Zoheir Khairy M A, Abd-Rabou Ahmed A, Darwish Ahmed M, Abdelhafez Mohamed A, Mahrous Karima F
Cell Biology Department, Biotechnology Research Institute, National Research Centre, Cairo, Egypt.
Hormones Department, Medical Research and Clinical Studies Institute, National Research Centre, Cairo, Egypt.
Front Oncol. 2022 Oct 5;12:998247. doi: 10.3389/fonc.2022.998247. eCollection 2022.
Liver cancer is the deadliest malignancy among common tumors. It is the top cause of cancer-related deaths in Egypt, and it is characterized by increasing occurrence among the population. The objective of this study was to determine the outcome of pre-treatment of IQGAP1-shRNA on induced mouse hepatocellular carcinoma model and evaluate the potency of this IQGAP1-shRNA plasmid to recover hepatic cancer as a new tool of cancer therapy. Therefore, we will use RNA interference (RNAi) technology to silence IQGAP1 oncogene to completely recover the chemically induced models for hepatic cancer by designing short RNAi specific for IQGAP1 gene in HCC cells and construct new vectors suitable for this purpose. We assigned mice into three groups: the first negative control group (NC) was injected with saline, the second control group was injected with shRNA (shNC), the third positive control group was injected with diethylnitrosamine (DENAA), and the fourth group was treated with the IQGAP1-shRNA prior to its exposure to DENA.
Our results revealed that the treated group with IQGAP1-shRNA with DENA developed very few cases of hepatic cancer when compared with the positive control group. The positive control group exhibited significant increases in the liver function level as well as a decrease in serum albumin levels when compared to both the treated and the negative control groups. The altered levels of the serum α-fetoprotein as well as of the tumor necrosis factor-alpha, and interleukin-4 in DENA-treated mice were significantly ameliorated by IQGAP1-shRNA administration. Flow cytometer analyses have indicated that the silencing of IQGAP1 cannot significantly modulate DENA-induced apoptosis in the circulating blood cells. Moreover, the elevated mRNA expression levels of IQGAP1, IQGAP3, KRas, HRas, interleukin-8, nuclear factor kappa B, caspase-3, caspase-9 and Bcl-2, were significantly decreased by the IQGAP1-shRNA treatment. However, the IQGAP2, DR4, DR5, p53 and BAX genes were found to be significantly up-regulated post-therapy. In agreement with these findings, IQGAP1-shRNA was able to modulate the DENA-induced histological changes in the mice liver which were represented by severe necrosis and hydropic degenerative changes.
Our study revealed that IQGAP1-shRNA was able to preserve hepatocyte integrity and the liver histological architecture through the regulation of the expression of IQGAPs, Ras, TRAILs and IL-8 receptors, as well as of pro-apoptotic and anti-apoptotic genes. Therefore, the silencing of IQGAP1 could be part of a promising therapeutic strategy against hepatic cancer.
肝癌是常见肿瘤中最致命的恶性肿瘤。它是埃及癌症相关死亡的首要原因,且在人群中的发病率呈上升趋势。本研究的目的是确定IQGAP1 - shRNA预处理对诱导型小鼠肝细胞癌模型的影响,并评估该IQGAP1 - shRNA质粒作为一种新的癌症治疗工具在恢复肝癌方面的效力。因此,我们将使用RNA干扰(RNAi)技术,通过设计针对肝癌细胞中IQGAP1基因的短RNAi来沉默IQGAP1癌基因,以完全恢复化学诱导的肝癌模型,并构建适用于此目的的新载体。我们将小鼠分为三组:第一组阴性对照组(NC)注射生理盐水,第二组对照组注射shRNA(shNC),第三组阳性对照组注射二乙基亚硝胺(DENAA),第四组在暴露于二乙基亚硝胺(DENA)之前用IQGAP1 - shRNA进行治疗。
我们的结果显示,与阳性对照组相比,用IQGAP1 - shRNA和DENA治疗的组发生肝癌的病例极少。与治疗组和阴性对照组相比,阳性对照组的肝功能水平显著升高,血清白蛋白水平降低。IQGAP1 - shRNA给药显著改善了DENA处理小鼠血清甲胎蛋白、肿瘤坏死因子 - α和白细胞介素 - 4水平的变化。流式细胞仪分析表明,IQGAP1的沉默不能显著调节循环血细胞中DENA诱导的细胞凋亡。此外,IQGAP1 - shRNA处理显著降低了IQGAP1、IQGAP3、KRas、HRas、白细胞介素 - 8、核因子κB、半胱天冬酶 - 3、半胱天冬酶 - 9和Bcl - 2的mRNA表达水平升高。然而,发现IQGAP2、DR4、DR5、p53和BAX基因在治疗后显著上调。与这些发现一致,IQGAP1 - shRNA能够调节DENA诱导的小鼠肝脏组织学变化,这些变化表现为严重坏死和水样变性改变。
我们的研究表明,IQGAP1 - shRNA能够通过调节IQGAPs、Ras、TRAILs和IL - 8受体以及促凋亡和抗凋亡基因的表达来维持肝细胞完整性和肝脏组织结构。因此,IQGAP1的沉默可能是一种有前景的肝癌治疗策略的一部分。
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