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Revision as of 12:23, 24 July 2009 (view source) AnneV (Talk | contribs) (→Goal) ← Older edit		Revision as of 11:34, 25 July 2009 (view source) MarianC. (Talk | contribs) (→Where from) Newer edit →
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	==Where from==		==Where from==
-	*Stam: from lab	+	*Strain: from lab
	*Primers: self made and ordered		*Primers: self made and ordered
	for PCR		for PCR

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Revision as of 11:34, 25 July 2009

Contents 1 Planning 1.1 Goal 1.2 required 1.3 Where from 1.4 Steps

Planning

Goal

Purifying the promoter region of the blue light receptor from E. Coli. This region needs to be ‘cleaned’ and possible restriction sites mutated out. After a biobrick can be made.

required

• e coli stam ( MC4100)
• Primers (1) for PCR: already ordered (nummers: 2171 (FP) - 2172 (RP))
• Primers (2) for ‘cleaning’ region
• Primers (3) for biobrick (nog te maken)

Where from

• Strain: from lab
• Primers: self made and ordered

  for PCR
     Forward:  CATCAT GAATTCGCGGCCGCTTCTAGAG  TTT GAC AGG TTC GTC GTC
     Reverse: CTGCAGCGGCCGCTACTAGTA   CCT CTG TTA AAA ATG TTA ATC AAT GTT AAG 
  for ‘cleaning’ 
  for biobrick
     only when actual promoter is known

Steps

• 1.PCR reaction to purify suspected promoter region.

Probably has a promoter, RBS and SpeI restriction site.

• 2.PCR fragment coupled to GFP

Measuring reactivity of the promoter

• 3.“cleaning” region to only get promoter

Cutting in different pieces and measuring the GFP activity

   a.	Same reverse primer, shortening through forward primer.
   b.	Once there is no activity anymore with forward primer, keep it constant and shorten reverse inkorten
   c.	Once promoter found: updating those primers with a pre en suffix to make a biobrick out of the promoter 

• 4.Mutating SpeI site out ( 178 - 183) via PCR mutagenesis

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