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Temporal and spatial expression of tissue inhibitors of metalloproteinases 1 and 2 (TIMP-1 and -2) in the bovine corpus luteum

机译:牛黄体中金属蛋白酶1和2(TIMP-1和-2)组织抑制剂的时空表达

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摘要

The matrix metalloproteinases (MMPs) and their endogenous inhibitors, tissue inhibitors of metalloproteinases (TIMPs), may mediate the dramatic structural and functional changes in the corpus luteum (CL) over the course of its life span. In addition to regulating MMP activity, TIMPs are also involved in a variety of cellular processes, including cell proliferation and steroidogenesis. In a series of initial studies, we determined that matrix metalloproteinase inhibitory activity was present in protein extracts from early (4 days old, estrus = day 0), mid (10–12 days old) and late (16 days old) CL (n = 3 for each stage). Reverse zymography revealed four metalloproteinase inhibitory protein bands with relative molecular masses that are consistent with those reported for TIMP-1 to -4. In order to gain a better understanding of TIMPs and their role in luteal function, we further characterized this inhibitory activity with a particular focus on the temporal and spatial expression of TIMP-1 and TIMP-2 in the bovine CL. Northern blotting revealed that the TIMP-1 transcript (0.9 kb) was expressed at a higher (p < 0.05) level in early and mid cycle CL than in the late stage. In contrast, two TIMP-2 mRNA species, one major 1 kb species and one minor 3.5 kb species, were significantly (p < 0.05) increased in the mid and late cycle CL than in the early. Western blotting analyses demonstrated no differences in TIMP-1 (29 kDa) protein levels between early and mid stages, while its levels decreased (p < 0.05) from the mid to late stage CL. Conversely, TIMP-2 (22 kDa) protein was detected at a low level in the early CL, but significantly (p < 0.05) increased in the mid and late stages. Immunohistochemistry revealed that both TIMP-1 and -2 were localized to large luteal cells from all three ages of CL. TIMP-1 was also localized in capillary smooth muscle cells, while TIMP-2 was restricted to the endothelial cells in the capillary compartment. In conclusion, the different temporal expression patterns of TIMP-1 and TIMP-2 suggest that TIMP-1 may be important for luteal formation and development, while TIMP-2 may play significant roles during luteal development and maintenance. Furthermore, the distinct localization of these two inhibitors in the vascular compartment indicates that they may serve diverse physiological functions during different stages of luteal angiogenesis.
机译:基质金属蛋白酶(MMP)及其内源性抑制剂,金属蛋白酶的组织抑制剂(TIMPs),可以介导黄体(CL)在其整个生命周期中发生巨大的结构和功能变化。除调节MMP活性外,TIMP还参与多种细胞过程,包括细胞增殖和类固醇生成。在一系列初步研究中,我们确定了早期(4天大,发情=第0天),中期(10-12天大)和晚期(16天大)CL(n)的蛋白质提取物中存在基质金属蛋白酶抑制活性。 =每个阶段3个)。反向酶谱法显示四个金属蛋白酶抑制蛋白带,其相对分子质量与TIMP-1至-4报道的相对分子质量一致。为了更好地了解TIMPs及其在黄体功能中的作用,我们进一步表征了这种抑制活性,特别关注TIMP-1和TIMP-2在牛CL中的时空表达。 Northern印迹显示,TIMP-1转录物(0.9 kb)在CL早期和中期CL中的表达水平高于后期(p <0.05)。相反,在周期中后期CL中,两种TIMP-2 mRNA种类,一种主要的1 kb种类和一种次要的3.5 kb种类比早期显着增加(p <0.05)。 Western印迹分析表明,早期和中期之间TIMP-1(29 kDa)蛋白水平没有差异,而从CL的中期到后期,其水平却下降了(p <0.05)。相反,在早期CL中检测到TIMP-2(22 kDa)蛋白水平较低,但在中晚期显着(p <0.05)增加。免疫组织化学显示,TIMP-1和-2均位于所有三个年龄的CL的大黄体细胞中。 TIMP-1也定位在毛细血管平滑肌细胞中,而TIMP-2限于毛细血管腔内的内皮细胞。总之,TIMP-1和TIMP-2的不同时间表达模式表明TIMP-1对黄体的形成和发育可能很重要,而TIMP-2在黄体的形成和维持中可能起重要作用。此外,这两种抑制剂在血管腔中的独特定位表明它们可能在黄体血管生成的不同阶段发挥多种生理功能。

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