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用单克隆抗雌激素亲和素对猕猴生殖道中雌激素受体进行免疫细胞化学定位。

Immunocytochemical localization of estrogen receptors in the macaque reproductive tract with monoclonal antiestrophilins.

作者信息

McClellan M C, West N B, Tacha D E, Greene G L, Brenner R M

出版信息

Endocrinology. 1984 Jun;114(6):2002-14. doi: 10.1210/endo-114-6-2002.

Abstract

Monoclonal antibodies to the estrogen receptor (anti-ER) were used to develop an immunocytochemical method to detect ERs in frozen sections of the macaque reproductive tract. Specific nuclear, but not cytoplasmic, staining occurred with two different methods: direct, in which an antiestrophilin -horseradish peroxidase conjugate was used as the first antibody, and indirect, in which a mixture of antiestrophilins was used in the first incubation step. Nuclear staining was absent when various control antibodies replaced the anti-ER. In uteri from spayed monkeys treated with estradiol (E2) for 14 days, nuclear staining was always present. In uteri from similar animals treated for an additional 14 days with E2 and progesterone, nuclear staining was almost completely absent. Mean endometrial nuclear ER levels, measured by an exchange assay, were 5-fold greater in the E2-treated than in the E2-plus progesterone-treated group. In addition, when samples of estrogenized uterus and oviduct were incubated for 60 min in vitro with 100 nM E2, the intensity of nuclear staining increased in parallel with an increase in the concentration of nuclear ER. The nuclei of stromal, smooth muscle, and epithelial cells of the estrogenized oviduct, cervix, and vagina as well as smooth muscle cells of the estrogenized myometrium were also receptor positive. Nontarget tissues, such as duodenum, colon, esophagus, and skeletal muscle, contained no cells that showed specific nuclear staining. Some staining of cytoplasmic and extracellular components occurred in all preparations. These latter reactions were nonspecific, because they were present in many nontarget tissues or when control antibodies replaced the anti-ER. With current methods, only nuclear ERs can be reliably localized in frozen sections of monkey tissues with monoclonal antiestrophilins .

摘要

利用雌激素受体单克隆抗体(抗ER)开发了一种免疫细胞化学方法,用于检测猕猴生殖道冰冻切片中的ER。两种不同方法均出现了特异性的细胞核染色,而非细胞质染色:直接法,即使用抗雌激素结合蛋白-辣根过氧化物酶偶联物作为一抗;间接法,即在第一步孵育中使用抗雌激素结合蛋白混合物。当各种对照抗体替代抗ER时,细胞核染色消失。在用雌二醇(E2)处理14天的去卵巢猴子的子宫中,始终存在细胞核染色。在用E2和孕酮再处理14天的类似动物的子宫中,细胞核染色几乎完全消失。通过交换测定法测得,E2处理组的平均子宫内膜细胞核ER水平比E2加孕酮处理组高5倍。此外,当雌激素化的子宫和输卵管样本在体外与100 nM E2孵育60分钟时,细胞核染色强度随着细胞核ER浓度的增加而平行增加。雌激素化的输卵管、子宫颈和阴道的基质、平滑肌和上皮细胞的细胞核以及雌激素化的子宫肌层的平滑肌细胞也呈受体阳性。非靶组织,如十二指肠、结肠、食管和骨骼肌,未发现有显示特异性细胞核染色的细胞。在所有制剂中均出现了一些细胞质和细胞外成分的染色。这些后期反应是非特异性的,因为它们存在于许多非靶组织中,或者当对照抗体替代抗ER时也会出现。使用当前方法,用单克隆抗雌激素结合蛋白只能在猴子组织的冰冻切片中可靠地定位细胞核ER。

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