Studying expression of IL-1β gene under the action of siRNA complexes with anti-influenza effect

E. Pashkov, A. V. Pak, N. Abramova, I. V. Yakovleva, N. Vartanova, E. Bogdanova, E. P. Pashkov, O. Svitich, V. Zverev
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Abstract

Influenza is one of the most urgent global health problems today. The influenza virus has immunosuppressive properties, which can lead to the development of secondary immunodeficiencies, interfering with the functioning of the interferon system activation, thus leading to impaired production of pro-inflammatory cytokines. IL-1 is the most important player in development of antiviral immunity. This cytokine plays an important role in boosting the expression of the MCP-1 and MCP-3 genes and maturation of macrophages and dendritic cells. Induction of IL-1 production occurs due to interaction of the ligand with Toll-like receptors. Currently, there is a lot of drugs aimed at the prevention and treatment of influenza infection. However, their use in some cases is difficult due to high mutational variability of the influenza virus, thus making it resistant to these drugs. Therefore, the issue of developing and creating effective methods to combat such infections is of particular importance. A promising approach to the treatment and prevention of viral respiratory infections may be connected with RNA interference. This process consists of degradation of foreign mRNA by small interfering RNA (siRNA) molecules. The aim of the present study was to evaluate expression of the IL-1 gene upon transfection of miRNA complexes directed to the cellular FLT4, Nup98, Nup205 genes. Evaluation of changed viral reproduction was carried out using titration by CPE virus-containing fluid. Expression level of the IL-1 gene was determined by means of real-time RT-PCR. Assessment of the changes in viral reproduction allowed us to reveal that the use of all the miRNA complexes directed to the cellular genes lead to a significant decrease in viral reproduction on the 1st day after infection. Usage of Nup205 + FLT4 and FLT4 + Nup205 + Nup98 complexes proved to cause a decrease in viral reproduction on the second day as well (p 0.05), as compared with nonspecific and viral controls. When analyzing expression profile of the IL-1 gene, an increase in its expression was observed on the 1st day for all miRNA complexes and on the 2nd and 3rd days for the Nup98 + FLT4 and Nup205 + Nup98 complexes. In the course of the study, it was found that suppression of the cellular genes FLT4, Nup98 and Nup205 activities, which are necessary for viral reproduction, led to a significant decrease in viral activity and an increase in IL-1 expression.
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研究抗流感siRNA复合物作用下IL-1β基因的表达
流感是当今最紧迫的全球卫生问题之一。流感病毒具有免疫抑制特性,可导致继发性免疫缺陷的发展,干扰干扰素系统激活的功能,从而导致促炎细胞因子的产生受损。IL-1在抗病毒免疫的发展中起着至关重要的作用。该细胞因子在促进巨噬细胞和树突状细胞MCP-1和MCP-3基因的表达和成熟中起重要作用。诱导IL-1的产生是由于配体与toll样受体的相互作用。目前,有很多药物旨在预防和治疗流感感染。然而,由于流感病毒的高度突变变异性,在某些情况下很难使用这些药物,从而使其对这些药物产生耐药性。因此,发展和创造有效的方法来对抗这种感染的问题是特别重要的。一种治疗和预防病毒性呼吸道感染的有希望的方法可能与RNA干扰有关。该过程由小干扰RNA (siRNA)分子降解外源mRNA组成。本研究的目的是评估转染指向细胞FLT4、Nup98、Nup205基因的miRNA复合物后IL-1基因的表达。用CPE含病毒液滴定法评价变异病毒的繁殖情况。real-time RT-PCR检测IL-1基因表达水平。对病毒繁殖变化的评估使我们发现,使用所有指向细胞基因的miRNA复合物导致感染后第1天病毒繁殖显著减少。与非特异性和病毒对照相比,Nup205 + FLT4和FLT4 + Nup205 + Nup98复合物的使用在第2天也导致病毒繁殖减少(p 0.05)。在分析IL-1基因的表达谱时,在所有miRNA复合物的第1天,以及Nup98 + FLT4和Nup205 + Nup98复合物的第2天和第3天,IL-1基因的表达均有所增加。在研究过程中发现,抑制病毒繁殖所必需的细胞基因FLT4、Nup98和Nup205的活性,导致病毒活性显著降低,IL-1表达增加。
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