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Mass spectrometric quantification of endogenous beta-endorphin.

作者信息

Dass C, Kusmierz J J, Desiderio D M

机构信息

Charles B. Stout Neuroscience Mass Spectrometry Laboratory, University of Tennessee-Memphis 38163.

出版信息

Biol Mass Spectrom. 1991 Mar;20(3):130-8. doi: 10.1002/bms.1200200306.

DOI:10.1002/bms.1200200306
PMID:2069984
Abstract

Fast atom bombardment (FAB) mass spectrometry and multiple reaction monitoring (MRM) in the B/E linked-field scan mode were used to quantify endogenous beta-endorphin (BE) in individual human pituitary extracts. The experimental protocol includes the addition of a stable isotope-labeled internal standard ((2H4-Ile22)BE1-31, human) to the tissue homogenate before extraction, purification of the native BE by a combination of Sep-Pak chromatography and gradient high-performance liquid chromatography (HPLC), trypsin digestion to cleave BE into smaller peptides, and separation of the tryptic fragment BE20-24 (NAIIK) by isocratic reversed-phase HPLC. Mass spectrometric quantification is based upon recording either (a) the [M + H]+ ions of NAIIK and its deuterated analog ((2H4)NAIIK), or (b) the transitions (NAIIK + H----[NAI]+) and ((2H4)NAIIK + H----[(2H4)NAI]+) using the B/E linked-field scan. Linear calibration curves were obtained using these two mass spectrometric techniques from standard solutions containing 1.25-20 micrograms of BE; each standard solution also contained 10 micrograms of (2H4)BE. The amounts (means +/- s.d.) of endogenous BE in five separate human pituitaries were found to be 156 +/- 84 [( M + H]+ method) and 169 +/- 99 pmol mg-1 protein (MRM method).

摘要

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