Purification, Characterization, andin vitroDifferentiation of Cytotrophoblasts from Human Term Placentae*

人胎盘催乳素 生物 合胞滋养细胞 胎盘催乳素 合胞体 胎盘 免疫过氧化物酶 滋养层 合胞滋养细胞 内分泌学 细胞滋养层 Percoll公司 胎膜 内科学 胎儿 分子生物学 体外 抗体 生物化学 免疫学 细胞 单克隆抗体 医学 怀孕 遗传学
作者
Harvey J. Kliman,John E. Nestler,EDUARDO SERMASI,Jean M. Sanger,Jerome F. Strauss
出处
期刊:Endocrinology [Oxford University Press]
卷期号:118 (4): 1567-1582 被引量:1578
标识
DOI:10.1210/endo-118-4-1567
摘要

Highly purified functional cytotrophoblasts have been prepared from human term placentae by adding a Percoll gradient centrifugation step to a standard trypsin-DNase dispersion method. The isolated mononuclear trophoblasts averaged 10 μm in diameter, with occasional cells measuring up to 20–30 μm. Viability was greater than 90%. Transmission electron microscopy revealed that the cells had fine structural features typical of trophoblasts. In contrast to syncytial trophoblasts of intact term placentae, these cells did not stain for hCG, human placental lactogen, pregnancy-specific α1-glycoprotein or low mol wt cytokeratins by immunoperoxidase methods. Endothelial cells, fibroblasts, or macrophages did not contaminate the purified cytotrophoblasts, as evidenced by the lack of immunoperoxidase staining with antibodies against vimentin or α1-antichymotrypsin. The cells produced progesterone (1 ng/106 cells-4 h), and progesterone synthesis was stimulated up to 8- fold in the presence of 25-hydroxycholesterol (20 μg/ml). They also produced estrogens (1360 pg/106 cells-4 h) when supplied with androstenedione (1 ng/ml) as a precursor. When placed in culture, the cytotrophoblasts consistently formed aggregates, which subsequently transformed into syncytia within 24–48 h after plating. Time lapse cinematography revealed that this process occurred by cell fusion. The presumptive syncytial groups were proven to be true syncytia by microinjection of fluorescently labeled y9-actinin, which diffused completely throughout the syncytial cytoplasm within 30 min. Immunoperoxidase staining of cultured trophoblasts between 3.5 and 72 h after plating revealed a progressive increase in cytoplasmic pregnancy-specific β1-glycoprotein, hCG, and human placental lactogen concomitant with increasing numbers of aggregates and syncytia. At all time points examined, occasional single cells positive for these markers were identified. RIA of the spent culture media for hCG revealed a significant increase in secreted hCG, paralleling the increase in hCG-positive cells and syncytia identified by immunoperoxidase methods. We conclude that human cytotrophoblasts differentiate in culture and fuse to form functional syncytiotrophoblasts. {Endocrinology118:1567–1582,1986)
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