Team:DTU-Denmark/Notebook/22 August 2013

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==Main purpose==
==Main purpose==
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*USER reaction
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*PCR for biobrick parts
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*gel purification of pZA21::ara with USER endings
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*colony PCR
==Who was in the lab==
==Who was in the lab==
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Gel purified the linearized plasmid pZA21::ara with USER endings
Gel purified the linearized plasmid pZA21::ara with USER endings
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===colony pPCR to verify AMO insert===
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===colony PCR to verify AMO insert===
Picked 10 colonies from yesterday's cloning for colony PCR. Diluted cells in 50 uL of MilliQ and took 1 uL as template
Picked 10 colonies from yesterday's cloning for colony PCR. Diluted cells in 50 uL of MilliQ and took 1 uL as template
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==Conclusion==
==Conclusion==
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=lab 115=
=lab 115=

Revision as of 17:50, 28 September 2013

22 August 2013

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Contents

lab 208


Main purpose


  • USER reaction
  • PCR for biobrick parts
  • gel purification of pZA21::ara with USER endings
  • colony PCR

Who was in the lab


Kristian, Henrike

Procedure


USER ligation and transformation

Redid for HAO and cyc in arabinose inducible pZA21::araBAD and for Nir fragments

PCR for Biobrick parts

Set up a new PCR reaction for Biobrick parts using HF buffer and 5% DMSO but no MgCl2. PCR was run on a touchdown program

primers: 53a, 53b

template: Sec2 miniprep

program:

temperature time cycles
98C 2:00 -
98C 0:10 10
63C 1:00 10
-0.5C per cycle
72C 1:00 10
98C 0:10 25
53C 1:00 25
72C 1:00 25
72C 5:00 -
10C hold -

Gel purification

Gel purified the linearized plasmid pZA21::ara with USER endings

colony PCR to verify AMO insert

Picked 10 colonies from yesterday's cloning for colony PCR. Diluted cells in 50 uL of MilliQ and took 1 uL as template

primers: 53a, 53b

program:

temperature time cycles
98C 10:00 -
98C 0:10 36
56C 0:30 36
72C 2:00 36
72C 5:00 -
10C hold -

Results


nanodrop measurement of ara spl plasmids

Nd ara spl.jpg

Conclusion


lab 115


Main purpose


Run Experiment 2 in two different samples anaerobically in order to characterize the behavior of E.coli.

Who was in the lab


Ariadni, Helen

Procedure


Adjusting the temperature at 36 degrees and calibrating the probes as described in Calibration protocol.


Following the protocol Experiment 2

Changing the steps :

6. 4 ml of the overnight culture growing in DM minimal medium

12. The OD was measured OD=0.261 in sample A and OD=0.263 in sample B.

19.

  • For sample A after taking the first sample, we continue with two more samples after 5 and 10 minutes. Then we add 2 ml of nitrite solution and continue by taking a sample after spiking. Then we took three more samples and after 15 minutes we spike with 2 ml of nitrite, and finally we took a last sample. The final OD measurement was OD=0.244 and the temperature was 36.8 degrees.
  • For sample B after taking the first sample, we continue with two more samples after 5 and 10 minutes. Then we add 1 ml of nitrite solution and continue by taking a sample after spiking. Then we took two more samples and after 10 minutes we spike with 4 ml of nitrite, and then there was a response after 12 minutes were finally we took one sample and after 5 minutes the last. The final OD measurement was OD=0.248 and the temperature was 36.4 degrees.

Results


Colorimetric results

Ranges

  • Measuring range 2-75 mg/L NH4-N
  • Measuring range 1-25 mg/L NO3-N
  • Measuring range 0.02-1 mg/L NO2-N


Standard solutions

  • Ammonium - 66.6 mg/L (expected 39 mg/L)
  • Nitrite - 0.72 mg/L (expected 0.5 mg/L)
  • Nitrate -


For Sample A

time nitrite (mg/L) nitrate (mg/L) ammonium (mg/L)
0 <0.02 <1 3.8
5 <0.02 <1 <2
10 <0.02 <1 0.3
spike 0.7 <1 <2
15 0.7 <1 0.7
20 0.71 <1 0.2
25 0.72 <1 <2
second spike 1.46 1.7 2.7
35 1.42 1.6 <2

For Sample B

time nitrite (mg/L) nitrate (mg/L) ammonium (mg/L)
0 <0.02 - <2
5 <0.02 - <2
10 <0.02 - <2
spike 0.36 - <2
15 0.4 - <2
20 0.4 <1 <2
second spike 2.12 2.3 <2
30 1.78 2.6 0.4
35 1.74 2.7 <2

N2O measurement

Dtu Experiment 2 round 2 --sample A.png Dtu Experiment 2 round 2 -- sample B.png

Conclusion

There was no response from native E.coli.



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