We analyzed four bulk and single-nuclei RNA-seq datasets for heart and kidney samples from Gene Expression Omnibus (Table 1). The first dataset (GSE14910) contains bulk RNA-seq data from 200 left ventricle samples harvested from subjects undergoing transplantation because of end-stage HF and 166 left ventricle control samples from unused donor hearts with normal heart function. The second dataset (GSE66494) contains bulk RNA-seq from 53 renal biopsies with CKD across 8 subtypes, histo-pathologically confirmed the existence of renal fibrosis, and 8 control kidney samples with normal kidney function. The third dataset, GSE183852, studies the differences between end-stage HF and normal control left ventricles. Technically, the GSE183852 dataset contains single-cell RNA sequencing of 7 samples and 38 samples (25 controls and 13 HF) using the snRNA sequencing method. We first filtered out the single-cell RNA sequencing data and kept the snRNA data, since the sample size for snRNA sequencing is larger in GSE183852. The fourth dataset (GSE195718) contains snRNA-seq data from 3 control kidney tissues and 6 fibrotic kidney tissues harvested from kidneys at the end stage of kidney transplantation. For bulk datasets, we normalized the data with the log2 method prior to downstream analysis. For single-cell datasets, we controlled the data quality using the Seurat package (15). Briefly, low-quality cells, defined by having fewer than 300 expressed genes, more than 2,500 expressed genes, or mitochondrial gene expression exceeding 5%, were excluded from the analysis. Detailed information about these datasets is provided in the following:

We downloaded 12,778 genes from the “Harmonizome 3.0” (https://maayanlab.cloud/Harmonizome/) as signature gene sets for inflammation and fibrosis.

To confirm if the inflammation-related and fibrosis-related gene hallmarks (h.all.v2023.1.Hs.symbols.gmt) were activated in HF and CKD, Gene Set Variation Analysis (GSVA) and Gene Set Enrichment Analysis (GSEA) were employed for heart and kidney bulk RNA sequencing data, respectively, using “GSVA” (16) and “clusterProfiler” (17) packages.

Moreover, Gene Ontology (GO) and Kyoto Encyclopedia of Genes and Genomes (KEGG) pathway analysis were performed with the “clusterProfiler” package to discover the main biological processes and pathways for the shared inflammatory fibrosis genes between HF and CKD.

The “Limma” R package was used to identify the differentially expressed genes (DEGs) in the GSE141910 and GSE66494 datasets. DEGs were defined as genes with an adjusted p-value < 0.05 and |fold change|≥ 0.75.

The Search Tool for the Retrieval of Interacting Genes/Proteins (STRING) database is a comprehensive database for connecting the known interactions among different genes and proteins. Herein, isolated genes were filtered out of the PPI plot with default parameters. Moreover, the Cytoscape software (version 3.10.3) was used to construct the gene network and choose the key genes with a connection degree number above 5.

First, the GSE66494 and GSE141910 datasets were merged and divided into the disease group and the control group. We used the “randomForest” R package to classify the disease and control groups. Next, we ranked the genes based on “mean decrease Gini” score and a score higher than 0.25 was considered significant between disease groups (HF and CKD) and the control group. In addition, the LASSO regression method, a more interpretable algorithm compared to Random Forest, was applied to identify significant genes in the merged datasets based on the assumption of a linear relationship between the features and the target. To control overfitting and select the regularization parameter (λ) in the LASSO model, we performed 10-fold cross-validation and chose the λ value that minimized the cross-validation error. Moreover, to assess model stability and ensure reproducibility of feature selection, the analysis was repeated using different random seeds, and the consistency of selected genes across runs was examined.

After preprocessing the snRNA data, the 2,000 most variable genes were selected using the FindVariableFeatures function to reduce the dimension and identify sub-clusters. Based on the scaled data, Principal Component Analysis (PCA) was performed with variable genes. Next, the RunHarmony function in the “harmony” package was adopted to correct the batch effects across the samples. Subsequently, the FindNeighbors and FindClusters functions were performed on the harmonized data to identify the clusters of the cells. The FindAllMarkers function was used to get the cluster-specific markers. The Wilcoxon’s rank-sum test with the Benjamini-Hochberg method was used to calculate p-values and adjusted p-values for comparing gene expression among the clusters. Cell types were annotated by mapping marker genes of each cluster to the reference genes from “CellMarkers 2.0” database (18) supplemented with literature.

The FindAllMarkers function in the “Seurat” R package was used to calculate gene expression differences in M1 macrophages between the HF and control groups. Subsequently, the clusterProfiler R package (V.4.7.1.2) was used to enrich pathways using “h.all.v2023.1.Hs.symbols.gmt” hallmark gene set. Pathways with an adjusted p-value of less than 0.05 were considered significant.

The Python tool “pySCENIC” is a pipeline used for inferring the importance of the transcription factors (TFs) and their target genes in a single-cell dataset with the Wilcoxon rank-sum test. Herein, we adopted it to discover the regulatory network connecting TFs to their genes in M1 and M2 macrophages. The importance of the regulon-gene connection above 1 was considered significant. Besides, the “AUCell” R package was employed to calculate the regulon activity score for each cell with the regulon list from “pySCENIC”. Furthermore, to identify modules with the most significant TF regulatory networks, the “dendextend” R package was used, and the “h” parameter was set to 5. Visualization of the modules based on the regulon activity score was performed using the “ComplexHeatmap” R package [30].

Since inflammatory fibrosis is driven by multiple cell types, the “CellChat” R package (version 2.1.2) was chosen to explore the possible interactions among cell types and compare the interaction differences among groups. Given that inflammation and fibrosis were the primary focus of this study, macrophages, fibroblasts, myo-fibroblasts, and SMCs were included in the analysis of cardiac fibrosis, while PTE cells and fibroblasts were included for renal fibrosis analysis. Due to limited cell numbers, macrophages were excluded from the fibrosis analysis. To investigate cellular crosstalk, ligand-receptor interactions were predicted using the CellChatDB.human database. Statistically significant interactions (p<0.05) were selected for downstream analysis, and communication networks were constructed and filtered according to the package’s standard tutorial for multiple dataset comparisons, applying all default parameters(https://htmlpreview.github.io/?https://github.com/jinworks/CellChat/blob/master/tutorial/Comparison_analysis_of_multiple_datasets.html).

Detailed primary mouse cardiac fibroblast isolation and culture is as described previously (19). Briefly, hearts from C57BL/6 wild-type male mice were collected, washed, cut into small pieces, and digested with Collagenase I (05172969103, Roche). Then the suspension of the digested mixture was centrifuged, and pellets were seeded in high-glucose DMEM (11965092, Gibco) with 10% fetal bovine serum (15140122, Gibco), 1% streptomycin (100 μg/mL), and penicillin (100 U/mL) (C0222, Beyotime) and cultured in a humidified incubator (37°C, 5% CO₂). After culturing for 6 hours, the suspensions were removed, and the cardiac fibroblasts adhered to the flasks. Cardiac fibroblasts were cultured in the aforementioned medium, and passages within 10 were used for formal experiments. For stimulation, cardiac fibroblasts were seeded into 12-well plates with a density of 1.5*10⁴/well and cultured overnight. Then replace the medium with 1% FBS, starving cells for 24 hours. For treatment, 100 ng/ml of IL-1β (200-10B, Peprotech) and 15 ng/ml TGF-β (100-21-2UG, Peprotech) were used to stimulate for 24 hours, respectively.

First, 9 ml blood was withdrawn from healthy male participants at room temperature. Next, lymphocyte separation medium (TBDTM-0050, TBD Science) was used for PBMC isolation, following the standard operating procedure. In short, 5 ml separation medium was mixed with 4 ml blood and centrifuged for 30 minutes at a speed of 600g. Isolate the PBMC layer for washing, then culturing or freezing. Subsequently, monocytes were isolated from thawed PBMCs using CD14 MicroBeads (130-050-201, Miltenyi Biotec) and a MACS separator (130-092-168, Miltenyi Biotec). Briefly, cells were incubated with CD14 MicroBeads in cold buffer (PBS/2 mM EDTA/0.5% BSA), washed, and passed through an LS column in a MACS separator. Unbound cells were removed with buffer washes, and CD14⁺ monocytes were eluted by plunger flushing.

Isolated monocytes were counted and seeded in a 24-well plate with a cell density of 4 * 10⁵/well in RPMI 1640 mixed with 10% FBS. Besides, human M-CSF (130-096-491, Miltenyi Biotec) (375 ng/mL) was supplemented to maintain macrophage status. For M1 polarization, cells were stimulated with 10 ng/mL lipopolysaccharide (L4391, Sigma) and 10 ng/mL interferon-γ (300-02; PeproTech) for 6 hours. Regarding M2 polarization, cells were treated with 20 ng/mL interleukin-4 (200-04; PeproTech) and 20 ng/mL interleukin-10 (200-10; PeproTech) for 6 hours.

The present study was approved by the local ethics committee of Ningbo Medical Centre Lihuili Hospital (KY2025SL157-01). Unaffected healthy kidney tissues were used from patients undergoing nephrectomy due to kidney cancer (distant from any cancer as confirmed by a blinded pathologist). Written informed consents were obtained from all patients according to the Declaration of Helsinki.

As reported previously (20, 21), CD10 is used for sorting PTE cells, and PDGFRβ⁺ cells are considered mesenchymal cells, acting as the main cellular source of fibrosis in the kidneys. Thus, to validate the results from snRNA data analysis, CD10⁺ and PDGFRβ⁺ were sorted based on the previous experience of our group (21). To ensure renal cells with fibrotic susceptibility, kidney tissues from individuals with long-term CKD (22) were adopted.

Briefly, kidney tissue from the donor (64 years old, male, estimated Glomerular Filtration Rate (eGFR): 34 ml/min/1.73 m²) was split into 0.5–1 mm³ pieces, and then the gentleMACS system (Miltenyi Biotec, Bergisch Gladbach, Germany) was used for preparing single-cell suspensions following recommended procedures. To sort the PTE cells, cells were pre-treated with Fc-block (TruStain anti-human, BioLegend, dilution: 1:50) for 30 minutes and subsequently incubated with CD10 (HI10a, BioLegend, dilution: 1:40), CD45 (HI30, BioLegend, dilution: 1:40), CD31 (WM59, BioLegend, dilution: 1:40), and CD235a (HI264, BioLegend, dilution: 1:50). Finally, CD10⁺/CD235a^-/CD31^-/CD45^-/DAPI^- cell subset was sorted using SONY SH800 cytometer (Supplementary Figure S1). PDGFRβ⁺ cell population from another donor (73 years old, male, eGFR: 42 ml/min/1.73 m²) was obtained with PDGFRβ antibody (MAB1263, R&D Systems, dilution: 1:100) and separated by magnetic microbeads (130-047-102, Miltenyi Biotec). Isolated renal PTE and mesenchymal cells were cultured in DMEM/F12 GlutaMAX™ medium (10565018, Gibco) supplemented with 10% fetal calf serum (A01125499, Gibco) and 1% streptomycin (100 μg/mL), and penicillin (100 U/mL) (C0222, Beyotime) in a humidified incubator (37 °C, 5% CO2). For subsequent experiments, both cell types were immortalized through lentiviral transduction of SV40LT (E5510S, New England Biolabs) and following our previous protocol (21). Immortalized cell types were cultured as mentioned above.

To generate a PHLDA1 KO in the human PTE line, a two-step lentiviral CRISPR/Cas9 system was used. LentiCas9-eGFP (63592, Addgene) was first transduced into cells. Then, the cells that expressed Cas9 were sorted according to eGFP fluorescence (lentiCas9-eGFP) strength. Afterwards, cells were transduced with lentiviral vectors encoding single-guide RNAs (sgRNAs) targeting PHLDA1: pLKO5.sgRNA.EFS.tRFP (57823, Addgene) backbone for sgRNA expression pLKO-PHLDA1-KO-tRFP targeting exon 1 or a non-targeting control sgRNA (pLKO-CRISPR-NT). All constructs expressed turboRFP (tRFP) to enable fluorescent selection of sgRNA-positive cells. Cells were collected based on tRFP signal. Genome editing and transfecting efficiency were confirmed by Sanger sequencing and Flow cytometry analysis (Supplementary Figure S2). sgRNA and non-targeting control sequence were provided in Supplementary Excel 1.

To induce cellular injury and evaluate transcriptional changes in PHLDA1-knockout and non-targeting control (NT) cells, cultures were exposed to 5 Gy X-ray irradiation for 10 minutes, three times per day, over a period of 3 days.

PDGFRβ⁺ cells were co-cultured for 3 days with day-3 PHLDA1-KO CD10⁺ PTE cells or PHLDA1-NT CD10⁺ PTE cells that had undergone X-ray exposure. Co-culture was performed using 0.4 μm transwells (TCS016006, JET, China). Following co-culture, cells were collected for analysis or prepared for staining.

Total RNA was isolated from cell lines using the RNA isolation kit (1051, Zymo Research) following the manufacturer’s protocol. 300ng RNA was used for the 200 µl cDNA synthesis. Moreover, real-time PCR was performed using SYBR Green Master Mix kit (A25778, Fisher Scientific), and results were calculated with the 2^^(-ΔΔCt) method. The primer sequences of all mentioned primers, in this study were provided in Supplementary Table S1.

Total RNA from NT and PHLDA1-KO PTE cells was isolated as mentioned above. For bulk mRNA sequencing (RNA-seq), 200 ng total RNA was used for library construction and sequencing was performed by Novogene (Cambridge, UK). Libraries were sequenced on Illumina NovaSeq 6000 flow cells (paired-end, 150bp). Provided FASTQ files were aligned using STAR; reads were counted using featureCounts with -p -t exon -O -g gene_id -s 0. Sequencing quality was assessed using FASTQC. DEGs were analysed with the “DESeq2” R package (23) and genes with adjusted p-value<0.05 and log2|fold change|≥ 1 were considered significant. Downstream settings for GO, KEGG, GSEA, and GSVA analysis were as described above.

Regarding protein isolation, cells were lysed in ice-cold RIPA buffer (89900, Thermo Scientific) (with protease/phosphatase inhibitors), incubated (30 min, 4°C), and centrifuged (12,000 rpm, 10 min). Protein concentration was determined via Bio-Rad DC™ Protein Assay (5000121, Bio-Rad). As for the western blot, SDS-PAGE gel was used for electrophoresis running, and proteins were transferred via the Turbo system (1704150, Bio-Rad). After transferring, the PVDF membrane was rinsed with TBS-T (Tris-buffered saline with 0.1% Tween-20) and blocked with 5% BSA in TBS-T for 1hour at room temperature. Next, the membrane was incubated with the PHLDA1 antibody (18263-1-AP, Proteintech, dilution: 1:2000), β-Tubulin antibody (2146S, Cell Signaling Technology, dilution: 1:1000), p65 (ab16502, Abcam, dilution: 1:2000), p-p65 (phospho S536) (ab28856, Abcam, dilution: 1:1000), and b-Actin (4967, Cell Signaling Technology, dilution: 1:1000) overnight at 4°C. Finally, blots were detected after incubation with the second antibody for 1 hour at room temperature.

Coverslips are sterilized, coated with 1:100 gelatin, and seeded with PDGFRβ+ cells with a density of 2*10⁴/well in 12 12-well plate, which are allowed to attach and grow. After treatment, cells were fixed using 3% paraformaldehyde, permeabilized with 0.1% Triton X-100 for 20 minutes, and blocked in 2% bovine serum, incubated with a primary antibody overnight at 4°C, washed with PBS, and subsequently incubated with the secondary antibody for 2 h. Primary antibodies include: α-SMA (F3777, Sigma, dilution: 1:100), COL1A1 (ab34710, Abcam, dilution: 1:100), PHLDA1 (sc-23866, Santa Cruz, dilution: 1:50), p65 (ab16502, Abcam, dilution: 1:300), VCAM1 (AF643, R&D Systems, dilution: 1: 400). Nikon A1R confocal microscope was used subsequently for taking images.

p65 overexpressed plasmids (pcDNA3.1-p65) and the empty vector (pcDNA3.1 -EV) were provided by GenePharma (Shanghai, China). Transfection of pcDNA3.1-EV and pcDNA3.1-p65 was performed by Lipofectamine 3000 (Thermo Fisher, Waltham, MA, USA) according to the manufacturer’s instructions.

RNA in situ hybridization (ISH) was performed on 4% formalin-fixed, paraffin-embedded tissue sections with the RNAScope Multiplex Detection Kit V2 (323100, ACD) according to the manufacturer’s guidelines. The RNAscope assay utilized the following probes (ACD): Hs-PHLDA1 (593561-C1), Hs-Col1a1 (1094101-C2), and Hs-p65 (490441-C3).