Team:Cambridge/Lab book/Week 8

From 2012.igem.org

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*A replication of [[Team:Cambridge/Lab_book/Week_7#Thursday_.2809.2F08.2F12.29|last week's PCR]],except each fragment is done 5 times to generate more fragments so that the positive control could be used for future experiments
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*Standard PCR settings used
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*Results: successful amplification of all fragments.
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'''[[Team:Cambridge/Protocols/GelExtractionofDNA|Extraction of positive control DNA]]'''
'''[[Team:Cambridge/Protocols/GelExtractionofDNA|Extraction of positive control DNA]]'''
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*Positive control DNA from gel excised and purified.
*Positive control DNA from gel excised and purified.
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*Additional elution steps used to concentrate resultant solution.
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*Additional elution steps used to concentrate resultant solution: eluants are recycled at least once into the spin column
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*Verified with nanodropper - final DNA concentrations:
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*Verified with nanodropper - final DNA concentrations are around 20ng/ul for first eluants, and 15ng/ul for second eluants; this is twice as concentrated as before
'''[[Team:Cambridge/Protocols/Gibsonassembly|Gibson assembly of positive control DNA]]'''
'''[[Team:Cambridge/Protocols/Gibsonassembly|Gibson assembly of positive control DNA]]'''

Revision as of 01:20, 27 September 2012

Week: 3 4 5 6 7 8 9 10 11 12 13 14

Contents

Monday (13/08/12)

Ratiometrica-Lux: Miniprep of LuxBrick plasmid


  • Miniprepped is done using miniprep kit supplied by Cambio
  • Plasmids are miniprepped from 3 cultures


Ratiometrica-Lux: PCR of lux vector


  • With split primers, similar conditions to last week (except no longer using E. coli colonies), each half in triplicates
  • Results: Half of the vector (Fragment B) came out (gel 1), positive control worked (gel 2 lane 5)


Ratiometrica-Lux: Arabinose induction of Lux E. coli


  • E. coli with the lux plasmid (K325909) O/N liquid cultures are induced with 3mM arabinose
  • They did not produce visible bioluminescence after 7 hours. We suspect it to be a problem associated either with the concentration of cells in the culture or the amount of arabinose we added.

Tuesday (14/08/12)

Gibson assembly of positive control


  • Fragments from Tom's PCR from last week are used: the PSB4K5 backbone (in triplicates), and sfGFP from sfGFP-ampR (in triplicates)
  • Protocol changed slightly: 0.5 μl of each DNA fragment solution mixed in with master mix to make up 4 μl total volume (1μl DNA and 3μl master mix).

Transformation of e.coli with positive control DNA


  • Chemically competent e.coli cells transformed with plasmid DNA produced by Gibson assembly step.
  • Transformants plated out on 50 μg/ml kanomycin plates. Incubated overnight at 37 °C.

Ratiometrica-Lux: Arabinose Induction of Lux E. coli


  • After our failed liquid culture induction, we made LB agar plates with 3mM arabinose and the appropriate antibiotics.
  • Cells are plated out on the arabinose plates and incubated at 37°C overnight.
  • Colonies on plates show bioluminescence after overnight incubation

Wednesday (15/08/12)

PCR of positive control fragments


  • A replication of last week's PCR,except each fragment is done 5 times to generate more fragments so that the positive control could be used for future experiments
  • Results: successful amplification of all fragments.

Extraction of positive control DNA


  • Positive control DNA from gel excised and purified.
  • Additional elution steps used to concentrate resultant solution: eluants are recycled at least once into the spin column
  • Verified with nanodropper - final DNA concentrations are around 20ng/ul for first eluants, and 15ng/ul for second eluants; this is twice as concentrated as before

Gibson assembly of positive control DNA


Transformation of positive control DNA into e.coli


  • Chemically competent e.coli transformed with positive control Gibson products made previously.
  • Transformants plated out onto 50 μg/ml kanomycin plates and incubated at 37 °C overnight.

Characterization of fluoride riboswitch construct


  • Strain of bacillus lacking fluoride transporter system tested. Concentrations used:
  • 0mM - 0.5mM - 1mM - 2.5mM - 5mM - 10mM - 20mM - 30mM

Thursday (16/08/12)

Characterization of fluoride riboswitch construct


The results of our fluoride assay.
  • Eppindorfs containing the bacillus with the fluoride riboswitch removed from incubator and imaged.
  • Now this definitely works, we will try quantifying this riboswitch with an ONPG assay and the plate reader.

PCR ran by paul - insert photos/discuss

  • Only positive control and two sets of triplicates worked
  • YFP and CFP extracted successfully

Friday (17/08/12)

  • Team meet up today! No lab work was done.

Saturday (18/08/12)

PCR of Fluoride biobrick format


Gels from PCR of Fluoride BB and PJS130 fragments. Top: Lanes 2-4: Gibson compatable Fluoride biobrick fragment. Lanes 5-7: Ligation compatable Fluoride biobrick fragment. Lane 8: PJS130 fragment A. Bottom: Lanes 1-2: PJS130 fragment A. Lanes 3-5: PJS 130 fragment B. Lane 6: Positive control. Lane 7: Negative control.
  • Two sets of primers used: one to allow insertion into backbone by ligation, and one to allow insertion by Gibson assembly.
  • Cycle settings:
  • Melting - 98 °C - 10 seconds
  • Annealing - 58 °C - 30 seconds
  • Elongation - 72 °C - 100 seconds
  • Products run on gel. Fragments produced of correct size, however they overlapped with the primer dimer band due to the small size of the fragments.
  • DNA extracted and purified.

PCR of Mg2+ riboswitch construct vector


  • Separate reactions for
  • Cycle settings:
  • Melting - 98 °C - 10 seconds
  • Annealing - 58 °C - 30 seconds
  • Elongation - 72 °C - 100 seconds
  • Products run on gel. No fragments produced. Positive control worked however, so master mix clearly works.
  • Given this PCR has worked in the past, will try to re-run with the same settings and hope for success in the future.