Expression of non-coding RNA snord105b in gastric cancer tissues, sera and its effect on proliferation of gastric cancer cells

Zhang Cong; Bai Hanyu; Wang Yaojie; Tian Guo; Liu Dongxin; Dai Suli; Liu Qingwei; Zhao Lianmei; Shan Baoen

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Expression of non-coding RNA snord105b in gastric cancer tissues, sera and its effect on proliferation of gastric cancer cells

VernacularTitle:非编码RNA snord105b在胃癌组织和血清中的表达及其对胃癌细胞增殖能力的影响
Author: ZHANG Cong ¹ ; BAI Hanyu ¹ ; WANG Yaojie ¹ ; TIAN Guo ² ; LIU Dongxin ³ ; DAI Suli ¹ ; LIU Qingwei ⁴ ; ZHAO Lianmei ¹ ; SHAN Baoen ¹
Author Information

1. Research Center, the Fourth Hospital of Hebei Medical University
2. b. Record Room, the Fourth Hospital of Hebei Medical University
3. Clinic Lab, the Health Care Center of Maternal and Child in Xinhua District
4. General Surgery, the Fourth Hospital of Hebei Medical University
Publication Type:Journal Article
Keywords: gastric cancer; non-coding RNA(ncRNA); snord105b; proliferation; biomarker
From: Chinese Journal of Cancer Biotherapy 2019;26(9):993-998
CountryChina
Language:Chinese
Abstract: Objective: To detect the expression of non-coding RNA snord105b in gastric cancer (GC) tissues, sera and cell lines, and its correlation with clinicopathological characteristics of patients with GC as well as its effect on the proliferation of GC cells. Methods: One hundred and twenty pairs of GC tissues and corresponding para-cancerous tissues from patients, who underwent surgery at Department of Surgery, the Fourth Hospital of Hebei Medical University between 2016 and 2017, were collected for this study. The presurgical sera samples from GC patients (n=50) and peripheral venous blood samples from healthy donors (n=30), as well as five gastric cancer cell lines (SGC-7901, AGS, MGC-803, BGC-823, HGC-27) and gastric mucosa normal epithelial GES-1 cells were also obtained. qPCR assay was adopted to detect the expression of snord105b in GC tissues, sera and cell lines. The correlation between snord105b and patients’clinicopathological features was investigated. MTS assay was adopted to detect the effect of snord105b silence or over-expressionon in vitro proliferation of four GC cells. Results: qPCR assay demonstrated that the expression of snord105b in GC tissues, sera and cell lines were significantly higher than that of para-cancerous tissues, sera from healthy donors and GES-1 cells (all P< 0.05). Expression level of snord105b was obviously associated with age,tumor size, differentiation and TNM stages of patients (all P<0.05). MTS assay demonstrated that knockdown of snord105b could suppress the proliferation of GC cells (P< 0.05), while forced-expression of snord105b could promote the proliferation of GC cells (P< 0.05). Conclusion: non-coding RNA snord105b aberrantly expressed in GC tissues, sera, and cells, and its expression was obviously correlated with patients’age, tumor size, differentiation and TNM stages. Snord105b could significantly promote the proliferation of GC cells, which may be used as a potential clinical biomaker for early diagnosis and prognosis of GC.
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