Construction and validation of ceRNA network for pyroptosis-related molecules during the acute phase of traumatic brain injury

doi:10.3877/cma.j.issn.2095-9141.2025.01.002

Abstract

Abstract:

Objective

To explore the temporal expression patterns of genes related to pyroptosis after traumatic brain injury （TBI） and construct a key molecular competitive endogenous RNA （ceRNA）network，providing a new perspective for further studying intervention targets of neuroinflammation during the acute phase of TBI.

Methods

A controlled cortical impact （CCI） mouse model was established，and groups were set up for sham surgery and different time points after TBI，including 0，1，2，3，4，6，12 h and 1，3，7 d post-injury （n=3 per group） for transcriptome sequencing. Mfuzz clustering analysis was used to explore the temporal expression characteristics of pyroptosis-related genes at the transcriptional level after TBI. Messenger RNA （mRNA） and long non-coding RNA （lncRNA） differentially expressed between TBI 12 h group and sham surgery group were screened. Based on bioinformatics methods，a competitive endogenous RNA （ceRNA） network was constructed using the“miRDB”，“Starbase”，and“LncBase v3.0” databases. The expression levels were verified through a single-cell dataset and RT-qPCR，and the direct binding of key molecules was validated using a dual-luciferase reporter assay.

Results

Pyroptosis-related genes exhibited two expression patterns after TBI，which reach their peak expression at 12 h and 3 d after TBI，respectively. Differential analysis between TBI 12 h group surgery and sham group identified 533 differentially expressed mRNA （432 upregulated and 101 downregulated） and 103 differentially expressed lncRNAs （51 upregulated and 52 downregulated），with Caspase-4，interleukin （IL）-1α，IL-1β，and IL-6 emerging as core pyroptosis mRNAs. The constructed ceRNA network comprised 4 lncRNAs （F630028O10Rik，F730311O21Rik，BE692007，and Mir17Hg），16 microRNAs （including mmumiR-466a-3p，etc.），and 4 core pyroptosis mRNAs （Caspase-4，IL-1α，IL-1β，and IL-6）. Single-cell dataset analysis confirmed the high expression of IL-1β during the acute phase of TBI. The dual-luciferase reporter gene assay verified the direct binding of F630028O10Rik/mmu-miR-466a-3p and mmu-miR-466a-3p/IL-1β. The relative luciferase activity of F630028O10Rik-WT and IL-1β-WT decreased by 16.5% and 27.1%，respectively （P＜0.05）.

Conclusion

The pyroptosis genes after TBI are divided into early genes （peak expression at 12 h） and late genes （peak expression at 3 d），which have different functions. A ceRNA network related to pyroptosis at 12 h after TBI was constructed，revealing that the IL-1β and its ceRNA regulatory axis （F630028O10Rik/miR-466a-3p/IL-1β） may play a central role in neuroinflammation during the acute phase （12 h） after TBI，providing new insights into intervention targets for the acute phase after TBI.

Key words: Traumatic brain injury, Neuroinflammation, Pyroptosis, Long non-coding RNA, Competing endogenous RNA

Yulian Zhang, Hanhan Dang, Chuanpeng Zhang, Kun He, Pengyu Chen, Yunsheng Zhang, Zai Wang, Li Zhang, Yanbing Yu. Construction and validation of ceRNA network for pyroptosis-related molecules during the acute phase of traumatic brain injury[J]. Chinese Journal of Neurotraumatic Surgery(Electronic Edition), 2025, 11(01): 5-16.

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Figures/Tables 8

References 24

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基因	引物序列
Caspase-4	F 5^’-GCTGATGCTGTCAAGCTGAG-3^’
	R5^’-GAGCCTCCTGTTTTGTCTCG-3^’
IL-1α	F 5^’-CGTCAAGCAACGGGAAGATT-3^’
	R5^’-ATCTGGGTTGGATGGTCTCTTC-3^’
IL-1β	F 5^’-TGTAATGAAAGACGGCACACC-3^’
	R5^’-TCTTCTTTGGGTATTGCTTGG-3^’
IL-6	F 5^’-GCTACCAAACTGGATATAATCAGGA-3^’
	R5^’-CCAGGTAGCTATGGTACTCCAGAA-3^’
F630028O10Rik	F 5^’-AGCTGAGTTGGACACTCTGTG-3^’
	R5^’-AGGCTATGTGCTCTGTCCTG-3^’
F730311O21Rik	F 5^’-CGCACGGTAACGTTTGGATG-3^’
	R5^’-GGCCAGATGAGTCCGACATT-3^’
Mir17hg	F 5^’-CACAGGTTGGGATTTGTCGC-3^’
	R5^’-GTGGAAATCGGCATCTTCAGC-3^’
BE692007	F 5^’-TGGGCACCGATCCTGACTAT-3^’
	R5^’-TTCTGTTGCTGTAACTGTAGCTT-3^’
GAPDH	F 5^’-AACTTTGGCATTGTGGAAGG-3^’
	R5^’-GGATGCAGGGATGATGTTCT-3^’

基因	引物序列
Caspase-4	F 5^’-GCTGATGCTGTCAAGCTGAG-3^’
	R5^’-GAGCCTCCTGTTTTGTCTCG-3^’
IL-1α	F 5^’-CGTCAAGCAACGGGAAGATT-3^’
	R5^’-ATCTGGGTTGGATGGTCTCTTC-3^’
IL-1β	F 5^’-TGTAATGAAAGACGGCACACC-3^’
	R5^’-TCTTCTTTGGGTATTGCTTGG-3^’
IL-6	F 5^’-GCTACCAAACTGGATATAATCAGGA-3^’
	R5^’-CCAGGTAGCTATGGTACTCCAGAA-3^’
F630028O10Rik	F 5^’-AGCTGAGTTGGACACTCTGTG-3^’
	R5^’-AGGCTATGTGCTCTGTCCTG-3^’
F730311O21Rik	F 5^’-CGCACGGTAACGTTTGGATG-3^’
	R5^’-GGCCAGATGAGTCCGACATT-3^’
Mir17hg	F 5^’-CACAGGTTGGGATTTGTCGC-3^’
	R5^’-GTGGAAATCGGCATCTTCAGC-3^’
BE692007	F 5^’-TGGGCACCGATCCTGACTAT-3^’
	R5^’-TTCTGTTGCTGTAACTGTAGCTT-3^’
GAPDH	F 5^’-AACTTTGGCATTGTGGAAGG-3^’
	R5^’-GGATGCAGGGATGATGTTCT-3^’

基因	假手术组（n=3）	TBI 12 h组（n=3）	t 值	P值
mRNA
Caspase-4	1.023±0.255	13.908±0.836	25.529	＜0.001
IL-1α	1.005±0.121	14.694±0.411	55.283	＜0.001
IL-1β	1.003±0.093	15.420±0.737	33.433	＜0.001
IL-6	1.000±0.027	106.223±9.835	18.530	＜0.001
lncRNA
F630028O10Rik	1.043±0.386	17.655±3.362	8.501	0.001
F730311O21Rik	1.057±0.415	3.100±1.081	3.058	0.038
Mir17hg	1.101±0.256	4.767±1.031	5.793	0.004
BE692007	1.027±0.284	2.061±0.717	2.317	0.081

基因	假手术组（n=3）	TBI 12 h组（n=3）	t 值	P值
mRNA
Caspase-4	1.023±0.255	13.908±0.836	25.529	＜0.001
IL-1α	1.005±0.121	14.694±0.411	55.283	＜0.001
IL-1β	1.003±0.093	15.420±0.737	33.433	＜0.001
IL-6	1.000±0.027	106.223±9.835	18.530	＜0.001
lncRNA
F630028O10Rik	1.043±0.386	17.655±3.362	8.501	0.001
F730311O21Rik	1.057±0.415	3.100±1.081	3.058	0.038
Mir17hg	1.101±0.256	4.767±1.031	5.793	0.004
BE692007	1.027±0.284	2.061±0.717	2.317	0.081

基因	空白对照组（n=3）	LPS模型组（n=3）	t 值	P值
mRNA
Caspase-4	1.004±0.116	8.487±0.880	14.636	＜0.001
IL-1α	1.002±0.083	18.680±1.286	23.800	＜0.001
IL-1β	1.005±0.122	20.129±0.914	35.854	＜0.001
IL-6	1.005±0.123	1113.774±116.101	16.601	＜0.001
lncRNA
F630028O10Rik	0.937±0.173	1.546±0.261	3.364	0.028
F730311O21Rik	1.003±0.091	2.446±0.762	3.266	0.031
Mir17hg	1.000±0.031	1.373±0.213	3.044	0.038
BE692007	1.004±0.103	2.923±0.323	9.740	0.001

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