Production of tissue inhibitors of metalloproteinases (TIMPs) by pig ovarian cells in vivo and the effect of TIMP-1 on steroidogenesis in vitro.

E. Shores, M. Hunter
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引用次数: 20

Abstract

Precisely which ovarian cells produce tissue inhibitors of metalloproteinases (TIMPs) is unclear. Although granulosa cells are reported to produce TIMPs, thecal TIMP production has not been investigated nor has the influence of TIMPs on theca cells. Furthermore, although periovulatory follicles have been examined, little is known about smaller ovarian follicles. Follicles >/= 2 mm in diameter were collected from Large White hybrid gilts on the day before predicted oestrus (n = 3) or after hCG treatment (n = 3) and divided into 1 mm size classes. Small (2 to < 5 mm) follicles were kept intact, whereas follicles >/= 5 mm were separated into follicular fluid, granulosa and theca cell compartments. After homogenization, TIMP-1, -2 and -3 were detected by reverse zymography. Theca cells (50 x 10(3) per well) were cultured with TIMP-1 (10, 100 or 200 ng ml(-1) with or without long-R3 insulin-like growth factor I (IGF-I)) in a serum-free system to investigate the effect on steroidogenesis and the number of cells. Both large and small pig follicles produced TIMPs and TIMP-1, -2 and -3 were detected in follicular fluid, granulosa and theca cell samples. There was a phase x tissue type interaction for the presence of both TIMP-1 and -2 (P < 0.03, P < 0.05, respectively), and TIMPs were detected in more granulosa and theca cell samples after hCG than during the follicular phase. The concentrations were influenced by the type of tissue (TIMP-1, P < 0.005; TIMP-2, P < 0.005, TIMP-3, P > 0.05), and the highest concentrations occurred in the theca tissue. There were tissue type x follicle size interactions for the presence of both TIMP-1 and -2 (P < 0.001). In vitro, TIMP-1 increased thecal steroidogenesis after 144 h (oestradiol, P < 0.05, progesterone, P < 0.001) but reduced the number of viable cells (P < 0.001). In conclusion, TIMP-1, -2 and -3 were present in large and small pig follicles and were produced by both granulosa and theca cells, although concentrations differed with the type of tissue. Production was regulated by factors including follicle size and phase of the oestrous cycle. In addition to controlling tissue remodelling, TIMP-1 may also regulate steroidogenesis.
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猪卵巢细胞体内金属蛋白酶组织抑制剂(timp)的产生及TIMP-1对体外类固醇生成的影响
确切地说,卵巢细胞产生金属蛋白酶组织抑制剂(TIMPs)尚不清楚。尽管有报道称颗粒细胞可产生TIMP,但尚未研究鞘膜TIMP的产生,也未研究TIMP对鞘膜细胞的影响。此外,虽然已经检查了排卵周卵泡,但对较小的卵巢卵泡知之甚少。在预测发情前一天(n = 3)或hCG治疗后(n = 3)收集直径为>/= 2mm的大白杂交后备母猪卵泡,并将其分为1 mm大小的组。小卵泡(2 ~ < 5mm)保持完整,而卵泡(>/= 5mm)被分离成卵泡液、颗粒和卵泡膜细胞室。匀浆后,反酶法检测TIMP-1、-2和-3。在无血清系统中,用TIMP-1(10、100或200 ng ml(-1)加或不加长r3胰岛素样生长因子I (IGF-I))培养caa细胞(每孔50 × 10(3)),观察其对甾体生成和细胞数量的影响。猪大、小卵泡均可产生timp,在卵泡液、颗粒和卵膜细胞样品中均检测到TIMP-1、-2和-3。TIMP-1和-2存在于x期组织型相互作用(P < 0.03, P < 0.05), hCG后颗粒和卵泡细胞样品中检测到的timp多于卵泡期。其浓度受组织类型的影响(TIMP-1, P < 0.005;TIMP-2, P < 0.005, TIMP-3, P < 0.05),且在卵膜组织中浓度最高。TIMP-1和-2存在组织型x卵泡大小相互作用(P < 0.001)。体外处理144 h后,TIMP-1增加了鞘内甾体生成(雌二醇,P < 0.05,孕酮,P < 0.001),但减少了活细胞数量(P < 0.001)。综上所述,TIMP-1、-2和-3均存在于猪的大卵泡和小卵泡中,并可由颗粒细胞和膜细胞产生,但其浓度随组织类型的不同而不同。生产受卵泡大小和发情周期等因素的调节。除了控制组织重塑,TIMP-1还可能调节类固醇生成。
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