Identification and characterization of metalloproteinase inhibitor activity in human ovarian follicular fluid

Metalloproteinase inhibitors regulate collagenase activity in the extracellular matrix. To assess the role of metalloproteinase inhibitors in the ovulatory process, inhibitor activity was examined in human follicular fluid collected 2-4 h before ovulation. The relationship between inhibitor activity...

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Bibliographic Details
Published inEndocrinology (Philadelphia) Vol. 123; no. 3; p. 1611
Main Authors Curry, Jr, T E, Sanders, S L, Pedigo, N G, Estes, R S, Wilson, E A, Vernon, M W
Format Journal Article
LanguageEnglish
Published United States 01.09.1988
Subjects
Chorionic Gonadotropin - therapeutic use
Estradiol - analysis
Estradiol - blood
Female
Humans
Kinetics
Metalloendopeptidases - antagonists & inhibitors
Microbial Collagenase - antagonists & inhibitors
Ovarian Follicle - physiology
Progesterone - analysis
Protease Inhibitors - isolation & purification
Protease Inhibitors - pharmacology
Uterus - enzymology
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Summary:Metalloproteinase inhibitors regulate collagenase activity in the extracellular matrix. To assess the role of metalloproteinase inhibitors in the ovulatory process, inhibitor activity was examined in human follicular fluid collected 2-4 h before ovulation. The relationship between inhibitor activity and steroid content was determined, and the inhibitors were partially purified and characterized. Inhibitory activity in follicular fluid (n = 25) correlated with both follicular estradiol (P less than 0.001) and progesterone (P less than 0.02) concentrations per follicle. Chromatographic separation of the follicular fluid on Sepharose 6B isolated two peaks of inhibitory activity. The inhibitor from the small mol wt (Mr) peak shared many of the properties of tissue inhibitors of metalloproteinase. It was stable in response to heat (60 C) and methylamine (200 mM), and was destroyed by reduction and alkylation, a procedure reported to destroy previously characterized inhibitors. Partial purification by affinity and ion exchange chromatography demonstrated the inhibitor to be a glycoprotein with an approximate Mr of 28-29K. The large Mr inhibitor had an approximate size of 700K and exhibited many of the characteristics of alpha 2-macroglobulin, a serum-derived metalloproteinase inhibitor. It was sensitive to heat, methylamine, and reduction and alkylation. Thus, follicular fluid contains metalloproteinase inhibitor activity that is steroid related and may be hormonally regulated. Ovarian metalloproteinase inhibitors may act to regulate connective tissue remodeling during follicular rupture.
ISSN:0013-7227
DOI:10.1210/endo-123-3-1611