Dzitoyeva Svetlana, Chen Hu, Manev Hari
Department of Psychiatry, Psychiatric Institute, University of Illinois at Chicago, 1601 West Taylor Street, MC912, Chicago, IL 60612, USA.
J Lipids. 2013;2013:864593. doi: 10.1155/2013/864593. Epub 2013 May 25.
Experiments were performed in 3T3-L1 preadipocytes differentiated in vitro into adipocytes. Cells were treated with olanzapine and a 5-lipoxygenase (5-LOX) activating protein (FLAP) inhibitor MK-886. Lipid content was measured using an Oil Red O assay; 5-LOX and FLAP mRNA content was measured using quantitative real-time PCR; the corresponding protein contents were measured using quantitative Western blot assay. Olanzapine did not affect the cell content of 5-LOX mRNA and protein; it decreased FLAP mRNA and protein content at day five but not 24 hours after olanzapine addition. In the absence of MK-886, low concentrations of olanzapine increased lipid content only slightly, whereas a 56% increase was induced by 50 μ M olanzapine. A 5-day cotreatment with 10 μ M MK-886 potentiated the lipid increasing action of low concentrations of olanzapine. In contrast, in the presence of 50 μ M olanzapine nanomolar and low micromolar concentrations of MK-886 reduced lipid content. These data suggest that FLAP system in adipocytes is affected by olanzapine and that it may modify how these cells respond to the second-generation antipsychotic drugs (SGADs). Clinical studies could evaluate whether the FLAP/5-LOX system could play a role in setting a variable individual susceptibility to the metabolic side effects of SGADs.
实验在体外分化为脂肪细胞的3T3-L1前脂肪细胞中进行。细胞用奥氮平和5-脂氧合酶(5-LOX)激活蛋白(FLAP)抑制剂MK-886处理。使用油红O测定法测量脂质含量;使用定量实时PCR测量5-LOX和FLAP mRNA含量;使用定量蛋白质免疫印迹测定法测量相应的蛋白质含量。奥氮平不影响5-LOX mRNA和蛋白质的细胞含量;在添加奥氮平后第5天它降低了FLAP mRNA和蛋白质含量,但在24小时时未降低。在不存在MK-886的情况下,低浓度奥氮平仅轻微增加脂质含量,而50 μM奥氮平诱导脂质含量增加56%。与10 μM MK-886共同处理5天增强了低浓度奥氮平增加脂质的作用。相反,在存在50 μM奥氮平的情况下,纳摩尔和低微摩尔浓度的MK-886降低了脂质含量。这些数据表明脂肪细胞中的FLAP系统受奥氮平影响,并且它可能改变这些细胞对第二代抗精神病药物(SGADs)的反应方式。临床研究可以评估FLAP/5-LOX系统是否可能在设定个体对SGADs代谢副作用的可变易感性中起作用。
