NDUFA12 as a functional target of the anticancer compound ertredin in human hepatoma cells as revealed by label-free chemical proteomics

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Title
NDUFA12 as a functional target of the anticancer compound ertredin in human hepatoma cells as revealed by label-free chemical proteomics
Author(s)
S I Park; S M Cho; S Atsumi; M Kawada; M Shibuya; Ju Yeon Lee; Jin Young Kim; H J Kwon
Bibliographic Citation
Journal of Proteome Research, vol. 23, no. 1, pp. 130-141
Publication Year
2024
Abstract
Many attempts have been made to develop new agents that target EGFR mutants or regulate downstream factors in various cancers. Cell-based screening showed that a natural small molecule, Ertredin, inhibited the growth of EGFRvIII mutant cancer cells. Previous studies have shown that Ertredin effectively inhibits anchorage-independent 3D growth of sphere-forming cells transfected with EGFRvIII mutant cDNA. However, the underlying mechanism remains unclear. In this study, we investigated the target protein of Ertredin by combining drug affinity-responsive target stability (DARTS) assays with liquid chromatography-mass spectrometry using label-free Ertredin as a bait and HepG2 cell lysates as a proteome pool. NADH dehydrogenase [ubiquinone] 1 alpha subcomplex subunit 12 (NDUFA12) was identified as an Ertredin-binding protein that was responsible for its biological activity. The interaction between NDUFA12 and Ertredin was validated by DARTS and cellular thermal shift assays. In addition, the genetic knockdown of the identified target, NDUFA12, was shown to suppress cell proliferation. NDUFA12 was identified as a biologically relevant target protein of Ertredin that is responsible for its antitumor activity, and these results provide insights into the role of NDUFA12 as a downstream factor in EGFRvIII mutants.
Keyword
ErtredinAnticancer agentTarget identificationDARTSLC?MS/MSCETSAMitochondria complex 1NDUFA12
ISSN
1535-3893
Publisher
Amer Chem Soc
Full Text Link
http://dx.doi.org/10.1021/acs.jproteome.3c00471
Type
Article
Appears in Collections:
1. Journal Articles > Journal Articles
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