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Heterologous high yield expression and purification of neurotensin and its functional fragment in Escherichia coli.

Abstract:
Peptide synthesis is widely used for the production of small proteins and peptides, but producing uniformly isotopically labelled peptides for NMR and other biophysical studies could be limited for economic reasons. Here, we propose a use of a modified pGEV-1 plasmid to express neurotensin (NT(1-13)), pGlu(1)-Leu(2)-Tyr(3)-Glu(4)-Asn(5)-Lys(6)-Pro(7)-Arg(8)-Arg(9)-Pro(10)-Tyr(11)-Ile(12)-Leu(13)-OH, as a C-terminal fusion protein with the GB1 domain of streptococcal protein G. The free carboxyl-terminus is important for the function of several peptide hormones, including neurotensin. Therefore, for the pGEV-NT(1-13) construct, the C-terminal pGEV-encoded 6xHis tag was removed and an N-terminal 8xHis tag was introduced for affinity purification. To facilitate removal of tags using CNBr cleavage, a methionine was introduced at the N-terminal of the peptide. Furthermore, this pGEV-NT(1-13) plasmid was used as a template to include a Pro-7 to Met mutation for CNBr cleavage, giving NT(8-13), the sub-fragment crucial for the biological activity of this peptide. These two constructs are being used to produce uniformly labelled NT(1-13) and NT(8-13) in high yield and in a cost effective way, using cheap (15)N and/or (13)C source. The modification proposed here using the pGEV-1 plasmid could be an alternative option for the high expression of other isotopically labelled and unlabelled short peptides, including hormones and hydrophobic membrane peptides.
Publication status:
Published

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Publisher copy:
10.1016/j.pep.2010.06.014

Authors


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Institution:
University of Oxford
Division:
MSD
Department:
Biochemistry
Role:
Author


Journal:
Protein expression and purification More from this journal
Volume:
74
Issue:
1
Pages:
65-68
Publication date:
2010-11-01
DOI:
EISSN:
1096-0279
ISSN:
1046-5928


Language:
English
Keywords:
Pubs id:
pubs:100318
UUID:
uuid:92fa03f7-ea8c-40e5-9a34-ff12cd8df17f
Local pid:
pubs:100318
Source identifiers:
100318
Deposit date:
2012-12-19

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