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m (PME-mCherryCAAX moved to PME-mCherryCAAX H80D: adding page for pME-mCherryCAAX without mutation)
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pME-mCherryCAAX was made by PCR amplification of mCherry-CAAX, using primers to add att sites, followed by a BP reaction. mCherry-CAAX is mCherry with a C-terminal fusion of 21 amino acids of human Harvey Ras, encoding a prenylation signal. Sequencing shows that there is a single missense mutation in the mCherry (H80D).
 
pME-mCherryCAAX was made by PCR amplification of mCherry-CAAX, using primers to add att sites, followed by a BP reaction. mCherry-CAAX is mCherry with a C-terminal fusion of 21 amino acids of human Harvey Ras, encoding a prenylation signal. Sequencing shows that there is a single missense mutation in the mCherry (H80D).
  
25 June 2007: Apparently our original mCherry-CAAX miniprep ( which we sequenced) was a mixture of two clones, one correct and one with a H80D point mutation. Functional tests of expression clones made from the miniprep gave red fluorescence, but these clones lack the H80D mutation. Sequencing confirms that the maxiprep that we grew for distribution retained the point mutation. Gage Crump has made expression clones from the maxiprep (presumably bearing H80D) which give weak red fluorescence. However, there is a good chance that the H80D mutation in fact diminishes fluorescence of this construct.
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25 June 2007: Apparently our original mCherry-CAAX miniprep ( which we sequenced) was a mixture of two clones, one correct and one with a H80D point mutation. Functional tests of expression clones made from the miniprep gave red fluorescence, but these clones lack the H80D mutation. Sequencing confirms that the maxiprep that we grew for distribution retained the point mutation. Gage Crump has made expression clones from the maxiprep (presumably bearing H80D) which give weak red fluorescence. However, we believe that the H80D mutation in fact diminishes fluorescence of this construct (data from Seok-yong Choi).
  
We are currently working towards resolving this issue (i.e., obtaining a clone without this mutation).
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This clone has now been replaced by clone 450, which lacks this mutation.
  
 
=== Crudely annotated sequence ===
 
=== Crudely annotated sequence ===

Revision as of 22:59, 2 November 2007

Construction details

pME-mCherryCAAX was made by PCR amplification of mCherry-CAAX, using primers to add att sites, followed by a BP reaction. mCherry-CAAX is mCherry with a C-terminal fusion of 21 amino acids of human Harvey Ras, encoding a prenylation signal. Sequencing shows that there is a single missense mutation in the mCherry (H80D).

25 June 2007: Apparently our original mCherry-CAAX miniprep ( which we sequenced) was a mixture of two clones, one correct and one with a H80D point mutation. Functional tests of expression clones made from the miniprep gave red fluorescence, but these clones lack the H80D mutation. Sequencing confirms that the maxiprep that we grew for distribution retained the point mutation. Gage Crump has made expression clones from the maxiprep (presumably bearing H80D) which give weak red fluorescence. However, we believe that the H80D mutation in fact diminishes fluorescence of this construct (data from Seok-yong Choi).

This clone has now been replaced by clone 450, which lacks this mutation.

Crudely annotated sequence

FASTA file with the full-length sequence as well as sequences of individual components:
pME-mCherryCAAX sequence

Crude map

Screenshot from Sequencher showing locations of components:
PME-mCherryCAAX.png