6 MiRNAs are critical components of competing endogenous RNA network in cells.
7 Via binding to complementary sites on mRNA 3ʹUTR, miRNAs promote mRNA degradation or inhibit mRNA translation to repress gene expression.
8 Dysregulation of miRNAs results in abnormal expression of target genes and is associated with cancer development.
9 Hundreds of cancer-associated miRNAs have been reported in colorectal cancer.
10,11 For example, miR-193a-3p, which is downregulated in BRAF-mutated colorectal cancers, inhibits colorectal cancer cell proliferation.
12 MiR-4449 is highly expressed in serum from patients with multiple myeloma compared with samples from healthy volunteers.
13 However, the precise function of miR-4449 in colorectal cancer is not known.
[Full text] High Expression of LINC01268 is Positively Associated with Hepatocellu
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[Full text] Regulation of Pancreatic Fibrosis by Acinar Cell-Derived Exosomal miR-
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G) The mRNA and (
H,
I) protein levels of CCND1 were determined by Real-Time qPCR and Western Blot analysis, respectively. (Note: “Con” indicated “Control”, “KD-L” indicated “Knock-down of LncRNA SNHG16” and “KD-L+KD-miR” suggested “both LncRNA SNHG16 and miR-17-5p ablation”). Each experiment repeated at least 3 times, and
P 0.05.
Knock-Down of LncRNA SNHG16 Inhibited OSCC Progression Through the miR-17-5p/CCND1 Axis
We next investigated whether LncRNA SNHG16 regulated OSCC development by targeting the miR-17-5p/CCND1 axis. To achieve this, the LncRNA SNHG16 silencing vectors, miR-17-5p inhibitor and CCND1 overexpression vectors were delivered into OSCC cells (Figure 6A and B), which were divided into four groups, including Control, KD-SNHG16, KD-SNHG16+miR-17-5p inhibitor, and KD-SNHG16+OE-CCND1. As expected, the data in Figure 6C and D showed that knock-down of LncRNA SNHG16 inhibited cell proliferation in OSCC cells, which were restored by silenci