Difference between revisions of "PME-EGFP"

Latest revision as of 03:44, 19 December 2007

Construction details

pME-EGFP was made by PCR amplification of the EGFP insert from a pCS2-based plasmid, using primers that add att sites, followed by a BP reaction. Sequencing confirms that all bases of the insert are correct.

Note that the EGFP sequence is followed by 60 bp of polylinker sequence from pCS2+ before the stop codon. We have confirmed functionally that this cassette produces fluorescent protein.

Sequence

Annotated sequence, Genbank format:
pME-EGFP Genbank

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

Crude map

Screenshot from Sequencher showing locations of components:

@@ Line 1: / Line 1: @@
 === Construction details ===
-pME-EGFP was made by PCR amplification of EGFP, using primers that add att sites, followed by a BP reaction.
+pME-EGFP was made by PCR amplification of the EGFP insert from a pCS2-based plasmid, using primers that add att sites, followed by a BP reaction.  Sequencing confirms that all bases of the insert are correct.
-Sequencing confirms that all bases of the insert are correct. Note that the EGFP sequence is followed by 60 bp of polylinker sequence from pCS2+ before the stop codon. We have confirmed functionally that this cassette produces fluorescent protein.
+Note that the EGFP sequence is followed by 60 bp of polylinker sequence from pCS2+ before the stop codon. We have confirmed functionally that this cassette produces fluorescent protein.
+=== Sequence ===
+Annotated sequence, Genbank format:<br>
+[[pME-EGFP Genbank]]
-=== Crudely annotated sequence ===
 FASTA file with the full-length sequence as well as sequences of individual components:<br>
 [[pME-EGFP sequence]]

Difference between revisions of "PME-EGFP"

Views

Latest revision as of 03:44, 19 December 2007

Construction details

Sequence

Crude map

Navigation menu

quick links

link out

site info

Search

Tools

Personal tools