MicroRNA-320–3p promotes the progression of acute pancreatitis by blocking DNMT3a-mediated MMP8 methylation in a targeted manner

MicroRNA-320–3p promotes the progression of acute pancreatitis by blocking DNMT3a-mediated MMP8 methylation in a targeted manner

In this research, we screened out two genes upregulated in mice with acute pancreatitis (AP) by gene sequencing: microRNA (miR)-320–3p and matrix metalloprotease 8 (MMP8). This study was designed to determine whether miR-320–3p and MMP8 participate in AP development and explore the mechanisms, with...

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Veröffentlicht in:Molecular immunology 2022-11, Vol.151, p.84-94
Hauptverfasser: Gu, Huan, Peng, Jie, Wang, Meng, Guo, Zimeng, Huang, Haosu, Yan, Lu
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Acute pancreatitis
DNA methylation
DNA methyltransferase 3a
Matrix metalloprotease 8
MicroRNA-320–3p
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creator Gu, Huan
Peng, Jie
Wang, Meng
Guo, Zimeng
Huang, Haosu
Yan, Lu
description In this research, we screened out two genes upregulated in mice with acute pancreatitis (AP) by gene sequencing: microRNA (miR)-320–3p and matrix metalloprotease 8 (MMP8). This study was designed to determine whether miR-320–3p and MMP8 participate in AP development and explore the mechanisms, with a new idea for clinical diagnosis and treatment of AP. Expression of miR-320–3p, DNA methyltransferase 3a (DNMT3a), and MMP8 in mouse pancreatic tissues and AR42J cells was tested by RT-qPCR and western blot assays. Pancreatic pathological changes, serum amylase and lipase, and inflammatory factors in mouse serum and cell supernatant were measured by hematoxylin-eosin staining, automation analyzer, and enzyme-linked immunosorbent assay, respectively. Cell proliferation and apoptosis were determined by CCK-8 assay and flow cytometry. The interaction between miR-320–3p, DNMT3a, and MMP8 was verified by luciferase activity assay, ChIP-qPCR, and MSP assay. High expression of miR-320–3p and MMP8, and low expression of DNMT3a were observed in pancreatic tissues of AP mice and caerulein-induced AP cellular model. Downregulation of miR-320–3p alleviated injury of mouse pancreas, reduced the levels of serum amylase and lipase, and blocked inflammatory factor levels in AP mice. In caerulein-induced AP cellular models, inhibiting miR-320–3p facilitated proliferation and inhibited apoptosis. Upregulation of MMP8 resulted in the opposite results, which could be reversed by simultaneous inhibition of miR-320–3p. miR-320–3p targeted DNMT3a, and downregulating miR-320–3p promoted DNMT3a expression. Moreover, DNMT3a promoted DNA methylation in MMP8 promoter region, thereby inhibiting MMP8 expression in AP mouse and cellular models. This research suggests that miR-320–3p inhibits DNMT3a to reduce MMP8 methylation and increase MMP8 expression, thereby promoting AP progression. •1 Upregulated miR-320–3p and MMP8 are found in AP mice and caerulein-induced AP cells.•2 Inhibition of miR-320–3p and MMP8 alleviates the symptoms of AP.•3 Low expression of DNMT3a is found in AP mice and caerulein-induced AP cell model.•4 miR-320–3p targets DNMT3a.•5. DNMT3a promotes MMP8 methylation and reduces MMP8 expression.
doi_str_mv 10.1016/j.molimm.2022.09.003
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This study was designed to determine whether miR-320–3p and MMP8 participate in AP development and explore the mechanisms, with a new idea for clinical diagnosis and treatment of AP. Expression of miR-320–3p, DNA methyltransferase 3a (DNMT3a), and MMP8 in mouse pancreatic tissues and AR42J cells was tested by RT-qPCR and western blot assays. Pancreatic pathological changes, serum amylase and lipase, and inflammatory factors in mouse serum and cell supernatant were measured by hematoxylin-eosin staining, automation analyzer, and enzyme-linked immunosorbent assay, respectively. Cell proliferation and apoptosis were determined by CCK-8 assay and flow cytometry. The interaction between miR-320–3p, DNMT3a, and MMP8 was verified by luciferase activity assay, ChIP-qPCR, and MSP assay. High expression of miR-320–3p and MMP8, and low expression of DNMT3a were observed in pancreatic tissues of AP mice and caerulein-induced AP cellular model. Downregulation of miR-320–3p alleviated injury of mouse pancreas, reduced the levels of serum amylase and lipase, and blocked inflammatory factor levels in AP mice. In caerulein-induced AP cellular models, inhibiting miR-320–3p facilitated proliferation and inhibited apoptosis. Upregulation of MMP8 resulted in the opposite results, which could be reversed by simultaneous inhibition of miR-320–3p. miR-320–3p targeted DNMT3a, and downregulating miR-320–3p promoted DNMT3a expression. Moreover, DNMT3a promoted DNA methylation in MMP8 promoter region, thereby inhibiting MMP8 expression in AP mouse and cellular models. This research suggests that miR-320–3p inhibits DNMT3a to reduce MMP8 methylation and increase MMP8 expression, thereby promoting AP progression. •1 Upregulated miR-320–3p and MMP8 are found in AP mice and caerulein-induced AP cells.•2 Inhibition of miR-320–3p and MMP8 alleviates the symptoms of AP.•3 Low expression of DNMT3a is found in AP mice and caerulein-induced AP cell model.•4 miR-320–3p targets DNMT3a.•5. 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Downregulation of miR-320–3p alleviated injury of mouse pancreas, reduced the levels of serum amylase and lipase, and blocked inflammatory factor levels in AP mice. In caerulein-induced AP cellular models, inhibiting miR-320–3p facilitated proliferation and inhibited apoptosis. Upregulation of MMP8 resulted in the opposite results, which could be reversed by simultaneous inhibition of miR-320–3p. miR-320–3p targeted DNMT3a, and downregulating miR-320–3p promoted DNMT3a expression. Moreover, DNMT3a promoted DNA methylation in MMP8 promoter region, thereby inhibiting MMP8 expression in AP mouse and cellular models. This research suggests that miR-320–3p inhibits DNMT3a to reduce MMP8 methylation and increase MMP8 expression, thereby promoting AP progression. •1 Upregulated miR-320–3p and MMP8 are found in AP mice and caerulein-induced AP cells.•2 Inhibition of miR-320–3p and MMP8 alleviates the symptoms of AP.•3 Low expression of DNMT3a is found in AP mice and caerulein-induced AP cell model.•4 miR-320–3p targets DNMT3a.•5. 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This study was designed to determine whether miR-320–3p and MMP8 participate in AP development and explore the mechanisms, with a new idea for clinical diagnosis and treatment of AP. Expression of miR-320–3p, DNA methyltransferase 3a (DNMT3a), and MMP8 in mouse pancreatic tissues and AR42J cells was tested by RT-qPCR and western blot assays. Pancreatic pathological changes, serum amylase and lipase, and inflammatory factors in mouse serum and cell supernatant were measured by hematoxylin-eosin staining, automation analyzer, and enzyme-linked immunosorbent assay, respectively. Cell proliferation and apoptosis were determined by CCK-8 assay and flow cytometry. The interaction between miR-320–3p, DNMT3a, and MMP8 was verified by luciferase activity assay, ChIP-qPCR, and MSP assay. High expression of miR-320–3p and MMP8, and low expression of DNMT3a were observed in pancreatic tissues of AP mice and caerulein-induced AP cellular model. Downregulation of miR-320–3p alleviated injury of mouse pancreas, reduced the levels of serum amylase and lipase, and blocked inflammatory factor levels in AP mice. In caerulein-induced AP cellular models, inhibiting miR-320–3p facilitated proliferation and inhibited apoptosis. Upregulation of MMP8 resulted in the opposite results, which could be reversed by simultaneous inhibition of miR-320–3p. miR-320–3p targeted DNMT3a, and downregulating miR-320–3p promoted DNMT3a expression. Moreover, DNMT3a promoted DNA methylation in MMP8 promoter region, thereby inhibiting MMP8 expression in AP mouse and cellular models. This research suggests that miR-320–3p inhibits DNMT3a to reduce MMP8 methylation and increase MMP8 expression, thereby promoting AP progression. •1 Upregulated miR-320–3p and MMP8 are found in AP mice and caerulein-induced AP cells.•2 Inhibition of miR-320–3p and MMP8 alleviates the symptoms of AP.•3 Low expression of DNMT3a is found in AP mice and caerulein-induced AP cell model.•4 miR-320–3p targets DNMT3a.•5. DNMT3a promotes MMP8 methylation and reduces MMP8 expression.</abstract><pub>Elsevier Ltd</pub><doi>10.1016/j.molimm.2022.09.003</doi><tpages>11</tpages></addata></record>
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subjects Acute pancreatitis
DNA methylation
DNA methyltransferase 3a
Matrix metalloprotease 8
MicroRNA-320–3p
title MicroRNA-320–3p promotes the progression of acute pancreatitis by blocking DNMT3a-mediated MMP8 methylation in a targeted manner
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