Ethanol inhibition of undifferentiated rat neural progenitor cell replication can be prevented by chlorogenic acid via the NFATc4/CSE signaling pathway

Sambantham Shanmugam; Dhyanesh Patel; Angelica L Rodriguez; Aashlesha Walchale; Xiaobo Liu; Susan E Bergeson; Lenin Mahimainathan; Madhusudhanan Narasimhan; George I Henderson

doi:10.1111/acer.15141

Ethanol inhibition of undifferentiated rat neural progenitor cell replication can be prevented by chlorogenic acid via the NFATc4/CSE signaling pathway

Alcohol Clin Exp Res (Hoboken). 2023 Aug;47(8):1530-1543. doi: 10.1111/acer.15141. Epub 2023 Jul 10.

Authors

Sambantham Shanmugam¹, Dhyanesh Patel¹, Angelica L Rodriguez¹, Aashlesha Walchale¹, Xiaobo Liu¹, Susan E Bergeson², Lenin Mahimainathan³, Madhusudhanan Narasimhan³, George I Henderson¹

Affiliations

¹ Department of Pharmacology and Neuroscience, TTUHSC, Lubbock, Texas, USA.
² Department of Cell Biology and Biochemistry, TTUHSC, Lubbock, Texas, USA.
³ Department of Pathology, University of Texas Southwestern Medical Center, Dallas, Texas, USA.

PMID: 37364904
DOI: 10.1111/acer.15141

Abstract

Background: Prenatal ethanol exposure hinders oxidative stress-mediated neuroblast/neural progenitor cell proliferation by inhibiting G1-S transition, a process vital to neocortical development. We previously showed that ethanol elicits this redox imbalance by repressing cystathionine γ-lyase (CSE), the rate-limiting enzyme in the transsulfuration pathway in fetal brain and cultured cerebral cortical neurons. However, the mechanism by which ethanol impacts the CSE pathway in proliferating neuroblasts is not known. We conducted experiments to define the effects of ethanol on CSE regulation and the molecular signaling events that control this vital pathway. This enabled us to develop an intervention to prevent the ethanol-associated cytostasis.

Methods: Spontaneously immortalized undifferentiated E18 rat neuroblasts from brain cerebral cortex were exposed to ethanol to mimic an acute consumption pattern in humans. We performed loss- and gain-of-function studies to evaluate whether NFATc4 is a transcriptional regulator of CSE. The neuroprotective effects of chlorogenic acid (CGA) against the effects of ethanol were assessed using ROS and GSH/GSSG assays as measures of oxidative stress, transcriptional activation of NFATc4, and expression of NFATc4 and CSE by qRT-PCR and immunoblotting.

Results: Ethanol treatment of E18-neuroblast cells elicited oxidative stress and significantly reduced CSE expression with a concomitant decrease in NFATc4 transcriptional activation and expression. In parallel, inhibition of the calcineurin/NFAT pathway by FK506 exaggerated ethanol-induced CSE loss. In contrast, NFATc4 overexpression prevented loss of ethanol-induced CSE. CGA increased and activated NFATc4, amplified CSE expression, rescued ethanol-induced oxidative stress, and averted the cytostasis of neuroblasts by rescuing cyclin D1 expression.

Conclusions: These findings demonstrate that ethanol can perturb CSE-dependent redox homeostasis by impairing the NFATc4 signaling pathway in neuroblasts. Notably, ethanol-associated impairments were rescued by genetic or pharmacological activation of NFATc4. Furthermore, we found a potential role for CGA in mitigating the ethanol-related neuroblast toxicity with a compelling connection to the NFATc4/CSE pathway.

Keywords: FASD; alcohol; neural progenitor cells; oxidative stress; transsulfuration pathway.

Abstract

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