A radioimmunoassay for fluorogestone acetate (FGA) and its application to the measurement of plasma FGA and progesterone in ewes treated with FGA-impregnated intravaginal sponges.

O Gaston-Parry, K Heasman, J K Nemorin, T J Robinson
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Abstract

Simultaneous concentrations of endogenous progesterone and exogenous FGA have been measured in ewes treated with FGA-impregnated intravaginal sponges at several times relative to the expected time of release of LH. First, a direct double antibody radioimmunoassay (RIA) for FGA, with good precision, sensitivity and reproducibility, was developed and validated. An oxime derivative was prepared and then conjugated to human serum albumen at the 3-position to produce the antigen. Antibodies raised in New Zealand White rabbits showed little cross-reactivity with related steroids. FGA was estimated in extracted and unextracted plasma; results were indistinguishable. Second, sponges impregnated with 40 mg FGA were inserted into 20 anoestrous crossbred ewes for 12 days; 500 i.u. pregnant mare serum gonadotrophin (PMSG) was injected at withdrawal. Similar sponges were reintroduced into four ewes at each of the intervals 1, 3, 5, and 7 days later; three ewes served as controls. Plasma concentrations of progesterone and FGA were estimated by RIA daily during treatment and at intervals of 2 h for 12 h and at 18 and 24 h after withdrawal. The plasma profiles of FGA during the two successive periods of insertion were remarkably similar. A concentration of 3.0 ng/ml (s.e.m. +/- 0.22) was attained on day 1, falling to 1.5 ng/ml (+/- 0.15) by day 4. Thereafter, the concentration was maintained at 1.1 ng/ml (+/- 0.08). Plasma progesterone concentrations were at basal levels of less than 0.2 ng/ml during the first (acyclic) period of sponge insertion. During the second (cyclic) period there was a marked difference related to the time of sponge insertion. Insertion on day 1 (before LH release) resulted in complete inhibition of luteal activity; insertion on day 3, 5 or 7 was followed by apparently normal luteal function. There was no evidence of any feedback mechanism of exogenous progestagen on endogenous progesterone and no interaction. It is concluded that a 12-day treatment is needed in cyclic ewes for full synchronization and that sponges impregnated with 40 mg FGA will maintain an effective plasma concentration of greater than 1 ng/ml to the end of this period.

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醋酸氟孕酮(FGA)的放射免疫测定及其在母羊阴道内浸渍氟孕酮海绵血浆FGA和孕酮测定中的应用
内源性孕酮和外源性FGA在母羊阴道内浸渍的海绵中同时浓度被测量,相对于LH的预期释放时间。首先,建立并验证了FGA直接双抗体放射免疫分析法(RIA),该方法具有良好的精密度、灵敏度和重复性。制备了肟衍生物,并在3位与人血清白蛋白偶联产生抗原。在新西兰大白兔中培养的抗体与相关类固醇没有交叉反应。估计提取血浆和未提取血浆的FGA;结果难以区分。其次,将海绵浸渍40 mg FGA,植入20只无情杂交母羊体内12 d;停药时注射妊娠母马血清促性腺激素(PMSG) 500 iu。在1、3、5和7 d后,将类似海绵重新引入4只母羊体内;三只母羊作为对照。在治疗期间每日、停药后每隔2 h、停药后12 h、停药后18 h和24 h用RIA测定血浆中黄体酮和FGA浓度。FGA在两个连续插入期间的等离子体谱非常相似。第1天的浓度为3.0 ng/ml (s.e.m. +/- 0.22),第4天降至1.5 ng/ml(+/- 0.15)。此后,浓度维持在1.1 ng/ml(+/- 0.08)。在海绵插入的第一个(无周期)期间,血浆孕酮浓度低于0.2 ng/ml的基础水平。在第二个(循环)周期中,与海绵插入时间有关的差异显着。在第1天(黄体生成素释放前)插入导致黄体活性完全抑制;植入后第3、5或7天黄体功能明显恢复正常。没有证据表明外源性孕激素对内源性孕激素有任何反馈机制,也没有相互作用。综上所述,周期母羊需要12天才能完全同步,海绵中浸透40 mg FGA将保持大于1 ng/ml的有效血药浓度,直至周期结束。
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A radioimmunoassay for fluorogestone acetate (FGA) and its application to the measurement of plasma FGA and progesterone in ewes treated with FGA-impregnated intravaginal sponges. Characterization of proteolytic and collagenolytic enzymes from the larvae of Lucilia cuprina, the sheep blowfly. Relationship between plasma zinc, angiotensin-converting enzyme, alkaline phosphatase and onset of symptoms of zinc deficiency in the rat. Effect of myiasis and acute restraint stress on plasma levels of immunoreactive beta-endorphin, adrenocorticotrophin (ACTH) and cortisol in the sheep. Group-specific and type-specific gel diffusion precipitin tests for bluetongue virus serotype 20 and related viruses.
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