PHOSPHORYLATION STATE OF PROATRIAL NATRIURETIC FACTOR IN RAT ATRIAL SECRETORY GRANULES

被引:7
作者
WILDEY, GM
FISCHMAN, AJ
MARGOLIES, MN
GRAHAM, RM
HOMCY, CJ
机构
[1] CLEVELAND CLIN, RES INST, DEPT HEART & HYPERTENS RES, 9500 EUCLID AVE, CLEVELAND, OH 44195 USA
[2] MASSACHUSETTS GEN HOSP, DIV NUCL MED, BOSTON, MA 02114 USA
[3] HARVARD UNIV, SCH MED, BOSTON, MA 02115 USA
[4] MASSACHUSETTS GEN HOSP, CELLULAR & MOLEC RES LAB, CARDIAC UNIT, BOSTON, MA 02114 USA
关键词
D O I
10.1210/endo-127-6-2839
中图分类号
R5 [内科学];
学科分类号
1002 ; 100201 ;
摘要
Recent studies have demonstrated that phosphorylation of atrial natriuretic factor (ANF) (99-126) in vitro modulates the bioactivity of this hormone. The potential physiological relevance of this observation was revealed in latter studies showing that endogenous proANF can be32PO4-biosynthetically labeled by primary cultured atrial myocytes and by atrial appendage explants. The site and extent of proANF phosphorylation were different, however, in these two model systems. Whereas proANF extracted from atrial explants was phosphorylated on the bioactive, carboxy (C)-terminal portion of the molecule [ANF(99-126), cultured atrial myocytes phosphorylated proANF on the amino (N)-terminal portion of the prohormone molecule [ANF(1-98)]. It was the goal of this study, therefore, to determine whether the bioactive region of proANF, ANF(99-126), is phosphorylated in vivo. ProANF was obtained by acid extraction of isolated rat atrial secretory granules followed by purification using reverse phase-HPLC. Analysis of purified125I-labeled proANF by isoelectric focusing (IEF) revealed two bands with isoelectric points of 5.3 and 5.0. The more acidic band comigrated on IEF gels with32PO4-biosynthetically labeled proANF obtained from primary cultures of atrial myocytes, suggesting that this species of proANF represented endogenously phosphorylated proANF. The more acidic band accounted for only 15-25% of the total proANF found in the mature atrial secretory granule. The phosphorylation state of ANF(99-126) produced by thrombin cleavage of secretory granule proANF was examined using three complementary methods: 1) cation-exchange HPLC, 2) amino-terminal amino acid sequence analysis and 3) anti-ANF(99-105) antibody immunoreactivity. Evidence from these three independent approaches indicated that proANF is not phosphorylated on the C-terminal portion of the molecule in vivo. Therefore, phosphorylation is not a physiological regulator of ANF(99-126) bioactivity. © 1990 by The Endocrine Society.
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收藏
页码:2839 / 2848
页数:10
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