RT Journal Article
SR Electronic
T1 Liberation from fibrogenesis or tumorigenesis via cellular senescence by a novel small molecule
JF bioRxiv
FD Cold Spring Harbor Laboratory
SP 2021.06.01.446522
DO 10.1101/2021.06.01.446522
A1 Moon Kee Meang
A1 Saesbyeol Kim
A1 Byung-Soo Youn
YR 2021
UL http://biorxiv.org/content/early/2021/07/16/2021.06.01.446522.abstract
AB Uncontrolled proliferative diseases such as fibrosis or cancers are fatal human disorders. Previously, we found that a chromone-scaffold derivative called ONG41008 had a strong anti-fibrotic effect on in vitro fibrogenesis as well as in a murine lung fibrosis model. It later occurred to our attention that while ONG41008 remarkably attenuated proliferation of diseased human lung myofibroblasts (DHLF), resulting in replicative senescence (RS) typified by cell flatness, normal human lung fibroblasts were not affected. Video demonstration revealed that RS was evident within 48hr after ONG41008 treatment. No ONG41008 affected activated caspase 3 and mitochondrial membrane potential in DHLF. An interactome study suggested that metabolic shift, chromatin remodeling, or cell cycle control may be required for the RS. This observation prompted us to be engaged in cellular senescence of tumor cells. Clearly, senescent cells were conspicuously but temporarily observed in A549, adenocarcinomic human alveolar epithelial cells, giving us confidence that dysregulated cell proliferation could be a common underlying principle conserved in both DHLF and A549. An early phase of stimulation of A549 by ONG41008 led to RS followed by multinucleation (MNC), which has been known to be oncogene-induced senescence (OIS). MNC was immediately followed by apoptosis. Concomitant with massive upregulation of p16 and translocation to the nuclei, complete cell death of the remaining A549 occurred. Induction and nuclear translocation of p21was also noted in both A549 and DHLF stimulated with ONG41008. No induction of TP53 was seen but phosphorylation of TP53 was substantially increased in A549. Both immunocytochemistry and western blots corroborated these common senescent imaging features. With comparative analyses, it is clear that ONG41008 exhibited much lesser toxicity on normal human lung fibroblast than SAHA (suberoylanilide hydroxamic acid) and Nintedanib. ONG41008 predominantly induced G2/M arrest in A549. Clear formation of MNC was noted in aggressive cancer cell lines involving MCF7 and PC3. A massive increase in NAD/NADH ratio was made by ONG41008, likely impacting mitochondrial function. This may explain how ONG41008 initiated OIS via ROS production in the recovered mitochondria. On the contrary, SAHA did not affect NAD/NADH ratio.Taken together, all these studies strongly suggest that ONG41008 is a potent inducer of RS or OIS, resulting in cessation of cell cycle are at G2/M cell cycle stages and/or systemic cell death. To our best knowledge, the liberation of uncontrolled proliferative cells from fibrogenesis or tumorigenesis by a small molecule in vitro is an unprecedented case. ONG41008 could be a potential and safe drug for a broad range of fibrotic diseases or tumorigenic diseases.Competing Interest StatementB-S Youn retain the shares of Osteoneurogen, M-K Meang retains a stock option, and SB Kim are employed by OsteoNeuroGen. The current contents of the ONG41008 data has been subjected to a Korean provisionary patent. CSChromone ScaffoldCSDChromone Scaffold DerivativesDHLFDiseased Human Lung Fibroblasts from IPF patientsNHLFNormal Human Lung FibroblastsRSReplicative SenescenceOISOncogene-Induced SenescenceMNCMultinucleationMTMPMitochondrial Membrane PotentialNADnicotinamide adenine dinucleotideNAMPTNicotinamide Phosphoribosyltransferase