Team:Bielefeld-Germany/Amsterdam/Labjournal
From 2012.igem.org
(Difference between revisions)
Line 33: | Line 33: | ||
<div id="anzeige"><h1>Summary of Week 24</h1> | <div id="anzeige"><h1>Summary of Week 24</h1> | ||
- | |||
</html> | </html> | ||
Revision as of 09:39, 26 October 2012
Labjournal
Summary of Week 24
Week 24 (10/08 - 10/14/12)
Weekly Seminar
Monday October 08th
All: Day off in Amsterdam!!!
Tuesday October 09th
Wednesday October 10th
- Team Shuttle Vector:
- Ligation of pSB1C3::BBa_K863202 construct in KRX cells was done.
- Team Cellulose Binding Domain:
- Gradient-PCRs of CBDcex_Freiburg; CBDclos_Freiburg; GFP_Freiburg and ecol_Freiburg (47 °C to 67°C)
- Product:
- CBDcex_Freiburg at all temperatures
- CBDclos_Freiburg at all temperatures
- GFP_Freiburg at all temperatures
- ecol_Freiburg at 53 °C to 61°C (best at 57 to 59 °C)
- pooled fractions for gel clean up
- Product:
- Gradient-PCRs of CBDcex_Freiburg; CBDclos_Freiburg; GFP_Freiburg and ecol_Freiburg (47 °C to 67°C)
- Team Site Directed Mutagenesis:
- Ordered Primers for the SDM of the illegal XbaI restriction site in the shuttle vector
- Team Cultivation and Purification:
- Made precultures of E. coli KRX with [http://partsregistry.org/wiki/index.php?title=Part:BBa_K863000 BBa_K863000] and [http://partsregistry.org/wiki/index.php?title=Part:BBa_K863005 BBa_K863005]for 19L fermentation (500mL preculture)
Thursday October 11th
- Team Cellulose Binding Domain:
- Clean-Up of the Gel-pieces (from PCR-products)
- Restriction of PCR-products (3h):
- GFP_Freiburg:
- XbaI+PstI Tango-Buffer for Ligation
- XbaI+AgeI Tango 4xAgeI for Assembly
- CBDclos/cex:
- NgoMIV+PstI P.4+BSA 2xPstI for Assembly
- GFP_Freiburg:
- Assembly and Ligation (1h with T4):
- GFP_Freiburg + CBDcex_Freiburg + J61101
- GFP_Freiburg + CBDclos_Freiburg + J61101
- GFP_Freiburg + J61101
- Transformation in E. coli KRX (3 µL, chemical):
- GFP_Freiburg + CBDcex_Freiburg + J61101
- GFP_Freiburg + CBDclos_Freiburg + J61101
- GFP_Freiburg + J61101
- All Transformations were plated on AMP-select-agar
- Team Cultivation and Purification
- 12 L Cultivation of E. coli KRX with [http://partsregistry.org/wiki/index.php?title=Part:BBa_K863000 BBa_K863000] and [http://partsregistry.org/wiki/index.php?title=Part:BBa_K863005 BBa_K863005]
- Settings:
- 12 L Cultivation of E. coli KRX with [http://partsregistry.org/wiki/index.php?title=Part:BBa_K863000 BBa_K863000] and [http://partsregistry.org/wiki/index.php?title=Part:BBa_K863005 BBa_K863005]
Bioengineering NFL 19L fermenter, autoinduction HSG medium, 60 µg/mL chloramphenicol, 19 L, 37 °C, stirrer on cascade to hold a pO2 of 50 %, airflow: 12 NL/m, 16 hours. HSG medium was choosen to get a high biomass concentration with hope for a higher amount of laccases.
- Made precultures of E. coli Rosetta Gami 2 containing [http://partsregistry.org/wiki/index.php?title=Part:BBa_K863012 BBa_K863012](09/09) and <partinfo>BBa_K863022</partinfo> (09/09) behind a constitutive promoter. (500mL preculture)
Friday October 12th
- Team Cellulose Binding Domain:
- A lot of colonies on all three dishes (J61101+GFP_Freibug;J61101+GFP_Freibug+CBDcex;J61101+GFP_Freibug+CBDclos)
- no obvious green fluorescence, not even at J61101+GFP
- Maybe the combination of J23100 and J61101 isn't strong enough to express a visible amount of GFP
- Colony-PCR of 16 colonies of every dish
- J61101 + GFP_Freiburg:
- 16/16 positive
- plated two on select-agar
- J61101 + GFP_Freiburg + CBDcex:
- 8/16 positve
- plated three on select-agar
- J61101 + GFP_Freiburg + CBDclos:
- 7/16 positive
- plated three on select-agar
- J61101 + GFP_Freiburg:
- A lot of colonies on all three dishes (J61101+GFP_Freibug;J61101+GFP_Freibug+CBDcex;J61101+GFP_Freibug+CBDclos)
- Team Shuttle Vector:
- The induction with 0.5% (v/v) methanol of P. pastoris GS115 cells with integrated BBa_K863204::GFP was started.
- Team Substrate Analysis:
- Since we have seen some new peaks after Estradiol treated with Laccases in the LC-MS, we wanted to have more degradation products to do an MS so we used a higher concentradion of Estradiol and Laccase and let them incubate for 66 hours.
- Team Cultivation and Purification
- 12L Cutlivations of E. coli KRX with [http://partsregistry.org/wiki/index.php?title=Part:BBa_K863000 BBa_K863000] and [http://partsregistry.org/wiki/index.php?title=Part:BBa_K863005 BBa_K863005] were harvested and stored at 4°C until purification.
- 12 L Cultivation of E. coli Rosetta Gami 2 containing [http://partsregistry.org/wiki/index.php?title=Part:BBa_K863012 BBa_K863012](09/09) and <partinfo>BBa_K863022</partinfo> (09/09)
- Settings:
Bioengineering NFL 19L fermenter, HSG medium, 60 µg/mL chloramphenicol, 300 µg/mL ampicillin, 12 L, 37 °C, stirrer on cascade to hold a pO2 of 50 %, airflow: 12 NL/m, 22-24 hours. HSG medium was chosen to get a high biomass concentration with hope for a higher amount of laccases.
Saturday October 13th
- Team Shuttle Vector:
- The P. pastoris GS115 cells integrated with BBa_K863204::GFP were also inducted with 0.5% (v/v) methanol (100%).
- Team Cultivation and Purification
- 12L Cutlivations of E. coli Rosetta Gami 2 containing [http://partsregistry.org/wiki/index.php?title=Part:BBa_K863012 BBa_K863012](09/09) and <partinfo>BBa_K863022</partinfo> (09/09) were harvested and stored at 4°C until purification.
Sunday October 14th
- Team Shuttle Vector:
- The P. pastoris GS115 cells integrated with BBa_K863204::GFP were also inducted with 0.5% (v/v) methanol (100%).
- Team Fungal and Plant Laccases:
- Team Cellulose Binding Domain:
- Tried to isolate all plates, but only got low concentrations (5 ng/µL - 20 ng/µL)
- plated eight different colonies for isolation
- Team Substrate Analysis:
- We took sample from the reaction of the 12th October.
Summary of Week 25
Week 25 (10/15 - 10/21/12)
Weekly Seminar
Monday October 15th
- Team Shuttle Vector:
- There are no colonies of pBS1C3::BBa_K863202 KRX transformantion.
- The P. pastoris GS115 cells integrated with BBa_K863204::GFP were harvested and the supernatant was examined on GFP by fluorescence. But there was no GFP. The next steps are: disrupt the cells and test the supernatant on GFP. Maybe the GFP could not be secreted.
- Team Fungal and Plant Laccases:
- Yeah, the yeast cells are growing.
- Team Cellulose Binding Domain:
- Tried to isolate the eight plated, but did get low concentrations again (except one J61101+GFP_Freiburg+CBDcex_Freiburg with conc >100 ng/µL)
- cleaned up some more PCR-products (GFP_Freiburg; CBDcex_Freiburg; CBDclos_Freiburg)
- Team Substrate Analysis: We stopped the reaction from the 12th October with Methanol and gave it to Dr. Marcus Persicke to measure the degradation on LC-MS
Tuesday October 16th
- Team Activity Tests:
- Today we received the samples from Team Cultivation & Purification. We are really motivated to measure the activity of our new produced enzymes. But before that we have to prepare the samples. This implied the determination of the protein concentration in each fraction, which we did today. The results are listed in the following table:
- Team Cellulose Binding Domain:
- Transformed B0034 into KRX
- Transformed J23100 into KRX
- Plated both on AMP-select-agar
- Plated one more Colony of J61101 + GFP_Freiburg and J61101 + GFP_Freiburg + CBDclos
region=DE Laccase] || 150 µL || |- |}
- Team Substrate Analysis: The Massspectrometry data showed two potential products after the Laccase treatment of Estradiol and Ethinyl estradiol but we unfortunatly could not identify them so we decided to do MS-MS on thoose. The products showed that after Laccase treatment both Estradiol and Ethinyl estradiol losses two H atoms which was new for us.
Wednesday October 17th
- Team Activity Tests:
- Before starting our activity assay we re-buffered the fractions we got from Team Cultivation and Purification. It took some time, that's why we had no time for activity analysis yet. But we prepared everything for the next day, including determining the protein concentration of the fractions after they have been re-buffered. This is what we got:
- Team Shuttle Vector:
- Genomic DNA isolation of yeast cells with integrated BBa_K863204::GFP construct was done with the Kit. For genotype characterisation an PCR with the praimer pair 5AOX-Genotyp-FW and TT-Genotyp-RV was done and the fragment size was determined.
- Team Fungal and Plant Laccases:
- YPD liquid culture was inoculated with one yeast colony (BBa_K863204::TV5) and incubated at 30°C and 150 rpm.
- Team Cellulose Binding Domain:
- Picked colonies of B0034 and J23100 and plated them on AMP selection agar for plasmid isolation
- Team Site Directed Mutagenesis:
- SDM-PCR of the Shuttle vector
- Added DpnI over night
Thursday October 18th
- Team Activity Tests:
- Finally the day had come to measure the activity of our own produced laccases. This activity assay should give information about the enzyme content in every fraction. To make the measurements comparable we applied the same protein amount in every sample. Again, we used our standard activity assay protocol, but this time we used the Britton-Robinson Buffer at pH 5. Also we applied 0.1 mM ABTS and measured over night.
- Team Cellulose Binding Domain:
- Isolated J23100 plasmid
- Digested J23100 with EcoRI and PstI
- Digested pSB1C3-Backbone with EcoRI and PstI
- Clean up of pSB1C3-BB and J23100 + RFP - Insert via Gel
- Ligation of J23100 and pSB1C3-BB
- Isolated B0034 plasmid
- Digested B0034 with SpeI and PstI
- Digested GFP_Freiburg-PCR-product with XbaI and PstI
- Digested an other fraction of the GFP_Freiburg-PCR-product with XbaI and AgeI
- Assembled (Ligation):
- B0034 with GFP_Freiburg
- B0034 with GFP_Freiburg and CBDcex_Freiburg
- B0034 with GFP_Freiburg and CBDclos_Freiburg
- Transformed these three into KRX
- Team Site Directed Mutagenesis:
- Bands of 19C-PRC-product in Gel at 7 kbp (which is correct)
- Clean-Up of 19C-PRC-product
- Transformation of the 19C-PRC-product in XL1 Blue
Friday October 19th
- Team Activity Tests:
- After getting our interesting activity measurement results, we had to figure out which fraction is going to be used in the following experiments and how much laccase it contains besides other proteins. We agreed, that the most active fraction contains 90 % laccase, which is commonly used in the literature. Since we applied the same protein amount of each fraction for the activity measurements, we made sure that the results really correspond to the amount of laccase. These are the most active fractions we have chosen with their contained laccase amount:
- ECOL: Fraction 50% 2 with a laccase concentration of 63,9 µg mL-1.
- BPUL: Fraction 50% 2 with a laccase concentration of 25,1 µg mL-1.
- BHAL: Fraction 5% 3 with a laccase concentration of 10,9 µg mL-1.
- TTHL: The best fraction of our TTHL laccase was fraction 50% 1 with a laccase concentration of 4,03 µg mL-1. In regard to Team Immobilization and Team Substrate Analysis we had to reach a higher amount of TTHL laccase. So we thought of combining two fractions. We chose the second best fraction of TTHL, which is 5% 3. To calculate the amount of contained laccase we had to compare the activity and reconsidered the slope. Since we stated the fraction with its highest activity as 90 % contained laccase, we calculated the amount of laccase regarding to that one. The following figure shows the slopes we got out of the activity from fraction 50% 1 and fraction 5% 3 (which is the second best). Accordingly to this, fraction 5% 3 contains 68,9% of laccase, which is 4,8 µg mL-1. In total, the composed fraction contains 4,4 µg mL-1.
- After getting our interesting activity measurement results, we had to figure out which fraction is going to be used in the following experiments and how much laccase it contains besides other proteins. We agreed, that the most active fraction contains 90 % laccase, which is commonly used in the literature. Since we applied the same protein amount of each fraction for the activity measurements, we made sure that the results really correspond to the amount of laccase. These are the most active fractions we have chosen with their contained laccase amount:
- Team Cellulose Binding Domain:
- Colony-PCR of B0034 + GFP_Freiburg; B0034 + GFP_Freiburg + CBDcex; B0034 + GFP_Freiburg + CBDcex_Freiburg; B0034 + GFP_Freiburg + CBDclos_Freiburg.
- All negative
- Restriction of Ecol_Freiburg with XbaI, AgeI and DpnI
- Colony-PCR of B0034 + GFP_Freiburg; B0034 + GFP_Freiburg + CBDcex; B0034 + GFP_Freiburg + CBDcex_Freiburg; B0034 + GFP_Freiburg + CBDclos_Freiburg.
- Team Site Directed Mutagenesis:
Saturday October 20th
Sunday October 21st
- Team Cellulose Binding Domain:
- Colonies PCRs of B0034 + GFP_Freiburg; B0034 + GFP_Freiburg + CBDcex_Freiburg; B0034 + GFP_Freiburg + CBDclos_Freiburg
- All negativ
- Transformed once again (with an mix of old an new GFP_Freiburg)
- Isolated plated colonies of transformed colonies (two GFP; two GFP+Cex; two GFP+Clos
- Restriction analysis showed only bands at 2K bp (pSB1C3+BBa_B0034 vector without insert)
- Colonies PCRs of B0034 + GFP_Freiburg; B0034 + GFP_Freiburg + CBDcex_Freiburg; B0034 + GFP_Freiburg + CBDclos_Freiburg
- Team Site Directed Mutagenesis:
- Isolated the plasmids of the six SDM-dishes
- Over-night digestion with NotI
Summary of Week 26
Week 26 (10/22 - 10/28/12)
Weekly Seminar
Monday October 22nd
- Team Cellulose Binding Domain:
- Sequencing of <partinfo>BBa_K863120</partinfo> in <partinfo>BBa_J61101</partinfo> showed a deletion within the ORF of the GFP; this seemed to be the reason that the colonies are not fluorescent.
- Gradient-PCR on <partinfo>BBa_I13522</partinfo> with GFP_Freiburg Pre- and Suffix Primers
- Worked fine. Clean up and digestion with XbaI and PstI
- Gradient-PCR on <partinfo>BBa_K863103</partinfo> with CBDcex_Freiburg and GFP_Freiburg_compl Primers
- One of 12 temperatures worked. Clean up and digestion with XbaI and PstI
- Gradient-PCR on <partinfo>BBa_K863113</partinfo> with CBDclos_Freiburg and GFP_Freiburg_compl Primers
- did not get product at all
- Ligation of the PCR products and GFP_Freiburg and CBDcex_Freiburg-GFP_Freiburg, respectively
- Transformation of both ligations
- Cells plated on selection agar
- Team Site Directed Mutagenesis:
- Stopped Digestion of the shuttle vector, but gel went wrong and the products were lost
Tuesday October 23rd
- Team Cellulose Binding Domain:
- Colony PCR of B0034 + GFP_Freiburg
- 14/24 positive
- Plated three on selection agar for plasmid isolation
- Colony PCR of B0034 + CBDcex-GFP_Freiburg
- 16/24 positive
- Plated three on selection agar for plasmid isolation
- Colony PCR of B0034 + GFP_Freiburg
Wednesday October 24th
- Team Cellulose Binding Domain:
- Isolated Plasmids containing B0034 + GFP_Freiburg &
- Digestion of pooled plasmids with XbaI and PstI
- Isolated Plasmids containing B0034 + CBDcex-GFP_Freiburg
- Digestion of pooled plasmids with XbaI and PstI
- Digestion of J23100 with SpeI and PstI
- Clean up of inserts (B0034 + GFP_Freiburg & B0034 + CBDcex-GFP_Freiburg) and Backbone (J23100) via gel
- Ligation of Backbone and the inserts
- Transformation and plted on selection agar
- Isolated Plasmids containing B0034 + GFP_Freiburg &
- Team Site Directed Mutagenesis:
- Digestion showed that all isolated colonies still have the illegal XbaI restriction side
Thursday October 25th
- Team Substrate Anaylsis: The MS-MS data arrived from Marcus Persicke. To ensure our measurements and discuss what happens after the Laccase treatment and on the ESI we decided to ask an organic chemistrer so we went to Prof. Dr. Dietmar Kuck whos expert on this field. Since he had less time to discuss we have only speculativ testifies.
Friday October 26th
Saturday October 27th
Sunday October 28th
55px |