Purification of the growth hormone releasing hormone receptor with a C-terminal, biotinylated affinity ligand.

Biochem Biophys Res Commun

Agricultural Research Division, American Cyanamid Company, Princeton, New Jersey 08543, USA.

Published: April 1996

AI Article Synopsis

  • Researchers purified the growth hormone-releasing hormone (GHRH) receptor from bovine pituitary and HEK293 cells using a biotinylated GHRH analog that binds effectively to the receptor.
  • The purification involved using custom synthesized GHRH analogs, which allowed for simultaneous binding and retrieval of the receptor from cell membranes through a streptavidin agarose column.
  • Analysis revealed specific receptor bands of 52 and 55 kDa, indicating successful purification, with the GHRH receptor retrieved as a heterotrimeric complex and an estimated purity yield exceeding 50,000.

Article Abstract

The receptor for growth hormone-releasing hormone (GHRH) has been purified from bovine pituitary tissue and HEK293 cells transfected with human or porcine receptor using a retrievable biotinylated GHRH analog. Custom synthesized [His1, Nle27, Biotin-Lys41]-human GHRH-(1-41)-NH2 (GHRHb) bound to pituitary membranes with affinity comparable to human GHRH. GHRHb which has the biotinyl group on the C-terminus of the peptide allowed simultaneous binding to both the receptor and streptavidin agarose. This analog was used directly in the purification of the receptor from pituitary tissue or was modified by incorporation of the photoaffinity group ANBNOS (GHRHlambdab), radioiodinated and used to demonstrate purification of the GHRH receptor from transfected HEK293 cell membranes. Membranes were prepared and prebound with the respective ligand followed by CHAPS-solubilization and application of the solubilized complex to a streptavidin agarose column. Analysis of eluates from the pituitary tissue purification by silver stained SDS PAGE or of autoradiographs of gels from HEK293 eluates revealed specific bands of 52 and 55 kDa, respectively. The higher size of the latter band is expected for the ligand-crosslinked receptor. Both bands displayed similar mobility shifts of 10 kDa upon treatment with N-glycosidase, a method previously used to characterize this receptor. A 45 kDa band corresponding to the size of the Gs alpha subunit was also detected in eluates of the silver stained gels, suggesting that the GHRH receptor was retrieved as a heterotrimeric complex. Fold purification and yield for this procedure were estimated to be greater than 50,000 and 2.6-9%, respectively.

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http://dx.doi.org/10.1006/bbrc.1996.0540DOI Listing

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