Estrogenic activity of E2-conjugated GLP-1 is mediated by intracellular endolysosomal acidification and estrone metabolism

Callum Coupland; Na Sun; Ahmed Khalil; Özüm Ezgi Karaoglu; Arkadiusz Liskiewicz; Daniela Liskiewicz; Gerald Grandl; Seun Akindehin; Gandhari Maity; Bin Yang; Brian Finan; Patrick Knerr; Jonathan D. Douros; Axel Walch; Richard DiMarchi; Matthias H. Tschöp; Timo D. Müller; Aaron Novikoff

doi:10.1016/j.molmet.2025.102136

Estrogenic activity of E2-conjugated GLP-1 is mediated by intracellular endolysosomal acidification and estrone metabolism

Callum Coupland, Na Sun, Ahmed Khalil, Özüm Ezgi Karaoglu, Arkadiusz Liskiewicz, Daniela Liskiewicz, Gerald Grandl, Seun Akindehin, Gandhari Maity, Bin Yang, Brian Finan, Patrick Knerr, Jonathan D. Douros, Axel Walch, Richard DiMarchi, Matthias H. Tschöp, Timo D. Müller, Aaron Novikoff

Medicine and Health

Research output: Contribution to journal › Article › peer-review

Abstract

Objective: Recent modifications to glucagon-like peptide 1 (GLP-1), known for its insulinotropic and satiety-inducing effects, have focused on conjugating small molecules to enable selective delivery into GLP-1R+ tissues to achieve targeted synergy and improved metabolic outcomes. Despite continued advancements in GLP-1/small molecule conjugate strategies, the intracellular mechanisms facilitating concurrent GLP-1R signaling and small molecule cargo release remain poorly understood. Methods: We evaluate an estradiol (E2)-conjugated GLP-1 (GLP-1-CEX/E2) for relative differences in GLP-1R signaling and trafficking, and elucidate endolysosomal dynamics that lead to estrogenic activity using various live-cell, reporter, imaging, and mass-spectrometry techniques. Results: We find GLP-1-CEX/E2 does not differentially activate or traffic the GLP-1R relative to its unconjugated GLP-1 backbone (GLP-1-CEX), but uniquely internalizes the E2 moiety and stimulates estrogenic signaling. Endolysosomal pH-dependent proteolytic activity likely mediates E2 moiety liberation, as evidenced by clear amplification in estrogenic activity following co-administration with lysosomal VATPase activator EN6. The hypothesized liberated metabolite from GLP-1-CEX/E2, E2-3-ether, exhibits partial estrogenic efficacy through ERα, and is predisposed toward estrone-3-sulfate conversion. Finally, we identify relative increases in intracellular E2, estrone, and estrone-3-sulfate following GLP-1-CEX/E2 incubation in GLP-1R+ cells, demonstrating proof-of-principle for desired cargo release. Conclusion: Together, our data suggest that GLP-1-CEX/E2 depends on GLP-1R trafficking and lysosome acidification for estrogenic efficacy, with a likely conversion of the liberated E2-3-ether metabolite into estrone-3-sulfate, resulting in a residual downstream flux into active estradiol. Our current findings aim to improve the understanding of small molecule targeting and the efficacy behind GLP-1/small molecule conjugates.

Original language	English
Article number	102136
Journal	Molecular Metabolism
Volume	96
DOIs	https://doi.org/10.1016/j.molmet.2025.102136
State	Published - Jun 2025

Keywords

Bioluminescence resonance energy transfer (BRET)
Estradiol
Glucagon-like peptide 1
Metabolomics
Peptide conjugation
Pharmacology

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10.1016/j.molmet.2025.102136

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Coupland, C., Sun, N., Khalil, A., Karaoglu, Ö. E., Liskiewicz, A., Liskiewicz, D., Grandl, G., Akindehin, S., Maity, G., Yang, B., Finan, B., Knerr, P., Douros, J. D., Walch, A., DiMarchi, R., Tschöp, M. H., Müller, T. D., & Novikoff, A. (2025). Estrogenic activity of E2-conjugated GLP-1 is mediated by intracellular endolysosomal acidification and estrone metabolism. Molecular Metabolism, 96, Article 102136. https://doi.org/10.1016/j.molmet.2025.102136

@article{da3cbdb00c644cc98b75ea14325e71ce,

title = "Estrogenic activity of E2-conjugated GLP-1 is mediated by intracellular endolysosomal acidification and estrone metabolism",

abstract = "Objective: Recent modifications to glucagon-like peptide 1 (GLP-1), known for its insulinotropic and satiety-inducing effects, have focused on conjugating small molecules to enable selective delivery into GLP-1R+ tissues to achieve targeted synergy and improved metabolic outcomes. Despite continued advancements in GLP-1/small molecule conjugate strategies, the intracellular mechanisms facilitating concurrent GLP-1R signaling and small molecule cargo release remain poorly understood. Methods: We evaluate an estradiol (E2)-conjugated GLP-1 (GLP-1-CEX/E2) for relative differences in GLP-1R signaling and trafficking, and elucidate endolysosomal dynamics that lead to estrogenic activity using various live-cell, reporter, imaging, and mass-spectrometry techniques. Results: We find GLP-1-CEX/E2 does not differentially activate or traffic the GLP-1R relative to its unconjugated GLP-1 backbone (GLP-1-CEX), but uniquely internalizes the E2 moiety and stimulates estrogenic signaling. Endolysosomal pH-dependent proteolytic activity likely mediates E2 moiety liberation, as evidenced by clear amplification in estrogenic activity following co-administration with lysosomal VATPase activator EN6. The hypothesized liberated metabolite from GLP-1-CEX/E2, E2-3-ether, exhibits partial estrogenic efficacy through ERα, and is predisposed toward estrone-3-sulfate conversion. Finally, we identify relative increases in intracellular E2, estrone, and estrone-3-sulfate following GLP-1-CEX/E2 incubation in GLP-1R+ cells, demonstrating proof-of-principle for desired cargo release. Conclusion: Together, our data suggest that GLP-1-CEX/E2 depends on GLP-1R trafficking and lysosome acidification for estrogenic efficacy, with a likely conversion of the liberated E2-3-ether metabolite into estrone-3-sulfate, resulting in a residual downstream flux into active estradiol. Our current findings aim to improve the understanding of small molecule targeting and the efficacy behind GLP-1/small molecule conjugates.",

keywords = "Bioluminescence resonance energy transfer (BRET), Estradiol, Glucagon-like peptide 1, Metabolomics, Peptide conjugation, Pharmacology",

author = "Callum Coupland and Na Sun and Ahmed Khalil and Karaoglu, \{{\"O}z{\"u}m Ezgi\} and Arkadiusz Liskiewicz and Daniela Liskiewicz and Gerald Grandl and Seun Akindehin and Gandhari Maity and Bin Yang and Brian Finan and Patrick Knerr and Douros, \{Jonathan D.\} and Axel Walch and Richard DiMarchi and Tsch{\"o}p, \{Matthias H.\} and M{\"u}ller, \{Timo D.\} and Aaron Novikoff",

note = "Publisher Copyright: {\textcopyright} 2025 The Author(s)",

year = "2025",

month = jun,

doi = "10.1016/j.molmet.2025.102136",

language = "English",

volume = "96",

journal = "Molecular Metabolism",

issn = "2212-8778",

publisher = "Elsevier GmbH",

}

Coupland, C, Sun, N, Khalil, A, Karaoglu, ÖE, Liskiewicz, A, Liskiewicz, D, Grandl, G, Akindehin, S, Maity, G, Yang, B, Finan, B, Knerr, P, Douros, JD, Walch, A, DiMarchi, R, Tschöp, MH, Müller, TD & Novikoff, A 2025, 'Estrogenic activity of E2-conjugated GLP-1 is mediated by intracellular endolysosomal acidification and estrone metabolism', Molecular Metabolism, vol. 96, 102136. https://doi.org/10.1016/j.molmet.2025.102136

TY - JOUR

T1 - Estrogenic activity of E2-conjugated GLP-1 is mediated by intracellular endolysosomal acidification and estrone metabolism

AU - Coupland, Callum

AU - Sun, Na

AU - Khalil, Ahmed

AU - Karaoglu, Özüm Ezgi

AU - Liskiewicz, Arkadiusz

AU - Liskiewicz, Daniela

AU - Grandl, Gerald

AU - Akindehin, Seun

AU - Maity, Gandhari

AU - Yang, Bin

AU - Finan, Brian

AU - Knerr, Patrick

AU - Douros, Jonathan D.

AU - Walch, Axel

AU - DiMarchi, Richard

AU - Tschöp, Matthias H.

AU - Müller, Timo D.

AU - Novikoff, Aaron

PY - 2025/6

Y1 - 2025/6

N2 - Objective: Recent modifications to glucagon-like peptide 1 (GLP-1), known for its insulinotropic and satiety-inducing effects, have focused on conjugating small molecules to enable selective delivery into GLP-1R+ tissues to achieve targeted synergy and improved metabolic outcomes. Despite continued advancements in GLP-1/small molecule conjugate strategies, the intracellular mechanisms facilitating concurrent GLP-1R signaling and small molecule cargo release remain poorly understood. Methods: We evaluate an estradiol (E2)-conjugated GLP-1 (GLP-1-CEX/E2) for relative differences in GLP-1R signaling and trafficking, and elucidate endolysosomal dynamics that lead to estrogenic activity using various live-cell, reporter, imaging, and mass-spectrometry techniques. Results: We find GLP-1-CEX/E2 does not differentially activate or traffic the GLP-1R relative to its unconjugated GLP-1 backbone (GLP-1-CEX), but uniquely internalizes the E2 moiety and stimulates estrogenic signaling. Endolysosomal pH-dependent proteolytic activity likely mediates E2 moiety liberation, as evidenced by clear amplification in estrogenic activity following co-administration with lysosomal VATPase activator EN6. The hypothesized liberated metabolite from GLP-1-CEX/E2, E2-3-ether, exhibits partial estrogenic efficacy through ERα, and is predisposed toward estrone-3-sulfate conversion. Finally, we identify relative increases in intracellular E2, estrone, and estrone-3-sulfate following GLP-1-CEX/E2 incubation in GLP-1R+ cells, demonstrating proof-of-principle for desired cargo release. Conclusion: Together, our data suggest that GLP-1-CEX/E2 depends on GLP-1R trafficking and lysosome acidification for estrogenic efficacy, with a likely conversion of the liberated E2-3-ether metabolite into estrone-3-sulfate, resulting in a residual downstream flux into active estradiol. Our current findings aim to improve the understanding of small molecule targeting and the efficacy behind GLP-1/small molecule conjugates.

AB - Objective: Recent modifications to glucagon-like peptide 1 (GLP-1), known for its insulinotropic and satiety-inducing effects, have focused on conjugating small molecules to enable selective delivery into GLP-1R+ tissues to achieve targeted synergy and improved metabolic outcomes. Despite continued advancements in GLP-1/small molecule conjugate strategies, the intracellular mechanisms facilitating concurrent GLP-1R signaling and small molecule cargo release remain poorly understood. Methods: We evaluate an estradiol (E2)-conjugated GLP-1 (GLP-1-CEX/E2) for relative differences in GLP-1R signaling and trafficking, and elucidate endolysosomal dynamics that lead to estrogenic activity using various live-cell, reporter, imaging, and mass-spectrometry techniques. Results: We find GLP-1-CEX/E2 does not differentially activate or traffic the GLP-1R relative to its unconjugated GLP-1 backbone (GLP-1-CEX), but uniquely internalizes the E2 moiety and stimulates estrogenic signaling. Endolysosomal pH-dependent proteolytic activity likely mediates E2 moiety liberation, as evidenced by clear amplification in estrogenic activity following co-administration with lysosomal VATPase activator EN6. The hypothesized liberated metabolite from GLP-1-CEX/E2, E2-3-ether, exhibits partial estrogenic efficacy through ERα, and is predisposed toward estrone-3-sulfate conversion. Finally, we identify relative increases in intracellular E2, estrone, and estrone-3-sulfate following GLP-1-CEX/E2 incubation in GLP-1R+ cells, demonstrating proof-of-principle for desired cargo release. Conclusion: Together, our data suggest that GLP-1-CEX/E2 depends on GLP-1R trafficking and lysosome acidification for estrogenic efficacy, with a likely conversion of the liberated E2-3-ether metabolite into estrone-3-sulfate, resulting in a residual downstream flux into active estradiol. Our current findings aim to improve the understanding of small molecule targeting and the efficacy behind GLP-1/small molecule conjugates.

KW - Bioluminescence resonance energy transfer (BRET)

KW - Estradiol

KW - Glucagon-like peptide 1

KW - Metabolomics

KW - Peptide conjugation

KW - Pharmacology

UR - http://www.scopus.com/inward/record.url?scp=105002755674&partnerID=8YFLogxK

U2 - 10.1016/j.molmet.2025.102136

DO - 10.1016/j.molmet.2025.102136

M3 - Article

AN - SCOPUS:105002755674

SN - 2212-8778

VL - 96

JO - Molecular Metabolism

JF - Molecular Metabolism

M1 - 102136

ER -

Estrogenic activity of E2-conjugated GLP-1 is mediated by intracellular endolysosomal acidification and estrone metabolism

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Keywords

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