Team:Leicester/Notebook

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Revision as of 00:15, 5 October 2013

iGEM Leicester Test Page 2012

Notebook

July
M T W T F S S
1 2 3 4 5 6 7
8 9 10 11 12 13 14
15 16 17 18 19 20 21
22 23 24 25 26 27 28
29 30 31
August
M T W T F S S
1 2 3 4
5 6 7 8 9 10 11
12 13 14 15 16 17 18
19 20 21 22 23 24 25
26 27 28 29 30 31
September
M T W T F S S
1
2 3 4 5 6 7 8
9 10 11 12 13 14 15
16 17 18 19 20 21 22
23 24 25 26 27 28 29 30

Making chloramphenicol agar plates

400ml agar
melt in microwave
Add 800ul of chloramphenicol to make 25ug/ml
Pour out into 20 petri dishes
Leave overnight to set on the bench

Transformation of RFP control plasmid

Keep competent cells on ice
Add 50ul of cells to 4 tubes
Add 1ul of resuspended DNA to 2 tubes
Add 1ul RFP to the other 2 tubes
Incubate for 30mins
Heat shock at 42 degrees for 60secs
Incubate on ice for 5mins
Add 200ul of SOC media
Incubate at 37degrees for 2hrs
Spread on 6 plates:
Positive control (normal plate)
Negative control (No plasmid)
20ul of 50pg/ul
200ul of 50pg/ul
20ul of 10pg/ul
200ul of 10pg/ul
leave plates on bench overnight

Count colonies on agar plates

Plate Colonies
Viability control Covered
Negative control 1 contaminant
20ul of 50pg/ul 135
20ul of 10pg/ul 96
200ul of 50pg/ul ~1600
200ul of 10pg/ul 944
Therefore there was 1.2x10^8 cfu/ug

Replate to get individual colonies

Take an individual colonies
Streak out onto new plate
Sterilize loop using bunsen burner
Incubate at 37 overnight

Incubate in broth

4ml of luria broth in 6 universals
Add 8ul of chloramphenicol
Pick single colony and put in broth (sterile technique)
Incubate overnight at 37 in shaker

Make agarose gel

20ml of 5xTBE
80ml of water
0.8g of agarose
(0.8% gel)
boil till all agarose dissolved
Cool
Add 5ul of ethidium bromide
Pour gel

Make buffer

50ml of 5xTBE
200ml of water

Isolating RFP plasmid

Add 1.5ml of overnight culture to epindorph
Centrifuge for 2mins
Remove supernatent
Repeat
Use thermo scientific mini kit
Measure concentration using nanodrop

Double digest

50ng of DNA
2ul of 3.1 buffer
1ul of each restriction (XbaI and PstIin the 6 samples, EcoRI and PstI in the 6 samples, 12 samples in total)
Water to make total volume to 20ul
Incubate at 60mins at 37
20mins at 80

Single digest

Digesting RFP plasmid again using a single restriction enzyme- XbaI
Digesting DNA samples 1-6
200ng of DNA is run
Volumes for digest:
Sample nr 1 2 3 4 5 6
DNA 0.7 0.7 0.8 1.3 1.2 2.6
Buffer 2 2 2 2 2 2
Water 16.3 16.3 16.2 15.7 15.8 14.4
Xbal 1 1 1 1 1 1
Buffer used was cutsmart
Incubate samples at 37C for 1h
2ul of orange G dye was added to each samples
Samples were then frozen overnight to run on gel on Monday

Make agarose gel

20ml 5xTBE
80ml water
1g of agarose
Boil in microwave 1 min at a time
Cool
Add 5ul ethidium bromide

Running single digested DNA from Friday

Gel didn't show the expected bands and was disregarded

Isolating Limonene biobrick

Use Bioline isolate II plasmid mini kit

no title

Sample Plasmid Volume(ul) DNA Concerntration(ng/nl)
1.1 40 131.8
1.2 40 77.1
1.3 46 56.8
1.4 39 109
1.5 41 129.1
1.6 32 93.3
measured DNA concentration using nanodrop

Restriction enzyme digest of the DNA samples

enzymes: XbaI, PstI
master mix:
Buffer - 14ul
H2O - 88.2ul
XbaI - 1.4ul
PstI - 1.4ul
Total volume - 105ul
Each sample contained 5ul of DNA and 15ul of the master mix.
The total amount of DNA in each sample was 200ng
To calculate it we divided 200ng by the concentration of each sample
The rest of the volume was made up with water to give a total of 5ul.
The samples were then incubated in a water bath at 37C for an hour

Agorose Gel preparation

20ml of 5xTBE
80ml of water
0.8g of agarose
Boil for 3 minutes, 1 minute at a time.
Let it cool and add 5ul of ethidium bromide.
Pour and let it set for 30 mins.
Adding dye and marker
Used orange g loading dye.
2ul to each sample
Used 1kb ladder, 5ul per 1 marker well.
Run the gel
Gel picture

Ran the gel from the 26/07/2013 again for 45min

Digestion of plasmid backbone (pSB1C3)

Three different reactions
Master Mix (changes were made from the protocol)
5ul NEB Buffer 3.1
0.5ul of EcoRI
0.5ul of PstI
19ul of dH2O
For each reaction add:
4ul of linearized backbone
4ul of enzyme master mix
digest at 37C for 30min
heat kill at 80C for 20min

Digestion of the limonene biobrick plasmid backbone (BBa_K118025)

Using clone 1.1 purified plasmid DNA
For the reaction adding:
5ul NEB Buffer 3.1
2ul of EcoRI
2ul of PstI
2.5ul of dH2O
38.5ul of DNA
digest at 37C for 30min
heat kill at 80C for 20min

Ligation of insert to vector

For this experiment, two separate samples will be run; a control and the actual ligation.
Calculate appropriate vector:insert ratio and convert to a 1:1 ratio
Add the following substances
11.1ul of dH2O
1ul of QS Ligase *
5ul of 4xQS Buffer (vortex before use)
Mix thoroughly by pipetting
Incubate at room temperature for 5 min to create cohesive ends
Run 2.5-5ul of the ligation mixture onto an agarose gel to check ligation efficiency against a known marker. Add 1ul of dye to aid the visualization of results.
Transform it into competent cells (E.coli)
*For the control, no QS Ligase is added but its equivalent volume (1ul) is made up by dH2O.
The results from the gel electrophoresis show four lanes; two 1kb markers on either end (the first and forth lane), one control (the second lane) and the actual ligation results (the third lane). The control has two bands which shows that it has not been ligated, one band is around the 2kb area which is lightly-staining and one band is heavy-staining around the 5kb area. The actual ligation shows a lightly-staining smear, conclusive with the formation of a plasmid. The results are sufficiently good to carry on with the next phase of the experiment - the transformation.

Transformation of the limonene Biobrick (BBa_K118025)

Ligated with the pSB1C3 vector (restriction sites EcoRI, PstI)
Protocol:
Start thawing the competent cells on ice
Seperate 4 pre-chilled eppendorf tubes;
Resistance/Viability test
Ligation experiment with 10ul DNA
Ligation experiment with 5ul DNA
Positive control using 1ul RFP
Add 50ul of thawed competent cells and then the aforementioned volume of DNA to each eppendorf tube.
For each eppendorf tube, pipette the solution gently to mix. Ensure the cells are kept on ice.
Close the tubes and incubate the cells on ice for 30 minutes
Heat shock the cells by immersion in a pre-heated water bath at 42'C for 60 seconds
Incubate the cells on ice for 5 minutes
Add the 200ul of SOC (SOB + 0.4g glucose) media to each tube
Incubate the cells at 37'C for 2 hours
Plate onto petri dishes (ensure your petri dishes are labelled correctly):
For eppendorf 1, plate 100ul onto a chloroamphenicol petri dish and another 100ul of the solution onto a LB (luria broth) petri dish
For eppendorf 2, plate 200ul and 20ul onto two separate chloroamphenicol petri dishes
For eppendorf 3, plate 200ul and 20ul onto two separate chloroamphenicol petri dishes
For eppendorf 4, plate 200ul and 20ul onto two separate chloroamphenicol petri dishes
Incubate the plates at 37'C overnight

Results from the Transformation of limonene Biobrick (BBa_K118025) to the pSB1C3 vector

  1. The Viability test showed colony growth on it, as expected
  2. The Resistance test showed no colony growth, as expected
  3. The ligation experiment with 10ul DNA showed no results for both the 20ul and 200ul plates. This was not expected.
  4. The ligation experiment with 5ul DNA showed no results for both the 20ul and 200ul plates. This was not expected.
  5. The positive RFP control showed red colonies, as expected.
Discussion: The results of the viability test indicates that the cells used were viable, and the resistance test indicated that the these cells did not have any intrinsic resistance to the chloroamphenicol antibiotic. The positive RFP control showed red colonies, which implies that the transformation was successful. Since our ligations showed no results, it can be assumed that there was a problem with the ligation experiment itself. Running the gel for Limonene biobrick digests (BBa_K118025) again for separation of the 2kb and 5kb fragment. Extracted the 5kb fragment using Bioline gel extraction kit.

Digestion of the chlorophenicol plasmid vector pSB1C3

Three different reactions
Master Mix (changes were made from the protocol)
5ul NEB Buffer 3.1
0.5ul of EcoRI
0.5ul of PstI
19ul of dH2O
For each reaction add:
4ul of linearized backbone
4ul of enzyme master mix
digest at 37C for 30min
heat kill at 80C for 20min

Ligation of the plasmid pSB1C3 with the purified limonene biobrick (plasmid pSB1C3)

For this experiment, two separate samples will be run; a control and the actual ligation.
Calculate appropriate vector:insert ratio and convert to a 1:1 ratio
volume of vector - 2ul
volume of insert - 0.8ul
Add the following substances
11.2ul of dH2O
1ul of QS Ligase *
5ul of 4xQS Buffer (vortex before use)
Mix thoroughly by pipetting
Incubate at room temperature for 5 min to create cohesive ends
Run 2.5-5ul of the ligation mixture onto an agarose gel to check ligation efficiency against a known marker. Add 1ul of dye to aid the visualization of results. Transform it into competent cells (E.coli)
*For the control, no QS Ligase is added but its equivalent volume (1ul) is made up by dH2O.

Transformation of the plasmid pSB1C3 and the limonene biobrick BBa_K118025

Start thawing the competent cells on ice
Seperate 4 pre-chilled eppendorf tubes;
  1. Resistance/Viability test
  2. Ligation experiment with 10ul DNA
  3. Ligation experiment with 5ul DNA
  4. Positive control using 1ul RFP
Add 50ul of thawed competent cells and then the aforementioned volume of DNA to each eppendorf tube.
For each eppendorf tube, pipette the solution gently to mix. Ensure the cells are kept on ice.
Close the tubes and incubate the cells on ice for 30 minutes
Heat shock the cells by immersion in a pre-heated water bath at 42'C for 60 seconds
Incubate the cells on ice for 5 minutes
Add the 200ul of SOC (SOB + 0.4g glucose) media to each tube
Incubate the cells at 37'C for 2 hours
Plate onto petri dishes (ensure your petri dishes are labelled correctly):
  1. For eppendorf 1, plate 100ul onto a chloroamphenicol petri dish and another 100ul of the solution onto a LB (luria broth) petri dish
  2. For eppendorf 2, plate 200ul and 20ul onto two separate chloroamphenicol petri dishes
  3. For eppendorf 3, plate 200ul and 20ul onto two separate chloroamphenicol petri dishes
  4. For eppendorf 4, plate 200ul and 20ul onto two separate chloroamphenicol petri dishes
Incubate the plates at 37'C overnight

Gel electrophoresis

Gel electrophoresis was done to confirm the presence of the purified DNA.
5ul of DNA was run, but after electrophoresis no band was present.
We assumed this was down to pippeting error and thus carried on with the transformation.

Results from the transformation plates

On the 01/08/2013 we plated the transformations containing the biobrick BBa_K118025.
Our transformations were successful
the plates contained different volumes of the transformation: 20ul and 200ul
the plate to test viability shows growth as expected
the plate to test resistance shows no growth as expected
there were two different different transformations that contained different volumes of ligated DNA, which were plated into different plates.
The 10ul ligated DNA plates showed growth
The RFP control plates showed growth as expected
the plates with the ligated DNA did not show growth as the RFP plates, this could be because the cells did not take up as much plasmid as the optimum RFP plasmid or not all the plasmid were ligated with the biobrick.
It is also important to notice that there is not much different in the number of colonies between the 5ul and 10ul plates.

Next steps

The presence of the limonene biobrick in the ligated product has to be confirmed. This would be done in 2 ways
a) Measurement of volatile organic compounds (VOC) - 3 separate groups of cells would be prepared for this experiment.
The first group would be transformed cells containing the ligated product.
The second group would be transformed cells containing only circularised pSB1C3 vector
The third group would just be competent cells
b) Miniprep of transformed cells containing the ligated product (from above results)

Digestion of pSB1C3 backbone

Master Mix (changes were made from the protocol)
5ul cut smart Buffer
0.5ul of XbaI
0.5ul of SpeI
19ul of dH2O
For each reaction add:
4ul of linearized backbone
4ul of enzyme master mix
digest at 37C for 30min
heat kill at 80C for 20min
this digestion was done as control to test if our colonies with the limonene biobrick is expressing limonene.

Circularisation of pSB1C3

For this experiment, two separate samples will be run; a control and the actual ligation.
Add the following substances
12ul of dH2O
1ul of QS Ligase*
2ul of the digested vector pSB1C3
5ul of 4xQS Buffer (vortex before use)
Mix thoroughly by pipetting
Incubate at room temperature for 5 min to create cohesive ends
Run 2.5-5ul of the ligation mixture onto an agarose gel to check ligation efficiency against a known marker. Add 5ul of dye to aid the visualization of results.
Transform it into competent cells (E.coli)

Gel Electrophoresis

Gel was run in order to confirm that the cirularisation experiment had worked.
The linearised pSB1C3 vector was used as a control.
The results showed that the circularisation experiment worked, as the linearised vector is represented on the gel while the circularised vector was cloudy and ran off the gel.

Transformation of circularised pSB1C3 vector

After confirming the presence of the circularised vector, it was transformed into competent cells
This was left to incubate overnight at 37 degrees Celsius

Reculturing of transformed cells

The transformed cells containing the ligated product from yesterday's experiment were recultured onto 2 agar plates.
The 2 plates were divided into 12 squares each.
Each square was streaked with colonies that were randomly chosen from the 5ul and 10ul plates.
The plates were then left on the bench for overnight incubation

Incubation in broth

The next day the some colonies from the recultured plates were incubated in broth.
This was done in preparation of the miniprep.

Isolation of ligated plasmid

The ligated plasmid- chloramphenicol backbone and limonene biobrick, were isolated from cells that were incubated overnight in broth by miniprep.
Protocols from both Bioline kit and Thermoscientific were used for the miniprep.
there were 6 tubes containing the plasmid.
The plasmid concentration in each of the 6 tubes were measured using nanodrop.
200ng of plasmid from each of the 6 different tube was used for digestion.
sample volume(ul) concentration (ng/ul) yield(ug)
5.1 99 75 7.4
5.2 100 44.2 4.4
5.3 98 46.7 4.6
10.1 46 61.8 2.84
10.2 44 77.1 3.39
10.3 47 13.7 0.64

Digestion of ligated plasmid

Master Mix (changes were made from the protocol)
2ul of NEB Buffer
1ul of EcoRI
1ul of PstI
varying concentration of dH2O and plasmid depending on overall concentration of plasmid in each tube.
Final volume of each of the 6 tubes was 20ul.

Gel Electrophoresis

The product of digestion was run on agarose gel
This was done in order to confirm the presence of the limonene biobrick
The lanes are in the following order:
Marker, Sample 5.1, Sample 5.2, Sample 5.3, Sample 10.1, Sample 10.2, Sample 10.3, Marker.
We were expecting to see a 2kb and 5kb band. These bands appeared for samples 5.1, 10.1,10.2 and 10.3. To further determine the composition of samples, we did a single digest on the samples.

Single digest

For samples 5.1, 10.1, 10.2 and 10.3 two single digests each were made with EcoRI and PstI, giving a total of 8 samples.
The samples are run on 0.8% agarose gel.

Running of an agarose gel

Running the gel for digests of samples 5.1, 10.1, 10.2 and 10.3 from the previous day.
expectation-7kb band, confirming the presence of the limonene biobrick (5kb) and chloramphenicol backbone (2kb)
The gel shows the presence of 7kb bands for both digests of samples 10.1, 10.2 and the 5.1 sample, which was expected.
No bands appeared for samples 5.1.
For samples 10.3 there is a 2kb band, indicating that with the ligation, the chloroamphenicol circulized.

Making chloroamphenicol agar plates

Making additional plates
400ml of agar
Melt in microwave
3mins on low -> shake
Repeat
2mins on low -> shake
Repeat
Add 800ul of chloroamphenicol at a concentration of 25 ul/ml
Pour out onto 20 petri dishes
Leave to set on bench

Plating out samples

Plating out samples 10.1, 10.2, 10.3 and 5.1 onto chloroamphenicol plates.
Grow overnight at 37C

Dillution of Herring sperm DNA

Dilutions were done in 3 sets: Samples 1-3 were diluted in 90ul of water, where 10ul of stock DNA was added from an overnight dilution of 100um of Herring sperm DNA in 900ul of water.
Samples 1s-3s were also diluted in 90ul of water, except the first 10um of DNA was taken from an undiluted stock Herring sperm DNA.
Samples 1 5/45- 3 5/45 were from a known concentration of DNA stock, where 5ul of DNA was added to 45ul of water.
sample concentration (ng/ul) 260/280 260/230
1kb 534 1.82 1.95
1 5/45 52.7 1.77 2.05
2 5/45 4.6 1.46 1.88
3 5/45 0.1 0.24 -0.29
Overnight
1 in 10 24.8 1.8 2.42
1 2.1 1.67 22.44
2 0.8 2.87 -3.99
Fresh Stock
1s 5341.8 1.78 2.15
2s 440.0 1.80 2.23
3s 45.1 1.83 2.26
concentration of DNA was measured using nanodrop.

Gel electrophoresis of Dilluted Herring sperm DNA

Lanes are: marker, 1 5/45, 2 5/45, 3 5/45, 1, 2, 3, 1s, 2s, 3s, lambda NT, lambda
Results are as expected. Lanes show that samples 1, 2 and 3 were degraded overnight, suggesting nuclease activity. Samples 1s, 2s and 3s are the fresh Herring sperm stock and show no degradation.

Making samples for DNA sequencing

Making chloroamphenicol/IPTG plates

400ml of agar
Boil for 3min x2
Boil for 2min x2
Cool to 40C
Add 800ul of chloroamphenicol at 25ug/ml
Add 400ul IPTG at 0.15mM
Makes 20 petri dishes

Streaked out samples of the limonene/pSB1C3 ligated plasmid

Streaked samples 5.1, 10.1, 10.2 and 10.3 onto the chloroamphenicol/IPTG plates
IPTG was used to induce the lac operon, and therefore induce limonene synthesis
Plates were labelled using special symbols by only one team member to ensure double-blinded test

Made polystyrene strips

--> include video here

Overnight culture preparation

To make glycerol broths, so sample can be frozen and preserved
Use four universal tubes, add:
4ml Luria Broth
8ul chloroamphenicol
Add bacteria from the original plates (sample 5.1, 10.1, 10.2 and 10.3 into a single tube each respectively)
*Each sample was also re-streaked on a chloroamphenicol plate to maintain current stock.

Isolating plasmid

From overnight culture, took 3ml of culture and centrifuged into pellet of samples 5.1, 10.1, 10.2, 10.3
Isolated the plasmid using omega bio-tek Plasmid mini kit I
Concentrations from nano drop are shown in the table below
Sample Volume(ul) Conc.(ng/ul) 260/280 260/230
5.1 92 65.8 1.87 1.75
10.1 88 36.9 1.80 1.77
10.2 89 48.3 1.79 1.98
10.3 94 17.4 1.84 1.59

Digesting the plasmids for restriction mapping

Digesting 200ng of DNA with SacI
1ul of SacI
2ul of NEB buffer 1.1
DNA volumes added for samples 5.1 to 10.3:
3ul; 5ul; 4ul; 11.5ul
Water added for samples 5.1 to 10.3:
14ul; 12ul; 13ul; 5.5ul
Digestion in 37C water bath for 30mins
Heat kill at 80C for 20mins

Running an agarose gel

Add 5ul of 6x orange G to each sample
1kb marker is used
Wells are loaded in the following order:
5ul of marker, 25ul of samples 5.1; 10.1; 10.2; 10.3, 5ul of marker
The lanes are as expected.
Samples 5.1, 10.1 and 10.3 were expected to show 3 fragments, sized 2070, 1890 and 1529bp. This is what is shown on the gel.
Sample 10.3 only has one SacI restriction site and when cut, a band of 2070bp is expected. That is also shown on the gel.

Glycerol stocks

Took 750ul from overnight culture and centrifuged at full speed for ~2 minutes
Supernatant was removed
Pellet resuspended in 375ul of HMFM
Samples were then frozen at -80

Sonicating Herring sperm DNA

The herring Sperm was to viscous, so to reduce viscosity the sonicator was used
1ml of core DNA used in 2 tubes, 1 control and 1 to go in the sonicator
The control tube was left on the bench at room temperature
The 2nd tube was put in the sonicator for the folowing times: 2mins, 2mins, 5mins, 5mins, 20mins, 20mins, 30mins
Each time both tubes were filmed to compare viscosity

Sonicating herring sperm DNA

Pipetting out sonicated samples every 30mins
Pipette 4ul of DNA into Son 1-6 every 30mins
Dilute 1ul of DNA from Son 1-6 in 9ul of 1xTE buffer to tubes 10xdil 1-6
Vortex each dilution thoroughly and centrifuge briefly.
Keep tubes on ice

Running an agarose gel for sonication analysis

To tubes 1-6, add 14 ul of sterile water and 5 ul of orange G dye and 1ul of DNA from Dil x10 1-6 appropriately. Centrifuge briefly. Keep on ice until loading.
Use 5 ul of 1kb marker on both ends
Add buffer so that wells in the tray and the tray itself are covered
Run at 80 V for an hour and a half (gel is 1.2%)

Making agar, chloroamphenicol and chloroamphenicol/IPTG plates

One container of 400 ml Luria Agar was melted down in the microwave. This is enough to make 20 agar petri dishes.
This was poured straight into 4 petri dishes to make agar plates
The remaining agar had 0.64 ul of chloroamphenicol added to it (concentration = 24 ug/ml), and was mixed thoroughly
The resulting solution was poured into 4 petri dishes, to make 4 chloroamphenicol agar plates
The remaining agar solution had 1.5 ul of IPTG added to it (concentration = 24 ug/ml)
This was mixed thoroughly, and then used to make up the remaining 12 chloroamphenicol/IPTG plates.

Agarose gel preparation

20 ml of 5 x TBE, 80 ml of distilled water and 0.8 g of agarose was added into a container.
The solution was boiled for 3 minutes, 1 minute at a time.
The solution was left to cool.
5 ul of ethidium bromide was added to the solution.
The solution was then poured into the gel plate and left to set for 30 minutes.

Dilutions of Herring Sperm DNA

Add 9ul of TE buffer to 6 epindorph tubes
Pipette 1ul of each sonicated DNA sample 1-6 into each buffer for a 10x dilution
vortex thoroughly and centrifuge briefly

Running dilutions on 0.8% gel

1ul of dilution was put in 14ul of water and 5ul of orange G, to make up a total volume of 20ul for each sample.
5ul of 1kb ladder was used on both ends as a marker

Testing for limonene

Took sample plates to chemistry lab

Serial dilution of herring sperm DNA

100ul DNA and 900ul TE to make master mix
5 independent samples 10ul each were taken from master mix
Each independent sample was diluted twice in 90ul of TE
20 dilution samples were then nanodropped to check dilution accuracy
Sample nr Concerntration(ng/ul) 260/280 260/230
nr. 1/1 529.9 1.81 2.26
nr. 1/2 52.1 1.86 2.32
nr. 2/1 454.3 1.81 2.28
nr. 2/2 46 1.82 2.23
nr. 3/1 457.3 1.83 2.28
nr. 3/2 529.9 1.81 2.26
nr. 4/1 522.8 1.82 2.27
nr. 4/2 47.3 1.87 2.26
nr. 5/1 481.4 1.82 2.28
nr. 5/2 40.8 1.84 2.35
Dilutions show accuracy
Master dilution is sonicated and every 30mins a 30ul sample is taken to dilute twice (10ul of DNA in 90ul of TE buffer)
6 30ul samples are taken
Samples are then run on a gel

Running the gel from sonication series

Samples were taken from sonicated tube every 30min intervals, a total of 6 samples.
Each was diluted 100 fold to get a concentration in the range of 40-50ng/ul
5ul of DNA was taken from the dilution, to which 10ul of sterile water and 5ul of orange G was added
Samples were run against a 1kb ladder and control herring sperm DNA, which was not sonicated.

Denaturing sonicated DNA

Denaturing DNA by heat shock for 10mins in a 95C heat block
Adding 5ul of OG dye

Running both denatured and sonicated samples on gel

For just the sonication samples 1-6, 5ul of OG and 10ul of sterile water was added to 5ul of DNA.
5ul of 1kb ladder was used for 3 wells each.
The last 6 wells after ladder are the denatured DNA samples.
We were expecting to see fragmentation for the denatured samples.
There is no significant difference in between the sonicated samples and the sonicated and denatured ones.
There is a slight decrease in bands depending on the sonication time interval.
Suggestions are to use ultra-sonification to view the effects focused just on the sample.

Making nutrient agar plates and broth

Making up broth and agar solution to grow P. putida in.
For agar plates:
9.2g of nutrient agar medium
400ml of distilled water
For broth:
3.2g of nutrient broth
400ml of distilled water
Both were autoclaved for 45mins
Agar was poured onto 16 plates

Plating out bacteria

Freeze dried P. putida was rehydrated using 1ml of nutrient broth
The culture was aseptically transferred back into the broth containing tube
Mix
From that tube, colonies were streaked onto 6 plates and left to incubate over night at 30C

Growing bacteria in broth

100ml of autoclaved broth was added to 2 flasks each
The broth tube, containing the bacteria, was divided between flasks
Flask were left to incubate at 30C on a shaker overnight

Reculturing Bacteria

The P. putida grew overnight, which proved that we had viable cells.
The bacteria was then re-streaked to single colonies and left to grow overnight in a 37C incubator.

Isolation of P. putida DNA

8 1.5ml samples were isolated from each of the 2 broths that were prepared yesterday.
The first few steps of CTAB protocol was used to prep cells for DNA isolation;
The 8 samples were spun down at 10000 rpm for 5 mins.
The supernatant was discarded.
cells were then resuspended in 1ml of TE.
740ul of this new mixture was transferred to 8 new eppendorf tubes.
20ul of lysozyme was added to each of these 8 samples.
A maxwell robot was then used to complete the DNA extraction process.

Hydrodynamic shearing of Herring Sperm DNA

A 20G syringe was used ~24 times to squirt the herring sperm DNA in order to make it less viscous.
30G syringe was also used
This method seems to work better than the sonification.

Measuring the concentrations of isolated P. putida DNA from the previous day

Measuring concentration using nanodrop
Blanking against buffer
Sample nr. Concerntration ng/ul 260/280 260/230
2 44 1.8 1.15
4 30.6 1.8 1.29
6 42.3 1.81 1.05
8 35.6 1.85 1.26
10 38.2 1.84 1.28
12 40.6 1.83 1.45
14 39.9 1.88 1.47
16 18.5 1.17 0.67

Preparing samples to run on 1% gel

500ng of each of the isolated P. putida DNA sample is run on gel
Volumes are adjusted to 20ul per well accordingly (includes DNA, sterile H2O and OG)
5ul of orange G dye is added to each sample
5ul of 1kb ladders are used
For sheared DNA, dilutions were loaded
1ul of DNA was diluted in 9ul of 1xTE buffer to make up 10x dilution
1ul from 10x dilution was put in 9ul of 1xTE buffer to make up 100x dilution
Dilutions were nanodropped and the concentration for 100 fold dilution was 121 ng/ul
200ng of herring sperm DNA was run on gel
One lane was left for control, non-sheared DNA, also 100 fold dilution

Running gel of P. putida DNA and Herring sperm DNA

Samples in lanes goes as follows: 1 Kb ladder, 2, 4, 6, 8, 10, 12, 14, 16, 1 kb ladder, 100x dilution of sheared herring sperm DNA, control 100x diluted herring sperm DNA

Running sonicated herring sperm DNA on 0.8% gel

3 lanes for running:
Sheared and sonicated
Unsheared and sonicated
Unsheared and unsonicated
5ul of 1kb marker is used
The DNA samples are diluted 100 fold and 200ng of sample is run.
Volume of sterile water is adjusted appropriately to make up 20ul of sample per well, including 5ul of orange G dye
Not visible on the computer file, but picture shows a very slight decrease in sheared/sonificated and unsheared/sonicated samples vs the unsheared/unsonificated control
The difference is not significant, but the viscosity has changed when mechanically spreading the DNA on polystyrene, though it is not that evident on the gel.

Making up a sheared/sonicated dilution to leave on bench overnight

500ul of sheared/sonicated DNA
500ul of 1xTE
Mix
Leave on bench overnight

Incubating sheared/sonicated dilution at 37C on a shaking rack

10ul of 1xTE added to 2ul of sheared/sonicated DNA
Mix
Incubated overnight at 37C on a shaking rack

Nanodropping overnight incubations of herring sperm DNA

Table representing the concentrations of herring sperm DNA before and after different treatments
Sample Concerntration
Sheared/Unsonicated (s.u.s) 17900ng/ul=17.9mg/ml
S.u.s 10fold dil. 1790.1ng/ul
S.u.s 100fold dil 152.6ng/ul
Sheared/Sonicated (s.s) 17667ng/ul=17.6mg/ml
S.s 10fold dil. 1766.7ng/ul
S.s 100fold dil. 156.2ng/ul
Sheared/sonicated overnight Concentration in the tube=Average of the two samples=16.9mg/ml
500ul(DNA) in 500ul(1xTE) 14485.9ng/ul
2ml(DNA) in 10ml(1xTE) 3883ng/ul
Concentrations decrease with dilutions
The stock concentration in sheared/sonicated tube varies slightly, when derived from measured dilution concentrations that were subjected to different treatments (i.e. overnight incubation), though they orignated from the same tube
Difference in concentration is not too significant though: proposed 17.6mg/ml vs 16.9mg/ml

Running overnight dilutions on gel

Lanes are as folllows: 1kb ladder, dilution 500ul DNA in 500 1xTE, dilution 2ml DNA in 10ml 1xTE, control unsheared/unsonicated 100 fold dilution.

Running 16s PCR of P. putida

Lanes are as follows: 100kb ladder, pcr samples 1, 2, 3, 4, 100kb ladder

Gel Extraction of PCR

Cut out the bright band
Use Thermo scientific geneJET extraction kit

Running DNA from purified gel

Lanes are as follows: 1kb ladder, samples 1+2, samples 3+4, 1kb ladder

Sent samples for sequencing

Sent sample to PNACL to be sequenced

First trial of polystyrene combustion with DNA

Tested with DNA covered strips and non DNA covered strips
Tested with 1, 2, 3, 6 strips at a time.
Burned with bunsen burner against a ruler to measure rate
+DNA burned with yellow flame, black smoke and left carbon residue
-DNA appeared to melt with into the more compact form of polystyrene and flame did not catch
Experiment is being redesigned to improve it as results were not as expected

Gel electrophoresis

Two different sets of gel were run due to the different fragment size of the PCR product.
Smaller fragments were run on a 2% agarose gel whilst larger fragments were run on a 1% gel.

DNA extraction from gel

Extracting previously run DNA from gel using Thermo Scientific GeneJet gel extraction kit and following its protocol.
Concentrations of DNA were measured by nanodrop
Sample B (Tod C gene) was not purified correctly, another PCR is needed. (Nanodrop shows contamination)
Table representing the concentration and volume of DNA isolated from samples
Sample Volume Concerntration ng/ul 260/280 260/230
A 48 19.3 2.02 0.03
C 50 27.7 1.88 0.04
D 49 26.9 1.71 0.05
E 50 20.5 1.98 0.03

Make 2% agarose gel

Run Tod operon ligation genes on the gel

1.5h at 70V

Isolate the DNA from gel

DNA isolated using Bioline Isolate II PCR and gel kit and following its protocol

Measuring concentration of DNA using nanodrop

Sample Volume Concerntration ng/ul 260/280 260/230
A1 30 14.7 1.81 1.41
A2 31 13 1.71 1.43
B1 30 23.6 1.93 1.02
B2 29 21.9 1.88 1.33
C1 29 14.7 1.83 0.63
C2 30 15.5 1.86 0.64

Preparing samples to be sent to be sequenced by PNACL

Repeating the combustion experiment

Blocks of both DNA and no DNA coating were made
Blocks are thicker than last experiment to observe the difference
Both DNA and no DNA blocks were sprayed with water and dried for equal treatment conditions

Second attempt at polystyrene combustion with DNA

Larger strips were used
DNA was spread on some and water was spread on some other
Strips were left to dry on the bench
some strips were cut from a block of polystyrene which was made with DNA
Each strip was burnt with a bunsen burner with a ruler and filmed to compare the rate of burning
Results were not as expected, DNA appeared to make no difference except a blacker remnant

Preparation of IPTG and Chloramphenicol plates

The IPTG/Chloramphenicol plates that were prepared earlier on (08/08/13) for the volatile organic compound (VOC) test were found to be contaminated.
Hence new plates had to be made using the below protocol;
PROTOCOL:
x2 400ml of already prepared and sterilized agar was obtained from the media kitchen.
The agar was microwaved using the lowest power level at 2-3 mins intervals until completely melted.
The x2 400ml agar were then placed in the 37 degrees room to cool.
After cooling, 800ul of cholramphenicol and 400ul of IPTG were added to one bottle whilst only 800ul of chloramphenicol was added to the second bottle.
The content of both agar bottles was then poured into petri dishes.
3 (chloramphenicol+ IPTG) plates were streaked with 5.1 ligated product (limonene biobrick and chloramphenicol backbone) from earlier and 3 others were streaked with 10.2 ligated product.
RFP colonies were streaked on 3 chloramphenicol resistance plates.
All 9 plates were Incubated overnight in a 37 degrees room.

Ligation of PCR products (TOD operon) using the Promega pGEM-T Vector System

The samples ligated were A (TODX), C (TODF) and E (TOBG)
The promega protocol was followed and it can be found at
http://www.promega.co.uk/resources/protocols/technical-manuals/0/pgem-t-and-pgem-t-easy-vector-systems-protocol/
To calculate the amount of DNA insert needed for each sample, we used the promega biomath calculator (www.promega.com/biomath). We used the 1:3 ratio of vector to insert.
Size of the PCR inserts (add 56bp to account for the primer)
TodX 544 + 56= 600
TodF 460+56= 516
TobG 807 + 56=863
Volume of DNA insert for each sample
A - 1.6ul
C - 1.1ul
E - 1.5ul
The samples were incubate at 4 degrees overnight to be transformed tomorrow morning.

Overnight Broth

RFP cells were incubated in luria broth in a 37 degrees shaker incubator
The cells would be minipreped tomorrow to serve as a backbone for the ligation of the TOD biobbricks.
How to make the broth
Using a 15ml centrifuge tube add:
5ml of luria broth
5ul of Chloramphenicol

Preparation of Ampicillin Resistance plates

Ampicillin resistance plates were made by adding 400ul of Ampicillin to 400ml of agar.
This would be used to grow the transformants of samples A,C and E (above) as pGEM-T Vector has AmpR gene.

Volatile organic compound (VOC) experiment of limonene biobrick/pBS1C3 backbone

9 plates were taken over to our chemistry department to measure the expression of limonene.
The equipment used for this assay is a Proton Transfer Reaction- Time of Flight Mass Spectrometer.
PLATES
3 plates of 5.1(see 05/08/13) ligated product
3 plates of 10.2 (see 05/08/13)ligated product
3 luria agar plates ( to be used as control, for blanking the equipment)

Miniprep of cells

The pSB1C3 RFP cells that were incubated in luria broth overnight yesterday, were minipreped using the OMEGA bio-tek protocol, in order to isolate plasmid of interest.
Nanodrop results
Sample Volume Concerntration ng/ul 260/280 260/230
1 40 56.2 1.89 1.95
2 40 62.3 1.88 2.02

Double Digest of the pSB1C3 miniprep

Samples 1 and 2 were transfered to new eppendorf tubes
In each tube it was added
39ul of DNA (miniprep)
1ul of XbaI
2ul of SpeI
6ul of cut smart buffer
12ul of sterile water
The samples were incubated at 37 degrees water buffer After the samples were incubated at 80 degrees to kill the enzymes

Transformation of TOD genes ligations done on the 02/09/13 using the pGEM-T Vector System I-A3600 (changes were made to the protocol)

Centrifuge the ligations reactions briefly.
Add 5ul of each ligation reaction to a sterile 1.5ml
Thaw the competent cells on ice. Mix the cells by gently flicking the tube.
Carefully transfer 100ul of the competent cells to the ligation reaction tubes.
Incubate the tubes on ice for 20 minutes
Heat-shock the cells for 45-50 seconds in a water bath at exactly 42C degrees. Do not Shake. Immediately return the tubes to ice for 2 minutes.
Add 950ul of room temperature SOC medium to the ligation reaction transformations. incubate for 1.5 hours at 37C with shaking.

Plating out the transformants

The transformants would be plated out on Ampicillin resistant plates that were prepared yesterday.
40ul of X-Gal and 20ul of of IPTG were streaked respectively unto the already made plates. (except the viability and resistance test plates) Below is a list of the plates that were made;
1)x2 plates of positive control (no PCR product)- 20ul and 200ul plates 2)x2 plates of Background control- 20ul and 200ul 3)x2 plates of ligated product 1 (L1) - A- 20ul and 200ul plates 4)x2 plates of L2- C -20ul and 200ul plates 5)x2 plates of L3- E - 20ul and 200ul plates 6)x2 transformation control - (50pg of puc19) - 20ul and 200ul plates 7)x1 Viability control (only luria broth)- 200ul of cells 8)x1 resistance control (Only Amp agar) - 200ul of cells
All 14 plates were incubated overnight at 37 degrees centigrade.

Transformation results

From the above results,colonies were found growing on the resistance control plate, which indicates that our competent cells already express ampicillin resistance, but this is not meant to be so. Hence in order to confirm that our results are reliable;
colonies would be randomly selected from each of the two plates (20ul and 200ul) for the 3 TOD genes
These colonies would be cultured in luria broth + Amp. This broth would be incubated overnight in a 37 degrees shaker incubator.

Gel Electrophoresis

The double digest (pSB1C3) from yesterday was run on a 1% gel.
This was done in order to confirm that the digest worked and also to purify the pSB1C3 vector.
From left to right
Sample 1.1 - track 2
Sample 1.2 - track 3
Sample 2.1 - track 4
Sample 2.2 - track 5
The 2 Kb bands are the pSB1C3 backbone
The 1 Kb bands are the RFP biobrick
The two higher bands in tracks 2 and 3 are plasmids that were not digested.

Gel purification of the pSB1C3 backbone and RFP biobrick

The Zymoclean Gel DNA recovery Kit was used to perform the purification and its protocol was followed.
However the elution step was changed to 12ul of elution buffer, and this step was repeated.
Nanodrop of the samples
Sample Volume Concerntration ng/ul 260/280 260/230
pSB1C3 1 20 34 1.67 0.92
pSB1C3 2 40 62.3 1.88 2.02
RFP 1 20 28.8 1.57 0.71
RFP 2 18.8 22.2 1.79 1.84

Double digest of TOD genes PCR products

Samples A (TodX), C (TodF) and E (ToBG) were digested with the enzymes XbaI and SpeI.
Protocol
Sample A C E
Volume (ul) 20 23.5 21
Spel (ul) 1 1 1
Xbal 0.5 0.5 0.5
Custmart Buffer 6 6 6
5m Tris Hcl (ul) 32.5 29 31.5
The samples were incubated at 37C for 90 minutes
Heat kill the enzymes by incubating the samples at 80C for 20 minutes

Ligation of the TOD genes (X, F and ToBG) to the pSB1C3 backbone

The pGEM-T Vector System was used, However changes were made to the protocol. The promega biomath caculator (www.promega.com/biomath) was used to work out the ratio of insert to vector. The DNA concentration of the TOD genes can be found at Lab work 28/09/2013. The DNA concentration of the pSB1C3 and the RFP biobrick can be found above. The amount of vector DNA was added at 50ng.
Samples A (TodX) C (TodF) E (ToBG) RFP-sample 2 (positive control) Background Control
@X Rapod ligation buffer (ul) 5 5 5 5 5
vector (pSB1c3-sample1) (ul) 1.6 1.6 1.6 1.6 1.6
T4 DNA ligase (ul) 1 1 1 1 1
PCR product (ul) 2.3 1.4 3.1 3.6 -
Deionized water for the final volume of 12 ul 2.1 3 1.3 0.8 4.4

Isolating microbes from CSE kits

We received some CSE kits from one of our participating schools.
It is to be noted that the polystyrene was not significantly degraded.
Distilled water was run down each of the 2 sides of the kit (the polystyrene and miscellanous sides)into 2 separate petri dishes.
a spreader was used to spread the sample from each of the petri dishes onto luria agar plates.
Thus each of the 2 samples from each CSE kit was incubated at 3 different temperatures (room temperature, 30 degrees and 37 degrees) Because we received 5 CSE kits, 30 plates were incubated.

Transformation of pSB1C3/TOD genes

Centrifuge the ligation
Add 6 ul of each ligation reaction to a sterile 1.5ml tube on ice
Thaw the cells on ice
Carefully transfer 50ul of cells to the ligation reaction. Gently flick the tubes and incubate on ice for 20 minutes.
Heat shock the cells for 45 seconds in a 42'C water bath. Do not shake. Immediately return the tubes to ice for 2 minutes.
Add 950 ul of SOC medium (at room temperature) to the ligation reactions. Incubate for 1.5 hours at 37'C on a shaker.
The controls for this experiment are the resistance and viability controls.
One tube has 50 ul of highly competent cells and SOC medium added to it.
The samples A (TodX), C (TodF), E(ToBG), positive control, and background control were plated on chlorophenicol resistant agar plates, at the volumes of 20ul and 200ul. A 100ul of only highly efficient cells and SOC medium was plated in a chlorophenicol plate and another 100ul was plated on a LB plate.

Isolate plasmid from overnight broth

The plasmids were isolated using the Omega Plasmid Mini Kit 1, and its protocol was followed.
Nanodrop results
Sample Volume Concerntration ng/ul 260/280 260/230
TodX 1 39 37.8 2.02 1.72
TodX 2 43.8 59.1 1.9 1.74
TodF 1 42 100.4 1.9 2.02
TodF 2 40.5 26.2 1.92 1.66
ToBG 1 45 53.2 1.94 1.67
ToBG 2 47 21.6 2.00 1.43

Double digest of isolated plasmid with SpeI and XbaI

Master mix for 12 reactions
36 ul of cut smart buffer
1.2 ul of XbaI
2.4 of SpeI
44.4 ul of 5mTris Hcl
Protocol
Sample DNA (ul) Master Mix (ul) 5mTris Hcl (ul) added to final volume of 30ul
TodX 1 13.2 9 7.8
TodX 2 8.5 9 12.5
TodF 1 8.5 9 19
TodF 2 5 9 2
ToBG 1 9.5 9 11.6
ToBG 2 23 9 0

Results from double digest of isolated plasmid with SpeI and XbaI

Experiment conducted on the 05/09/13

Results from the transformation of pSB1C3/TOD genes

Experiment conducted on the 05/09/13
The positive RFP control showed colony growth on both the 20 ul and the 200 ul plates, but showed a mix of red and white colonies.
The background control also showed colony growth, which was not expected.
Upon further investigation, it was discovered the XbaI and SpeI have complementary sticky ends which could result in re-circularisation of the vector backbone to itself. This explains the presence of white colonies on the RFP positive control and the growth on the background control. To identify if this has occurred, another double digest will be carried out.
The samples A (TodX), C (TodF) and E(ToBG) all showed colony growth for the 20 ul and the 200 ul plates.

Miniprep of overnight broth

Following on from 06/09/13 result,overnight broth was prepared yesterday from the single colonies that had grown on each of the 2 plates shown on 06/09/13.
The broth, which contains cells that have been transformed with pSB1C3/TOD genes, was minipreped using the Omega Bio-Tek kit.
This would enable us to confirm which cells have the recircularised plasmid and those with the ligated product.

Measurement of DNA concentration

Sample Volume Concerntration ng/ul 260/280 260/230
TOD X1 31.6 86.5 1.87 1.92
TOD X2 31.7 58.7 1.89 1.26
TOD X3 32.7 56.6 1.91 1.88
TOD X4 31.6 55.8 1.88 1.65
TOD X5 31.7 44.4 1.87 1.78
TOD X6 31.7 70.5 1.88 1.88
Sample Volume Concerntration ng/ul 260/280 260/230
TOD F1 32.4 39.6 1.91 1.59
TOD F2 33.7 49.4 1.91 1.65
TOD F3 32.3 47.4 1.89 1.71
TOD F4 31.6 43.7 1.94 1.73
TOD F5 36.5 57 1.89 1.50
TOD F6 38 59.4 1.89 1.61
TOD G1 36.8 72.5 1.89 1.51
TOD G2 44.7 1.90 1.90 1.65
TOD G3 33.7 50.2 1.90 1.46
TOD G4 41.9 55 1.93 1.35
TOD G5 34 43 1.96 1.54
TOD G6 35 48 1.89 1.72
DNA concentration was measured using Nanodrop.

Double Digestion of pSB1C3/TOD genes

The pSB1C3/TOD genes were double digested with (XbaI and SpeI) & (EcoRI and PstI)
The master mix for the (XbaI and SpeI) was;
60ul of cut smart buffer 5ul of XbaI 10ul of SpeI 273ul of 5M Tris
The master mix for the (EcoRI and PstI) was;
60ul of cut smart buffer 5ul of XbaI 5ul of SpeI 278ul of 5M Tris
All 36 tubes were incubated overnight in 37 degrees room.
Tomorrow the plasmids that were isolated from the miniprep would be run on a 1% agarose gel to distinguish between cells that have the pSB1C3/TOD genes from those that have the recircularised pSB1C3 vector.
Meanwhile the plasmids from the miniprep were sent for sequencing this afternoon.

Dissolution of polystyrene in Limonene

This experiment was set up to decide how much limonene can economically dissolve polystyrene.
MATERIALS USED
20ml solution of 25% limonene.
8cm x 5cm x 2cm polystyrene block (thus volume of 80cm^3)
RESULT
It took ~33 minutes for the block to be completely dissolved

Dissolution of polystyrene

a 20ml solution of 50% Limonene was made to determine if the dissolution of polystyrene from 09/09/13 would occur faster.
as predicted, the 8cm x 5cm x 2cm PS block was completely dissolved in 9 minutes.

Gel electrophoresis

The samples from the double digest on 09/09/13 were run to confirm if the digestion worked.
From the results, we would also be able to distinguish between cells that have been successfully transformed with the ligated pSB1C3/TOD genes from those with the recircularised pSB1C3.
Results of the Gel electrophoresis
TODX Gel
Wells order: TODX1 (SpeI/XbaI), TODX1 (EcoRI/PstI); TODX2 (SpeI/XbaI), TODX2 (EcoRI/PstI); TODX3 (SpeI/XbaI), TODX3 (EcoRI/PstI); TODX4 (SpeI/XbaI), TODX4 (EcoRI/PstI); TODX5 (SpeI/XbaI), TODX5 (EcoRI/PstI); TODX6 (SpeI/XbaI), TODX6 (EcoRI/PstI). The expected results were that the we would see the TODX genes drop off in separate band in all the digestions in its respective size (600bp). However as it can be seen in the picture above only the samples cut with SpeI and XbaI had two fragments and they are the wrong size (~ 1Kb). The samples TODX (1, 2 and 6) were sent to be sequenced before the digestions and it showed that the pSB1C3 plasmid re-circularized. This is because the two enzymes have complementary sticky ends.
TODF
Wells order: TODF1 (SpeI/XbaI), TODF1 (EcoRI/PstI); TODF2 (SpeI/XbaI), TODF2 (EcoRI/PstI); TODF3 (SpeI/XbaI), TODF3 (EcoRI/PstI); TODF4 (SpeI/XbaI), TODF4 (EcoRI/PstI); TODF5 (SpeI/XbaI), TODF5 (EcoRI/PstI); TODF6 (SpeI/XbaI), TODF6 (EcoRI/PstI). This shows the same results as TODX above.
TOBG
Wells order: TOBG1 (SpeI/XbaI), TOBG1 (EcoRI/PstI); TOBG2 (SpeI/XbaI), TOBG2 (EcoRI/PstI); TOBG3 (SpeI/XbaI), TOBG3 (EcoRI/PstI); TOBG4 (SpeI/XbaI), TOBG4 (EcoRI/PstI); TOBG5 (SpeI/XbaI), TOBG5 (EcoRI/PstI); TOBG6 (SpeI/XbaI), TOBG6 (EcoRI/PstI). This shows the same results as TODX above.

Nanodrop of the pGEM-T plasmids that were ligated with the TOD operon genes and the pSB1C3 backbone

Sample Volume Concerntration ng/ul 260/280 260/230
TodX 1 25.8 37.4 1.84 1.52
TodX 2 35 61.3 1.82 1.74
TodF 1 37.8 99.4 1.83 1.99
TodF 2 22.7 25.7 1.76 1.60
ToBG 1 31.4 51.7 1.84 1.57
ToBG 2 20.1 21.9 1.83 1.26
pSB1C3 1 10.3 31.8 1.65 1.44
pSB1C3 1 19 40.9 1.81 1.71

Double Digestions of the plasmids above

Sample DNA Volume Buffer Xbal Pstl dH2O to reach final volume of 60 ul
TodX 45.5 6 1 1 6.5
TodF 49.6 6 1 1 2.4
TodG 42.9 6 1 1 9.1
pSB1C3 25 6 1 1 27

Gel electropheresis of the double digestion performed in the 10/09/13

The picture above shows that the double digestion hasn't worked as expected. Different reasons of why it hasn't worked were discussed and the reason agreed was that the PStI enzyme was not working properly.

Isolate plasmid from overnight culture

Using Omega mini prep kit protocol
Samples:
TODF 1,2,3,
TODX 1, 2, 3
TOBG 1, 2, 3,
RFP 1, 2, 3
Sample Volume (ul) Concerntration (ng/ul)
TODF1 43 120
TODF2 43 98.8
TODX1 42 399.3
TODX2 44 442.2
TODX3 43 417.5
TODG1 43 262.4
TODG2 47 319.2
TODG3 41 338.4
RFP1 41 77.7
RFP2 41 32.7
RFP3 42 59

Glycerol stocks

Took 750ul from overnight culture and centrifuged at full speed for ~2 minutes
Supernatant was removed
Pellet resuspended in 375ul of HMFM
Samples were then frozen at -80

Gel Purification of the pGEM-T pasmid double digestions ran in the 11/09/13

The gel was purified by using the The Zymoclean Gel DNA recovery Kit and its protocol was followed.
Nanodrop Results
Sample Volume Concerntration ng/ul 260/280 260/230
TodX 48.5 7.1 1.83 0.72
Todf 45.5 21.7 1.89 1.19
TodBG/td> 47.7 9 1.77 0.70
pSB1C3 (RFP) 46.2 7.3 1.81 0.16

Digestion of the samples purified with the enzyme PstI-HF and XbaI

Two single digestions were set up to test if one of the enzymes was not working properly.
DNA volume (ul) Volume Custmart Buffer enzyme volume dH20 added to total volume of 60 ul
TODX 23 6 1 30
TODF 22.5 6 1 30.5
TOBG 22 6 1 31
pSB1C3 (RFP) 20.5 6 1 32.5
Gel image of the above double digestion Gel order: TODX, TODX, TODF, TODF, TOBG, TOBG, pSB1C3, pSB1C3 (XbaI); TODX, TODF, TOBG, pSB1C3 (PstI) The picture above shows that the assumption that one of the enzymes did not working properly was wrong, as it shows the same result as the gel run on the 11/09/13.

Double digestion of the isolated pGEM plasmids ligated with the TOD operon genes (X, F and TOBG)

As the digestions with the plasmids that were stored in the freezer did not work new digestins were set up with the isolated plasmids from the overnight culture.
The pGEM-T plasmid contain the restrictions sites for PstI and SpeI, which are also present in the amplified TOD operon gene and the pSB1C3 plasmid.
To avoid the recircularization of the pSB1C3 backbone when ligating the genes with this plasmid, the double digestion was set up with the enzymes PstI and XbaI.
Another double digestion with EcoRI and SpeI was set up to test if the restrictions sites present in the TOD genes are not mutated. If the bands in the gel shows a linear band, it can be assumed that the enzymes cut the pGEM plasmids in its PstI and SpeI restriction sites.
Master Mix of the PstI/XbaI double digestion 30 ul of cut samart buffer
5 ul of PstI
5 ul of XbaI
58 ul of dH2O
9.8 ul of the master mix were added to each reaction.
2 ug DNA of each sample were digested.
Protocol
Sample DNA volume (ul) dH20 (ul) addded to the final volume of 30 ul
TODF1 16.5 3.5
TODF2 20.2 0
TODX1 5 15.2
TODX2 4.2 16
TODFX3 4.8 15.4
TODFG1 7.6 12.6
TODFG2 6.3 13.9
TODFG3 5.9 14.3
Master Mix of the EcoRI/SpeI double digestion Only samples TODX1, TODX2 and TODX3 were used for this digestion
15 ul of cutsmart buffer
2.5 ul of EcoRI
2.5 ul of SpeI
106 ul of dH2O
25 ul of Master Mix was added to each reaction.
Sample DNA volume (ul) dH20 (ul) addded to the final volume of 30 ul
TODX1 5 25
TODX2 4.2 0.8
TODFX3 4.8 0.2
The digestion was left overnight in the 37C room.
Heat kill at 80C for 20 minutes.

Chemistry Lab Results

Two experiments were run in the chemistry lab.
Polystyrene Combustion
Two pieces of normal packaging polystyrene were burnt, which showed the flammability of polystyrene.
After two blocks of polystyrene made form the sugar given to the Leicester iGEM team by Jablite. One of them had DNA incorporated and the other had no DNA. We were able to establish that the polystyrene sugar provided to us from Jablite already had fire retardant chemicals incorporated, which did not allow us to test if DNA could work as a fire retardant for polystyrene.
Polystyrene dissolution in limonene

Gel electropheresis of pGEM-T vectors with the TOD genes

Gel order: TodX1, TodX2, TodX3, TodF1, TodF2, TobG1, TobG2, TobG3 (all cut with (XbaI/PstI); TodX1, TodX2, TodX3 (this were cut with EcoRI/SpeI)
The gel shows that once again the expected genes were not cut out from the plasmid. This could be because the restriction sites were mutated when they were cloned.

Digesting pSB1C3 backbone

Digesting for ligation with the already digested Tod operon PCR products
Following the iGEM official protocol
Using EcoRI-HF and PstI-HF
Exluding the DpnI from the master mix and adjusting the volume of water accordingly
Protocol can be found at: [1]

Ligation of digested pSB1C3 backbone to Tod F, X and Tob G

Using Promega protocol to which changes were made
Reagents Tod F Tod X Tod G Postive Control Background Control
2x Rapid Ligation buffer 5ul 5ul 5ul 5ul 5ul
pSB1C3 digest (50ng) 2ul 2ul 2ul 2ul 2ul
PCR Product 3.3ul 3ul 3.8ul - -
Control insert DNA - - - 2ul -
T4 DNA ligase 1ul 1ul 1ul 1ul 1ul
Deinoized water for final volume of 10ul - - - - 1ul
Mix reactions by pipetting. Incubate the reactions for 1h at room temperature.
Control insert DNA from the transformation efficiency kit provided by iGEM

Transformation of TOD genes ligations with the digested pSB1C3 using the pGEM-T Vector System I-A3600 (changes were made to the protocol)

Centrifuge the ligations reactions briefly.
Add 5ul of each ligation reaction to a sterile 1.5ml
Thaw the competent cells on ice. Mix the cells by gently flicking the tube.
Carefully transfer 50ul of the competent cells to the ligation reaction tubes.
Incubate the tubes on ice for 20 minutes
Heat-shock the cells for 45-50 seconds in a water bath at exactly 42C degrees. Do not Shake. Immediately return the tubes to ice for 2 minutes.
Add 900ul of room temperature SOC medium to the ligation reaction transformations. incubate for 1.5 hours at 37C with shaking.

Digestion of the TOD genes PCR products

The PCR products of TODX, TODF and TOBG were digested with the enzymes EcoRI-HF and PstI-HF.
Protocol
Sample DNA volume (ul) custmart buffer (ul) EcoRl (ul) Pstl (ul) dH20 (ul)
TODX 8.7 2 0.5 0.5 8.3
TODF 8.3 2 0.5 0.5 8.7
TOBG 8 2 0.5 0.5 9
The samples were incubated for 1 hour at 37C.
Heat kill the enzymes at 80C for 20 minutes.

Running the backbone and RFP on gel

on 1% gel to check if the gel extraction worked.
gel shows that extraction worked
2kb band representing the backbone is visible as well as 1kb representing the RFP

Digestion of the pGEM plasmid gel extracted on the 13/09/13

The samples were digested with the enzymes EcoRI-HF and PstI-HF
Master Mix for 8 reactions
16 ul of cutsmart buffer
4 ul of EcoRI
4 ul of PstI
88 ul of dH2O
14 ul of master mix was added to each reaction

Results from previous day

Background control plate had growth, which was not expected. This suggests that pSB1C3 backbone religated.
It was also thought that the Tod genes used were not from the PCR fusion experiment.
Same experiment done again, with a new set of Tod genes from a PCR fusion.
For digestion of backbone, already digested backbone from 01/08/2013 was used, which was digested with EcoRI and PstI.

Incubation of bacteria from the plates of previous day for mini prep

12 single colonies were picked from each plate and put into 15ml of broth
36 tubes were left incubating overnight at 37C

Sending pGEM-T vector with Tod insert clones to sequencing by PNACL

Digestion of new fusion PCR Tod genes

Digestion with EcorI-HF and PstI-HF using Cutsmart buffer
500ng of DNA was digested from the following Tod DNA concentrations:
Sample Concerntration ng/ul 260/280 260/230
TodX 49.5 1.89 1.99
Todf 33.9 1.98 1.68
Tod B 37.4 1.82 1.70
Volumes for double digest:
Sample DNA Buffer Water EcorI-HF PstI-HF
Tod X 10.1ul 3ul 15.9 0.5 0.5
Tod F 13.4ul 3ul 12.6 0.5 0.5
Tod B 14.7ul 3ul 11.3 0.5 0.5
Incubation at 37C for 30min
Heat kill at 80C for 20min

Ligation of Tod genes and pSB1C3 backbone

For background control, just the pSB1C3 backbone was used
For positive control, RFP plasmid from transformation efficiency kit provide by iGEM was used
Quick stick ligase was used and a different protocol from previous day
Bioline Quick Stick Ligase protocol:
Combine the vector and the insert in the appropriate ratio to make up no more than 100ng of DNA
Adjust volume to 14ul with ddH2O
Add 1ul of QS ligase
Add 5ul of 4x QS Buffer (vortex before use)
Mix thoroughly before pipetting
Incubate at room temperature for 5min
The volumes for ligation:
Sample DNA ul Vector(pSB1C3) ul QS ligase ul Buffer ul H20 ul
Tod X 0.9 2 1 5 5.1
Tod F 0.8 2 1 5 5.2
Tod B 1 2 1 5 5
Postive Control 1 2 1 5 5
Background Control 1 2 1 5 5

Transformation of TOD genes ligations with the digested pSB1C3 using the pGEM-T Vector System I-A3600 (changes were made to the protocol)

Centrifuge the ligations reactions briefly.
Add 5ul of each ligation reaction to a sterile 1.5ml
Thaw the competent cells on ice. Mix the cells by gently flicking the tube.
Carefully transfer 50ul of the competent cells to the ligation reaction tubes.
Incubate the tubes on ice for 20 minutes
Heat-shock the cells for 45-50 seconds in a water bath at exactly 42C degrees. Do not Shake. Immediately return the tubes to ice for 2 minutes.
Add 900ul of room temperature SOC medium to the ligation reaction transformations. incubate for 1 hour at 37C with shaking.

Plating out transformants on chloroamphenicol plates

Plating out a total of 10 plates, 2 for each sample
20ul and 200ul were plated from each sample
Plates were left over night at 37C.

Making and running an agarose gel

Making a 3% agarose gel to run Tod PCR fusion genes from 17/09
This is to determine that the digestion works
Running the gel with digested and undigested samples to observe the difference
Digested samples were taken from the digestions the Tod genes from previous day
100ng of both samples were run against a 100kb ladder
Rows are as follow:100bp ladder, undigested x, digested x, undigested b, digested b, undigested f, digested f

For selection of individual colonies

DNA isolation from PCR products

Isolating DNA using Omega nucleic acid purification kit and following its protocol.
Isolated DNA from all of the samples B and F and samples X3, 5, 6, 7, 8, 10, 12.
Selection was made by looking at gel pictures and selecting samples with visible bands.

Nanodropping the samples for concentration

Sample nr Volume ul Concerntration ng/ul 260/280 260/230
X3 41 11.3 1.87 1.29
X5 47 12.2 1.78 1.22
X6 34 12.9 1.79 1.22
X7 45 8 1.71 0.96
X8 43 10.5 1.88 1.2
X10 44 9 1.88 1.2
X12 45 12.8 1.70 1.40
F1 44.5 11.2 1.69 1.22
F2 44 9.1 1.88 1.20
F3 45.2 10.6 1.77 0.99
F4 43.7 9.7 1.82 1.10
F5 45.2 10.6 1.67 1.19
F6 45.4 9.6 1.82 0.85
F7 46 11 1.76 1.14
F8 46 11.7 1.73 1.24
F9 42.4 10.5 1.83 1.32
F10 46 11 1.93 1.39
F11 45.5 10.3 1.82 1.18
F12 45.5 14.9 1.83 1.32
B1 45 6.9 1.56 0.86
B2 46 10.5 1.64 1.17
B3 46 10 1.78 1.41
B4 47 11.5 1.70 1.35
B5 47 10.4 1.84 1.25
B6 47 8.6 1.96 1.33
B7 47 9.7 1.74 1.01
B8 46 12.4 1.58 1.22
B9 45 10.5 1.58 1.05
B10 46 11.1 1.73 1.32
B11 46 10.2 1.87 1.56
B12 46 12.1 1.75 1.38

Sending isolated DNA to be sequenced by PNACL

Sending 4 samples from each operon that showed highest DNA concentration: B5, 4, 9, 12; F8, 1, 10, 12; X3, 5, 6, 12.

Preparing overnight broths

Preparing broths from individual colonie plates from previous day
Selecting 4 colonies from each that showed highest DNA concentration from nanodrop: B5, 4, 9, 12; F8, 1, 10, 12; X3, 5, 6, 12.

Miniprep from overnight broths

DNA is isolated using Omega Miniprep kit and its protocol is followed

Nanodropping the isolated DNA

Sample Volume Concerntration ng/ul 260/280 260/230
X12 90 13.5 1.86 1.38
X3 43 13.6 2.12 1.34
X5 45 16 2.08 1.64
X6 44 19.1 2.04 1.59
B4 93 11.1 1.73 1.28
B5 87 9.5 1.99 1.34
B9 43 13.1 2.14 1.43
B12 43 14.9 1.99 1.34
F1 92 17.6 1.91 1.15
F8 93 17.6 1.85 1.70
F10 91 12.4 1.99 1.30
F12 41 18.5 2.06 1.71

Double digest of isolated DNA

Digesting with EcorI-HF/PstI-HF and XbaI/PstI to see if DNA incorporated insert has the biobrick prefix and suffix present.
Gel to be run in the 23/09/13

Gel Results from the digestion performed on the 20/09/13

Gel Order: X3 (E/P), X3 (X/P); X5 (E/P), X5 (X/P); X6 (E/P), X6 (X/P); X12 (E/P), X12 (X/P); F1 (E/P), F1 (X/P);
The gel shows that digestions were successful as every sample dropped the inserted gene. Gel Order: F8 (E/P), F8 (X/P); F10 (E/P), F10 (X/P); F12 (E/P), F12 (X/P); B4 (E/P), B4 (X/P); B5 (E/P), B5 (X/P); B9 (E/P), B9 (X/P); B12 (E/P), B12 (X/P).
Same result as the gel above

Evaporation of isolated plasmids and re-suspended in 1xTE

The samples were evaporated with a vacuum evaporator.
The samples were re-suspended in 20 ul of 1xTE.
Sample Volume Concerntration ng/ul 260/280 260/230
X3 20 12.1 1.49 1.44
X5 20 15.6 1.63 1.45
X6 20 25.2 1.63 1.46
B4 20 12.1 1.49 1.44
B9 20 16.3 1.63 1.45
B12 20 26.3 1.87 1.05
F1 20 38.9 1.83 1.57
F10 20 33.6 1.67 1.4
F12 20 6.5 1.48 1.10

Luria Agar plates

Luria agar plates were made for the plating of the CSE kits that arrived.

Plating out the CSE kits

The CSE kits that arrived yesterday were plated out. The polystyrene and the miscellaneous part were plated on two plates,one was incubated at room temperature and the other at 37C.

Overnight cultures

Overnight cultures of the biobricks samples were set up to prepare glycerol cultures tomorrow. The samples were F1, F10, F12, X3,X5, X6, B4, B9 and B12. These samples were sequenced and they had no mutations.

Glycerol Stocks

Glycerol stocks were made from the samples F1, F10, F12, X3,X5, X6, B4, B9 and B12. These samples were sequenced and they had no mutations.