Weems Y S, Lennon E, Uchima T, Raney A, Goto K, Ong A, Zaleski H, Weems C W
Department of Human Nutrition Food, and Animal Sciences, University of Hawaii, Honolulu, HI 96822, USA.
Prostaglandins Other Lipid Mediat. 2008 Feb;85(1-2):33-41. doi: 10.1016/j.prostaglandins.2007.10.003. Epub 2007 Oct 24.
Nitric oxide (NO) has been reported to be luteolytic in vitro and in vivo in cows. However, an NO donor reversed PGF2alpha-induced inhibition of rat luteal progesterone secretion in vitro and an NO donor or endothelin-1 stimulated bovine luteal tissue secretion of prostaglandins E (PGE; PGE1, PGE2) in vitro without affecting progesterone or PGF2alpha secretion. In addition, chronic infusion of an NO donor into the interstitial tissue of the ovarian vascular pedicle adjacent the luteal-containing ovary prevented the decline in circulating progesterone, while a nitric oxide synthase (NOS) inhibitor did not affect luteolysis. The objective of this experiment was to determine whether an NO donor or NOS inhibitor infused chronically intrauterine adjacent to the luteal-containing ovary during the ovine estrous cycle was luteolytic or antiluteolytic. Ewes were treated either with vehicle (N=5), diethylenetriamine (DETA-control for DETANONOate; N=5), (Z)-1-[2-(2-aminoethyl)-N-(2-ammonioethyl)amino]diazen-1-ium-1,2-diolate (DETANONOate-long acting NO donor; N=6), l-arginine (N=5), l-nitro-arginine methyl ester (l-NAME-NOS inhibitor; N=6), or NG-monomethyl-l-arginine acetate (l-NMMA; NOS inhibitor; N=5) every 6h from 2400h (0h) on day 8 through 1800h on day 18 of the estrous cycle. Jugular venous blood and inferior vena cava plasma via a saphenous vein cathether 5cm anterior to the juncture of the ovarian vein and inferior vena cava were collected every 6h for analysis for progesterone and PGF2alpha and PGE, respectively, by RIA. Corpora lutea were collected at 1800h on day 18 and weighed. Weights of corpora lutea were heavier (P< or =0.05) in DETANONOate-treated ewes when compared to vehicle, DETA, l-arginine, l-NAME, or l-NMMA-treated ewes, l-arginine luteal weights were heavier than vehicle, DETA, l-arginine, l-NAME, or l-NMMA-treated ewes, and luteal weights of vehicle, DETA, l-NAME, or l-NMMA-treated ewes did not differ amongst each other (P> or =0.05). Profiles of progesterone in jugular venous blood on days 8-18 differed (P< or =0.05) in DETANONOate-treated ewes when compared to vehicle, DETA, l-arginine, l-NMMA or l-NAME-treated ewes, which did not differ (P> or =0.05) amongst each other. The PGE:PGF2alpha ratio profile in inferior vena cava plasma of DETANONOate-treated ewes was increased (P< or =0.05) when compared to all other treatment groups. In a second experiment, conversion of [3H PGE2] to [3H PGF2alpha] by day 15 ovine caruncular endometrium in vitro was determined in vehicle, DETA, or DETANONOate-treatment groups. Conversion of [3H PGE2] to [3H PGF2alpha] was decreased (P< or =0.05) only by DETANONOate. It is concluded that NO is not luteolytic during the ovine estrous cycle, but may instead be antiluteolytic and prevent luteolysis by altering the PGE:PGF2alpha ratio secreted by the uterus.
据报道,一氧化氮(NO)在奶牛体内外具有溶黄体作用。然而,一种NO供体可逆转PGF2α在体外对大鼠黄体孕酮分泌的抑制作用,且一种NO供体或内皮素-1在体外可刺激牛黄体组织分泌前列腺素E(PGE;PGE1、PGE2),而不影响孕酮或PGF2α的分泌。此外,向含黄体卵巢相邻的卵巢血管蒂间质组织中慢性注入NO供体可防止循环孕酮水平下降,而一氧化氮合酶(NOS)抑制剂对黄体溶解无影响。本实验的目的是确定在绵羊发情周期中,向含黄体卵巢相邻的子宫内慢性注入NO供体或NOS抑制剂是否具有溶黄体或抗溶黄体作用。从发情周期第8天的2400时(0时)至第18天的1800时,每隔6小时给母羊分别注射溶媒(N = 5)、二乙烯三胺(DETA,DETANONOate的对照;N = 5)、(Z)-1-[2-(2-氨乙基)-N-(2-氨乙基)氨基]重氮-1,2-二醇盐(DETANONOate,长效NO供体;N = 6)、L-精氨酸(N = 5)、L-硝基精氨酸甲酯(L-NAME,NOS抑制剂;N = 6)或NG-单甲基-L-精氨酸乙酸盐(L-NMMA,NOS抑制剂;N = 5)。每隔6小时通过位于卵巢静脉与下腔静脉交界处前方5cm处的大隐静脉导管采集颈静脉血和下腔静脉血浆,分别用放射免疫分析法测定孕酮、PGF2α和PGE。在第18天的1800时采集黄体并称重。与溶媒、DETA、L-精氨酸、L-NAME或L-NMMA处理的母羊相比,DETANONOate处理的母羊黄体重量更重(P≤0.05);L-精氨酸处理的母羊黄体重量比溶媒、DETA、L-精氨酸、L-NAME或L-NMMA处理的母羊更重;溶媒、DETA、L-NAME或L-NMMA处理的母羊黄体重量彼此之间无差异(P≥0.05)。与溶媒、DETA、L-精氨酸、L-NMMA或L-NAME处理的母羊相比,DETANONOate处理的母羊在第8 - 18天颈静脉血中的孕酮水平曲线存在差异(P≤0.05),而溶媒、DETA、L-精氨酸、L-NMMA或L-NAME处理的母羊之间无差异(P≥0.05)。与所有其他处理组相比,DETANONOate处理的母羊下腔静脉血浆中PGE:PGF2α比值曲线升高(P≤0.05)。在第二个实验中,测定了溶媒、DETA或DETANONOate处理组中第15天绵羊肉阜子宫内膜在体外将[3H PGE2]转化为[3H PGF2α]的情况。仅DETANONOate可使[3H PGE2]向[3H PGF2α]的转化减少(P≤0.05)。结论是,在绵羊发情周期中,NO不具有溶黄体作用,反而可能具有抗溶黄体作用,并通过改变子宫分泌的PGE:PGF2α比值来防止黄体溶解。
