Tumor Targeting via siRNA-COG3 to Suppress Tumor Progression in Mice and Inhibit Cancer Metastasis and Angiogenesis in Ovarian Cancer Cell Lines.

Janat Ijabi, Roghayeh Ijabi, Parisa Roozehdar, Zachary A Kaminsky, Hemen Moradi-Sardareh, Najmeh Tehranian, Naveed Ahmed
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Abstract

Background: The COG complex is implicated in the tethering of retrograde intra-Golgi vesicles, which involves vesicular tethering and SNAREs. SNARE complexes mediate the invasion and metastasis of cancer cells through MMPs which activate growth factors for ECM fragments by binding to integrin receptors. Increasing MMPs is in line with YKL40 since YKL40 is linked to promoting angiogenesis through VEGF and can increase ovarian cancer (OC) resistance to chemotropic and cell migration.

Objective: The aim of this study is an assessment of siRNA-COG3 on proliferation, invasion, and apoptosis of OC cells. In addition, siRNA-COG3 may prevent the growth of OC cancer in mice with tumors.

Methods: Primary OC cell lines will be treated with siRNA-COG3 to assay YKL40 and identified angiogenesis by Tube-like structure formation in HOMECs. The Golgi morphology was analyzed using Immunofluorescence microscopy. Furthermore, the effects of siRNA-COG3 on the proliferation and apoptosis of cells were evaluated using MTT and TUNEL assays. Clones of the HOSEpiC OC cell line were subcutaneously implanted in FVB/N mice. Mice were treated after two weeks of injection of cells using siRNA-COG3. Tumor development suppression was detected by D-luciferin. RT-PCR and western blotting analyses were applied to determine COG3, MT1- MMP, SNAP23, and YKL40 expression to investigate the effects of COG3 gene knockdown.

Results: siRNA-COG3 exhibited a substantial effect in suppressing tumor growth in mice. It dramatically reduced OC cell proliferation and triggered apoptosis (all p < 0.01). Inhibition of COG3, YKL-40, and MT1-MPP led to suppression of angiogenesis and reduction of microvessel density through SNAP23 in OC cells.

Conclusion: Overall, by knockdown of the COG3 gene, MT1-MMP and YKL40 were dropped, leading to suppressed angiogenesis along with decreasing migration and proliferation. SiRNACOG3 may be an ideal agent to consider for clinical trial assessment therapy for OC, especially when an antiangiogenic SNAR-pathway targeting drug.

通过 siRNA-COG3 靶向肿瘤,抑制小鼠肿瘤进展并抑制卵巢癌细胞系的癌症转移和血管生成
背景:COG复合体参与了高尔基体内囊泡的逆行拴系,其中涉及囊泡拴系和SNARE。SNARE复合物通过MMPs介导癌细胞的侵袭和转移,MMPs通过与整合素受体结合激活ECM碎片的生长因子。增加 MMPs 与 YKL40 相符,因为 YKL40 与通过血管内皮生长因子促进血管生成有关,可增加卵巢癌(OC)对趋化因子和细胞迁移的抵抗力:本研究旨在评估 siRNA-COG3 对 OC 细胞增殖、侵袭和凋亡的影响。此外,siRNA-COG3 还能阻止肿瘤小鼠中 OC 癌细胞的生长:方法:用 siRNA-COG3 处理原代 OC 细胞系,以检测 YKL40,并通过 HOMECs 中管状结构的形成确定血管生成。使用免疫荧光显微镜分析高尔基体的形态。此外,还使用 MTT 和 TUNEL 检测法评估了 siRNA-COG3 对细胞增殖和凋亡的影响。HOSEpiC OC 细胞系克隆被皮下植入 FVB/N 小鼠体内。注射细胞两周后,用 siRNA-COG3 处理小鼠。用D-荧光素检测肿瘤发生抑制情况。结果:siRNA-COG3 在抑制小鼠肿瘤生长方面有显著效果。结果表明:siRNA-COG3 在抑制小鼠肿瘤生长方面有显著效果,它能显著减少 OC 细胞增殖并引发细胞凋亡(均 p < 0.01)。抑制 COG3、YKL-40 和 MT1-MPP 可通过 SNAP23 抑制 OC 细胞的血管生成并降低微血管密度:总之,通过敲除 COG3 基因,MT1-MMP 和 YKL40 的作用减弱,从而抑制了血管生成,同时降低了迁移和增殖。SiRNA-COG3可能是临床试验评估治疗OC的理想药物,尤其是抗血管生成SNAR通路靶向药物。
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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