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大鼠卵巢胶原分解活性的体内测量。

In vivo measurement of rat ovarian collagenolytic activities.

作者信息

Hirsch B, Leonhardt S, Jarry H, Reich R, Tsafriri A, Wuttke W

机构信息

Department of Obstetrics and Gynecology, University of Gottingen, Germany.

出版信息

Endocrinology. 1993 Dec;133(6):2761-5. doi: 10.1210/endo.133.6.8243302.

Abstract

Ovarian collagenases are necessary for the process of ovulation, and they are believed to be activated by the preovulatory LH surge. This information is largely based on in vitro investigations in which the balance between inhibitory and stimulatory principles involved in the activation of collagenase are largely disrupted. Therefore, we developed a simple and reliable method to measure collagenolytic activity in vivo in freely moving rats. By the use of a microdialysis system, a peptide coupled with methyl-coumarin is perfused into the bursa of the ovary. Collagenolytic enzymes cleave this peptide, and the cleaved fragments rediffuse into the microdialysis system. The effluent is collected in fractions, and the peptide-methyl-coumarin complex is cleaved, which results in liberation of fluorescent methyl-coumarin. This assay is linear over a wide range of collagenolytic activity, and other proteases, such as trypsin or plasmin, do not give any fluorescent signal. In proestrous rats, collagenolytic activity increases after the onset of the preovulatory LH surge. In animals in which the LH surge was disrupted by the surgical procedure but had a normal proestrous PRL surge, neither progesterone nor collagenolytic activity increased in the perfusate fluid. This indicates that it is only LH, not PRL, that activates follicular collagenolytic enzymes. Similar results were obtained in immature PMSG/hCG-treated animals. Using a well established zymographic assay, these results were confirmed, and it was further demonstrated that type I and type IV collagenase are active in the rat ovary.

摘要

卵巢胶原酶是排卵过程所必需的,据信它们由排卵前促黄体生成素(LH)峰激活。该信息主要基于体外研究,而在这些研究中,胶原酶激活过程中涉及的抑制性和刺激性原理之间的平衡被大大破坏。因此,我们开发了一种简单可靠的方法来测量自由活动大鼠体内的胶原溶解活性。通过使用微透析系统,将与甲基香豆素偶联的肽灌注到卵巢囊中。胶原溶解酶切割该肽,切割后的片段再扩散回微透析系统。流出物按组分收集,肽 - 甲基香豆素复合物被切割,从而导致荧光甲基香豆素的释放。该测定在广泛的胶原溶解活性范围内呈线性,而其他蛋白酶,如胰蛋白酶或纤溶酶,不会产生任何荧光信号。在动情前期大鼠中,排卵前LH峰开始后胶原溶解活性增加。在通过手术破坏LH峰但动情前期催乳素(PRL)峰正常的动物中,灌注液中的孕酮和胶原溶解活性均未增加。这表明激活卵泡胶原溶解酶的仅为LH,而非PRL。在未成熟的孕马血清促性腺激素(PMSG)/人绒毛膜促性腺激素(hCG)处理的动物中也获得了类似结果。使用成熟的酶谱分析方法证实了这些结果,并进一步证明I型和IV型胶原酶在大鼠卵巢中具有活性。

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