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Evaluation of the Influence of Adalimumab on the Expression Profile of Leptin-Related Genes and Proteins in Keratinocytes Treated with Lipopolysaccharide A

机译:用脂多糖A处理瘦蛋白相关基因和蛋白质表达谱的评价

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摘要

Psoriasis is a disease with a proinflammatory base, in which an increased expression of leptin, tumor necrosis factor alpha (TNF-α), interleukin (IL) IL-12/23, IL-6, is observed. A drug used in the treatment of psoriasis of moderate and acute strength is the monoclonal antibody anti-TNF–adalimumab. The goal of this study was to evaluate the influence of adalimumab on changes in the expression profile of leptin-related genes in human keratinocyte cells exposed to lipopolysaccharide A and analyze if adalimumab acts via leptin pathways. The evaluation of changes of the pattern of genes connected with leptin and proteins coded by them was marked in a culture of human keratinocytes (HaCaT) exposed to 1 µg/mL lipopolysaccharide A (LPS) for 8 h in order to induce the inflammatory process, then to 8 µg/mL of adalimumab for 2.8 and 24 h in comparison with the control (cells not treated with the substances). The techniques used were mRNA microarray, Real-Time Quantitative Reverse Transcription Reaction (RTqPCR), Enzyme-Linked Immunosorbent Assay (ELISA), as well as transfections of HaCaT culture with leptin small interfering RNA (siRNA) in order to see whether adalimumab works through pathways dependent on leptin. A statistically lower expression of leptin and its receptors was observed under the influence of the drug, independent of the exposition time of keratinocytes to adalimumab. In the cells transfected with leptin siRNA, a lower concentration of JAK2 and STAT3 proteins was observed, which confirms that adalimumab works through pathways dependent on leptin. Adalimumab has a modulatory effect on the gene expression pattern and the proteins coded by them connected with leptin in keratinocytes treated with LPS in vitro.
机译:牛皮癣是一种患有促炎基质的疾病,其中观察到瘦素,肿瘤坏死因子α(TNF-α),白细胞介素(IL)IL-12/23,IL-6的增加。用于治疗中等和急性强度的牛皮癣的药物是单克隆抗体抗TNF-唑类吸收。本研究的目的是评估Adalimalab对脂多糖细胞中瘦蛋白相关基因表达谱的变化的影响,并分析Adalimalab通过瘦素途径作用。对与它们编码的瘦素和蛋白质相连的基因模式的变化的评估标记为暴露于1μg/ ml脂多糖A(LPS)的人角蛋白细胞(HACAT)的培养物中,以诱导炎症过程,然后与对照(用物质未处理的细胞)相比,达到2.8和24小时的8μg/ ml催留剂。使用的技术是mRNA微阵列,实时定量逆转录反应(RTQPCR),酶联免疫吸附测定(ELISA),以及用瘦素小干扰RNA(siRNA)的HACAT培养物转染,以便看Adalimalab是否通过倾向依赖于瘦素。在药物的影响下,观察到静息表达和其受体的表达,与阿塔洛单细胞的曝光时间无关。在用瘦素siRNA转染的细胞中,观察到较低浓度的JAK2和STAT3蛋白质,这证实了Adalimalab通过依赖于瘦素的途径作用。 Adalimumab对基因表达模式的调节效果和由它们在体外用LPS处理的角质形成细胞中与瘦素连接的蛋白质进行调节效果。

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