Identification of Heme Oxygenase-1 as a Putative DNA-Binding Protein

Author:

Scaffa Alejandro,Tollefson George A.ORCID,Yao Hongwei,Rizal Salu,Wallace Joselynn,Oulhen Nathalie,Carr Jennifer F.ORCID,Hegarty KatyORCID,Uzun Alper,Dennery Phyllis A.ORCID

Abstract

Heme oxygenase-1 (HO-1) is a rate-limiting enzyme in degrading heme into biliverdin and iron. HO-1 can also enter the nucleus and regulate gene transcription independent of its enzymatic activity. Whether HO-1 can alter gene expression through direct binding to target DNA remains unclear. Here, we performed HO-1 CHIP-seq and then employed 3D structural modeling to reveal putative HO-1 DNA binding domains. We identified three probable DNA binding domains on HO-1. Using the Proteinarium, we identified several genes as the most highly connected nodes in the interactome among the HO-1 gene binding targets. We further demonstrated that HO-1 modulates the expression of these key genes using Hmox1 deficient cells. Finally, mutation of four conserved amino acids (E215, I211, E201, and Q27) within HO-1 DNA binding domain 1 significantly increased expression of Gtpbp3 and Eif1 genes that were identified within the top 10 binding hits normalized by gene length predicted to bind this domain. Based on these data, we conclude that HO-1 protein is a putative DNA binding protein, and regulates targeted gene expression. This provides the foundation for developing specific inhibitors or activators targeting HO-1 DNA binding domains to modulate targeted gene expression and corresponding cellular function.

Funder

Institutional Development Award (IDeA) from the NIGMS of NIH

Ralph and Marian Falk Medical Research Trust Bank of America, N.A., Trustee

Warren Alpert Foundation of Brown University

Publisher

MDPI AG

Subject

Cell Biology,Clinical Biochemistry,Molecular Biology,Biochemistry,Physiology

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