Experimental Validation of the Neurotrophic Factor-α1 Binding Site on the Serotonin Receptor 1E (HTR1E) Responsible for β-Arrestin Activation and Subsequent Neuroprotection

Creators: Yang, Xuyu¹; Lee, Joo-Youn^{2, 3}; Kim, Soo-Kyung²; Loh, Y. Peng¹; Goddard, William A.²

1. Eunice Kennedy Shriver National Institute of Child Health and Human Development
2. California Institute of Technology
3. Korea Research Institute of Chemical Technology

Abstract

Stress, such as neuroexcitotoxicity and oxidative stress, as well as traumatic brain injury, will result in neurodegeneration. Deciphering the mechanisms underlying neuronal cell death will facilitate the development of drugs that can promote neuronal survival and repair through neurogenesis. Many growth and trophic factors, including transforming growth factors (TGFs), insulin-like growth factors (IGFs), epidermal growth factor (EGF), fibroblast growth factor 2 (FGF2), and brain-derived neurotrophic factor (BDNF), are known to play a role in neuroprotection and neurogenesis. Neurotrophic factor-α1 (NF-α1), also known as carboxypeptidase E (CPE), has been shown experimentally to have neuroprotective activity, acting extracellularly, independent of its intracellular enzymatic function in prohormone processing. We previously reported experiments and molecular dynamics (MD) simulations showing that a 200 amino acid segment of NF-α1/CPE interacts with the serotonin receptor 1E (HTR1E) to protect human neurons against oxidative and neuroexcitotoxic stress via β-arrestin and extracellular signal-regulated kinase (ERK) signaling. We report here validation of our previously predicted binding site with a series of 16 carboxypeptidase E (CPE) mutants, identifying 3 mutants that substantially decrease the binding to HTR1E. We then carried out pERK studies to show that these 3 mutants also dramatically reduce β-arrestin activation. This was followed by MD simulations of 8 selected mutants, finding that the same 3 most dramatically reduced binding of the mutated CPE to 5-HTR1E. Then, we examined the binding of β-arrestin to these 3 (after phosphorylating the intracellular Ser and Thr) and found that the predicted binding decreased dramatically. Then, we examined the predicted activation of the β-arrestin by these 3 and found a dramatic decrease, just as in the pERK experiments. We consider that these experiments and simulations fully validate the predicted binding site for CPE, identifying the key amino acid residues critical for binding and biological activity. This provides the target for experiments and in silico computational screening to identify small molecules to replace the CPE protein as novel drugs to protect human neurons against oxidative/neuroexcitotoxic stress via β-arrestin/ERK signaling.

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Acknowledgement

We would like to thank Dr. Bryan Roth, UNC, North Carolina for providing 5-HTR1E stable cells and V. K. Sharma, NICHD for helpful discussions.

Funding

This research was supported by the Intramural Research Program of the Eunice Kennedy Shriver National Institute of Child Health and Human Development (NICHD), National Institutes of Health, USA. The Caltech team received support from the NIH (R01HL155532 and R35HL150807). The KRICT team was supported by the KRICT intramural funding (grant number KK2432-10) and the National Research Council of Science and Technology (NST) from the Korean Government (grant number CAP23011-200).

Contributions

X.Y. and J.-Y.L. contributed equally to this change work. Y.P.L. designed the experimental research part of the project. W.A.G. designed the MD part of the project. X.Y. performed the experimental research and analyzed the experimental data. J.-Y.L. carried out the MD studies. W.A.G. and Y.P.L. wrote the paper with X.Y., J.-Y.L., and S.-K.K.

Supplemental Material

The Supporting Information is available free of charge at https://pubs.acs.org/doi/10.1021/acsomega.4c05367.

Methods and materials, HTLA cells transfected with plasmids expressing WT-CPE or each of the CPE mutants; Western blot analysis of pERK1/2 and tERK levels in HTR1E stable HEK293 cells treated with the medium obtained from CPE or vector transfected cells; structural analysis of intracellular loops (ICL1, ICL2, and ICL3) of 5-HTR1E upon CPE mutant binding. rmsd plots for eight CPE mutants/5-HTR1E/β-arrestin 1 complex of 100 ns MD simulations (PDF)

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