黄体酮调节绵羊子宫胎盘组织中组织非特异性碱性磷酸酶(TNSALP)的表达和活性。

IF 6.3 Q1 AGRICULTURE, DAIRY & ANIMAL SCIENCE
Claire Stenhouse, Katherine M Halloran, Emily C Hoskins, Robyn M Moses, Guoyao Wu, Heewon Seo, Gregory A Johnson, Larry J Suva, Dana Gaddy, Fuller W Bazer
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引用次数: 0

摘要

背景:组织非特异性碱性磷酸酶(TNSALP;由ALPL基因编码)在出生后的磷酸盐稳态调节中起着至关重要的作用,但TNSALP的活性和表达在妊娠期间如何调节在很大程度上仍是未知的。本研究测试了孕酮(P4)和/或干扰素tau(IFNT)调节绵羊妊娠期间TNSALP活性的假设:在实验 1 中,母羊配种后在妊娠的前 8 天每天肌肉注射玉米油载体(CO)或 25 毫克黄体酮(P4),并在妊娠的第 9、12 或 125 天切除子宫。在实验 2 中,母羊在发情周期的第 7 天安装宫内导管,从第 8 天到第 15 天每天肌肉注射 50 毫克 P4(CO)和/或 75 毫克孕酮受体拮抗剂(RU486)(CO),从第 11 天到第 15 天每天两次宫内注射对照蛋白(CX)或 IFNT(25 µg/uterine horn/d)(治疗组:P4+CX;P4+IFNT;RU486+P4+CX;RU486+P4+IFNT),并在第 16 天切除子宫:在实验 1 中,在第 12 天时,服用 P4 的母羊子宫内膜的 ALPL mRNA 表达量高于服用 CO 的母羊。在第12天,与服用CO的母羊相比,服用P4的母羊子宫内膜和子宫肌层的上皮、基质层和血管内皮的TNSALP活性更高。第125天,TNSALP活性定位于子宫上皮细胞和内皮细胞,与P4处理无关。P4处理过的母羊胎盘中的TNSALP活性更高,P4处理过的母羊内皮细胞和胴体组织中也检测到了TNSALP活性,而CO处理过的母羊则没有。在实验 2 中,服用 RU486 + P4 + CX 的母羊子宫内膜匀浆的 TNSALP 活性低于服用 P4 + CX 和 P4 + IFNT 的母羊。与其他处理组相比,RU486 + P4 + CX 处理组母羊腺上皮中层和深层的免疫活性 TNSALP 蛋白更强。与其他治疗组相比,RU486 + P4 + CX 治疗组母羊子宫内膜深层腺上皮顶端表面的酶活性更高:这些结果表明,P4(而非 IFNT)可调节 TNSALP 在子宫胎盘组织中的表达和活性,并有可能有助于调节磷酸盐的可用性,而磷酸盐的可用性对妊娠期间胎儿的发育至关重要。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Progesterone regulates tissue non-specific alkaline phosphatase (TNSALP) expression and activity in ovine utero-placental tissues.

Background: Tissue non-specific alkaline phosphatase (TNSALP; encoded by the ALPL gene) has a critical role in the postnatal regulation of phosphate homeostasis, yet how TNSALP activity and expression are regulated during pregnancy remain largely unknown. This study tested the hypothesis that progesterone (P4) and/or interferon tau (IFNT) regulate TNSALP activity during pregnancy in sheep.

Methods: In Exp. 1, ewes were bred and received daily intramuscular injections of either corn oil vehicle (CO) or 25 mg progesterone in CO (P4) for the first 8 days of pregnancy and were hysterectomized on either Day 9, 12, or 125 of gestation. In Exp. 2, ewes were fitted with intrauterine catheters on Day 7 of the estrous cycle and received daily intramuscular injections of 50 mg P4 in CO and/or 75 mg progesterone receptor antagonist (RU486) in CO from Days 8 to 15, and twice daily intrauterine injections of either control proteins (CX) or IFNT (25 µg/uterine horn/d) from Days 11 to 15 (treatment groups: P4 + CX; P4 + IFNT; RU486 + P4 + CX; and RU486 + P4 + IFNT) and were hysterectomized on Day 16.

Results: In Exp. 1, endometria from ewes administered P4 had greater expression of ALPL mRNA than ewes administered CO on Day 12. TNSALP activity appeared greater in the epithelia, stratum compactum stroma, and endothelium of the blood vessels in the endometrium and myometrium from ewes administered P4 than ewes administered CO on Day 12. On Day 125, TNSALP activity localized to uterine epithelial and endothelial cells, independent of P4 treatment. TNSALP activity in placentomes appeared greater in P4 treated ewes and was detected in endothelial cells and caruncular tissue in P4 treated but not CO treated ewes. In Exp. 2, endometrial homogenates from ewes administered RU486 + P4 + CX had lower TNSALP activity those for P4 + CX and P4 + IFNT ewes. Immunoreactive TNSALP protein appeared greater in the mid- and deep-glandular epithelia in RU486 + P4 + CX treated ewes as compared to the other treatment groups. Enzymatic activity appeared greater on the apical surface of the deep glandular epithelia in endometria from ewes treated with RU486 + P4 + CX compared to the other treatment groups.

Conclusions: These results suggest that P4, but not IFNT, regulates the expression and activity of TNSALP in utero-placental tissues and has the potential to contribute to the regulation of phosphate availability that is critical for conceptus development during pregnancy.

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