[The influence of Ras-associated binding protein 23 knockdown on the migration and invasion of esophageal squamous cell carcinoma cells and its mechanism].

Q3 Medicine
G Ma, H Liang, R P Zhang, Y Sun
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Immunohistochemistry (IHC) was used to detect the RAB23 protein expressions in 106 pairs of ESCC and adjacent normal tissues, as well as in the lymph glands and primary tumor tissues of 33 patients with positive lymph nodes and 10 patients with negative lymph nodes. Endogenous RAB23 expression was transiently depleted using siRNAs (si-NC, si-RAB23-1, and si-RAB23-9) or stably reduced using shRNAs (sh-NC and sh-RAB23) in ESCC KYSE30 and KYSE150 cells, and the knockdown efficiency was tested using Western blot assays. Cell counting kit-8 assays and mouse xenograft models were used to test the proliferation of ESCC cells<i>.</i> Transwell assays and tail vein-pulmonary metastasis models in immunocompromised mice were used to examine the migration and invasion of ESCC cells. Cell adhesion assays were used to test the adhesion of ESCC cells. RNA-seq assays were used to analyze how RAB23 knockdown influenced the expression profile of ESCC cells and the implicated signal pathways were confirmed using Western blot assays. <b>Results:</b> The RAB23 mRNA expression in 16 cases of ESCC tissues was 0.009 7±0.008 9, which was markedly higher than that in adjacent normal tissues (0.003 2±0.003 7, <i>P</i>=0.006). GEO analysis on RAB23 expressions in ESCC and adjacent normal tissues showed that the RAB23 mRNA level in ESCC tissues (4.30±0.25) was remarkably increased compared with their normal counterparts (4.10±0.17, <i>P=</i>0.037). Among the 106 pairs of ESCC and tumor-adjacent normal tissues, 51 cases exhibited low expression of RAB23 and 55 cases showed high expression of RAB23, whereas in the paired tumor-adjacent normal tissues 82 cases were stained weakly and 24 strongly for RAB23 protein. These results indicated that RAB23 expression was markedly increased in ESCC tissues (<i>P</i><0.001). Additionally, only 1 out of 33 primary ESCC tissues with positive lymph nodes showed low RAB23 protein expression. On the other hand, 7 samples of primary ESCC tissues with negative lymph nodes were stained strongly for RAB23 while its level in the other 3 samples was weak. These results showed that RAB23 expression was remarkably increased in primary ESCC tissues with positive lymph nodes compared with those with negative lymph nodes (<i>P</i>=0.024). Further tests showed that 32 out of 33 positive lymph nodes were stained strongly for RAB23, whereas no negative lymph nodes (<i>n</i>=10) exhibited high expression of RAB23 (<i>P</i><0.001). Both transient and stable knockdown of endogenous RAB23 expression failed to cause detectable changes in the proliferation of KYSE30 cells <i>in vitro</i> and <i>in vivo</i>, but attenuated the migration and invasion of KYSE30 cells as well as the invasion of KYSE150 cells. RAB23 knockdown was found to significantly decrease the number of adhesive KYSE30 cells in the sh-RAB23 group (313.75±89.34) compared with control cells in the sh-NC group (1 030.75±134.29, <i>P</i><0.001). RAB23 knockdown was also found to significantly decrease the number of adhesive KYSE150 cells in the sh-RAB23 group (710.5±31.74) compared with the number of control cells in the sh-NC group (1 005.75±61.09, <i>P</i><0.001). RNA-seq assays demonstrated that RAB23 knockdown using two siRNAs targeting RAB23 mRNA markedly impaired focal adhesion-related signal pathways, and decreased the levels of phosphorylated FAK (p-FAK) and phosphorylated paxillin (p-paxillin) in KYSE30 and KYSE150 cells. <b>Conclusions:</b> Significantly increased RAB23 in ESCC tissues positively correlates with lymph node metastasis. 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引用次数: 0

Abstract

Objective: To investigate the role and the mechanism of Ras-associated binding protein23 (RAB23) in the migration and invasion of esophageal squamous cell carcinoma (ESCC) cells. Methods: RAB23 mRNA levels were measured in 16 pairs of ESCC and adjacent normal tissues via real-time polymerase chain reactions. RAB23 mRNA levels in the ESCC and adjacent normal tissues of dataset GSE20347 deposited in the Gene Expression Omnibus (GEO) database were also analyzed. Immunohistochemistry (IHC) was used to detect the RAB23 protein expressions in 106 pairs of ESCC and adjacent normal tissues, as well as in the lymph glands and primary tumor tissues of 33 patients with positive lymph nodes and 10 patients with negative lymph nodes. Endogenous RAB23 expression was transiently depleted using siRNAs (si-NC, si-RAB23-1, and si-RAB23-9) or stably reduced using shRNAs (sh-NC and sh-RAB23) in ESCC KYSE30 and KYSE150 cells, and the knockdown efficiency was tested using Western blot assays. Cell counting kit-8 assays and mouse xenograft models were used to test the proliferation of ESCC cells. Transwell assays and tail vein-pulmonary metastasis models in immunocompromised mice were used to examine the migration and invasion of ESCC cells. Cell adhesion assays were used to test the adhesion of ESCC cells. RNA-seq assays were used to analyze how RAB23 knockdown influenced the expression profile of ESCC cells and the implicated signal pathways were confirmed using Western blot assays. Results: The RAB23 mRNA expression in 16 cases of ESCC tissues was 0.009 7±0.008 9, which was markedly higher than that in adjacent normal tissues (0.003 2±0.003 7, P=0.006). GEO analysis on RAB23 expressions in ESCC and adjacent normal tissues showed that the RAB23 mRNA level in ESCC tissues (4.30±0.25) was remarkably increased compared with their normal counterparts (4.10±0.17, P=0.037). Among the 106 pairs of ESCC and tumor-adjacent normal tissues, 51 cases exhibited low expression of RAB23 and 55 cases showed high expression of RAB23, whereas in the paired tumor-adjacent normal tissues 82 cases were stained weakly and 24 strongly for RAB23 protein. These results indicated that RAB23 expression was markedly increased in ESCC tissues (P<0.001). Additionally, only 1 out of 33 primary ESCC tissues with positive lymph nodes showed low RAB23 protein expression. On the other hand, 7 samples of primary ESCC tissues with negative lymph nodes were stained strongly for RAB23 while its level in the other 3 samples was weak. These results showed that RAB23 expression was remarkably increased in primary ESCC tissues with positive lymph nodes compared with those with negative lymph nodes (P=0.024). Further tests showed that 32 out of 33 positive lymph nodes were stained strongly for RAB23, whereas no negative lymph nodes (n=10) exhibited high expression of RAB23 (P<0.001). Both transient and stable knockdown of endogenous RAB23 expression failed to cause detectable changes in the proliferation of KYSE30 cells in vitro and in vivo, but attenuated the migration and invasion of KYSE30 cells as well as the invasion of KYSE150 cells. RAB23 knockdown was found to significantly decrease the number of adhesive KYSE30 cells in the sh-RAB23 group (313.75±89.34) compared with control cells in the sh-NC group (1 030.75±134.29, P<0.001). RAB23 knockdown was also found to significantly decrease the number of adhesive KYSE150 cells in the sh-RAB23 group (710.5±31.74) compared with the number of control cells in the sh-NC group (1 005.75±61.09, P<0.001). RNA-seq assays demonstrated that RAB23 knockdown using two siRNAs targeting RAB23 mRNA markedly impaired focal adhesion-related signal pathways, and decreased the levels of phosphorylated FAK (p-FAK) and phosphorylated paxillin (p-paxillin) in KYSE30 and KYSE150 cells. Conclusions: Significantly increased RAB23 in ESCC tissues positively correlates with lymph node metastasis. Depleted RAB23 expression attenuates focal adhesion-related signal pathways, thus impairing the invasion, metastasis, and adhesion of ESCC cells.

[Ras相关结合蛋白23敲除对食管鳞癌细胞迁移和侵袭的影响及其机制]。
研究目的研究 Ras 相关结合蛋白 23(RAB23)在食管鳞状细胞癌(ESCC)细胞迁移和侵袭中的作用及其机制。研究方法通过实时聚合酶链反应测定16对ESCC和邻近正常组织的RAB23 mRNA水平。还分析了基因表达总库(GEO)数据库中数据集 GSE20347 中 ESCC 和邻近正常组织的 RAB23 mRNA 水平。免疫组织化学(IHC)检测了106对ESCC和邻近正常组织以及33例淋巴结阳性患者和10例淋巴结阴性患者的淋巴腺和原发肿瘤组织中的RAB23蛋白表达。在 ESCC KYSE30 和 KYSE150 细胞中使用 siRNA(si-NC、si-RAB23-1 和 si-RAB23-9)瞬时清除内源性 RAB23 表达,或使用 shRNA(sh-NC 和 sh-RAB23)稳定降低内源性 RAB23 表达,并使用 Western 印迹检测敲除效率。细胞计数试剂盒-8测定和小鼠异种移植模型用于检测ESCC细胞的增殖情况。透孔试验和免疫缺陷小鼠尾静脉-肺转移模型用于检测 ESCC 细胞的迁移和侵袭。细胞粘附试验用于检测 ESCC 细胞的粘附性。用 RNA-seq 分析法分析 RAB23 敲除如何影响 ESCC 细胞的表达谱,并用 Western 印迹法确认其中涉及的信号通路。结果16 例 ESCC 组织中 RAB23 mRNA 的表达量为 0.009 7±0.008 9,明显高于邻近正常组织(0.003 2±0.003 7,P=0.006)。GEO分析显示,ESCC组织中RAB23 mRNA水平(4.30±0.25)明显高于正常组织(4.10±0.17,P=0.037)。在106对ESCC和肿瘤相邻正常组织中,51例RAB23低表达,55例RAB23高表达,而在肿瘤相邻正常组织中,82例RAB23蛋白弱染色,24例强染色。这些结果表明,RAB23在ESCC组织中的表达明显增加(PP=0.024)。进一步检测显示,33个阳性淋巴结中有32个被RAB23强染,而没有阴性淋巴结(10个)表现出RAB23的高表达(体外和体内,但减弱了KYSE30细胞的迁移和侵袭以及KYSE150细胞的侵袭。与 sh-NC 组的对照细胞(1 030.75±134.29,PPConclusions)相比,RAB23 敲除组(313.75±89.34)的粘附 KYSE30 细胞数量显著减少:ESCC组织中RAB23的显著增加与淋巴结转移呈正相关。RAB23的表达减少了与病灶粘附相关的信号通路,从而损害了ESCC细胞的侵袭、转移和粘附。
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来源期刊
中华肿瘤杂志
中华肿瘤杂志 Medicine-Medicine (all)
CiteScore
1.40
自引率
0.00%
发文量
10433
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