CHO-flp-In Cells

Further tasks:

  • get cells 90% confluence
  • freeze cells

2012-06-22

Topic: Planning the antibody construct

Investigators: Maria, Sascha


Aim: Draft for gene construct, searching appropriate Fc-part


Date/Time: 2012-06-22, 14:00 - 16:30


Materials:

  • Databases
  • Paper


Method:

reviewing of sequences



Results:

  • nucleotide sequence of human C-kappa1 gene


Further tasks:

  • further search for sequences

2012-06-27

Topic: Planning the antibody construct

Investigators: Sascha, Maria


Aim: Draft for gene construct


Date/Time: 2012-06-28,17:30-23:45


Materials:

  • Databases
  • Geneious
  • Paper


Method:

Planning and reviewing of sequence



Results:

  • antibody construct with exon/intron structure


Further tasks:

  • meeting with Dr. Kappel (Monday) and Prof. Lenhard (Wednesday) for clarification of exon/intron structure
  • further control
  • ordering of gene synthesis

Topic: Primer-Design for GATC-sequencing of pcDNA5-FRT and pOG44; vectors for stable transfection

Investigators: Sascha, Maria, Tarek


Aim: Primer-Design for pcDNA5-FRT and pOG44


Materials:

  • lablife: sequences of invitrogen vectors pcDNA5-FRT and pOG44
  • Oligocalc to calculate Tm of primers based on GATC-requirements
  • Geneious

Results:

  • forward-primer for CMV-promotor in pcDNA5-FRT and pOG44
  • reverse-primer for pcDNA5-FRT in hygromycin at N-terminus
  • reverse-primer for pOG44 in N-terminus of flp-gene


Further tasks:

  • ordering of primers at GATC
  • preparation of pcDNA5-FT, pOG44 and ordered primers based on requirements of GTAC

Virus

2012-06-07

Topic: Primer design -Cloning: Sortase-Tag an VP2 + PCR for VP2 with Kozak-sortase_tag-myc_tag

Investigators: Kathi, Laura, Tobias, Xenia

Aim: Primer design of VP2 region

Materials:

  • Vector:P10_pSB1C3_001_CMV_DARPin_ML_VP2/3_587KO_6xHis
  • Sortase-sequence: amino acid sequence: LTAPG translated to gene sequence: CTTACAGCCCCAGGA
  • restriction sites: NgoMIV

Method: Geneious

Results:

  • f_Primer_preNgoMIV+SortaseMotiv1+VP2
  • r_Primer_VP2_1

Further tasks:

  • check the primer

Changes:

  • primer for cmv region:
  • include restriction sites SpeI and XbalI, remove NgoMIV

2012-06-14

Topic: Primer design - Cloning: Sortase-Tag an VP2 + PCR for VP2 with Kozak-sortase_tag-myc_tag

Investigators: Kathi, Laura, Tobias and Xenia

Aim:

Change primer of 2012-06-07, generate primers for the cmv region + cmv-suffix with SpeI restriction site, include XbaI restriction site in VP2-prefix include myc-tag

Materials:

  • Vector:P10_pSB1C3_001_CMV_DARPin_ML_VP2/3_587KO_6xHis
  • Sortase-sequence: amino acid sequence: LTAPG translated to gene sequence: CTTACAGCCCCAGGA
  • Kozak-sequence: gccgcc
  • restriction sites: SpeI and XbaI

Method: Geneious

Results:

  • f_Primer_preXba1 with overhang of: kozak+SortaseMotiv1+myc-tag+VP2 (forward primer)
  • r_Primer_VP2_1 (reverse primer)
  • f_Primer_XbaI+cmv (forward primer)
  • r_Primer_CMV+suf (reverse primer)
  • location: directory: VIRUS/complete

Further tasks:

  • control
  • improvements
  • order

2012-06-19

Topic: Primer design - Cloning: Sortase-Tag linked on VP2 + PCR for VP2 with Kozak-sortase_tag-myc_tag

Investigators: Kathi, Laura, Tobias, Xenia

Aim: change primers of 2012-06-14

Materials:

  • vector:P10_pSB1C3_001_CMV_DARPin_ML_VP2/3_587KO_6xHis
  • sortase-sequence: amino acid sequence: LTAPG translated to gene sequence: CTTACAGCCCCAGGA
  • kozak-sequence: gccgcc
  • restriction sites: SpeI and XbalI

Method:Geneious

Results:

  • f_Primer_preXba1 with overhang: kozak+SortaseMotiv1+myc-tag+VP2 (forward primer)
  • r_Primer_VP2_1-Temp. 80.3 °C (reverse primer)
  • f_Primer_XbaI+Überhang_cmv (forward primer)
  • r_Primer_CMV+suf (reversed)+ overhang (reverse primer)
  • location: directory: VIRUS/complete

Further tasks:

  • control
  • improvements

2012-06-22

Topic: Primer design - Cloning: Sortase-Tag an VP2 + PCR for VP2 with Kozak-sortase_tag-myc_tag

Investigators: Kathi, Laura, Tobias, Xenia

Aim:

  • change primer of 2012-06-19
  • trim primer: r_Pst_Primer_VP2_1+overhang-to reduce temperature uo to 68 °C
  • remove primers for cmv region

Materials:

  • Vector: p10_pSB1C3_001_CMV_DARPin_ML_VP2/3_587KO_6xHis
  • Sortase-sequence: amino acid sequence: LTAPG translated to gene sequence: CTTACAGCCCCAGGA
  • Kozak-sequence: gccgcc
  • restriction sites: XbaI in forward primer for VP2 region

Method:Geneious

Results:

  • prf_XbaI_kozak_SortaseMotivN_myc_VP2 (forward primer)
  • prr_VP2_PstI_Temp68 (reverse primer)
  • location: directory geneious VIRUS/complete

Further tasks:

  • control of the primer

2012-06-28

Topic: TAE-buffer

Investigator:Xenia

Aim: TAE-buffer(50x)- 1l

Materials:

242 g tris base

57.1 mL glacial acetic acid

100 mL 0.5 M EDTA

add 1 L Millipore -water

Further tasks:

  • Agarose gel electrophoresis

2012-06-29

Topic: Primer solution

Investigator:Kathi

Aim: primer solution in 100 µM

Materials:

  • prr_VP2_PstI_Temp68 ad 394 µL Aqua dest
  • prf_XbaI_kozak_SortaseMotivN_myc_VP2 ad 178 µL Aqua dest

Results:

  • prf_XbaI_kozak_SortaseMotivN_myc_VP2 --> c=100 µM
  • prr_VP2_PstI_Temp68 --> c=100 µM

Further tasks:

  • PCR