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被单克隆抗体识别的蜕膜细胞特异性表面抗原:组织和物种分布

Decidual cell-specific surface antigen(s) recognized by monoclonal antibodies: tissue and species distribution.

作者信息

Kearns M, Parhar R S, Lala P K

出版信息

J Immunol. 1985 Aug;135(2):1046-52.

PMID:2409134
Abstract

Decidual cells are direct descendants of endometrial stromal cells and the ultimate progeny of bone marrow-derived precursors. In view of their bone marrow genealogy and demonstrated immunoregulatory role during pregnancy, this study attempted to identify a lineage-specific differentiation marker(s) on murine decidual cells with the hope of tracing their developmental pathway and exploring their familial relationship to other lymphomyeloid cells. Two protein A-binding, IgG2b isotype monoclonal antibodies (secreted by clones 16F12 and 2G4F8) were raised by immunizing virgin CBA mice with syngeneic decidual cells. The presence and the density of the antigenic marker(s) recognized by these antibodies were examined by radioautography on various cell types in single cell suspensions of the decidua, placenta, and lymphomyeloid organs after a sandwich labeling with hybridoma supernatants followed by 125I-protein A. Both antibodies appeared to recognize antigen(s) unique for the decidual cell lineage in mice, humans, and rats. The incidence of antigen-bearing decidual cells increased with gestational age in CBA, C3H, and CD1 mice between days 8 and 14, and in humans between 6 and 10.5 wk; in rats, however, some decline was noted between days 8 and 14. The binding was always higher with 16F12 than with 2G4F8 supernatants. No significant binding of either antibody to trophoblast cells of the placenta or leukocytes within the decidua was noted in any of the above mouse strains or species. Little or no labeling of any cell type was seen on lymphomyeloid cells of the virgin or pregnant CBA mice, but a consistent labeling of a rare blast-type cell in the blood was observed with both antibodies, raising the possibility that this cell may represent the circulating precursor of the decidual cell lineage. It remains to be investigated whether these antibodies are recognizing the same or different differentiation antigen(s) on the decidual cells, and whether a conservation of this antigen(s) during speciation signifies its functional importance.

摘要

蜕膜细胞是子宫内膜基质细胞的直接后代,也是骨髓衍生前体细胞的最终子代。鉴于其骨髓谱系以及在妊娠期间所表现出的免疫调节作用,本研究试图在小鼠蜕膜细胞上鉴定一种谱系特异性分化标志物,以期追踪其发育途径并探究其与其他淋巴髓样细胞的家族关系。通过用同基因蜕膜细胞免疫未交配的CBA小鼠,产生了两种与蛋白A结合的IgG2b同种型单克隆抗体(由克隆16F12和2G4F8分泌)。在用杂交瘤上清液进行夹心标记,随后用125I-蛋白A处理后,通过放射自显影检查蜕膜、胎盘和淋巴髓样器官单细胞悬液中各种细胞类型上这些抗体所识别的抗原标志物的存在情况和密度。两种抗体似乎都能识别小鼠、人类和大鼠蜕膜细胞谱系特有的抗原。在CBA、C3H和CD1小鼠中,8至14天之间以及人类6至10.5周之间,带有抗原的蜕膜细胞的发生率随胎龄增加;然而,在大鼠中,8至14天之间观察到一些下降。16F12的结合总是比2G4F8上清液的结合更高。在上述任何小鼠品系或物种中,均未观察到两种抗体与胎盘滋养层细胞或蜕膜内白细胞有明显结合。在未交配或怀孕的CBA小鼠的淋巴髓样细胞上几乎没有或没有观察到任何细胞类型的标记,但两种抗体均观察到血液中一种罕见的原始型细胞有一致的标记,这增加了这种细胞可能代表蜕膜细胞谱系循环前体的可能性。这些抗体是否识别蜕膜细胞上相同或不同的分化抗原,以及这种抗原在物种形成过程中的保守性是否表明其功能重要性,仍有待研究。

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