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针对参与前列腺腺癌细胞与成骨细胞旁分泌相互作用的胰岛素样生长因子结合蛋白的蛋白水解活性。

Proteinolytic activity against IGF-binding proteins involved in the paracrine interactions between prostate adenocarcinoma cells and osteoblasts.

作者信息

Koutsilieris M, Polychronakos C

机构信息

Hormonal Bioregulation Laboratory, Research Center, Laval University Hospital Center, (C.H.U.L.), Quebec, Canada.

出版信息

Anticancer Res. 1992 May-Jun;12(3):905-10.

PMID:1377896
Abstract

PA-III rat prostate adenocarcinoma cells are capable of inducing osteoblastic reaction after inoculation onto rat skeleton. In this study PA-III cells and osteoblast-derived rat osteosarcoma cells (UMR 106 cells) were employed to characterize the cellular interactions in the PA-III cell-induced bone tumors, in vitro. Insulin-like growth factor-I (IGF-I) and conditioned media (CM) of UMR 106 cells stimlated tritiated-thymidine incorporation into the DNA of PA-III cells growing in serum-free media. This effect was inhibited by monoclonal anti-hIGF-I antibody. In addition PA-III cell CM contained proteinolytic activity for the IGF-binding proteins of UMR 106 cell CM (IGFBP-1 and -2). This proteinase activity hydrolyzed also benzyloxycarbonyl-lysine thiobenzyl ester (BLT) and its action on IGFBPs and BLT was inhibited by benzamidine and aprotinin. Proteinase activity of PA-III cell CM when bound covalently to tritiated-dilsopropylfluoro-phosphate (DFP) and then analyzed on SDS-PAGE gel electrophoresis, revealed the presence of radioactivity linked with a 35 kDa protein band. This proteinase was eluted in the void volume of the G-50 sephadex column and was retained on and eluted from p-benzamidine affinity column. The 35 kDa proteinase was retained on and was eluted from cartridges of the C18 silica by 80% acetonitrile over 0.1% trifuroacetic acid. This partially purified material hydrolyzed BLT substrate and IGFBPs of UMR 106 cell CM and its effect was inhibited by benzamidine and aprotinin. These data indicate that PA-III cell CM contains a 35 kDa proteinase capable of digesting the IGFBPs and thus increases the bioavailability of osteoblast-derived IGFs. This mechanism may participate in the pathophysiology of the PA-III cell-induced bone tumor and its subsequent osteoblastic reaction.

摘要

PA - III大鼠前列腺腺癌细胞接种到大鼠骨骼后能够诱导成骨反应。在本研究中,使用PA - III细胞和成骨细胞来源的大鼠骨肉瘤细胞(UMR 106细胞)在体外表征PA - III细胞诱导的骨肿瘤中的细胞相互作用。胰岛素样生长因子 - I(IGF - I)和UMR 106细胞的条件培养基(CM)刺激了在无血清培养基中生长的PA - III细胞的DNA掺入氚标记的胸腺嘧啶核苷。这种作用被单克隆抗人IGF - I抗体抑制。此外,PA - III细胞CM对UMR 106细胞CM的IGF结合蛋白(IGFBP - 1和 - 2)具有蛋白水解活性。这种蛋白酶活性也能水解苄氧羰基 - 赖氨酸硫代苄酯(BLT),其对IGFBPs和BLT的作用被苯甲脒和抑肽酶抑制。当PA - III细胞CM与氚标记的二异丙基氟磷酸酯(DFP)共价结合,然后在SDS - PAGE凝胶电泳上进行分析时,蛋白酶活性显示存在与35 kDa蛋白带相关的放射性。这种蛋白酶在G - 50葡聚糖凝胶柱的空体积中被洗脱,并保留在对氨基苯甲脒亲和柱上并从中洗脱。35 kDa蛋白酶保留在C18硅胶柱上,并通过80%乙腈在0.1%三氟乙酸中从柱中洗脱。这种部分纯化的物质水解了UMR 106细胞CM的BLT底物和IGFBPs,其作用被苯甲脒和抑肽酶抑制。这些数据表明,PA - III细胞CM含有一种35 kDa的蛋白酶,能够消化IGFBPs,从而增加成骨细胞来源的IGFs的生物利用度。这种机制可能参与PA - III细胞诱导的骨肿瘤及其随后的成骨反应的病理生理学。

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