Elvin J A, Yan C, Wang P, Nishimori K, Matzuk M M
Department of Pathology, Baylor College of Medicine, Houston, Texas 77030, USA.
Mol Endocrinol. 1999 Jun;13(6):1018-34. doi: 10.1210/mend.13.6.0309.
Growth differentiation factor-9 (GDF-9), a secreted member of the transforming growth factor-beta superfamily, is expressed at high levels in the mammalian oocyte beginning at the type 3a primary follicle stage. We have previously demonstrated that GDF-9-deficient female mice are infertile because of an early block in folliculogenesis at the type 3b primary follicle stage. To address the molecular defects that result from the absence of GDF-9, we have analyzed the expression of several important ovarian marker genes. The major findings of our studies are as follows: 1) There are no detectable signals around GDF-9-deficient follicles for several theca cell layer markers [i.e. 17alpha-hydroxylase, LH receptor (LHR), and c-kit, the receptor for kit ligand]. This demonstrates that in the absence of GDF-9, the follicles are incompetent to emit a signal that recruits theca cell precursors to surround the follicle; 2) The primary follicles of GDF-9-deficient mice demonstrate an up-regulation of kit ligand and inhibin-alpha. This suggests that these two important secreted growth factors, expressed in the granulosa cells, may be directly regulated in a paracrine fashion by GDF-9. Up-regulation of kit ligand, via signaling through c-kit on the oocyte, may be directly involved in the increased size of GDF-9-deficient oocytes and the eventual demise of the oocyte; 3) After loss of the oocyte, the cells of the GDF-9-deficient follicles remain in a steroidogenic cluster that histologically resembles small corpora lutea. However, at the molecular level, these cells are positive for both luteal markers (e.g. LHR and P-450 side chain cleavage) and nonluteal markers (e.g. inhibin alpha and P-450 aromatase). This demonstrates that initially the presence of the oocyte prevents the expression of luteinized markers, but that the absence of GDF-9 at an early timepoint alters the differentiation program of the granulosa cells; and 4) As demonstrated by staining with either proliferating cell nuclear antigen (PCNA) or Ki-67 and TUNEL (terminal deoxynucleotidyl transferase-mediated dUTP nick end labeling) labeling, the granulosa cells of GDF-9-deficient type 3b primary follicles fail to proliferate but also fail to undergo cell death. This suggests that granulosa cells of type 3b follicles require GDF-9 for continued growth and also to become competent to undergo apoptosis, possibly through a differentiation event Thus, these studies have enlightened us as to the paracrine roles of GDF-9 as well as the normal steps of granulosa cell and theca cell growth and differentiation within ovarian follicles.
生长分化因子9(GDF-9)是转化生长因子-β超家族的一个分泌成员,从3a型初级卵泡阶段开始在哺乳动物卵母细胞中高水平表达。我们之前已经证明,GDF-9缺陷型雌性小鼠不育,原因是卵泡发生在3b型初级卵泡阶段早期受阻。为了探究GDF-9缺失导致的分子缺陷,我们分析了几个重要的卵巢标记基因的表达。我们研究的主要发现如下:1)在GDF-9缺陷型卵泡周围,几种卵泡膜细胞层标记物[即17α-羟化酶、促黄体生成素受体(LHR)和kit配体的受体c-kit]没有可检测到的信号。这表明在没有GDF-9的情况下,卵泡无法发出招募卵泡膜细胞前体围绕卵泡的信号;2)GDF-9缺陷型小鼠的初级卵泡显示kit配体和抑制素-α上调。这表明在颗粒细胞中表达的这两种重要的分泌生长因子可能受到GDF-9以旁分泌方式的直接调控。通过卵母细胞上的c-kit信号传导,kit配体的上调可能直接参与了GDF-9缺陷型卵母细胞大小的增加以及卵母细胞最终的死亡;3)卵母细胞丢失后,GDF-9缺陷型卵泡的细胞仍处于类固醇生成簇中,在组织学上类似于小黄体。然而,在分子水平上,这些细胞对黄体标记物(如LHR和P-450侧链裂解酶)和非黄体标记物(如抑制素α和P-450芳香化酶)均呈阳性。这表明最初卵母细胞的存在阻止了黄体化标记物的表达,但早期GDF-9的缺失改变了颗粒细胞的分化程序;4)通过增殖细胞核抗原(PCNA)或Ki-67染色以及TUNEL(末端脱氧核苷酸转移酶介导的dUTP缺口末端标记)标记显示,GDF-9缺陷型3b型初级卵泡的颗粒细胞无法增殖,但也不会发生细胞死亡。这表明3b型卵泡的颗粒细胞需要GDF-9来持续生长,并且可能通过分化事件来具备凋亡能力。因此,这些研究让我们了解了GDF-9的旁分泌作用以及卵巢卵泡内颗粒细胞和卵泡膜细胞生长与分化的正常步骤。
