Tissue prothrombinase activity in myometrium from timed-pregnant rats.

Mark Phillippe, Diana F Bradley, Kathrynn Phillippe, Daniel Engle
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引用次数: 7

Abstract

Objective: Fgl2 and thrombin potentially play roles during inflammation-induced preterm delivery. These studies sought to demonstrate functional prothrombinase enzyme activity in rat uterus, consistent with the expression of Fgl2 in this tissue.

Methods: Myometrial and other tissue obtained from non-pregnant and timed-pregnant rats was homogenized in Tris-buffered saline. Prothrombinase activity was determined based on the kinetic metabolism of a chromogenic thrombin substrate. Homogenates were incubated with prothrombin followed by the addition of the thrombin substrate. Thrombin activity was determined by comparing tissue activity to a standard curve generated using 0.01 to 0.04 units of active thrombin. Western blot studies were also performed to confirm tissue prothrombinase activity in myometrial homogenates. Prothrombin was incubated with tissue homogenates; the reactions were then terminated with sodium dodecyl sulfate (SDS) loading buffer.

Results: Prothrombinase activity in myometrial tissue was observed to be 0.047 to 0.077 U thrombin/10 min/microg protein. Heat denaturation and calcium removal eliminated prothrombinase activity, whereas the addition of Factor V enhanced activity. The Western blots confirmed the presence of prothrombin, the anticipated prethrombin fragments, and thrombin. Consistent with the enzyme studies, the thrombin band formed upon incubation with myometrial homogenates from pregnant and nonpregnant rats. In contrast, the thrombin band was not apparent with removal of calcium, heat denaturation and treatment with serine protease inhibitors.

Conclusions: In summary, these studies have confirmed functionally active prothrombinase activity in rat myometrium, supporting the hypothesis that Fgl2 is expressed in this tissue.

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定时妊娠大鼠肌层组织凝血酶原活性。
目的:Fgl2和凝血酶可能在炎症性早产中发挥作用。这些研究试图证明大鼠子宫中凝血酶原活性的功能,与Fgl2在该组织中的表达一致。方法:取未妊娠大鼠和定时妊娠大鼠的子宫肌层及其他组织,用tris缓冲盐水匀浆。根据显色凝血酶底物的动力学代谢测定凝血酶原活性。匀浆与凝血酶原孵育,然后加入凝血酶底物。凝血酶活性通过将组织活性与使用0.01至0.04单位活性凝血酶生成的标准曲线进行比较来确定。Western blot研究也证实了组织凝血酶原在子宫肌层匀浆中的活性。凝血酶原用组织匀浆孵育;然后用十二烷基硫酸钠(SDS)负载缓冲液终止反应。结果:肌组织凝血酶原活性为0.047 ~ 0.077 U凝血酶/10 min/ μ g蛋白。热变性和脱钙消除了凝血酶原的活性,而添加因子V则增强了活性。Western blots证实存在凝血酶原、预期的凝血酶前片段和凝血酶。与酶的研究一致,凝血酶带是在怀孕和未怀孕大鼠的子宫内膜匀浆孵育后形成的。相比之下,去除钙、热变性和丝氨酸蛋白酶抑制剂处理后,凝血酶带不明显。结论:综上所述,这些研究证实了大鼠肌层具有功能活性的凝血酶原活性,支持Fgl2在该组织中表达的假设。
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