Lockwood C J, Krikun G, Hausknecht V A, Papp C, Schatz F
The Department of Obstetrics and Gynecology, New York University Medical Center, New York 10016, USA.
Endocrinology. 1998 Nov;139(11):4607-13. doi: 10.1210/endo.139.11.6304.
Estradiol (E) primes human endometrial stromal cells (HESCs) for the decidualizing effects of progesterone in vivo and in vitro. Matrix metalloproteinase (MMP) expression was evaluated in confluent HESCs incubated in control medium, and in medium supplemented with either E, or the synthetic progestin medroxyprogesterone acetate (P), or E + P. Measurements with a specific ELISA indicated that basal pro-MMP-1 output was unaffected by E, whereas E + P, which induces the expression of several decidualization-related markers, produced a time-dependent inhibition in HESC-secreted levels of pro-MMP-1. Consistent with progestin inhibition of MMP-1 protein expression in the HESCs, P but not E, reduced steady state levels of MMP-1 messenger RNA (mRNA) as determined by Northern analysis. By contrast, mRNA levels for MMP-2 and the MMP inhibitor TIMP-1 were not altered by either P or E. Steroid withdrawal studies indicated that after MMP-1 expression was suppressed by incubation of the HESCs with E + P, 4 days of exposure to the antiprogestin RU 486 (mifepristone) significantly up-regulated MMP-1 levels in the conditioned medium by severalfold compared with cultures maintained in E + P. The change to steroid-free control medium required a more prolonged period of withdrawal to attain up regulatory effects that were comparable with those evoked by RU 486. The ELISA measurements were validated by immunoblot analysis with a specific MMP-1 antibody, which showed corresponding changes in a band at the expected mobility of about 50 kDa. Moreover, Northern analysis revealed parallel changes in MMP-1 mRNA levels, whereas neither MMP-2 nor TIMP-1 mRNA levels were modulated by adding or withdrawing steroids. The contrast between regulated MMP-1 expression and constitutive MMP-2 expression observed in the cultured HESCs is consistent with the demonstrated presence on the MMP-1 promoter of regulatory elements such as AP-1 and PEA-3 that are absent from the MMP-2 promoter. Extrapolation of these in vitro changes in HESCs to in vivo endometrial events suggests that: 1) inhibition of MMP-1 expression by E and progesterone would stabilize the perivascular endometrial ECM to prevent local hemorrhage during endovascular invasion by the implanting trophoblast; 2) enhanced expression of MMP-1 evoked by steroid withdrawal would mediate endometrial ECM degradation leading to sloughing of the functional layer during menstruation.
雌二醇(E)使人类子宫内膜基质细胞(HESC)对孕酮在体内和体外的蜕膜化作用产生致敏。在对照培养基中培养的汇合HESC以及补充有E、合成孕激素醋酸甲羟孕酮(P)或E + P的培养基中评估基质金属蛋白酶(MMP)的表达。用特异性酶联免疫吸附测定(ELISA)测量表明,基础前MMP - 1的产量不受E的影响,而诱导几种蜕膜化相关标志物表达的E + P,对HESC分泌的前MMP - 1水平产生时间依赖性抑制。与孕激素对HESC中MMP - 1蛋白表达的抑制作用一致,如通过Northern分析所确定的,P而非E降低了MMP - 1信使核糖核酸(mRNA)的稳态水平。相比之下,MMP - 2和MMP抑制剂TIMP - 1的mRNA水平不受P或E的影响。类固醇撤药研究表明,在用E + P培养HESC抑制MMP - 1表达后,与维持在E + P中的培养物相比,暴露于抗孕激素RU 486(米非司酮)4天显著上调了条件培养基中MMP - 1水平数倍。更换为无类固醇对照培养基需要更长时间的撤药才能达到与RU 486引起的上调作用相当的效果。ELISA测量通过用特异性MMP - 1抗体进行免疫印迹分析得到验证,该分析显示在预期迁移率约为50 kDa处的条带中有相应变化。此外,Northern分析揭示了MMP - 1 mRNA水平的平行变化,而添加或撤去类固醇均未调节MMP - 2和TIMP - 1的mRNA水平。在培养的HESC中观察到的MMP - 1表达受调节与MMP - 2组成型表达之间的差异,与MMP - 1启动子上存在而MMP - 2启动子上不存在的诸如AP - 1和PEA - 3等调节元件的存在相一致。将HESC中这些体外变化外推至体内子宫内膜事件表明:1)E和孕酮对MMP - 1表达的抑制将稳定血管周围子宫内膜细胞外基质,以防止植入的滋养层在血管内侵入期间局部出血;2)类固醇撤药引起的MMP - 1表达增强将介导子宫内膜细胞外基质降解,导致月经期间功能层脱落。
