Long non-coding RNA-AK138945 regulates myocardial ischemia-reperfusion injury via the miR-1-GRP94 signaling pathway

2.1 A mouse model of myocardial ischemia-reperfusion injury

C57BL/6 mice from Liaoning Changsheng Biotechnology Co., Ltd., aged between 8 to 10 weeks and weighing between 22 g and 25 g, were selected for animal experiments. The left anterior descending (LAD) artery coronary artery of the mouse was occluded for 50 minutes using a 7-0 ligature followed by a reperfusion period of 48 hours. (Animal Experimental Ethical Inspection Protocol No. HMUIRB3021619).

2.2 Echocardiographic analysis

Mice were intraperitoneally injected with 2, 2, 2-tribromoethanol (200 mg/kg; Sigma, St. Louis, Missouri, USA) for anesthesia, and their chests were depilated. The mice were then fixed supine on the operating table, and a proper amount of coupling agent was applied to the chest. The scanning probe was used to record the left ventricular electrocardiogram through the chest wall ultrasound and M-mode echocardiogram. Fractional shortening (FS) and ejection fraction (EF) were determined as the indicators of cardiac function.

2.3 Cell culture and cell dosing

Following the procedure described in our previous study^[16], neonatal mouse (C57BL/6) ventricular cells (NMVCs) were treated with hydrogen peroxide (100 μmol/L, Cat#323381, Sigma-Aldrich, USA ) for 48 hours to simulate MIRI in vitro. The NMVCs were incubated with GRP94 inhibitor PU-WS13 (5 μmol/L; Cat#58687, MedChemExpress, USA) for 48 hours.

2.4 Construction and transfection of lncRNA siRNA and plasmid

siRNA targeting lncRNA-AK138945 (5’-GAAGAGGUAUUGAAUGCUA-3’) was purchased from Ribobio (Guangzhou, Guangdong Province, China) and transfected into NMVCs following the manufacturer’s instructions.

2.5 CCK8 assay

Cell counting kit-8 (CCK8, CK04-500T, Dojindo, Japan) was used to measure cell viability under different conditions. NMVCs were cultured in 96-well culture clusters (about 1 × 10⁴ per well), followed by transfection with lncRNA-AK138945 specific siRNA for 48 hours. The CCK8 reagent (20 μL) and DMEM (180 μL) were added to each well and incubated for 1-4 hours. The absorbance was measured at 450 nm using an Infinite m200pro microplate spectrophotometer (Tecan, Salzburg, Austria).

2.6 Live/Dead cell staining

The cardiomyocytes were seeded on the cover glass of a 24-well culture plate. Forty-eight hours after transfection, live and dead cells were detected using the “Live/Dead Viability/Cytotoxicity Assay Kit” (Invitrogen, Shanghai, China) according to the manufacturer’s instructions. A fluorescence microscope (Olympus, Tokyo, Japan) was used to acquire images.

2.7 TUNEL assay

Terminal deoxynucleotide transferase dUTP nick end labeling (TUNEL) staining was used to evaluate the apoptosis of cultured cardiomyocytes. Briefly, NMVCs cultured on coverslips in 24-well plates were fixed in 4% paraformaldehyde. TUNEL staining was conducted using the in-situ cell death detection kit (Minneapolis, MN, USA) according to the manufacturer’s protocol. The numbers of TUNEL-positive cells and the total cells were counted under confocal microscopy.

2.8 Western blot

Total proteins extracted from NMVCs or mouse left ventricular tissue samples were transferred to a nitrocellulose membrane (Life Science, Überlingen, Germany) using SDS-PAGE (10%-15%). The membrane was sealed with 5% skimmed milk, and incubated overnight at 4°C with antibodies against GRP94 (Cat#20292, Cell Signaling Technology), Caspase9 (Cat#9504, Cell Signaling Technology), Caspase3 (Cat#9662, Cell Signaling Technology), Bcl2 (Cat#3498, Cell Signaling Technology), Bad (Cat#A19595, ABclonal Technology), or β-actin purchased from ZSGB-BIO (Beijing, China). Then, the membrane was washed with PBST and incubated with a secondary antibody (Alexa Fluor, Molecular Probes, Eugene, OR, USA) in the dark for 50 minutes. Odyssey v1.2 software (LI-COR Biosciences, Lincoln, NB, USA) was used to quantify the immunoblot bands. The results were normalized to the band density of β-actin.

2.9 Quantitative real-time PCR (qRT-PCR)

Total RNA was isolated from myocardial tissue and neonatal cardiomyocytes using TRIzol reagent (Invitrogen, Camarillo, CA, USA). The RNA concentration was measured by a NanoDrop 8000 spectrophotometer (Thermo Scientific, Wilmington, DE, USA). The RNA was reverse transcribed into cDNA using a reverse transcription kit (Dalian, China). Real-time quantitative PCR was performed on the Thermocycler ABI 7500 fast real-time PCR system (Applied Biosystems, Carlsbad, California, USA). The sequences of the primer pairs used in our study are:

ZFAS1-forward, 5’-AGCGTTTGCTTTGTTCCC-3’, reverse5’-CTCCCTCGATGCCCTTCT-3’; AK138945-forward, 5’-AGCCCAGGAACAAATGCAGAA-3’, reverse, 5’-TCAACGTCACACTTCATGATGGA-3’; CDR1as-forward, 5’-TCTGCTCGTCTTCCAACATC-3’, reverse, 5’-AGATCAGCACACTGGAGAC-3’; p-ACTB-forward, 5’-ACTGCCGCATCCTCTTCCT-3’; reverse, 5’-TCAACGTCACACTTCATGATGGA-3’; miR-1a-3p-forward, 5’-GGCGTGGAATGTAAAGAA-3’, reverse, 5’-CGGCAATTGCACTGGATA-3’, miR-1a-3p-RT,5’-GTCGTAT CCAGTGCGTGTCGTGGAGTCGGCAATTGCACTGGATACG ACATACATAC-3’; U6-forward, 5’-GCTTCGGCAGCACATATAC TAAAAT-3’, reverse, 5’-CGCTTCACGAATTTGCGTGTCAT-3’, U6-RT, 5’-GCTTCGGCAGCACATATACTAAAAT-3’; FOXO3-forward, 5’-CCGTGAGCAAGCCGTGTACTG-3’, reverse, 5’-TATCCAGCAGGTCGTCCATGAGG-3’; GRP94-forward, 5’-ATGAAGGCACAAGCATACCAGACG-3’, reverse5’-TCATCTTCCTTAATCCGCCGCAAC-3’.

2.10 Dual-luciferase reporter gene assay

HEK293T cells were transfected with miR-1a-3p mimic (20 μmol/L), blank, miR-1a-3p inhibitor, negative control mimic (NC) or negative control inhibitor (NC inhibitor) and plasmid (0.5 μg). Forty-eight hours after transfection, luciferase activity was measured on a fluorometer (Promega, Madison, Wisconsin, USA) using the Dual Luciferase Reporter Assay Kit (Promega, Madison, Wisconsin, USA).

2.11 Data and statistical analysis

The experimental data are expressed as mean ± standard error (mean ± SEM) and were statistically analyzed by one-way analysis of variance for multiple group comparisons and t-test for two-group comparisons (GraphPad Prism 8.0 California, United States). P < 0.05 was considered statistically significant.

3.1 Downregulation of lncRNA-AK138945 in MIRI hearts and hydrogen peroxide treated cardiomyocytes

To explore the regulatory mechanisms underlying MIRI, we first established a mouse model of MIRI. Comparative analysis revealed a marked reduction in both EF and FS in the MIRI group compared to the Sham group (Fig. 1A). Moreover, the expression levels of pro-apoptotic proteins, including Caspase3, Caspase9, and Bad, were significantly increased in the MIRI group compared to the Sham group (Fig. 1B-D). Subsequently, we assessed the expression levels of circRNA-CDR1as, lncRNA-ZFAS1, and lncRNA-AK138945. We observed a substantial increase in the expression levels of circRNA-CDR1as and lncRNA-ZFAS1 in both the heart tissue of MIRI mice and H₂O₂-treated cardiomyocytes, whereas the expression level of lncRNA-AK138945 was markedly reduced (Fig. 1E and F). These findings suggest a significant decrease in the expression level of lncRNA-AK138945 during MIRI, indicating its potential regulatory role in his pathological condition.

Fig. 1

Expression of lncRNA-AK138945 in a mouse model of myocardial ischemia-reperfusion injury (MIRI). (A) Significant decreases in ejection fraction (EF) and fractional shortening (FS) in MIRI mice compared to the control group, indicating the successful establishment of the MIRI model. ^**vs. Sham, P< 0.01, Sham, N = 6; MIRI, N = 4. (B-D) Western blot analysis on the expression levels of apoptotic proteins Caspase 9, Caspase 3, and Bad in myocardial tissue. ^*vs. Sham, P< 0.05; ^**vs. Sham, P< 0.01, N = 3-5. (E) qPCR analysis on the expression of lncRNA-AK138945 in neonatal mouse cardiomyocytes after hydrogen peroxide treatment ^*vs. Control, P< 0.05; ^**vs. Control, P< 0.01, N = 3. (F) Changes of lncRNA-AK138945 expression in cardiac tissue of MIRI model. ^*vs. Sham, P< 0.05; ^**vs. Sham, P< 0.01; ^***vs. Sham, P< 0.001, N = 3-4.

3.2 Knockdown of lncRNA-AK138945 induces cardiomyocyte apoptosis

To further explore the impact of lncRNA-AK138945 on MIRI, we designed and validated a siRNA targeting lncRNA-AK138945 (siAK138945) and confirmed its efficiency in knockdown (Fig. 2A). Comparative analysis revealed a noticeable reduction in cell viability following the knockdown of lncRNA-AK138945 relative to the control group (Fig. 2B). Moreover, silencing lncRNA-AK138945 increased the ratio of Tunel-positive cells (Fig. 2C), indicating apoptotic cell death. This was further evidenced by the increased cell death rate in siAK138945-treated cardiomyocytes, as revealed by Live/Dead cell staining experiments (Fig. 2D). These findings indicate that knockdown of lncRNA-AK138945 can induce cardiomyocyte apoptosis. To corroborate this inference mechanistically, we examined the effects of lncRNA-AK138945 on apoptosis-related proteins in cardiomyocytes. Noticeably, lncRNA-AK138945 knockdown elevated the levels of pro-apoptotic proteins like Bad, Caspase9, and Caspase3 and reduced the expression of anti-apoptotic protein Bcl-2 (Fig. 3A-D). These data collectively indicate that decreased expression of lncRNA-AK138945 may contribute to MIRI via regulating myocardial cell apoptosis.

Fig. 2

LncRNA-AK138945 knockdown facilitates cardiomyocyte apoptosis. (A) Verification of lncRNA-AK138945 knockdown efficiency by its siRNA (siAK138945) ^** vs. Control, P< 0.01; ^###vs. +siAK138945, P< 0.001, N = 3. (B) Reduced cardiomyocyte viability by siAK138945, as measured by CCK8 assay. ^***vs. Control, P< 0.001; ^###vs. +siAK138945, P< 0.001, N = 6. (C) siAK138945 increased cardiomyocyte apoptosis by siAK138945 as unveiled by Tunel staining. ^**vs. Control, P< 0.01; ^##vs. +siAK138945, P< 0.01, N = 3. (D) siAK138945 increased cardiomyocyte death, as demonstrated by survival/death (Live/Dead) staining. Red fluorescence represents dead cells, and green fluorescence represents live cells. ^*vs. Control, P< 0.05; ^#vs. +siAK138945, P< 0.05, N = 3.

Fig. 3

LncRNA-AK138945 knockdown anomaly alters the expression of apoptosis-related proteins in cardiomyocytes. (A-C) LncRNA-AK138945 knockdown by siAK138945 increases the expression levels of apoptotic proteins Caspase3, Caspase9, and Bad in cardiomyocytes. ^*vs. Control, P< 0.05; ^**vs. Control, P< 0.01; ^***vs. Control, P< 0.001; ^#vs. +siAK138945, P< 0.05; ^##vs. +siAK138945, P< 0.01, N = 3-4. (D) siAK138945 significantly reduced the expression of Bcl2. ^***vs. Control, P< 0.001; ^#vs. +siAK138945, P< 0.05, N = 5.

3.3 MiR-1a-3p is a direct target of lncRNA-AK138945

Subsequently, we endeavored to elucidate why the decreased expression of lncRNA-AK138945 induces myocardial damage. To this end, we conducted an analysis and prediction of microRNAs that can potentially be regulated by lncRNA-AK138945 using a bioinformatics database (http://bibiserv.techfak.uni-bielefeld.de/rnahybrid). Our analysis revealed that lncRNA-AK138945 has the potential to interact with miR-1a-3p, as depicted in Fig. 4A. To confirm the direct interaction between lncRNA-AK138945 and miR-1a-3p, we both cloned the wild-type and mutant miR-1a-3p containing the binding site for lncRNA-AK138945 into a luciferase reporter vector. Then, we co-transfected these constructs with miR-1a-3p, blank, miR-1a-3p inhibitor, NC, and NC inhibitor into HEK293T cells and evaluated the effects of miR-1a-3p on luciferase activity. Comparative analysis revealed a significant reduction in the luciferase activity of lncRNA-AK138945 in the miR-1a-3p group compared to the NC group, and this reduction was restored after mutation of the binding site (Fig. 4B). Moreover, we observed a significant increase in the level of miR-1a-3p following lncRNA-AK138945 knockdown (Fig. 4C). These results collectively indicate that miR-1a-3p is a direct target of lncRNA-AK138945.

Fig. 4

Experimental verification of miR-1a-3p as a downstream target of lncRNA-AK138945. (A) The predicted binding sites between miR-1a-3p and lncRNA-AK138945. (B) Luciferase reporter gene activity. ^***vs. NC, P< 0.001, N = 3. (C) Upregulation of miR-1a-3p expression following lncRNA-AK138945 knockdown. ^*vs. +siNC, P< 0.05; ^**vs. +siNC, P< 0.01, N = 3-6. (D-E) Downregulation of GRP94 expression post-lncRNA-AK138945 knockdown. ^**vs. Control, P< 0.01; ^***vs. Control, P< 0.001; ^#vs. +siAK138945, P< 0.05; ^## vs. +siAK138945, P< 0.01, N = 5-6.

We next proceeded to uncover the underlying downstream molecular mechanism of lncRNA-AK138945. Our previous study had already identified miR-1a-3p as a key regulator of MIRI by targeting GRP94^[15]. Therefore, we further explored the regulatory relationship between lncRNA-AK138945 and GRP94. As depicted in Fig. 4D and Fig. 4E, lncRNA-AK138945 knockdown markedly reduced the expression of GRP94 at both mRNA and protein levels compared to the siNC group. These findings strongly suggest the existence of the lncRNA-AK138945-miR-1a-3p-GRP94 regulatory pathway during MIRI.

3.4 Inhibition of GRP94 induces myocardial cell apoptosis

GRP94 serves as a type of molecular chaperone, actively participating in the ER quality control system and regulating the ER stress signaling pathway. Following myocardial ischemia-reperfusion, there is a notable increase in GRP94 levels^[17]. To further investigate the relationship between GRP94 and apoptosis during MIRI, we utilized PU-WS13, a potent GRP94-specific Hsp90 inhibitor with purine scaffolds^[18], in our experiments. Upon administration of PU-WS13, there was a significant increase in the expression levels of pro-apoptotic proteins in the H₂O₂-treated cardiomyocytes, accompanied by a decrease in the expression level of anti-apoptotic proteins (Fig. 5A-D).

Fig. 5

Inhibition of GRP94 induces cardiomyocyte apoptosis. (A-C) After treatment with a GRP94 inhibitor, the expression of apoptosis-related proteins Caspase3, Caspase9 and Bad was increased. ^***vs. Control, P< 0.001; ^#vs. H₂O₂, P< 0.05, ^##vs. H₂O₂, P< 0.01, N = 3-6. (D) The expression of anti-apoptotic protein Bcl2 was reduced after treatment with GRP94 inhibitor. ^**vs. Control, P< 0.01; ^#vs. H₂O₂, P< 0.05, N = 6.

3.5 Effect of transcription factor FOXO3 on the AK138945-miR-1-GRP94 signaling pathway

To further elucidate the upstream mechanism of lncRNA-AK138945 in regulating MIRI, we used the Jaspar database (http://jaspar.genereg.net/) to predict the potential transcription factors of lncRNA-AK138945. As illustrated in Supplementary Material 1, we identified 12 potential FOXO3 recognition/binding sites in the lncRNA-AK138945 sequence, suggesting that FOXO3 may play a role in regulating the lncRNA-AK138945-miR-1-GRP94 signaling pathway. It has been reported that FOXO3 deficiency can lead to increased oxidative damage and decreased myocardial function following acute ischemia-reperfusion injury^[19]. Furthermore, our analysis revealed a significant reduction in the expression of FOXO3 during MIRI, further corroborating these findings (Fig. 6A). Subsequently, we constructed a FOXO3 overexpression plasmid and confirmed its efficiency (Fig. 6B). Notably, FOXO3 overexpression significantly increased the expression levels of lncRNA-AK138945 and GRP94, while inhibiting the expression of miR-1a-3p (Fig. 6C-E). This finding suggests that FOXO3 exerts a regulatory effect on the lncRNA-AK138945-miR-1-GRP94 signaling pathway.

Fig. 6

Effect of transcription factor FOXO3 on the AK138945-miR-1-GRP94 signaling pathway. (A) The expression of FOXO3 in myocardial tissue. ^***vs. Sham, P< 0.001, Sham, N = 4; MIRI, N = 4. (B) Verification of FOXO3 overexpression efficiency. ^***vs. Control, P< 0.001; ^#vs. FOXO3, P< 0.05, N = 4. (C-D) The expression levels of lncRNA-AK138945 and GRP94 are up-regulated after FOXO3 overexpression. ^*vs. Control, P< 0.05; ^***vs. Control, P< 0.001; ^#vs. FOXO3, P< 0.05; ^##vs. FOXO3, P< 0.01, N = 6. (E) FOXO3 overexpression downregulates the expression level of miR-1a-3p. ^**vs. Control, P< 0.01; ^#vs. FOXO3, P< 0.05, N = 6.