In vitro study of the expression of autophagy genes ATG101, mTOR and AMPK in breast cancer with treatment of lactoferrin and in silico study of their communication networks and protein interactions

IF 4.3 3区 材料科学 Q1 ENGINEERING, ELECTRICAL & ELECTRONIC
Atefeh Mashhadi Kholerdi , Fatemeh Moradian , Havva Mehralitabar
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Abstract

Autophagy is a new window of science that has been noticed due to the importance of specific therapies in cancer. In this study, the effect of lactoferrin (Lf) on the expression level of ATG101, mTOR and AMPK genes in breast cancer cell line MCF7, as well as the interaction between lactoferrin protein and their protein were investigated. The expression level of the genes was measured using a real-time PCR method. PDB, UniProt, KEGG, and STRING databases and ClusPro webserver and PyMol software were used in silico study. The results showed that the expression level of the ATG101 gene in treatment with concentrations of 100, 400, 600, and 800 μg/ml Lf decreased by 0.05, 0.13, 0.54 and 0.77, respectively. The expression level of the mTOR gene in treatment with concentrations of 100, 400, 600, and 800 μg/ml Lf decreased by 0.07, 0.05, 0.13, and 0.49 times respectively. The level of the AMPK gene expression in treatment with concentrations of 100, 400, 600, and 800 μg/ml Lf decreased by 0.05, 0.01, 0.06, and 0.03, respectively. Virtualization of the interaction of Lf protein with ATG101, mTOR and AMPK proteins by Pymol software showed that the N lobe region of Lf interacted with the HORMA domain of ATG101 protein, the fat domain of mTOR protein, and the CTD domain of AMPK protein. Although Lf was not able to increase the expression of autophagy-inducing genes, it may be able to induce autophagy through protein interaction by activating or inhibiting proteins related to autophagy regulation.

体外研究乳铁蛋白治疗乳腺癌时自噬基因 ATG101、mTOR 和 AMPK 的表达情况,并对它们的通讯网络和蛋白质相互作用进行硅学研究。
自噬是一扇新的科学之窗,因其在癌症特定疗法中的重要性而备受关注。本研究探讨了乳铁蛋白(Lf)对乳腺癌细胞株 MCF7 中 ATG101、mTOR 和 AMPK 基因表达水平的影响,以及乳铁蛋白与这些基因之间的相互作用。这些基因的表达水平是通过实时 PCR 方法测定的。研究中使用了 PDB、UniProt、KEGG 和 STRING 数据库以及 ClusPro 网络服务器和 PyMol 软件。结果表明,浓度为 100、400、600 和 800 μg/ml 的 Lf 处理后,ATG101 基因的表达水平分别下降了 0.05、0.13、0.54 和 0.77。在 100、400、600 和 800 μg/ml Lf 浓度下,mTOR 基因的表达水平分别下降了 0.07、0.05、0.13 和 0.49 倍。100、400、600 和 800 μg/ml Lf 浓度处理的 AMPK 基因表达水平分别下降了 0.05、0.01、0.06 和 0.03 倍。Pymol软件对Lf蛋白与ATG101蛋白、mTOR蛋白和AMPK蛋白相互作用的虚拟分析表明,Lf的N叶区与ATG101蛋白的HORMA结构域、mTOR蛋白的脂肪结构域和AMPK蛋白的CTD结构域相互作用。虽然Lf不能增加自噬诱导基因的表达,但它可能通过蛋白相互作用,激活或抑制与自噬调控相关的蛋白,从而诱导自噬。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
CiteScore
7.20
自引率
4.30%
发文量
567
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