The antimicrobial peptide gramicidin S alters proliferation and inhibits adhesion of L929 cell line fibroblasts

49 Pub Date : 2023-08-11 DOI:10.26565/2075-3810-2023-49-04

N. M. Alabedalkarim, V. P. Berest, N. M. Moiseieva, G. Bozhok, T. P. Bondarenko

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Abstract

Background: Natural antimicrobial peptides are used in the fight against pathogens resistant to existing synthetic antibiotics. The non-specific mechanism of cytostatic action of antimicrobial peptides, in particular gramicidin S, against bacteria is also effective for damaging the cells of neoplasms. The existence of such a property in a registered antibiotic will indicate its antineoplastic potential and can be used to expand the spectrum of its therapeutic application. Aim of work is to clarify the possible antitumor effect of the antimicrobial peptide gramicidin S. Materials and Methods: Using the methods of confocal laser microscopy and light microscopy, the morphological and functional features of connective tissue cells under the influence of gramicidin S in the concentration range 0.5–50 μg/ml were studied using L929 fibroblasts cell culture. The cell area, nucleus area, and nucleus-to-cytoplasm ratio were determined. To study the migratory and proliferative activity of cells in vitro, the “scratch assay” was used, the confluency of the monolayer of cells was evaluated, morphometric studies were performed, and the relative area of the scratch was measured after 24, 48, and 72 hours. Results: The lytic effect of gramicidin S in a concentration of 50 μg/ml on L929 cells was established, in concentrations of 0.5 μg/ml and 5.0 μg/ml, the antibiotic increases the synthetic activity of cells and stimulates the proliferation of fibroblasts in a monolayer. Cell anisomorphism is more pronounced in the presence of 5.0 μg/ml gramicidin S added to the culturing medium during monolayer formation, while a one-third of the cells in the sample form a population that is morphologically different from other cells in the culture. The addition of gramicidin S at non-lytic concentrations of 0.5 and 5.0 μg/ml to unattached fibroblasts reliably inhibits monolayer formation. Under the influence of 5.0 μg/ml gramicidin S, the rate of monolayer formation is low, even despite the significant content of cells with a high nuclear-cytoplasmic ratio. The kinetics of filling the cell monolayer defect using the “scratch assay” shows that GS in concentrations of 0.5 and 5.0 μg/ml can control the migratory and proliferative properties of L929 cells. Conclusions: The effect of gramicidin S on the morphometric parameters of cells depends on the concentration of the peptide and the cell status in the culture. GS corrupts the adhesive properties of L929 fibroblasts in monolayer cell culture and the rate of cell monolayer formation. Cells at the stage of attachment and monolayer formation were most sensitive to non-lytic concentrations of GS. Inhibition of the adhesive properties of connective tissue cells by gramicidin S is a new non-canonical effect of a known antimicrobial drug, which may indicate the possibility of using gramicidin S as an anti-neoplasm agent.

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抗菌肽格拉西汀 S 可改变 L929 细胞系成纤维细胞的增殖并抑制其粘附性

背景：天然抗菌肽被用于对抗对现有合成抗生素具有抗药性的病原体。抗菌肽（特别是γ-蓟素 S）对细菌的非特异性细胞抑制作用机制也能有效地破坏肿瘤细胞。注册抗生素中存在这种特性将表明其具有抗肿瘤潜力，可用于扩大其治疗应用范围。这项工作的目的是阐明抗菌肽格拉西汀 S 可能具有的抗肿瘤作用：采用激光共聚焦显微镜和光学显微镜的方法，以 L929 成纤维细胞为研究对象，研究了浓度为 0.5-50 μg/ml 的皂苷 S 影响下结缔组织细胞的形态和功能特征。测定了细胞面积、细胞核面积和细胞核与细胞质的比例。为了研究细胞在体外的迁移和增殖活性，使用了 "划痕试验"，评估了单层细胞的汇合度，进行了形态计量学研究，并在 24、48 和 72 小时后测量了划痕的相对面积。结果浓度为 50 μg/ml 的桔皮素 S 对 L929 细胞有溶解作用，浓度为 0.5 μg/ml 和 5.0 μg/ml 的抗生素能提高细胞的合成活性，刺激单层成纤维细胞的增殖。在单层细胞形成过程中，如果在培养基中加入 5.0 μg/ml 的霉素 S，细胞的异形性会更加明显，同时样本中三分之一的细胞会形成与培养物中其他细胞形态不同的细胞群。在未附着的成纤维细胞中加入非溶解浓度为 0.5 和 5.0 μg/ml 的桔皮素 S 可有效抑制单层细胞的形成。在 5.0 μg/ml 革兰氏染色素 S 的影响下，单层形成率很低，即使细胞中含有大量核-胞质比很高的细胞。利用 "划痕试验 "填补细胞单层缺陷的动力学表明，浓度为 0.5 和 5.0 μg/ml 的 GS 可控制 L929 细胞的迁移和增殖特性。结论霉素 S 对细胞形态参数的影响取决于肽的浓度和细胞在培养过程中的状态。GS 会破坏单层细胞培养中 L929 成纤维细胞的粘附特性和细胞单层形成率。处于附着和单层形成阶段的细胞对非溶解浓度的 GS 最为敏感。革兰氏阴性菌素 S 对结缔组织细胞粘附性的抑制作用是一种已知抗菌药物的新的非典型效应，这可能预示着将革兰氏阴性菌素 S 用作抗肿瘤药物的可能性。

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