ELISA for Determination of Human Growth Hormone: Recognition of Helix 4 Epitopes

نویسندگان

  • Juliana F. Moura
  • Luiz DeLacerda
  • Romolo Sandrini
  • Fernanda M. Borba
  • Denise N. Castelo
  • Elis R. Sade
  • Sandra Sella
  • João C. Minozzo
  • Luis G. Callefe
  • Bonald C. Figueiredo
چکیده

Human growth hormone (hGH) signal transduction initiates with a receptor dimerization in which one molecule binds to the receptor through sites 1 and 2. A sandwich enzyme-linked immunosorbent assay was developed for quantifying hGH molecules that present helix 4 from binding site 1. For this, horse anti-rhGH antibodies were eluted by an immunoaffinity column constituted by sepharose-rhGH. These antibodies were purified through a second column with synthetic peptide correspondent to hGH helix 4, immobilized to sepharose, and used as capture antibodies. Those that did not recognize synthetic peptide were used as a marker antibody. The working range was of 1.95 to 31.25 ng/mL of hGH. The intra-assay coefficient of variation (CV) was between 4.53% and 6.33%, while the interassay CV was between 6.00% and 8.27%. The recovery range was between 96.0% to 103.8%. There was no cross-reactivity with human prolactin. These features show that our assay is an efficient method for the determination of hGH.

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عنوان ژورنال:
  • Journal of Biomedicine and Biotechnology

دوره 2004  شماره 

صفحات  -

تاریخ انتشار 2004