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细胞表面维生素D结合蛋白(GC球蛋白)源自血浆。

Cell surface vitamin D-binding protein (GC-globulin) is acquired from plasma.

作者信息

Guoth M, Murgia A, Smith R M, Prystowsky M B, Cooke N E, Haddad J G

机构信息

Department of Medicine, University of Pennsylvania School of Medicine, Philadelphia 19104.

出版信息

Endocrinology. 1990 Nov;127(5):2313-21. doi: 10.1210/endo-127-5-2313.

DOI:10.1210/endo-127-5-2313
PMID:2226317
Abstract

Vitamin D-binding protein (DBP) is an abundant plasma protein. The observation of immunodetectable, cell-associated DBP on peripheral blood mononuclear cells and placental cytotrophoblasts had presented the question of the origin, function, and precise subcellular localization of cell-associated DBP. Using anti-human DBP F(ab')2 with fluorescence-activated cytometric analysis and immunogold electron microscopy, we detected DBP on the plasmalemma of U937 cells, a monoblastic, histiocytic cell line grown in media supplemented with fetal calf serum (FCS). DBP was then removed from FCS by actin affinity chromatography followed by anti-DBP immunoaffinity chromatography. U937 cells in this DBP-free medium exhibited nearly identical growth rates to cells grown in medium containing native FCS. However, in contrast to cells grown with native FCS, those grown for seven to eight generations with DBP-free FCS exhibited less cell-surface DBP as quantified by fluorescence-activated cytometric analysis (73% decrease) and immunoelectron microscopy (88% decrease). DBP mRNA could not be detected in U937 cells, placental tissues, freshly prepared resting and stimulated B and T lymphocytes, or lymphocyte-derived cell lines by Northern analysis. In addition, using the sensitive reverse transcriptase/polymerase chain reaction assay no DBP fragments were detectable in U937 cells. We conclude that U937 cell-associated DBP is exogenously derived from plasma and is located on the plasmalemma. Based upon this conclusion, we postulate that specific binding sites for DBP may exist on the plasma membranes of certain cell types.

摘要

维生素D结合蛋白(DBP)是一种丰富的血浆蛋白。在外周血单核细胞和胎盘细胞滋养层细胞上观察到可免疫检测的、与细胞相关的DBP,这就提出了细胞相关DBP的起源、功能和精确亚细胞定位的问题。我们使用抗人DBP F(ab')2进行荧光激活细胞分析和免疫金电子显微镜观察,在U937细胞的质膜上检测到了DBP,U937细胞是一种在添加了胎牛血清(FCS)的培养基中生长的单核细胞、组织细胞系。然后通过肌动蛋白亲和层析继以抗DBP免疫亲和层析从FCS中去除DBP。在这种不含DBP的培养基中培养的U937细胞的生长速率与在含有天然FCS的培养基中培养的细胞几乎相同。然而,与用天然FCS培养的细胞相比,用不含DBP的FCS培养七至八代的细胞,通过荧光激活细胞分析(减少73%)和免疫电子显微镜观察(减少88%)定量显示,其细胞表面DBP较少。通过Northern分析,在U937细胞、胎盘组织、新制备的静息和刺激的B淋巴细胞和T淋巴细胞或淋巴细胞衍生细胞系中均未检测到DBP mRNA。此外,使用灵敏的逆转录酶/聚合酶链反应检测法,在U937细胞中未检测到DBP片段。我们得出结论,U937细胞相关的DBP是外源性来源于血浆,且位于质膜上。基于这一结论,我们推测某些细胞类型的质膜上可能存在DBP的特异性结合位点。

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