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鸡骨髓单核细胞系HD-11中25-羟基维生素D3 1-羟化反应的亚细胞定位及部分纯化

Subcellular localization and partial purification of the 25-hydroxyvitamin D3 1-hydroxylation reaction in the chick myelomonocytic cell line HD-11.

作者信息

Shany S, Ren S Y, Arbelle J E, Clemens T L, Adams J S

机构信息

Department of Medicine, Cedars-Sinai Research Institute, University of California Los Angeles School of Medicine.

出版信息

J Bone Miner Res. 1993 Mar;8(3):269-76. doi: 10.1002/jbmr.5650080304.

DOI:10.1002/jbmr.5650080304
PMID:8384398
Abstract

Hypercalcemia in human granuloma-forming diseases like sarcoidosis results from the endogenous overproduction of 1,25-dihydroxyvitamin D [1,25-(OH)2D] by disease-activated tissue macrophages. The recent identification of an immortalized chick myelomonocytic cell line, HD-11, that constitutively expresses a 25-hydroxyvitamin D (25-OHD) 1-hydroxylation reaction has alleviated dependence on studying primary macrophage cultures with no replicative potential in vitro. In these experiments we established conditions for the maximal expression of the HD-11 cell 25-OHD3-1-hydroxylation reaction and localized this activity to the mitochondrial fraction. On a per cell basis, the activity of HD-11 cell 25-OHD3 1-hydroxylation reaction was comparable to that in primary cultures of chick renal tubular epithelial cells, which express the authentic renal 25-OHD3 1-hydroxylase. Maximal product yield was achieved after incubation of HD-11 cells with 200 nM 25-OHD3 for 3 h. Although adherent monolayers possessed 3- to 4-fold more capacity for hormone production than cells in suspension, suspended cells exhibited easily detectable 25-OHD3 catalytic activity (0.58 +/- 0.08 pmol per 10(6) cells per h; +/- SEM), 50% of which remained solubilized in a sonicate of suspended cells cleared of nuclei and plasma membrane. Subcellular localization disclosed 91% of the residual activity to be concentrated in the mitochondrial subfraction. A detergent-solubilized extract of this mitochondrial subfraction contained 1.9 +/- 0.3 pmol 1,25-(OH)2D3 synthetic capacity per mg protein. The catalytic activity (1-hydroxylase activity) was concentrated 20.2-fold after chromatography on octyl-amino agarose and was associated with 0.054 nmol cytochrome P450 per mg protein.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

在结节病等人类肉芽肿形成性疾病中,高钙血症是由疾病激活的组织巨噬细胞内源性过量产生1,25 - 二羟基维生素D [1,25-(OH)2D] 所致。最近鉴定出一种永生化的鸡骨髓单核细胞系HD - 11,其组成性表达25 - 羟基维生素D(25 - OHD)1 - 羟化反应,这减少了对体外无复制潜力的原代巨噬细胞培养物研究的依赖。在这些实验中,我们确定了HD - 11细胞25 - OHD3 - 1 - 羟化反应最大表达的条件,并将该活性定位于线粒体部分。以每个细胞计算,HD - 11细胞25 - OHD3 1 - 羟化反应的活性与鸡肾小管上皮细胞原代培养物中的活性相当,后者表达真正的肾25 - OHD3 1 - 羟化酶。用200 nM 25 - OHD3孵育HD - 11细胞3小时后可实现最大产物产量。尽管贴壁单层细胞产生激素的能力比悬浮细胞高3至4倍,但悬浮细胞仍表现出易于检测到的25 - OHD3催化活性(每10(6)个细胞每小时0.58±0.08 pmol;±SEM),其中50%仍可溶解在去除细胞核和质膜的悬浮细胞超声裂解物中。亚细胞定位显示91%的残余活性集中在线粒体亚组分中。该线粒体亚组分的去污剂溶解提取物每毫克蛋白质含有1.9±0.3 pmol 1,25-(OH)2D3合成能力。在辛基氨基琼脂糖上进行层析后,催化活性(1 - 羟化酶活性)浓缩了20.2倍,并与每毫克蛋白质0.054 nmol细胞色素P450相关。(摘要截断于250字)

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