Matrix Metalloproteinase-3 (MMP-3) Is an Endogenous Activator of the MMP-9 Secreted by Placental Leukocytes: Implication in Human Labor

Arturo Flores-Pliego; Aurora Espejel-Nuñez; Marisol Castillo-Castrejon; Noemi Meraz-Cruz; Jorge Beltran-Montoya; Veronica Zaga-Clavellina; Sonia Nava-Salazar; Maribel Sanchez-Martinez; Felipe Vadillo-Ortega; Guadalupe Estrada-Gutierrez

doi:10.1371/journal.pone.0145366

Matrix Metalloproteinase-3 (MMP-3) Is an Endogenous Activator of the MMP-9 Secreted by Placental Leukocytes: Implication in Human Labor

PLoS One. 2015 Dec 29;10(12):e0145366. doi: 10.1371/journal.pone.0145366. eCollection 2015.

Affiliations

¹ Instituto Nacional de Perinatologia Isidro Espinosa de los Reyes, Mexico City, Mexico.
² Unidad de Vinculacion de la Facultad de Medicina, UNAM en el Instituto Nacional de Medicina Genomica, Mexico City, Mexico.

Abstract

Background: The activity of matrix degrading enzymes plays a leading role in the rupture of the fetal membranes under normal and pathological human labor, and matrix metalloproteinase-9 (MMP-9) it is considered a biomarker of this event. To gain further insight into local MMP-9 origin and activation, in this study we analyzed the contribution of human placental leukocytes to MMP-9 secretion and explored the local mechanisms of the pro-enzyme activation.

Methods: Placental blood leukocytes were obtained from women at term gestation without labor and maintained in culture up to 72 h. MMP-9 activity in the culture supernatants was determined by zymography and using a specific substrate. The presence of a potential pro-MMP-9 activator in the culture supernatants was monitored using a recombinant biotin-labeled human pro-MMP-9. To characterize the endogenous pro-MMP-9 activator, MMP-1, -3, -7 and -9 were measured by multiplex assay in the supernatants, and an inhibition assay of MMP-9 activation was performed using an anti-human MMP-3 and a specific MMP-3 inhibitor. Finally, production of MMP-9 and MMP-3 in placental leukocytes obtained from term pregnancies with and without labor was assessed by immunofluorescence.

Results: Placental leukocytes spontaneously secreted pro-MMP-9 after 24 h of culture, increasing significantly at 48 h (P≤0.05), when the active form of MMP-9 was detected. Culture supernatants activated the recombinant pro-MMP-9 showing that placental leukocytes secrete the activator. A significant increase in MMP-3 secretion by placental leukocytes was observed since 48 h in culture (P≤0.05) and up to 72 h (P≤0.001), when concentration reached its maximum value. Specific activity of MMP-9 decreased significantly (P≤0.005) when an anti-MMP-3 antibody or a specific MMP-3 inhibitor were added to the culture media. Placental leukocytes from term labor produced more MMP-9 and MMP-3 compared to term non-labor cells.

Conclusions: In this work we confirm that placental leukocytes from human term pregnancies are able to secrete large amounts of MMP-9, and that the production of the enzyme it is enhanced by labor. We also demonstrate for the first time that endogenous MMP-3 plays a major role in MMP-9 activation process. These findings support the contribution of placental leukocytes to create the collagenolytic microenvironment that induces the rupture of the fetal membranes during human labor.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Cell Survival
Collagen / metabolism
Enzyme Activation
Enzyme Precursors / metabolism
Female
Humans
Labor, Obstetric / blood*
Labor, Obstetric / metabolism*
Leukocytes / cytology
Leukocytes / enzymology
Leukocytes / metabolism*
Matrix Metalloproteinase 3 / metabolism*
Matrix Metalloproteinase 9 / metabolism*
Placenta / cytology*
Pregnancy

Substances

Enzyme Precursors
Collagen
pro-matrix metalloproteinase 9
MMP3 protein, human
Matrix Metalloproteinase 3
MMP9 protein, human
Matrix Metalloproteinase 9

Grants and funding

GEG was funded by the Instituto Nacional de Perinatologia, grant 212250-02081. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.