Uterine kallikrein and arterial bradykinin activities and uterine arterial proliferation in response to acute estradiol-17β exposure in ovariectomized ewes

去卵巢大鼠 内分泌学 内科学 缓激肽 子宫 激肽释放酶 雌激素 生物 子宫内膜 子宫内 医学 怀孕 受体 胎儿 生物化学 遗传学
作者
L A Lekatz,P Shukla,M A Vasquez Hidalgo,S O'Rourke,J Haring,G P Dorsam,A T Grazul-Bilska,K A Vonnahme
标识
DOI:10.1016/j.domaniend.2022.106748
摘要

• Exposure to estradiol-17β in ovariectomized ewes tended to increase kallikrein specific activity in carcuncular tissue. • Uterine arteries from ovariectomized ewes treated with estradiol-17β for 24 and 48 h had greater sensitivity to bradykinin, via the bradykinin receptor 2, than uterine arteries from ewes with 0 or 12 h estradiol-17β exposure. Estradiol-17β (E2) increases kallikrein in rodent and human reproductive tissues. Kallikrein specific activity is increased in the porcine uterus when conceptus E2 is secreted at maternal recognition of pregnancy. When kallikrein acts on kininogen to liberate bradykinin, angiogenic and vasoactive factors are released. The uterus of ovariectomized ewes administered E2 undergoes rapid vascular changes via different patterns of angiogenic and vasoactive factors. Our hypothesis was that E2 would increase the specific activity and protein secretion of tissue kallikrein in endometrial explants culture media (ECM) and ewes exposed to E2 would have uterine arteries that would be more sensitive to the vasodilatory effects of bradykinin. Ovariectomized ewes received 100 mg of E2 implants for 0, 12, 24, or 48 h. After treatment, uterine weights were determined, and caruncles were processed for ECM. Uterine weights and uterine weight per ewe body weight were significantly greater in the 12 and 24 h ewes compared with the 0 h ewes, with the 48 h ewes being similar to the 24 h ewes. There were no statistically significant differences in caruncular tissue kallikrein protein secretion among the treatment groups. There was a tendency ( P = 0.09) for duration of E2 exposure to influence tissue kallikrein specific activity where kallikrein activity was greater ( P ≤ 0.05) in the 12 and 48 h ewes compared with the 0 h ewes, with 24 h ewes being intermediate (unprotected F test). Uterine arteries from ewes with E2 for 24 and 48 h had more sensitivity to bradykinin, via the bradykinin receptor 2, than uterine arteries from ewes with 0 or 12 h E2 exposure. We fail to reject our hypothesis as E2 did elicit a positive response in tissue kallikrein specific activity and bradykinin response. Further investigations are needed to determine how kallikrein and bradykinin may be involved in vascular remodeling of the ovine uterus.

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