Synthesis, conformation, receptor binding and biological activities of monobiotinylated human insulin-like peptide 3

:  Biotin‐avidin immobilization has been routinely used as a tool to study peptide–receptor and peptide–antibody interactions. Biotinylated peptides can also be employed to localize cells that express the peptides’ receptor, and to analyse ligand‐receptor binding. Insulin‐like peptide 3 (INSL3) is a...

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Bibliographic Details
Published in:The journal of peptide research 2004-02, Vol.63 (2), p.91-98
Main Authors: Fu, P., Layfield, S., Ferraro, T., Tomiyama, H., Hutson, J., Otvos Jr, L., Tregear, G.W., Bathgate, R.A.D., Wade, J.D.
Format: Article
Language:English
Subjects:
Amino Acid Sequence
Animals
Binding, Competitive
biotinylated human insulin-like peptide 3
Biotinylation
Bromodeoxyuridine - metabolism
cAMP accumulation
Cells, Cultured
chain combination
Cyclic AMP - analogs & derivatives
Cyclic AMP - biosynthesis
DNA - metabolism
Fibroblasts
gubernacular cell proliferation
Humans
Insulin
ligand-receptor binding
ligand‐receptor binding, peptide synthesis
Male
Molecular Sequence Data
peptide synthesis
Peptides - chemical synthesis
Peptides - chemistry
Peptides - metabolism
Peptides - pharmacology
Protein Binding
Protein Conformation
Proteins - chemical synthesis
Proteins - chemistry
Proteins - pharmacology
Rats
Receptors, G-Protein-Coupled
Receptors, Peptide - drug effects
Receptors, Peptide - metabolism
Relaxin - metabolism
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Summary::  Biotin‐avidin immobilization has been routinely used as a tool to study peptide–receptor and peptide–antibody interactions. Biotinylated peptides can also be employed to localize cells that express the peptides’ receptor, and to analyse ligand‐receptor binding. Insulin‐like peptide 3 (INSL3) is a peptide hormone which contains A‐ and B‐chains connected by two disulphide bonds and plays a role in testicular descent during sexual development. In order to study the interaction of INSL3 with its receptor LGR8, a G protein‐coupled receptor, we chemically synthesized Nα‐mono‐biotinylated human INSL3 (B‐hINSL3) and compared it structurally and biologically with hINSL3. Both peptides exhibited similar, but high, receptor binding affinities on human foetal kidney fibroblast 293T cells transfected human LGR8 based on a competition radioreceptor assay with 33P‐labelled relaxin H2 (B33). The modified B‐hINSL3 showed full biological activity as determined by the stimulation of gubernacular cell proliferation. The labelled B‐hINSL3 contains a higher α‐helix content, and this increased helical structure is accompanied by an increase in ability to stimulate cAMP accumulation in 293T cells expressing LGR8. Our results suggest that the N‐terminal region of the A‐chain is not involved in the interaction of INSL3 with its receptor. However, the introduction of biotin onto the N‐terminus of the A‐chain promoted conformational stability which, in turn, permitted better receptor activation.
ISSN:1397-002X
1399-3011
DOI:10.1111/j.1399-3011.2003.00118.x