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马中黄体溶解和循环 PGF2α、孕酮、LH 和雌二醇之间的相关关系。

Luteolysis and associated interrelationships among circulating PGF2α, progesterone, LH, and estradiol in mares.

机构信息

Eutheria Foundation, Cross Plains, WI, USA.

出版信息

Domest Anim Endocrinol. 2011 Nov;41(4):174-84. doi: 10.1016/j.domaniend.2011.06.003. Epub 2011 Jul 21.

Abstract

The changing concentrations and temporal relationships among a PGF2α metabolite (PGFM), progesterone (P(4)), LH, and estradiol-17β (E(2)) before, during, and after luteolysis were studied in 10 mares. Blood samples were collected every hour for ≥4 d beginning on day 12 after ovulation. The luteolytic period extended from a decrease in P(4) at a common transitional hour (Hour 0) at the end of preluteolysis and beginning of luteolysis to a defined ending when P(4) reached 1 ng/mL. The length of luteolysis was 22.9 ± 0.9 h, contrasting with 2 d in published P(4) profiles from sampling every 6 to 24 h. In mares with complete data for Hours -40 to -2 (n = 6), PGFM concentrations remained below assay sensitivity (n = 2) or two or three small pulses (peak, 29 ± 4 pg/mL) occurred. During luteolysis, the pulses became more prominent (peak, 193 ± 36 pg/mL). Rhythmicity of PGFM pulses was not detected by a pulsatility program during preluteolysis but was detected in seven of nine mares during luteolysis and postluteolysis combined. The nadir-to-nadir interval for LH pulses and the peak-to-peak interval between adjacent pulses were longer (P < 0.05) during preluteolysis than during luteolysis (nadir to nadir, 5.2 ± 0.3 h vs 3.6 ± 0.4 h; peak to peak, 9.4 ± 1.0 h vs 4.7 ± 0.5 h). Unlike reported findings in cattle, concentrations of P(4) decreased linearly within the hours of each PGFM pulse during luteolysis, and a positive effect of an LH pulse on P(4) and E(2) concentration was not detected. The reported balancing of P(4) concentrations between a negative effect of PGF2α and a positive effect of LH in heifers was not detected in mares.

摘要

我们研究了 10 匹母马在排卵后第 12 天开始的≥4 天内,PGF2α 代谢产物(PGFM)、孕酮(P4)、LH 和雌二醇-17β(E2)在黄体溶解前、溶解期间和溶解后的浓度变化及其时间关系。每隔 1 小时采集 1 次血样。黄体溶解期从黄体溶解前和黄体溶解开始时的 P4 下降的共同过渡小时(0 小时)开始,到 P4 达到 1ng/mL 时定义的结束时间结束。黄体溶解期为 22.9±0.9 小时,与发表的每隔 6 到 24 小时采样的 P4 曲线相比,持续时间为 2 天。在有从 -40 小时到 -2 小时完整数据的 6 匹母马中(n=6),PGFM 浓度低于检测限(n=2),或者发生了 2 或 3 个小脉冲(峰值,29±4pg/mL)。在黄体溶解期间,脉冲变得更加明显(峰值,193±36pg/mL)。在黄体溶解前,脉冲性程序未检测到 PGFM 脉冲的节律性,但在黄体溶解和黄体溶解后联合期间,9 匹母马中有 7 匹检测到。LH 脉冲的峰峰间隔和相邻脉冲的峰谷间隔在黄体溶解前(峰谷间隔,5.2±0.3h 比黄体溶解期间(峰谷间隔,3.6±0.4h)更长(P<0.05);峰值间隔,9.4±1.0h 比黄体溶解期间(峰值间隔,4.7±0.5h)更长)。与牛的报告结果不同,在黄体溶解期间,每个 PGFM 脉冲期间 P4 浓度呈线性下降,并且未检测到 LH 脉冲对 P4 和 E2 浓度的正效应。在母马中,也未检测到报道的 PGF2α 的负效应和 LH 的正效应之间 P4 浓度的平衡作用。

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