Effects of In Utero EtOH Exposure on 18S Ribosomal RNA Processing: Contribution to Fetal Alcohol Spectrum Disorder

Nune Darbinian; Gary L Gallia; Armine Darbinyan; Ekaterina Vadachkoria; Nana Merabova; Amos Moore; Laura Goetzl; Shohreh Amini; Michael E Selzer

doi:10.3390/ijms241813714

Effects of In Utero EtOH Exposure on 18S Ribosomal RNA Processing: Contribution to Fetal Alcohol Spectrum Disorder

Int J Mol Sci. 2023 Sep 5;24(18):13714. doi: 10.3390/ijms241813714.

Authors

Nune Darbinian¹, Gary L Gallia², Armine Darbinyan³, Ekaterina Vadachkoria¹, Nana Merabova^{1

4}, Amos Moore¹, Laura Goetzl⁵, Shohreh Amini⁶, Michael E Selzer^{1

7}

Affiliations

¹ Center for Neural Repair and Rehabilitation Shriners Hospitals Pediatric Research Center, Lewis Katz School of Medicine, Temple University, Philadelphia, PA 19140, USA.
² Department of Neurosurgery, Johns Hopkins Hospital, Baltimore, MD 21287, USA.
³ Department of Pathology, Yale University School of Medicine, New Haven, CT 06520, USA.
⁴ Medical College of Wisconsin-Prevea Health, Green Bay, WI 54304, USA.
⁵ Department of Obstetrics & Gynecology, University of Texas, Houston, TX 77030, USA.
⁶ Department of Biology, College of Science and Technology, Temple University, Philadelphia, PA 19122, USA.
⁷ Departments of Neurology and Neural Sciences, Lewis Katz School of Medicine at Temple University, Philadelphia, PA 19140, USA.

Abstract

Fetal alcohol spectrum disorders (FASD) are leading causes of neurodevelopmental disability. The mechanisms by which alcohol (EtOH) disrupts fetal brain development are incompletely understood, as are the genetic factors that modify individual vulnerability. Because the phenotype abnormalities of FASD are so varied and widespread, we investigated whether fetal exposure to EtOH disrupts ribosome biogenesis and the processing of pre-ribosomal RNAs and ribosome assembly, by determining the effect of exposure to EtOH on the developmental expression of 18S rRNA and its cleaved forms, members of a novel class of short non-coding RNAs (srRNAs). In vitro neuronal cultures and fetal brains (11-22 weeks) were collected according to an IRB-approved protocol. Twenty EtOH-exposed brains from the first and second trimester were compared with ten unexposed controls matched for gestational age and fetal gender. Twenty fetal-brain-derived exosomes (FB-Es) were isolated from matching maternal blood. RNA was isolated using Qiagen RNA isolation kits. Fetal brain srRNA expression was quantified by ddPCR. srRNAs were expressed in the human brain and FB-Es during fetal development. EtOH exposure slightly decreased srRNA expression (1.1-fold; p = 0.03). Addition of srRNAs to in vitro neuronal cultures inhibited EtOH-induced caspase-3 activation (1.6-fold, p = 0.002) and increased cell survival (4.7%, p = 0.034). The addition of exogenous srRNAs reversed the EtOH-mediated downregulation of srRNAs (2-fold, p = 0.002). EtOH exposure suppressed expression of srRNAs in the developing brain, increased activity of caspase-3, and inhibited neuronal survival. Exogenous srRNAs reversed this effect, possibly by stabilizing endogenous srRNAs, or by increasing the association of cellular proteins with srRNAs, modifying gene transcription. Finally, the reduction in 18S rRNA levels correlated closely with the reduction in fetal eye diameter, an anatomical hallmark of FASD. The findings suggest a potential mechanism for EtOH-mediated neurotoxicity via alterations in 18S rRNA processing and the use of FB-Es for early diagnosis of FASD. Ribosome biogenesis may be a novel target to ameliorate FASD in utero or after birth. These findings are consistent with observations that gene-environment interactions contribute to FASD vulnerability.

Keywords: 18S Ribosomal RNA; FASD; Ribosomal RNA processing; alcohol; brain development; exosomes; neurons; srRNA.

Abstract

Grants and funding