Tagless LysoIP for immunoaffinity enrichment of native lysosomes from clinical samples

Daniel Saarela; Pawel Lis; Sara Gomes; Raja S Nirujogi; Wentao Dong; Eshaan S Rawat; Sophie Glendinning; Karolina Zeneviciute; Enrico Bagnoli; Rotimi Fasimoye; Cindy Lin; Kwamina Nyame; Fanni A Boros; Friederike Zunke; Frederic Lamoliatte; Sadik Elshani; Matthew Jaconelli; Judith Jm Jans; Margriet A Huisman; Christian Posern; Lena M Westermann; Angela Schulz; Peter M van Hasselt; Dario R Alessi; Monther Abu-Remaileh; Esther M Sammler

doi:10.1172/JCI183592

Tagless LysoIP for immunoaffinity enrichment of native lysosomes from clinical samples

Daniel Saarela, Pawel Lis, Sara Gomes, Raja S Nirujogi, Wentao Dong, Eshaan S Rawat, Sophie Glendinning, Karolina Zeneviciute, Enrico Bagnoli, Rotimi Fasimoye, Cindy Lin, Kwamina Nyame, Fanni A Boros, Friederike Zunke, Frederic Lamoliatte, Sadik Elshani, Matthew Jaconelli, Judith Jm Jans, Margriet A Huisman, Christian PosernLena M Westermann, Angela Schulz, Peter M van Hasselt, Dario R Alessi, Monther Abu-Remaileh, Esther M Sammler

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

Abstract

Lysosomes are implicated in a wide spectrum of human diseases, including monogenic lysosomal storage disorders (LSDs), age-associated neurodegeneration, and cancer. Profiling lysosomal content using tag-based lysosomal immunoprecipitation (LysoTagIP) in cell and animal models has substantially moved the field forward, but studying lysosomal dysfunction in patients remains challenging. Here, we report the development of the ‘tagless LysoIP’ method, designed to enable the rapid enrichment of lysosomes, via immunoprecipitation, using the endogenous integral lysosomal membrane protein TMEM192, directly from clinical samples and human cell lines (e.g., induced pluripotent stem cell–derived neurons). Isolated lysosomes were intact and suitable for subsequent multimodal omics analyses. To validate our approach, we applied the tagless LysoIP to enrich lysosomes from peripheral blood mononuclear cells derived from fresh blood of healthy donors and patients with CLN3 disease, an autosomal recessive neurodegenerative LSD. Metabolic profiling of isolated lysosomes revealed massive accumulation of glycerophosphodiesters (GPDs) in patients’ lysosomes. Interestingly, a patient with a milder phenotype and genotype displayed lower accumulation of lysosomal GPDs, consistent with their potential role as disease biomarkers. Altogether, the tagless LysoIP provides a framework to study native lysosomes from patient samples, identify disease biomarkers, and discover human-relevant disease mechanisms.

Original language	English
Article number	e183592
Journal	Journal of Clinical Investigation
Volume	135
Issue number	4
Early online date	26 Dec 2024
DOIs	https://doi.org/10.1172/JCI183592
Publication status	Published - 17 Feb 2025

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183592.2-20250214121652-covered-e0fd13ba177f913fd3156f593ead4cfdFinal published version, 2.13 MBLicence: CC BY

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Saarela, D., Lis, P., Gomes, S., Nirujogi, R. S., Dong, W., Rawat, E. S., Glendinning, S., Zeneviciute, K., Bagnoli, E., Fasimoye, R., Lin, C., Nyame, K., Boros, F. A., Zunke, F., Lamoliatte, F., Elshani, S., Jaconelli, M., Jans, J. J., Huisman, M. A., ... Sammler, E. M. (2025). Tagless LysoIP for immunoaffinity enrichment of native lysosomes from clinical samples. Journal of Clinical Investigation, 135(4), Article e183592. https://doi.org/10.1172/JCI183592

@article{4e82df91818143f2a4d6956ce90ca2ee,

title = "Tagless LysoIP for immunoaffinity enrichment of native lysosomes from clinical samples",

abstract = "Lysosomes are implicated in a wide spectrum of human diseases, including monogenic lysosomal storage disorders (LSDs), age-associated neurodegeneration, and cancer. Profiling lysosomal content using tag-based lysosomal immunoprecipitation (LysoTagIP) in cell and animal models has substantially moved the field forward, but studying lysosomal dysfunction in patients remains challenging. Here, we report the development of the {\textquoteleft}tagless LysoIP{\textquoteright} method, designed to enable the rapid enrichment of lysosomes, via immunoprecipitation, using the endogenous integral lysosomal membrane protein TMEM192, directly from clinical samples and human cell lines (e.g., induced pluripotent stem cell–derived neurons). Isolated lysosomes were intact and suitable for subsequent multimodal omics analyses. To validate our approach, we applied the tagless LysoIP to enrich lysosomes from peripheral blood mononuclear cells derived from fresh blood of healthy donors and patients with CLN3 disease, an autosomal recessive neurodegenerative LSD. Metabolic profiling of isolated lysosomes revealed massive accumulation of glycerophosphodiesters (GPDs) in patients{\textquoteright} lysosomes. Interestingly, a patient with a milder phenotype and genotype displayed lower accumulation of lysosomal GPDs, consistent with their potential role as disease biomarkers. Altogether, the tagless LysoIP provides a framework to study native lysosomes from patient samples, identify disease biomarkers, and discover human-relevant disease mechanisms.",

author = "Daniel Saarela and Pawel Lis and Sara Gomes and Nirujogi, {Raja S} and Wentao Dong and Rawat, {Eshaan S} and Sophie Glendinning and Karolina Zeneviciute and Enrico Bagnoli and Rotimi Fasimoye and Cindy Lin and Kwamina Nyame and Boros, {Fanni A} and Friederike Zunke and Frederic Lamoliatte and Sadik Elshani and Matthew Jaconelli and Jans, {Judith Jm} and Huisman, {Margriet A} and Christian Posern and Westermann, {Lena M} and Angela Schulz and {van Hasselt}, {Peter M} and Alessi, {Dario R} and Monther Abu-Remaileh and Sammler, {Esther M}",

note = "Publisher Copyright: {\textcopyright} 2024, Saarela et al.",

year = "2025",

month = feb,

day = "17",

doi = "10.1172/JCI183592",

language = "English",

volume = "135",

journal = "Journal of Clinical Investigation",

issn = "0021-9738",

publisher = "American Society for Clinical Investigation",

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Saarela, D, Lis, P, Gomes, S, Nirujogi, RS, Dong, W, Rawat, ES, Glendinning, S, Zeneviciute, K, Bagnoli, E, Fasimoye, R, Lin, C, Nyame, K, Boros, FA, Zunke, F, Lamoliatte, F, Elshani, S, Jaconelli, M, Jans, JJ, Huisman, MA, Posern, C, Westermann, LM, Schulz, A, van Hasselt, PM, Alessi, DR, Abu-Remaileh, M & Sammler, EM 2025, 'Tagless LysoIP for immunoaffinity enrichment of native lysosomes from clinical samples', Journal of Clinical Investigation, vol. 135, no. 4, e183592. https://doi.org/10.1172/JCI183592

TY - JOUR

T1 - Tagless LysoIP for immunoaffinity enrichment of native lysosomes from clinical samples

AU - Saarela, Daniel

AU - Lis, Pawel

AU - Gomes, Sara

AU - Nirujogi, Raja S

AU - Dong, Wentao

AU - Rawat, Eshaan S

AU - Glendinning, Sophie

AU - Zeneviciute, Karolina

AU - Bagnoli, Enrico

AU - Fasimoye, Rotimi

AU - Lin, Cindy

AU - Nyame, Kwamina

AU - Boros, Fanni A

AU - Zunke, Friederike

AU - Lamoliatte, Frederic

AU - Elshani, Sadik

AU - Jaconelli, Matthew

AU - Jans, Judith Jm

AU - Huisman, Margriet A

AU - Posern, Christian

AU - Westermann, Lena M

AU - Schulz, Angela

AU - van Hasselt, Peter M

AU - Alessi, Dario R

AU - Abu-Remaileh, Monther

AU - Sammler, Esther M

PY - 2025/2/17

Y1 - 2025/2/17

N2 - Lysosomes are implicated in a wide spectrum of human diseases, including monogenic lysosomal storage disorders (LSDs), age-associated neurodegeneration, and cancer. Profiling lysosomal content using tag-based lysosomal immunoprecipitation (LysoTagIP) in cell and animal models has substantially moved the field forward, but studying lysosomal dysfunction in patients remains challenging. Here, we report the development of the ‘tagless LysoIP’ method, designed to enable the rapid enrichment of lysosomes, via immunoprecipitation, using the endogenous integral lysosomal membrane protein TMEM192, directly from clinical samples and human cell lines (e.g., induced pluripotent stem cell–derived neurons). Isolated lysosomes were intact and suitable for subsequent multimodal omics analyses. To validate our approach, we applied the tagless LysoIP to enrich lysosomes from peripheral blood mononuclear cells derived from fresh blood of healthy donors and patients with CLN3 disease, an autosomal recessive neurodegenerative LSD. Metabolic profiling of isolated lysosomes revealed massive accumulation of glycerophosphodiesters (GPDs) in patients’ lysosomes. Interestingly, a patient with a milder phenotype and genotype displayed lower accumulation of lysosomal GPDs, consistent with their potential role as disease biomarkers. Altogether, the tagless LysoIP provides a framework to study native lysosomes from patient samples, identify disease biomarkers, and discover human-relevant disease mechanisms.

AB - Lysosomes are implicated in a wide spectrum of human diseases, including monogenic lysosomal storage disorders (LSDs), age-associated neurodegeneration, and cancer. Profiling lysosomal content using tag-based lysosomal immunoprecipitation (LysoTagIP) in cell and animal models has substantially moved the field forward, but studying lysosomal dysfunction in patients remains challenging. Here, we report the development of the ‘tagless LysoIP’ method, designed to enable the rapid enrichment of lysosomes, via immunoprecipitation, using the endogenous integral lysosomal membrane protein TMEM192, directly from clinical samples and human cell lines (e.g., induced pluripotent stem cell–derived neurons). Isolated lysosomes were intact and suitable for subsequent multimodal omics analyses. To validate our approach, we applied the tagless LysoIP to enrich lysosomes from peripheral blood mononuclear cells derived from fresh blood of healthy donors and patients with CLN3 disease, an autosomal recessive neurodegenerative LSD. Metabolic profiling of isolated lysosomes revealed massive accumulation of glycerophosphodiesters (GPDs) in patients’ lysosomes. Interestingly, a patient with a milder phenotype and genotype displayed lower accumulation of lysosomal GPDs, consistent with their potential role as disease biomarkers. Altogether, the tagless LysoIP provides a framework to study native lysosomes from patient samples, identify disease biomarkers, and discover human-relevant disease mechanisms.

U2 - 10.1172/JCI183592

DO - 10.1172/JCI183592

M3 - Article

C2 - 39724071

SN - 0021-9738

VL - 135

JO - Journal of Clinical Investigation

JF - Journal of Clinical Investigation

IS - 4

M1 - e183592

ER -

Tagless LysoIP for immunoaffinity enrichment of native lysosomes from clinical samples

Abstract

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