Highly sensitive in vitro bioassay for luteinizing hormone and chorionic gonadotropin allowing their measurement in plasma.

Reproduction & Fertility Pub Date : 2021-11-11 eCollection Date: 2021-12-01 DOI:10.1530/RAF-21-0045
Danièle Klett, Yves Combarnous
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引用次数: 2

Abstract

In previous studies, we had shown the synergistic effect of 10-5 M forskolin (FSK) on the detection threshold of the cyclic AMP response to luteinizing hormones (LH) and chorionic gonadotropins (CG) from various species in the mouse Leydig tumor cell (mLTC) cell line. Independently, we started to study the effect of 10-12-10-6 M oxytocin (OXT) also on the cyclic AMP response to LH and CG preparations on these same cells and found an amplifying effect on the luminescence response caused by gonadotropins. The aim was then to explore the effects of 10-12-10-6 M OXT on the gonadotropin-induced cAMP response, in the presence or absence of 10 µM FSK to optimize the assay down to a sensitivity compatible with the detection of the circulating concentrations of these hormones in various species. Finally, the optimization relies on three independent phenomena: (1) the inhibition of nucleotide phosphodiesterase by IBMX (3-isobutyl-1-methylxanthine) to avoid cAMP degradation; (2) the strong synergy of 10 µM forskolin with low concentrations of LH or CG during the 1-h luminescence measurement; (3) the stimulatory effect of 10-8M OXT on the amplitude of transfected cAMP-sensitive luciferase response. By doing this, the detectable concentrations are at the 1-10 pg/well (pM range) for the LHs and CGs from various species. The bioactivities of circulating LHs and CGs in blood or urine are therefore expected to be measurable in 10 µL-plasma samples from mammalian species and maybe others. Indeed, a preliminary study with equine and donkey plasma samples shows that the measured bioactivity was fully inhibited by a specific MAB against the receptor-binding region of equine LH (eLH) and equine CG (eCG), thus eliminating a possible response due to interfering substances other than eLH or eCG. From these data, it is expected that the bioactivity profiles of these hormones will be measurable in the blood of human, equine, and ovine species and very likely in rodents, ruminants, and hopefully in most other mammalian species.

Lay summary: Luteinizing hormone (LH) plays a central role in controlling ovary and testicle functions in many animals, including humans. The highly sensitive method, known as an assay, described in this paper, measures the biological activity of LH in the blood of mammals. The assay is performed in culture of cells derived from mouse testicles in the presence of factors that diminish the detection threshold for LH. The knowledge of the bioactive LH concentration dynamics in the blood is very informative about the reproductive status of male and female mammals. This new in vitro bioassay provides a powerful tool to get this information.

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高灵敏度的体外生物测定黄体生成素和绒毛膜促性腺激素,使其在血浆中测量。
在之前的研究中,我们在小鼠Leydig肿瘤细胞(mLTC)细胞系中发现了10-5 M forskolin (FSK)对不同种类黄体生成素(LH)和绒毛膜促性腺激素(CG)的环AMP反应检测阈值的协同作用。我们独立开始研究10-12-10-6 M催产素(OXT)对这些细胞对LH和CG制剂的循环AMP反应的影响,发现对促性腺激素引起的发光反应有放大作用。然后,目的是探索在10µM FSK存在或不存在的情况下,10-12-10-6 M OXT对促性腺激素诱导的cAMP反应的影响,以优化分析,使其灵敏度与检测不同物种中这些激素的循环浓度相兼容。最后,优化依赖于三个独立的现象:(1)IBMX(3-异丁基-1-甲基黄嘌呤)抑制核苷酸磷酸二酯酶以避免cAMP降解;(2) 10µM福斯克林与低浓度LH或CG在1 h的发光测量中具有较强的协同作用;(3) 10-8M OXT对转染camp敏感荧光素酶反应幅度的刺激作用。通过这样做,来自不同物种的LHs和cg的可检测浓度在1-10 pg/well (pM范围)。因此,血液或尿液中循环LHs和cg的生物活性有望在哺乳动物和其他物种的10 μ l血浆样本中测量。事实上,对马和驴血浆样本的初步研究表明,针对马LH (eLH)和马CG (eCG)受体结合区域的特异性MAB完全抑制了测量到的生物活性,从而消除了eLH或eCG以外的干扰物质可能引起的反应。根据这些数据,预计这些激素的生物活性将在人类、马和羊的血液中被测量,并且很可能在啮齿动物、反刍动物以及大多数其他哺乳动物物种中被测量。摘要:黄体生成素(LH)在包括人类在内的许多动物的卵巢和睾丸功能控制中起着重要作用。高灵敏度的方法,被称为化验,在本文中描述,测量生物活性的LH在哺乳动物的血液。该试验是在小鼠睾丸细胞的培养中进行的,存在降低LH检测阈值的因素。血液中生物活性LH浓度的动态变化对雄性和雌性哺乳动物的生殖状况有重要的信息。这种新的体外生物测定提供了一个强大的工具来获得这些信息。
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