Team:Braunschweig/Notebook-content
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The very first step of our lab work was to obtain all genes encoding the six subunits of the methane monooxygenase (mmoX, mmoY, mmoB, mmoZ, mmoD, mmoC) which catalyzes the conversion of the greenhouse gas methane to methanol, a natural intermediate of the cellular metabolism. Unfortunately, even though most of the MMO subunits are described in the iGEM Registry, most of them were not available in stock. Therefore, we isolated them directly from <i>Methylococcus capsulatus</i> str. Bath via PCR using appropriate self-designed primers. However, the sequence of the initial subunits mmoC, mmoX, mmoY and mmoZ contained various restriction sites within the genes (mostly PstI). In order to receive the RFC10 standard these were removed by using mutation PCR. We then cloned them into the pSB1C3 shipping vector to put them at disposal of the community of all future iGEM teams. <br> | The very first step of our lab work was to obtain all genes encoding the six subunits of the methane monooxygenase (mmoX, mmoY, mmoB, mmoZ, mmoD, mmoC) which catalyzes the conversion of the greenhouse gas methane to methanol, a natural intermediate of the cellular metabolism. Unfortunately, even though most of the MMO subunits are described in the iGEM Registry, most of them were not available in stock. Therefore, we isolated them directly from <i>Methylococcus capsulatus</i> str. Bath via PCR using appropriate self-designed primers. However, the sequence of the initial subunits mmoC, mmoX, mmoY and mmoZ contained various restriction sites within the genes (mostly PstI). In order to receive the RFC10 standard these were removed by using mutation PCR. We then cloned them into the pSB1C3 shipping vector to put them at disposal of the community of all future iGEM teams. <br> | ||
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Revision as of 11:44, 17 October 2014
Experiments
1. Obtaining the MMO genes
The very first step of our lab work was to obtain all genes encoding the six subunits of the methane monooxygenase (mmoX, mmoY, mmoB, mmoZ, mmoD, mmoC) which catalyzes the conversion of the greenhouse gas methane to methanol, a natural intermediate of the cellular metabolism. Unfortunately, even though most of the MMO subunits are described in the iGEM Registry, most of them were not available in stock. Therefore, we isolated them directly from Methylococcus capsulatus str. Bath via PCR using appropriate self-designed primers. However, the sequence of the initial subunits mmoC, mmoX, mmoY and mmoZ contained various restriction sites within the genes (mostly PstI). In order to receive the RFC10 standard these were removed by using mutation PCR. We then cloned them into the pSB1C3 shipping vector to put them at disposal of the community of all future iGEM teams.
For detailed information, take a look at our Lab notebook → E. 1 Isolation of sMMO genes from M. capsulatus.
2. His-tagging
Now that we had successfully isolated the genes for all the MMO subunits, our next goal was to proof that we were able to produce all of them in the well characterized and easily manageable model organism Escherichia coli. In order to check for expression later on, we added a His-tag at the C-terminus of each subunit by using appropriate PCR-primers. Afterwards, we put them under control of the inducible lac-promoter (R0011), a weak ribosome binding site (B0032) and a double terminator (B0015).
For detailed information, take a look at our Lab notebook → E. 2 HIS-Tagging of mmo genes.
3. Expression of His-construct
Plasmids containing the final His-tagged constructs were then transformed into chemo-competent E. coli cells and the single tagged subunits were expressed by induction with IPTG. To isolate the soluble and inclusion protein fractions, the cells were harvested and pelleted by centrifugation.
SDS-PAGE followed by an immunostain via His-tag was performed in order to verify the expression of the subunits. Unfortunately, only two subunits were detectable (MMOC and MMOX).
For the purpose of producing all of the MMO subunits efficiently we tested the coexpression of different combinations of known chaperone proteins. With their help the E. coli cells were able to express each of the six MMO subunits in soluble form. Hence, we are the first to efficiently produce all of these MMO subunits in the heterologous organism E.coli.
For detailed information, take a look at our Lab notebook → E. 5 Expression of HIS-constructs.
4. Construction of the mmo construct
After ensuring that all the subunits of the MMO were producible in E. coli using the right combination of chaperones, we decided to assemble all of them in one construct, thus creating our methane degrading E. cowli! In order to allow a subsequent induction of our final construct containing all six of the MMO subunit genes we again used the lac-promotor in combination with a weak RBS and a double terminator. In order to make sure that every subunit-encoding gene is translated, a single RBS is inserted upstream of every gene.
In order to allow a subsequent induction of our final construct containing all six of the MMO subunit genes we again used the lac-promotor in combination with a weak RBS and a double terminator. In order to make sure that every subunit-encoding gene is translated, a single RBS is inserted upstream of every gene.
For detailed information, take a look at our Lab notebook → E. 3 Cloning of final construct.
5. Expression of the mmo construct
To analyse the functionality of the final construct we cultivated our E.cowli in a converted anareobic jar filled with a 2% methane atmosphere for 6 h. In order to proof the activity of the enzyme complex we measured the decrease of the methane concentration over a time period of 3 h with an MQ-4 semiconductor sensor for natural gas, a kind gift from iGEM Team Aachen.
For detailed information, take a look at our Lab notebook → E. 5 Expression of mmo construct.
6. Preparation of competent cells with chaperones
For our coexpression experiments we used different combination of chaperones. Therefore, we created a stock of competent E. coli cells, that were made chemically competent after transformation with the different chaperone constructs.
For detailed information, take a look at our Lab notebook → E. 6 Preparing of competent cells with chaperones.
7. Rumen fluid experiments
In order to test our constructs under realistic conditions, we performed various rumen fluid experiments. Fresh rumen fluid was kindly provided by the Institute of Animal Nutrition, Friedrich-Loeffler-Institute (FLI), Federal Research Institute for Animal Health, Braunschweig and steril filtrated. We then used this steril fluid to analyse our E.Cowli’s chances in the cow’s rumen.
For detailed information, take a look at our Lab notebook → E. 7 Rumen fluid experiments
8. Entrapping of E. coli
Based on our first rumen fluid experiments, we have learnt that E. coli is not capable to grow on rumen fluid. In order to improve the chances of survivial of our E. cowli, as well as, to find a media to transport our E. cowli into thr cow's rumen we tested the impact of entrapment of E. cowli in alginate beads and analysed its growth.
For detailed information, take a look at our Lab notebook → E. 8 Entrapping of E. coli.
9. ILS
In this year’s iGEM competition the first international Interlab Measurement Study was introduced to obtain fluorescence data for three specific genetic devices expressing GFP. Even though we did not sign up for the track “Measurement” of the iGEM competition and therefore were not obliged to participate in this Interlab Measurement Study, we voluntarily took part as one of 45 teams worldwide. In addition to the general requirements we also completed the second “extra credit” assignment by building and testing all three devices expressing RFP instead of GFP and compared the fluorescence of both fluorescence proteins.
For detailed information, take a look at our Lab notebook → Interlab Study.
Protocols
Recipes for Solutions and Media
16 g | Bacto tryptone |
10 g | Bacto yeast extract |
5 g | NaCl |
were dissolved in 1 L dH2O, the pH was adjusted to 7.0.
For solid medium 12 g of Bacto agar (per Liter) was added.
10 g | Bacto tryptone |
5 g | Bacto yeast extract |
10 g | NaCl |
were dissolved in 1 L dH2O, the pH was adjusted to 7.0.
For solid medium 12 g of Bacto agar (per Liter) was added.
0,8 % (w/v) | NaCl |
0,02 % (w/v) | KCl |
0,144 % (w/v) | Na2HPO4 · 2 H2O |
0,024 % (w/v) | KH2HPO4 |
1 g | MgSO4 · 7 H2O |
0.2 g | CaCl2 · 6 H2O |
2 mL | Chelated Iron Solution |
1 g | KNO3 |
0.5 mL | Trace Element Solution |
0.272 g | KH2PO4 |
0.717 g | Na2HPO4 · 12 H2O |
12.5 g | Purified Agar |
1 L | Distilled deionized water |
Adjust pH to 6.8.
0.1 g | Ferric (III) ammonium citrate |
0.2 g | EDTA, sodium salt |
0.3 mL | HCl (concentrated) |
100 mL | distilled deionizied water |
500 mg | EDTA |
200 mg | FeSO4 · H2O |
10 mg | ZnSO4 · 7 H2O |
3 mg | MnCl2 · 4 H2O |
30 mg | H3BO3 |
20 mg | CoCl2· 6 H2O |
1 mg | CoCl2· 6 H2O |
2 mg | NiCl2 · 6 H2O |
3 mg | Na2MoO4 · 2 H2O |
1 L | Distilled water |
242 g | 2 M Tris base |
51,1 mL | glacial acetic acid (17,4 M) |
200 mL | 100 mM EDTA (pH 8) |
were dissolved in 1 L dH2O.
Loading buffer for gel electrophoresis
A 0.2 M EDTA and 0.05 % (w/v) orange G or bromphenoleblue solution was prepared in 50 % glycerine.
Ampicillin stock solution
10 g ampicillin sodium salt was dissolved in 100 mL dH2O, sterile filtered, aliquoted and stored at -20 °C.
Kanamycin stock solution
5 g kanamycin sulfate was dissolved in 100 mL dH2O, sterile filtered, aliquoted and stored at -20 °C.
Chloramphenicol stock solution
3.4 g chloramphenicol was dissolved in 100 mL Ethanol, sterile filtered, aliquoted and stored at -20 °C.
Tetracyclin stock solution
5 g Tetracyclin was dissolved in 100 mL Ethanol, sterile filtered aliqoted and stored at -20 °C.
0.3 g | CaCl2 |
0.6 g | potassiumacetate |
1.2 g | RbCl |
1 g | MnCl2 · 4H2O |
15 ml | glycerin |
were dissolved in dH2O and diluted to a final volume of 100 mL. The pH was adjusted and the solution sterile filtered.
2.2 g | CaCl2 |
0.12 g | potassiumacetate |
0.21 g | morphoslinopropanesulfuricacid |
15 ml | glycerin |
were dissolved in dH2O and diluted to a final volume of 100 mL. The pH was adjusted and the solution sterile filtered.
10 % (w/v) | SDS |
50 % (w/v) | Glycerine |
0.02 % (w/v) | Bromphenol blue |
15 % (w/v) | Beta-Mercaptoethanol |
30 % (w/v) | Acrylamide |
0.8 (w/v) | Bisacrylamide |
List of used strains
Strain | Genotype | Risk Group | Risk to Humans |
---|---|---|---|
E. coli XL1-Blue-MRF‘ | endA1 gyrA96(nalR) thi-1 recA1 relA1 lac glnV44 F'[ ::Tn10 proAB+ lacIq Δ(lacZ)M15 Amy CmR] hsdR17(rK- mK+) | S1 | Non-pathogenic, may cause irritation to skin, eyes and respiratory tract, may affect kidneys |
Methylococcus capsulatus | wildtype | S1 | Non-pathogenic, may cause irritation to skin, eyes and respiratory tract, may affect kidneys |
E. coli BL21 DE3 | F– ompT gal dcm lon hsdSB(rB- mB-) λ(DE3 [lacI lacUV5-T7 gene 1 ind1 sam7 nin5] | S1 | Non-pathogenic, may cause irritation to skin, eyes and respiratory tract, may affect kidneys |
E. coli JM109 | endA1 glnV44 thi-1 relA1 gyrA96 recA1 mcrB+ Δ(lac-proAB) e14- [F' traD36 proAB+ lacIq lacZΔM15] hsdR17(rK-mK+) | S1 | Non-pathogenic, may cause irritation to skin, eyes and respiratory tract, may affect kidneys |
The primer sequences that were used.
E. coli Culture ConditionsFor the cultivation of E. coli 2xYT medium was used. If necessary 1 µL/mL of an antibiotic stock solution was added. The cultures were incubated at 37 °C and in case of liquid cultures shaken at 250 rpm.
Methylococcus capsulatus Culture ConditionsFor the cultivation of M. capsulatus NMS medium was used. The cultures were incubated at 42 °C at 50 % methane atmosphere.
Measurement of Growth CurvesOvernight cultures in 2xYT medium containing the appropriate antibiotic were inoculated directly from -80 °C glycerol cell stock. Cells were grown in non-baffled-flasks at 37 °C and 250 rpm. The next day, main cultures in 2xYT medium containing the appropriate antibiotic were inoculated from overnight cultures to an OD600 0.1. Cells were grown in non-baffled flasks at 37°C and 250 rpm. Samples from each flask were taken at appropriate time points depending on the growth phase of the cells. Optical density was measured at a wavelength of 600 nm. Cells were left to grow until the stationary phase was reached.
Preparation of chemically competent cells100 mL of 2xYT media containing required antibiotic were inoculated and incubate at 37 °C and 250 rpm until OD600 0.5. Subsequently the cells were incubated on ice for 15 minutes and then centrifuged at 4 °C and 400 rpm for 5 minutes. The excess was discarded and the pellets resuspended in 7.5 mL ice cold TFB1. Afterwards the solution is incubated on ice for 90 minutes and then centrifuged for 5 minutes at 4000 rpm. Finally the pellets were resuspended, aliquoted and quick-frozen in liquid nitrogen. The vials were stored at -80°C.
CryopreservationThe respective strain was grown on 2xYT medium at 37 °C and 250 rpm overnight. Afterwards a 20 % Glycerin solution was prepared with the liquid culture, aliquoted, shock frozen and stored at -80 °C.
Minipreparation of Plasmid DNAMiniprep was done with Plasmid DNA purification Kit by Macherey-Nagel following the manufacturer’s protocol. First 3-5 mL of the cell suspension were spun down for 10 minutes (5000 g). For the alkaline lysis of the DNA the pellet was resuspended in 250 μL Resuspension Buffer A1. 250 μL of Lysis Buffer A2 was added and incubated at RT for 5 min. 300 μL of Neutralization Buffer A3 was added to stop the reaction. As final step of the alkaline lysis the mixtures was centrifuged at 10.000 x g for 10 minutes. Afterwards the NucleoSpin Column was loaded with 750 μL lysate and then centrifuged for 1 minute (10.000 x g). Subsequently the DNA was washed with 500 μL Wash Buffer and centrifuged again for 1 minute (10.000 x g). The DNA was the precipitated with the Ethanol containing wash buffer and separated by another centrifugation (1 min, 10000 x g) and dried. At last the DNA was eluted with 50 μL elution buffer, which was pre-heated to 60 °C, and incubated for 5 min. The eluted DNA was separated from the matrix by a final centrifugation step (1 min, 5000 x g).
Colony PCRAfter successful transformation single colonies were picked and analyzed by colony PCR. Therefore each colony was picked from the original plate with a pipette tip and dipped into the PCR-mix. Afterwards the pipette tip was used to inoculate a second agarplate. PCR fragments were analyzed via gelectrophoresis.
Component | μl per 10 μL reaction batch |
GoTaq Buffer flexi green | 2 |
dNTP mix | 0.2 |
MgCl2 (25 mM) | 0.8 |
Primer 1 | 0.5 |
Primer 2 | 0.5 |
Promega GoTaq polymerase | 0.05 |
H2O | 5.95 |
Temperature [°C] | Time | Cycles |
95 | 2 min | 1 |
94 | 15 s | 30 |
52 | 20 s | |
72 | 60 s | |
72 | 10 min | 1 |
Component | μl per 20 μl reaction batch |
Nuclease- free water | add 20 |
5x Phusion HF | 4 |
10 mM dNTPs | 0.4 |
10 μM forward primer | 1 |
10 μM reverse primer | 1 |
Template DNA | Variable: 1 pg - 10 ng |
Phusion DNA polymerase | 0.2 |
Temperatur [°C] | Time | Cycles |
98 | 30 s | 1 |
98 | 10 s | 30 |
50 - 60 depending on primer | 30 s | |
72 | 30 s/kb | |
72 | 10 min | 1 |
Gel electrophoresis
Depending on the size of the DNA fragments a 0.8 to 2 % agarose gel with 0.2 µg/mL ethidiumbromide was used. The gel was placed in an electrophoresis chamber and covered in 1x TAE buffer. Subsequently DNA samples mixed with loading buffer were loaded to the gel pockets and separated at 80-120 V for about 1 h. Last the gel was photographed for documentation.
Gel Slice Preparation10 µL of 6x loading buffer were added to digested DNA und mixed. The sample was loaded onto a 1 % agarose gel and separated via gel electrophoresis at 75 mA for 20-40 min depending on the size of the DNA. For gel extraction the gel was visualized on an UV-lightsource and the appropriate bands were cut using the x-tracta™ Gel Extractor tool (Promega). Gel purification was carried out using the Macherey-Nagel Nucleospin Gel and PCR Clean-up Kit.
Cloning
Restriction digestFor restriction of vector and insert DNA approximately 1000 ng purified DNA, 5 µL 10x buffer and 1 µL of each of the two restriction enzymes were mixed in a 1.5 mL reaction tube. The amount of DNA used depended on the size of the desired fragment. Water was added to a final volume of 50 µL. Restriction was carried out at 37 °C for 1 h. The reaction was stopped by inactivating the enzymes at 80 °C for 20 min.
- PstI/EcoRI HF: NE 2.1
- PstI/SpeI HF: NE 2.1
- PstI/XbaI: NE 3.1
- all other combinations: NEB CutSmart Buffer
For the desphosphorylation of vector DNA 5.56 µL Antarctic Phos Reaction Buffer (NEB) and 0.5 µL Antarctic Phosphatase (NEB) were added to the digestet DNA and mixed. DNA was incubated at 37 °C for 60 min. After 30 min of incubation 0.5 µL Antarctic Phosphatase was added to the DNA and mixed.
DNA PurificationAfter desphosphorylation the vector DNA was purified using the Macherey-Nagel Nucleospin Gel and PCR Clean-up Kit.
LigationFor ligation of the constructed plasmid 50 ng vector DNA, 3 times as much insert DNA, 2 µL T4 Ligase Buffer (NEB), 0.5 µL T4 Ligase (NEB) and water added to a final volume of 20 µL were mixed in 1.5 mL reaction tube. Ligation was carried out at 16 °C over night. The reaction was stopped by inactivating the enzymes at 65 °C for 20 min.
Transformation of chemocompetent cells via heatshockOne -80 °C glycerol stock of chemocompetend cells was thawed on ice. 10 µL of the ligated DNA was prepared in a 1.5 mL reaction tube. 50 µL of the cells were added and incubated for 20 min on ice. The mixture was then heat shocked at 42 °C for 1 min and cooled on ice for 2 min. 1 mL SOC-medium was added and the cells were incubated for 1 h at 37 °C while shaken at 600 rpm. 100 µL of the cell suspension were plated on a 2xYT agar plate with the according antibiotic (chloramphenicol or ampicillin) and incubated at 37 °C over night.
Expression of the His-constructs
50 ml 2xYT over night cultures of cells expressing HIS-tagged subunits of the MMO were inoculated from Glycerinstocks. After 24 h a main culture of 500 ml 2xYT-Ca-Glucose-Medium was inoculated to a starting OD600 of 0,1 and cultivated at 37 °C and 250 rpm. Induction to a concentration of 100μM IPTG between OD 0,4-0,6. After induction the culutures were cultivated at 30 °C. 1mL of an arabinose solution (200 mg/mL) was added after 2 h and 4 h. After 6 h and 24 h after induction with IPTG 250 ml of the cells were harvested, centrifuged (13,000 g, 10 min) and the supernatant was discarded. The expression of the HIS-tagged subunits of the MMO was analyzed by using SDS-PAGE and Coomassie or Immunostaining respectively.
Expression of the mmo-construct
5 ml 2xYT over night cultures of cells expressing the MMO were inoculated from Glycerinstocks. After 24 h a main culture of 50 ml 2xYT-Ca-arabinose (4 mg/mL)-Medium was inoculated to a starting OD600 of 0,1 and cultivated at 37 °C and 250 rpm. Induction to a concentration of 100μM IPTG between OD 0,4-0,6. After induction the culutures were cultivated at 30°C. 1mL of an arabinose solution (200 mg/mL) was added after 2 h and 4 h. The complete culture was harvested after 6 h.
Isolation of the soluble and inclusion fraction
The pellets harvested after 24 hours after induction with IPTG was resuspended in 5 ml PBS each. The cells were disrupted by sonification for 1 min and afterwards centrifuged for 15 min (800 g , 4 °C). The supernatant was transferred into a new 15 ml falcon and centrifuged for 30 min (6000 g, 4°C). The obtained supernatant contains MMO-subunits which are solubly produced. The pellet obtained after the first centrifugation step was resuspended in 10 ml PBS and again centrifuged for 15 min (6000 g, 4 °C). After the supernatant has been discarded this step has been repeated (resuspension in 10 ml PBS and centrifugation step). After the supernatant has been discarded the pellet was then resuspended in 2 ml PBS 8 M Urea added. The suspension was then transferred into a 2 ml Eppendorf tube and centrifuged for 20 min (11000 g, 4 °C). The obtained supernatant contains MMO-subunits which are produced in inclusion bodies.
The soluble fraction and inclusion body fraction was stored at -20 °C and later analysed using SDS-PAGE and Coomassie or Immunostaining respectively.
SDS-Page
The samples were mixed with 1x Laemmli Buffer with beta-Mercaptoethanol and heated for 10 min to 95 °C. The Gel was loaded with 10 μl of the prepared samples and run at 200 V for 50 min.
Coomassie Staining
After the SDS-PAGE has been executed the gel is put into a glass petridish filled with Coomassie Brilliant Blue coloring suspension and boiled up for a couple of second. The gel was incubated in the coloring suspension on a rocker for 10 min until the coloring was sufficient. Afterwards the gel was destained using destaining suspension and again boiled up for a couple of seconds and incubated on the rocker for an hour. The gel was stored in water until it was fully destained.
Western Blot
Blotting with Trans-blot SD semi dry transfer cell:
Order from top to bottom:
- filter paper
- gel
- blot-membrane
- filter paper
Activation of blot-membrane with MeOH (100 %). Filter paper are moistened with running buffer
Run of blot: 15V for 30 min
Immunostain
After having executed the Blot, the membrane was blocked with milk powder for 1 hour on a rocker. After 2 washing steps with PBS (0,1 %) (1x short, 1x for 5 min) the membrane was incubated for an hour in the first antibody solution on the rocker (Qiagen Anti Penta his (mouse) 1:2000). Again there was a washing step with PBS (1x short, 1x for 5 min). The membrane was then incubated for an hour in the second antibody solution (Dianova Goat anti Mouse IgG AP-conjugated 1:30.000, Predilution of antibody already 1:30) on the rocker. After the incubation the membrane was washed 3 times with PBST (2x short, 1x for 10 min) and twice washed with substrate buffer (1x short, 1 x for 5 min). The blot is then incubated in substrate buffer with NBT and BCIP (1: 100 in substrate buffer) until bands are visible (1-20 min). Afterwards the blot was washed twice with water (1x short, 1x for 5 min) and dried between two filterpapers.
sMMO activity assay
50 mL bacterial suspension was cultured as described in “Expression of the mmo-construct”. The culture was diluted to OD600 4 and centrifuged and washed twice with 0,9 % saline solution. The bacterial pellet was resuspended in 50 mL NMS-Medium. The methane measurement was performed in a modified anaerobic jar. Therefore the solution was placed into the anaerobic jar and was treated with methane and compressed air in order to obtain an atmosphere with 2 % methane. The methane concentration was detected with an “MQ-4 Semiconductor Sensor“ for 10.000 sec. A converted anaerobic jar in combination with a methane sensor was used for measurements.
For the measurements we used the sensor MQ-4 Semiconductor Sensor for Natural Gas by Henan Hanwei Electronics. Its function is based on SnO2 whose low conductivity rises with higher concentrations of combustible gases like methane or propane. This sensitivity for methane and its low costs made it perfect for our do it yourself methane measuring system. The data from the sensor were processed by a Sainsmart nano V3.0 device, a smaller variant of the Arduino board.
To get the right methane concentration for each experiment we used flow controllers to set up the respective flow rates for methane, air and carbon dioxide which were then conducted through the anaerobic jar for 10 minutes until a homogenous methane atmosphere was formed.
When the atmosphere needed was generated and all vents were closed the anaerobic jar was placed in an incubator set to correct temperature. For some experiments a magnetic stirrer was also placed in the incubator to keep the homogenity of the culture and the atmosphere in the jar. The sensor was connected to the Arduino board which was then plugged into the PC outside the incubator via USB cable.
We used a modified version of the Serial Client programmed by Michael Osthege from iGEM Aachen converting the processed signal of the Arduino board into a visual graph and a exportable table file. For the experiments, we filled the jar with a defined atmosphere of 2% methane in 98% air until the sensor displayed a stable methane concentration which was then set as 2%.The subsequently measured data were considered in relation to this value. Measurements were started after the sensor had adapted to humidity and temperature in the anaerobic jar. After the measurement the jar was filled with compressed air to define a zero-point.
Entrapment of E. coli
50 mL of an overnight culutre was pelletized. The pellet was washed twice in 0,9 % saline solution resuspended and diluted to OD600 4 in 10 mL 0,9 % saline solution. 1,5 g alginate was solved in 40 mL ddH2O and was briefly boiled up. The alginate solution was mixed with all requiered antibiotics and arabinose (4 mg/mL). The whole solution was cooled and mixed with 10 mL bacterial 0,9 % saline solution. Beads were droped with a transfer pipette into a 0,05 M CaCl2 solution. The CaCl2 solution was decanted after 10 min.
Counting of cells with Thoma counting plate
Cell culture is placed on the plate and covered with a cover plate.
Sizes of the counting plate: depth: 0.02 mm area: 0.0025 mm².
(Volume of a C-field: 0,0005 mm³ ).
The number of cells per mL was calculated accordingly.
Cultivation on rumen fluid agar plates
We prepared agar plates with different concentrations of sterile filtrated rumen fluid, each with and without supplementation of glucose (100 mM). One half of each of these plates was inoculated with unsterile rumen fluid and the other one with E. coli. The plates were incubated over night at 37°C.