Hobisch A, Ramoner R, Fuchs D, Godoy-Tundidor S, Bartsch G, Klocker H, Culig Z
Department of Urology, University of Innsbruck, Innsbruck A-6020, Austria.
Clin Cancer Res. 2001 Sep;7(9):2941-8.
The levels of interleukin-6 (IL-6) are frequently elevated in sera from patients with advanced prostate carcinoma. Our main objective was to investigate changes in responsiveness to IL-6 and/or androgen that occur in LNCaP cells after long-term treatment with IL-6. This in vitro model could be of clinical relevance because of its similarity with late-stage prostate carcinoma.
LNCaP human prostate cancer cells were treated with IL-6 at a concentration of 5 ng/ml. After 20 passages, the new subline LNCaP-IL-6+ has been established. Passages 20-40 are referred to as low passages (LP) and passages 41-73 as high passages (HP). LNCaP cells passaged at the same time in the absence of IL-6 were used as controls (LNCaP-IL-6-). Cells were counted after treatment with either IL-6 or the synthetic androgen methyltrienolone (R1881), and cell cycle analysis was performed. Binding of IL-6 or R1881 was assessed by radioligand binding assays. Reporter gene activity was measured by chloramphenicol acetyltransferase assay. Prostate-specific antigen in LNCaP-IL-6+ supernatants was measured by an enzyme immunoassay. Expression of IL-6 mRNA and protein was assessed by reverse transcription-PCR and ELISA, respectively.
The basal proliferation rate in HP LNCaP-IL-6+ cells was higher than that in LNCaP-IL-6- cells. IL-6 inhibited proliferation of LNCaP-IL-6- cells but not that of either LP or HP of LNCaP-IL-6+ cells. This inability to elicit a growth-inhibitory response was associated with lack of effect on cell cycle distribution in the LNCaP-IL-6+ subline. In parallel, IL-6 binding decreased gradually during long-term IL-6 treatment and, in HP, reached only 33% of the levels measured in controls. Binding of radiolabeled androgen increased 2-fold in HP LNCaP-IL-6+ cells. Reporter gene assays revealed that R1881, at nanomolar concentrations, was a more potent androgen receptor activator in LNCaP-IL-6+ than in LNCaP-IL-6- cells. However, androgen- and IL-6-induced prostate-specific antigen secretion decreased in long-term IL-6-treated cells. IL-6 cDNA fragments were detected by reverse transcription-PCR in HP LNCaP-IL-6+ cells but not in controls or LP. IL-6 protein was first detected in passage 36 of LNCaP-IL-6+ cells, and it increased in HP.
Long-term treatment of LNCaP human prostate cancer cells with IL-6 leads to abolishment of inhibitory growth response. In contrast to control cells, the LNCaP-IL-6+ subline expresses IL-6 mRNA and protein.
晚期前列腺癌患者血清中白细胞介素-6(IL-6)水平常升高。我们的主要目的是研究长期用IL-6处理后LNCaP细胞中对IL-6和/或雄激素反应性的变化。这个体外模型因其与晚期前列腺癌的相似性而可能具有临床相关性。
用浓度为5 ng/ml的IL-6处理LNCaP人前列腺癌细胞。传代20次后,建立了新的亚系LNCaP-IL-6+。第20 - 40代称为低代(LP),第41 - 73代称为高代(HP)。同时在无IL-6条件下传代的LNCaP细胞用作对照(LNCaP-IL-6-)。用IL-6或合成雄激素甲基三烯olone(R1881)处理细胞后进行细胞计数,并进行细胞周期分析。通过放射性配体结合试验评估IL-6或R1881的结合。通过氯霉素乙酰转移酶试验测量报告基因活性。用酶免疫测定法测量LNCaP-IL-6+上清液中的前列腺特异性抗原。分别通过逆转录PCR和ELISA评估IL-6 mRNA和蛋白的表达。
HP LNCaP-IL-6+细胞的基础增殖率高于LNCaP-IL-6-细胞。IL-6抑制LNCaP-IL-6-细胞的增殖,但不抑制LNCaP-IL-6+细胞的LP或HP代细胞的增殖。这种无法引发生长抑制反应与对LNCaP-IL-6+亚系细胞周期分布无影响有关。同时,在长期IL-6处理期间,IL-6结合逐渐减少,在HP代时仅达到对照中测量水平的33%。放射性标记雄激素在HP LNCaP-IL-6+细胞中的结合增加了2倍。报告基因试验显示,在纳摩尔浓度下,R1881在LNCaP-IL-6+细胞中比在LNCaP-IL-6-细胞中是更有效的雄激素受体激活剂。然而,在长期用IL-6处理的细胞中,雄激素和IL-6诱导的前列腺特异性抗原分泌减少。通过逆转录PCR在HP LNCaP-IL-6+细胞中检测到IL-6 cDNA片段,但在对照或LP代细胞中未检测到。在LNCaP-IL-6+细胞的第36代首次检测到IL-6蛋白,并且在HP代中增加。
用IL-6长期处理LNCaP人前列腺癌细胞导致抑制性生长反应消失。与对照细胞相比,LNCaP-IL-6+亚系表达IL-6 mRNA和蛋白。
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