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北京大学学报(医学版) ›› 2026, Vol. 58 ›› Issue (3): 616-623. doi: 10.19723/j.issn.1671-167X.2026.03.023

• 论著 • 上一篇    下一篇

LncRNA DANCR调节miR-656/BMPR1A轴对脑胶质瘤细胞恶性行为的影响

王欧洋, 朱鹏磊, 林杰, 吴昊*()   

  1. 温州市人民医院神经外科,浙江温州 325006
  • 收稿日期:2024-04-18 出版日期:2026-06-18 发布日期:2026-03-13
  • 通讯作者: 吴昊
  • 基金资助:
    温州市科技局课题(Y2023462)

Effect of LncRNA DANCR on the immune microenvironment of glioma cells by regulating the miR-656/BMPR1A axis

Ouyang WANG, Penglei ZHU, Jie LIN, Hao WU*()   

  1. Department of Neurosurgery, Wenzhou People' s Hospital, Wenzhou 325006, Zhejiang, China
  • Received:2024-04-18 Online:2026-06-18 Published:2026-03-13
  • Contact: Hao WU
  • Supported by:
    the Wenzhou Science and Technology Bureau in 2023(Y2023462)

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摘要:

目的: 探讨长链非编码RNA(long non-coding RNA,LncRNA)分化拮抗非蛋白编码RNA(differentiation antagonizing non-protein coding RNA,DANCR)调节微小RNA-656(miR-656)/骨形态发生蛋白受体1A(bone morphogenetic protein receptor type 1A,BMPR1A)轴对脑胶质瘤细胞免疫微环境的影响。方法: 实时荧光定量聚合酶链式反应(quantitative real-time polymerase chain reaction,qRT-PCR)检测脑胶质瘤细胞中DANCR、miR-656、BMPR1A的表达水平。通过转染或共转染至U87细胞,分为沉默(short hairpin, sh)-DANCR组、过表达(plasmid cytome galoirus, pc)DNA 3.1DANCR组、阴性对照(negative control, NC)sh组、pcDNA 3.1组、sh-DANCR+miR-656抑制剂组、sh-DANCR+NC抑制剂组、sh-DANCR+pcDNA 3.1 BMPR1A组、sh-DANCR+pcDNA 3.1组,并以未处理的U87细胞为空白组。CCK8检测U87细胞增殖;Transwell实验检测侵袭与迁移;流式细胞仪检测细胞凋亡;qRT-PCR检测细胞中DANCR、miR-656、BMPR1A mRNA表达;DANCR与miR-656靶向关系通过双荧光素酶验证;BMPR1A及免疫逃逸因子[程序性死亡受体1(programmed death-1,PD-1)和程序性死亡配体1(programmed death-ligand 1, PD-L1)]通过Western blot检测。结果: U87、A172、LN229和U251细胞较NHA细胞中DANCR、BMPR1A mRNA表达显著增加,miR-656表达显著降低(P<0.05);与空白组、sh-DANCR组相比,sh-DANCR组U87细胞增殖率,侵袭、迁移数,DANCR、BMPR1A mRNA、BMPR1A、PD-1、PD-L1表达显著降低,凋亡率、miR-656表达显著增加(P<0.05);与pcDNA 3.1组相比,pcDNA 3.1 DANCR组U87细胞增殖率,侵袭、迁移数,DANCR、BMPR1A mRNA、BMPR1A、PD-1、PD-L1表达显著增加,凋亡率、miR-656表达显著降低(P<0.05);与sh-DANCR+NC抑制剂组相比,sh-DANCR+miR-656抑制剂组U87细胞增殖率,侵袭、迁移数,BMPR1A mRNA、BMPR1A、PD-1、PD-L1表达显著增加,凋亡率、miR-656表达显著降低(P<0.05),DANCR表达的差异无统计学意义(P>0.05);与sh-DANCR+pcDNA 3.1组相比,sh-DANCR+pcDNA 3.1 BMPR1A组U87细胞增殖率,侵袭、迁移数,BMPR1A mRNA、BMPR1A、PD-1、PD-L1表达显著增加,凋亡率显著降低(P<0.05),miR-656表达、DANCR表达差异无统计学意义(P>0.05)。DANCR、miR-656具有靶向负调节关系。结论: LncRNA DANCR调节miR-656/BMPR1A轴改善脑胶质瘤细胞免疫微环境,抑制癌细胞恶性行为发展。

关键词: LncRNA DANCR, miR-656/BMPR1A轴, 脑胶质瘤细胞, 免疫微环境, 恶性行为发展

Abstract:

Objective: To investigate the effect of long non-coding RNA (LncRNA) differentiation antagonizing non-protein coding RNA (DANCR) on the immune microenvironment of glioma cells by regulating the miR-656/bone morphogenetic protein receptor type 1A (BMPR1A) axis. Methods: The expression levels of DANCR, miR-656 and BMPR1A in glioma cells were detected by quantitative real-time polymerase chain reaction (qRT-PCR). The U87 cells were transfected or co-transfected to form the following groups: sh-DANCR (transfected with sh-DANCR), overexpression (pcDNA 3.1) DANCR (transfected with pcDNA 3.1 DANCR), NC sh (transfected with negative control sh), pcDNA 3.1 (transfected with pcDNA 3.1 vector), sh-DANCR + miR-656 inhibitor (co-transfected with sh-DANCR and miR-656 inhibitor), sh-DANCR + NC inhibitor (co-transfected with sh-DANCR and NC inhibitor), sh-DANCR + pcDNA 3.1 BMPR1A (co-transfected with sh-DANCR and pcDNA 3.1 BMPR1A), and sh-DANCR + pcDNA 3.1 (co-transfected with sh-DANCR and pcDNA 3.1 BMPR1A). The untreated U87 cells were used as the blank group. The proliferation of U87 cells was detected by CCK-8; invasion and migration were detected by Transwell assay; apoptosis was detected by flow cytometry; the expression of DANCR, miR-656, and BMPR1A mRNA in cells was detected by qRT-PCR; the targeting relationship between DANCR and miR-656 was verified by dual-luciferase; and BMPR1A and immune escape factors [programmed death receptor 1 (PD-1) and programmed death-ligand 1 (PD-L1)] were detected by Western blot. Results: The mRNA expressions of DANCR and BMPR1A in U87, A172, LN229 and U251 cells were significantly increased, while the expression of miR-656 was significantly decreased compared with those in NHA cells (P < 0.05). Compared with the blank group and sh-DANCR group, the proliferation rate, invasion, migration number, DANCR, BMPR1A mRNA, BMPR1A, PD-1, PD-L1 expression of U87 cells in the sh-DANCR group were obviously reduced, while the apoptosis rate and miR-656 expression were obviously increased (P < 0.05). Compared with the pcDNA 3.1 group, the proliferation rate, invasion, migration number, DANCR, BMPR1A mRNA, BMPR1A, PD-1, and PD-L1 expression of U87 cells in the pcDNA 3.1 DANCR group were obviously increased, while the apoptosis rate and miR-656 expression were obviously reduced (P < 0.05). Compared with the sh-DANCR +NC inhibitor group, the proliferation rate, invasion, migration number, BMPR1A mRNA, BMPR1A, PD-1, and PD-L1 expression of U87 cells in the sh-DANCR+miR-656 inhibitor group were obviously increased, and the apoptosis rate and miR-656 expression were obviously reduced (P < 0.05), while the expression of DANCR was not obvious (P>0.05). Compared with the sh-DANCR+pcDNA 3.1 group, the proliferation rate, invasion, migration number, BMPR1A mRNA, BMPR1A, PD-1, and PD-L1 expression of U87 cells in the sh-DANCR+pcDNA 3.1 BMPR1A group obviously increased, and the apoptosis rate obviously decreased (P < 0.05), while here was no statistically obvious difference in miR-656 expression and DANCR expression (P>0.05). DANCR and miR-656 had a targeted negative regulatory relationship. Conclusion: LncRNA DANCR improves the immune microenvironment of glioma cells and inhibits the malignant behavior development of cancer cells by regulating the miR-656/BMPR1A axis.

Key words: LncRNA DANCR, MiR-656/BMPR1A axis, Glioma cells, Immune microenvironment, Malignant behavior development

中图分类号: 

  • R739.41

表1

qRT-PCR引物序列"

Primer name Orientation Sequence(5′ to 3′)
DANCR Forward GCGCCACTATGTAGCGGGTT
Reverse TCAATGGCTTGTGCCTGTAGTT
miR-656 Forward GTCAGAAAATGGAGTAACCTTA
Reverse GTCAGAAAATGGAGTAACCTTA
BMPR1A Forward TAGTTCGCTGAACCAATAAAGG
Reverse GTCAGAAAATGGAGTAACCTTA
β-actin Forward GCTAATATCTATAATC
Reverse GAGGCTATCTTCATAGAT
U6 Forward CTCGCTTCGGCAGCACA
Reverse AACGCTTCACGAATTTGCGT

表2

比较细胞中DANCR、miR-656、BMPR1A mRNA的表达"

Group DANCR miR-656 BMPR1A mRNA
NHA 0.94±0.10 0.92±0.10 1.02±0.11
LN229 1.51±0.16* 0.66±0.07* 1.41±0.15*
U251 1.55±0.16* 0.62±0.07* 1.47±0.15*
A172 1.62±0.17* 0.58±0.06* 1.57±0.16*
U87 2.03±0.21* 0.42±0.05* 2.03±0.21*

表3

各组U87细胞增殖率的变化"

Group Proliferation rate/%
Blank 94.22±4.51
NC sh 94.11±4.49
sh-DANCR 47.52±4.82a,b
pcDNA 3.1 94.24±4.49
pcDNA 3.1 DANCR 125.34±6.85c
sh-DANCR+NC inhibitor 47.67±4.79
sh-DANCR+miR-656 inhibitor 72.14±7.31d
sh-DANCR+pcDNA 3.1 47.72±4.81
sh-DANCR+pcDNA 3.1 BMPR1A 72.54±7.38e

图1

观察U87细胞侵袭变化"

图2

观察U87细胞迁移变化"

表4

U87细胞侵袭、迁移数变化"

Groups Invasion count Migration count
Blank 112.46±11.34 102.61±10.47
NC sh 108.94±11.27 105.81±10.62
sh-DANCR 70.88±7.18a, b 51.46±5.24a, b
pcDNA 3.1 111.74±11.20 104.55±10.53
pcDNA 3.1 DANCR 150.54±15.21c 145.84±14.75c
sh-DANCR+NC inhibitor 71.44±7.21 52.37±5.31
sh-DANCR+miR-656 inhibitor 108.72±11.04d 91.48±9.25d
sh-DANCR+pcDNA 3.1 71.67±7.20 52.53±5.29
sh-DANCR+pcDNA 3.1 BMPR1A 109.34±11.07e 91.66±9.28e

图3

观察U87细胞凋亡变化"

表5

U87细胞各组细胞的凋亡率"

Group Apoptosis rate/%
Blank 12.51±1.28
NC sh 12.63±1.29
sh-DANCR 37.82±3.86a, b
pcDNA 3.1 12.58±1.28
pcDNA 3.1 DANCR 7.67±0.79c
sh-DANCR+NC inhibitor 37.64±3.79
sh-DANCR+miR-656 inhibitor 21.04±2.18d
sh-DANCR+pcDNA 3.1 37.74±3.82
sh-DANCR+pcDNA 3.1 BMPR1A 21.17±2.24e

表6

U87细胞DANCR、miR-656、BMPR1A mRNA表达变化"

Group DANCR miR-656 BMPR1A mRNA
Blank 1.05±0.11 0.98±0.10 0.94±0.10
NC sh 1.06±0.11 1.02±0.11 0.98±0.10
sh-DANCR 0.45±0.05a, b 1.67±0.18a, b 0.55±0.06a, b
pcDNA 3.1 0.97±0.10 0.92±0.10 1.05±0.11
pcDNA 3.1 DANCR 1.55±0.16c 0.57±0.06c 1.72±0.18c
sh-DANCR+NC inhibitor 0.48±0.05 1.64±0.18 0.58±0.06
sh-DANCR+miR-656 inhibitor 0.46±0.05 1.08±0.11d 0.88±0.09d
sh-DANCR+pcDNA 3.1 0.47±0.05 1.62±0.18 0.56±0.06
sh-DANCR+pcDNA 3.1 BMPR1A 0.42±0.05 1.59±0.11 0.83±0.09e

图4

DANCR、miR-656结合位点"

表7

DANCR、miR-656靶向关系"

Group relative luciferase activity
NC mimics+DANCR-WT 1.07±0.11
miR-656 mimics+DANCR-WT 0.62±0.07a
NC mimics+DANCR-MUT 1.03±0.11
miR-656 mimics+DANCR-MUT 1.06±0.11

图5

细胞中BMPR1A、PD-1、PD-L1蛋白表达"

表8

U87细胞BMPR1A、PD-1、PD-L1表达变化"

Groups BMPR1A/β-actin PD-1/β-actin PD-L1/β-actin
Blank 1.24±0.13 0.83±0.09 0.77±0.08
NC sh 1.27±0.13 0.87±0.09 0.71±0.08
sh-DANCR 0.65±0.07a,b 0.41±0.05a,b 0.34±0.04a,b
pcDNA 3.1 1.25±0.13 0.85±0.09 0.75±0.08
pcDNA 3.1 DANCR 1.68±0.17c 1.37±0.14c 1.14±0.12c
sh-DANCR+NC inhibitor 0.68±0.07 0.48±0.05 0.36±0.04
sh-DANCR+miR-656 inhibitor 0.92±0.10d 0.78±0.08d 0.64±0.07d
sh-DANCR+pcDNA 3.1 0.65±0.07 0.46±0.05 0.37±0.04
sh-DANCR+pcDNA 3.1 BMPR1A 0.97±0.10e 0.72±0.08e 0.66±0.07e
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ISSN 1671-167X
CN 11-4691/R
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