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雌二醇激活的甲胎蛋白抑制子宫对雌激素的反应。

Estradiol-activated alpha-fetoprotein suppresses the uterotropic response to estrogens.

作者信息

Mizejewski G J, Vonnegut M, Jacobson H I

出版信息

Proc Natl Acad Sci U S A. 1983 May;80(9):2733-7. doi: 10.1073/pnas.80.9.2733.

Abstract

The binding of estrogen to alpha-fetoprotein (AFP) in the plasma cannot account for the impaired estrogen response seen in immature rodents because estradiol (E2) doses that far exceed the total body burden of AFP will stimulate only modest uterine growth. We investigated this phenomenon in immature female mice by determining their uterine weights 23 hr after intraperitoneal injection of estrogens or AFP or both. Administration of either 0.5 micrograms of E2 or 10 ng of moxestrol (MOX) approximately doubled the uterine weight. Giving 1 microgram of AFP 1 hr before injection of either estrogen did not alter that response. Combining the E2 and AFP just prior to injection resulted in decreased uterine growth (34% inhibition). Preincubating the estrogens with purified AFP (0.1-50 micrograms) did not affect the growth response to moxestrol but markedly decreased the response to E2. This was not due to sequestering of hormone because maximal reduction of the E2 response (ca. 65% inhibition) required only 1.0 microgram of AFP (AFP/E2 molar ratio, 1:130), and higher AFP doses inhibited less. About 40% of the growth elicited by injection of either 0.5 micrograms of E2 or 10 ng of MOX was inhibited when these doses were preceded by injection of the preincubated AFP/E2 mixture but not when preceded by either of the components. In each experiment, the mitotic index of luminal epithelium was affected to the same degree as uterine weight. AFP and E2 incubated for 1 hr thus produce a potent inhibitor of estrogen-stimulated mitotic activity and growth. This inhibitor might act upon estrogen-responsive cells at specific sites at which competition by an inactive component of AFP can block the process.

摘要

血浆中雌激素与甲胎蛋白(AFP)的结合无法解释在未成熟啮齿动物中观察到的雌激素反应受损现象,因为远远超过AFP全身负荷的雌二醇(E2)剂量只会刺激适度的子宫生长。我们通过在腹腔注射雌激素或AFP或两者后23小时测定未成熟雌性小鼠的子宫重量,对这一现象进行了研究。注射0.5微克E2或10纳克莫昔司琼(MOX)均可使子宫重量增加约一倍。在注射任何一种雌激素前1小时给予1微克AFP不会改变这种反应。在注射前将E2和AFP混合会导致子宫生长减少(抑制34%)。将雌激素与纯化的AFP(0.1 - 50微克)预孵育不会影响对莫昔司琼的生长反应,但会显著降低对E2的反应。这并非由于激素的隔离,因为E2反应的最大降低(约65%抑制)仅需要1.0微克AFP(AFP/E2摩尔比为1:130),更高的AFP剂量抑制作用较小。当在注射0.5微克E2或10纳克MOX之前先注射预孵育的AFP/E2混合物时,约40%的生长受到抑制,而在注射其中任何一种成分时则不会。在每个实验中,腔上皮的有丝分裂指数与子宫重量受到的影响程度相同。因此,AFP和E2孵育1小时会产生一种有效的雌激素刺激有丝分裂活性和生长的抑制剂。这种抑制剂可能作用于雌激素反应细胞的特定部位,在这些部位AFP的无活性成分的竞争可以阻断这一过程。

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