TAR DNA-binding protein 43 inhibits inflammatory response and protects chondrocyte function by modulating RACK1 expression in osteoarthritis

Yongming Huang; Qiming Huang; Haitao Su; Xiujun Mai; Enhui Feng; Zhenwu Cao; Xiuyun Zeng

doi:10.1016/j.biopha.2016.11.037

TAR DNA-binding protein 43 inhibits inflammatory response and protects chondrocyte function by modulating RACK1 expression in osteoarthritis

Biomed Pharmacother. 2017 Jan:85:362-371. doi: 10.1016/j.biopha.2016.11.037. Epub 2016 Nov 24.

Authors

Yongming Huang¹, Qiming Huang², Haitao Su³, Xiujun Mai³, Enhui Feng³, Zhenwu Cao³, Xiuyun Zeng³

Affiliations

¹ Department of orthopedics, The Second Clinical Medical College of Guangzhou University of Chinese Medicine, No. 12 Jichang Road of Baiyun District, Guangzhou, 510405, PR China. Electronic address: huang163huang@163.com.
² Joy Phosphor (Beijing) Biomedical Technologies Co., Ltd, Jinqiu International Mansion A1305, No. 6 Zhichun road, Haidian district, Beijing 100088, PR China.
³ Department of orthopedics, The Second Clinical Medical College of Guangzhou University of Chinese Medicine, No. 12 Jichang Road of Baiyun District, Guangzhou, 510405, PR China.

PMID: 27890430
DOI: 10.1016/j.biopha.2016.11.037

Abstract

Background: TAR DNA-binding protein-43 (TDP-43, transactive response DNA binding protein 43kDa) accumulates in the cytoplasm of affected neurons and glia, as large inclusions of stress granules (SGs). However, the mechanism of TDP-43 interaction with the target genes and its specific role in osteoarthritis (OA) progression is still unknown. The goal of this study was to identify the role of TDP-43 in OA progression by modulating its target genes.

Methods: MSCs were transfected with TDP-43 gene lentivirus. The role of elevated TDP-43 expression in the differentiation of MSCs to chondrocytes was investigated. Cell function assay was used to evaluate the proliferation and apoptosis of Human chondrocytes (HCs) co-cultured with MSC. Truncated TDP-43/p35 expression and SGs formation in HCs were identified using cyto-immunofluorescence assay. Critical genes mediating apoptotic and proliferative signaling in HCs were measured using co-culturing MSC assays. The phosphorylation of key kinases was analyzed using the HTRF phosphokinase assay, and the expression of key genes in proliferative and apoptotic signaling transduction pathways was detected using qRT-PCR.

Results: The MSCs differentiated into HCs after transfection of TDP-43 genes. The TDP-43 can degrade truncated TDP-43/p35, and promote SGs formation and HCs proliferation, and inhibit HCs apoptosis after co-culturing with MSCs. TDP-43 overexpression in MSCs promoted high expression of RACK1 and promoted phosphorylation of key kinases in HCs. Critical genes were highly expressed in P38 MAPK/MKK3 proliferative signaling, but not in P38 MAPK/JNK MAPK signaling.

Conclusions: The chondrogenically differentiation of MSCs was not influenced by transfection of TDP-43 genes, and promoted HCs growth after co-culturing with HCs. The data indicated that TDP-43/p35 contributed to SGs formation by promoting RACK1 expression. The study sheds new light on post-transcriptional regulation and apoptosis in OA by RACK1, which is a potential treatment strategy for OA.

Keywords: Ariticular cartilage; Gene; Osteoarthritis; RACK1 expression; TDP-43.

MeSH terms

Animals
Cell Proliferation / physiology
Chondrocytes / physiology*
Coculture Techniques
DNA-Binding Proteins / genetics
DNA-Binding Proteins / metabolism*
GTP-Binding Proteins / genetics
GTP-Binding Proteins / metabolism*
Gene Expression Regulation
Humans
Inflammation / metabolism*
Mesenchymal Stem Cells
Neoplasm Proteins / genetics
Neoplasm Proteins / metabolism*
Osteoarthritis / metabolism*
Phosphorylation
RNA
Receptors for Activated C Kinase
Receptors, Cell Surface / genetics
Receptors, Cell Surface / metabolism*
Signal Transduction

Substances

DNA-Binding Proteins
Neoplasm Proteins
RACK1 protein, human
Receptors for Activated C Kinase
Receptors, Cell Surface
TARDBP protein, human
RNA
GTP-Binding Proteins