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Elucidating the Molecular Pathway through which L-Lactate potentiates NMDAR Signaling

The role of L-Lactate has expanded from an energy metabolite to a signaling molecule in
neurons. Studies have shown that L-Lactate plays a role in neuroprotection and in
NMDAR-dependent long-term memory formation. The aim of this dissertation is to
characterize the role of L-Lactate as a signaling molecule and understand the molecular mechanism through which L-Lactate potentiates NMDAR signal. Using mass spectrometry, I monitored the time-dependent changes in the phosphoproteome of cortical neuronal cultures in response to Lactate. The phosphoproteomic analysis highlighted a number of cytoskeletal proteins involved in synapse remodeling as well as axon guidance that were regulated by L-Lactate. In addition, I found that L-Lactate
induced phosphorylation of proteins involved in the MAPK pathway, as reported in an earlier study. I hypothesize the involvement of CaMKII in this mechanism. CaMKII is one of the most abundant kinases in the brain and plays a role in learning and memory via interaction with NMDAR. Using CaMKII inhibitors and mutants of the NMDAR subunit GluN2B, the findings in this dissertation provide evidence for the involvement of CaMKII, specifically, the interaction between CaMKIIa and GluN2B, as a requirement for the L-Lactate mediated potentiation of NMDAR signal.
In addition, to gain insight into the evolution of lactate from a metabolite to a signaling
molecule, this study explores the evolution of glutamate as a signaling molecule in
multicellular organisms so it may serve as a model for evolution of metabolites like
lactate into signaling molecules. For this purpose, the model organism Hydra was used, since it belongs to phylum Cnidaria, evolutionarily one of the first phyla to have a
nervous system. In order to explore whether glutamate receptors, particularly, NMDAR
are functionally expressed in Hydra and are localized in neurons, a line of transgenic
Hydra expressing a calcium indicator (GCaMP6s) in neurons was generated. With the transgenic Hydra line, I attempted to measure the in vivo response of neurons in Hydra to glutamate. This study highlights several ground work experiments with an extensive discussion of implications and challenges and an outlook for future investigations.

Identiferoai:union.ndltd.org:kaust.edu.sa/oai:repository.kaust.edu.sa:10754/660266
Date06 1900
CreatorsMahmood, Hanan S.
ContributorsMagistretti, Pierre J., Biological and Environmental Science and Engineering (BESE) Division, Gojobori, Takashi, Moran, Xose Anxelu G., Martin, Jean-Luc
Source SetsKing Abdullah University of Science and Technology
LanguageEnglish
Detected LanguageEnglish
TypeDissertation
Rights2022-12-26, At the time of archiving, the student author of this dissertation opted to temporarily restrict access to it. The full text of this dissertation will become available to the public after the expiration of the embargo on 2022-12-26.

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