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催乳素通过因肌浆网钙ATP酶2b过度表达而增加内质网含量来刺激前列腺细胞增殖。

Prolactin stimulates prostate cell proliferation by increasing endoplasmic reticulum content due to SERCA 2b over-expression.

作者信息

Crépin Alexandre, Bidaux Gabriel, Vanden-Abeele Fabien, Dewailly Etienne, Goffin Vincent, Prevarskaya Natalia, Slomianny Christian

机构信息

Inserm, U800, Laboratoire de Physiologie Cellulaire, Equipe Labellisée par la Ligue Contre le Cancer, Villeneuve d'Ascq, F-59655 France.

出版信息

Biochem J. 2007 Jan 1;401(1):49-55. doi: 10.1042/BJ20060870.

Abstract

Prolactin (PRL) has been shown to be involved in the differentiation and proliferation of numerous tissues, including the prostate gland. Moreover, variations in [Ca2+]ER (calcium concentration within the endoplasmic reticulum) may play a role in cell growth. However, few studies have focused on the regulation of calcium homoeostasis by prolactin. The present study evaluates the regulation of calcium pools as well as the possible role of [Ca2+]ER variations as a signal for growth modulation by PRL. We show that PRL stimulates the proliferation of normal SV40 immortalized epithelial prostate (PNT1A) cells with a maximum effect at a dose of 100 ng/ml. We also show that 100 ng/ml PRL increases the [Ca2+]ER when measured either by indirect quantification with Fura-2AM after application of 1 mM thapsigargin or by direct quantification with Mag-Fura-2AM within the endoplas-mic reticulum. Western blot analysis shows that the SERCA 2b (sarcoendoplasmic calcium ATPase 2b) is over-expressed in PNT1A cells treated with 100 ng/ml PRL for 24 h. A small inter-fering RNA SERCA 2a/b, used to down-regulate endogenous SERCA 2b expression, reduced both PNT1A cell proliferation and [Ca2+]ER. We thus identify [Ca2+]ER and SERCA 2b as protagonists in PRL-induced proliferation.

摘要

催乳素(PRL)已被证明参与包括前列腺在内的众多组织的分化和增殖。此外,内质网内的钙浓度([Ca2+]ER)变化可能在细胞生长中发挥作用。然而,很少有研究关注催乳素对钙稳态的调节。本研究评估了钙池的调节以及[Ca2+]ER变化作为催乳素调节生长信号的可能作用。我们发现,催乳素能刺激正常SV40永生化前列腺上皮细胞(PNT1A)的增殖,在剂量为100 ng/ml时效果最佳。我们还发现,当通过应用1 mM毒胡萝卜素后用Fura-2AM进行间接定量测量或在内质网内用Mag-Fura-2AM进行直接定量测量时,100 ng/ml的催乳素会增加[Ca2+]ER。蛋白质印迹分析表明,在用100 ng/ml催乳素处理24小时的PNT1A细胞中,肌浆内质网钙ATP酶2b(SERCA 2b)过度表达。一种用于下调内源性SERCA 2b表达的小干扰RNA SERCA 2a/b,降低了PNT1A细胞的增殖和[Ca2+]ER。因此,我们确定[Ca2+]ER和SERCA 2b是催乳素诱导增殖的主要因素。

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