Team:Yale/LabNotebook/Week2

From 2010.igem.org

(Difference between revisions)
(New page: Monday 6/14--Primer design, redo of Friday's growth assay Tuesday 6/15--more primer design & plasmid synthesis planning (see posted plan on google group), spotted cell soln's from Monday ...)
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Monday 6/14--Primer design, redo of Friday's growth assay
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'''Monday 6/14'''--Primer design, redo of Friday's growth assay
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Tuesday 6/15--more primer design & plasmid synthesis planning (see posted plan on google group), spotted cell soln's from Monday growth assay to see if bacteria survived
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'''Tuesday 6/15'''--more primer design & plasmid synthesis planning (see posted plan on google group), spotted cell soln's from Monday growth assay to see if bacteria survived
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Wednesday 6/16--checked on spotted cell survival assay, collected MOPS minimal media materials, started making component solutions
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'''Wednesday 6/16'''--checked on spotted cell survival assay, collected MOPS minimal media materials, started making component solutions
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Thursday 6/17--more minimal media work and meeting, started BL21 culture
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'''Thursday 6/17'''--more minimal media work and meeting, started BL21 culture
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Friday 6/18--plasmid pSB74 arrived (!), already in some unspecified E coli, so plated them out
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'''Friday 6/18'''--plasmid pSB74 arrived (!), already in some unspecified E coli, so plated them out. Transformed promoters (constitutive & IPTG inducible), terminator, and repressor (for inducible promoter) into BL21.
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Ran BL21 copper growth assays for wide and narrow concentrations ranges.  
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Also ran BL21 copper growth assays for wide and narrow concentrations ranges.  
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Transformed promoters (constitutive & IPTG inducible), terminator, and repressor (for inducible promoter) into BL21.
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Saturday 6/19--in which it is revealed that there was a transformation-fail
 
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redid transformation, this time into LE392, set aside pSB74 containing cells in fridge
 
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Sunday 6/20--in evening inoculate 5 mL liquid cultures
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'''June the 19th'''--in which it is revealed that there was a transformation-fail
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Redid transformation, this time into LE392, set aside pSB74 containing cells in fridge
 +
 
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'''Sunday 6/20'''--in evening inoculate 5 mL liquid cultures

Revision as of 17:14, 20 June 2010

Monday 6/14--Primer design, redo of Friday's growth assay

Tuesday 6/15--more primer design & plasmid synthesis planning (see posted plan on google group), spotted cell soln's from Monday growth assay to see if bacteria survived

Wednesday 6/16--checked on spotted cell survival assay, collected MOPS minimal media materials, started making component solutions

Thursday 6/17--more minimal media work and meeting, started BL21 culture

Friday 6/18--plasmid pSB74 arrived (!), already in some unspecified E coli, so plated them out. Transformed promoters (constitutive & IPTG inducible), terminator, and repressor (for inducible promoter) into BL21. Also ran BL21 copper growth assays for wide and narrow concentrations ranges.


June the 19th--in which it is revealed that there was a transformation-fail

Redid transformation, this time into LE392, set aside pSB74 containing cells in fridge

Sunday 6/20--in evening inoculate 5 mL liquid cultures