High-fidelity CRISPR/Cas9- based gene-specific hydroxymethylation rescues gene expression and attenuates renal fibrosis.
Xingbo XuXiaoying TanBjoern TampeTim WilhelmiMelanie S HulshoffShoji SaitoTobias MoserRaghu KalluriGerd HasenfussElisabeth M ZeisbergMichael ZeisbergPublished in: Nature communications (2018)
While suppression of specific genes through aberrant promoter methylation contributes to different diseases including organ fibrosis, gene-specific reactivation technology is not yet available for therapy. TET enzymes catalyze hydroxymethylation of methylated DNA, reactivating gene expression. We here report generation of a high-fidelity CRISPR/Cas9-based gene-specific dioxygenase by fusing an endonuclease deactivated high-fidelity Cas9 (dHFCas9) to TET3 catalytic domain (TET3CD), targeted to specific genes by guiding RNAs (sgRNA). We demonstrate use of this technology in four different anti-fibrotic genes in different cell types in vitro, among them RASAL1 and Klotho, both hypermethylated in kidney fibrosis. Furthermore, in vivo lentiviral delivery of the Rasal1-targeted fusion protein to interstitial cells and of the Klotho-targeted fusion protein to tubular epithelial cells each results in specific gene reactivation and attenuation of fibrosis, providing gene-specific demethylating technology in a disease model.
Keyphrases
- genome wide
- gene expression
- crispr cas
- dna methylation
- genome wide identification
- genome editing
- copy number
- cancer therapy
- drug delivery
- transcription factor
- dna damage
- systemic sclerosis
- genome wide analysis
- bone marrow
- dna repair
- cell proliferation
- mesenchymal stem cells
- idiopathic pulmonary fibrosis
- cell therapy
- circulating tumor