Macrophage elastase (MMP12) critically contributes to the development of subretinal fibrosis

Caijiao Yi; Jian Liu; Wen Deng; Chang Luo; Jinyan Qi; Mei Chen; Heping Xu

doi:10.1186/s12974-022-02433-x

Macrophage elastase (MMP12) critically contributes to the development of subretinal fibrosis

J Neuroinflammation. 2022 Apr 5;19(1):78. doi: 10.1186/s12974-022-02433-x.

Authors

Caijiao Yi¹, Jian Liu², Wen Deng¹, Chang Luo¹, Jinyan Qi¹, Mei Chen³, Heping Xu^{4

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Affiliations

¹ Aier School of Ophthalmology, Central South University, Changsha, 410000, China.
² Aier Institute of Optometry and Vision Science, Changsha, 410000, China.
³ The Wellcome-Wolfson Institute for Experimental Medicine, School of Medicine, Dentistry and Biomedical Sciences, Queen's University Belfast, 97 Lisburn Road, Belfast, BT9 7BL, UK.
⁴ Aier School of Ophthalmology, Central South University, Changsha, 410000, China. heping.xu@qub.ac.uk.
⁵ Aier Institute of Optometry and Vision Science, Changsha, 410000, China. heping.xu@qub.ac.uk.
⁶ The Wellcome-Wolfson Institute for Experimental Medicine, School of Medicine, Dentistry and Biomedical Sciences, Queen's University Belfast, 97 Lisburn Road, Belfast, BT9 7BL, UK. heping.xu@qub.ac.uk.

Abstract

Background: Macular subretinal fibrosis is the end-stage complication of neovascular age-related macular degeneration (nAMD). We previously developed a mouse model of two-stage laser-induced subretinal fibrosis that mimics closely the dynamic course of macular fibrosis in nAMD patients. This study was aimed to understand the molecular mechanism of subretinal fibrosis.

Methods: Subretinal fibrosis was induced in C57BL/6J mice using the two-stage laser-induced protocol. Twenty days later, eyes were collected and processed for RNA sequencing (RNA-seq) analysis. DESeq2 was used to determine the differentially expressed genes (DEGs). Gene Ontology (GO) and KEGG were used to analyze the enriched pathways. The expression of the selected DEGs including Mmp12 was verified by qPCR. The expression of MMP12 in subretinal fibrosis of mouse and nAMD donor eyes was examined by immunofluorescence and confocal microscopy. The expression of collagen 1, αSMA and fibronectin and cytokines in bone marrow-derived macrophages from control and subretinal fibrosis mice were examined by qPCR, immunocytochemistry and Luminex multiplex cytokine assay. The MMP12 specific inhibitor MMP408 was used to evaluate the effect of MMP12 on TGFβ-induced macrophage-to-myofibroblast transition (MMT) in vitro and its role in subretinal fibrosis in vivo.

Results: RNA-seq analysis of RPE-choroid from subretinal fibrosis eyes uncovered 139 DEGs (fold change log2(fc) ≥ 0.5, FDR < 0.05), including 104 up-regulated and 35 were down-regulated genes. The top 25 enrichment GO terms were related to inflammation, blood vessels/cardiovascular development and angiogenesis. One of the most significantly upregulated genes, Mmp12, contributed to 12 of the top 25 GO terms. Higher levels of MMP12 were detected in subretinal fibrotic lesions in nAMD patients and the mouse model, including in F4/80⁺ or Iba1⁺ macrophages. BMDMs from subretinal fibrosis mice expressed higher levels of MMP12, collagen-1, αSMA and fibronectin. MMP408 dose-dependently suppressed TGFβ-induced MMT in BMDMs. In vivo treatment with MMP408 (5 mg/kg) significantly reduced subretinal fibrosis accompanied by reduced F4/80⁺ macrophage infiltration.

Conclusions: MMP12 critically contributes to the development of subretinal fibrosis, partially through promoting MMT.

Keywords: Age-related macular degeneration; Inflammation; Macular fibrosis; Matrix metalloproteinase-12; RNA sequencing.

MeSH terms

Animals
Fibrosis
Humans
Matrix Metalloproteinase 12* / genetics
Mice
Mice, Inbred C57BL
Retina* / pathology

Substances

Matrix Metalloproteinase 12
matrix metallopeptidase 12, mouse

Abstract

MeSH terms

Substances

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