SorLA regulates the activity of lipoprotein lipase by intracellular trafficking

Stine C Klinger; Simon Glerup; Merete K Raarup; Muriel C Mari; Mette Nyegaard; Gerbrand Koster; Thaneas Prabakaran; Björn Stefan Nilsson; Maj M Kjaergaard; Oddmund Bakke; Anders Nykjær; Gunilla Olivecrona; Claus Munck Petersen; Morten Schallburg Nielsen

doi:10.1242/jcs.072538

SorLA regulates the activity of lipoprotein lipase by intracellular trafficking

Stine C Klinger, Simon Glerup, Merete K Raarup, Muriel C Mari, Mette Nyegaard, Gerbrand Koster, Thaneas Prabakaran, Björn Stefan Nilsson, Maj M Kjaergaard, Oddmund Bakke, Anders Nykjær, Gunilla Olivecrona, Claus Munck Petersen, Morten Schallburg Nielsen

Publikation: Bidrag til tidsskrift › Tidsskriftartikel › Forskning › peer review

58 Citationer (Scopus)

Abstract

Many different tissues and cell types exhibit regulated secretion of lipoprotein lipase (LPL). However, the sorting of LPL in the trans Golgi network has not, hitherto, been understood in detail. Here, we characterize the role of SorLA (officially known as SorLA-1 or sortilin-related receptor) in the intracellular trafficking of LPL. We found that LPL bound to SorLA under neutral and acidic conditions, and in cells this binding mainly occurred in vesicular structures. SorLA expression changed the subcellular distribution of LPL so it became more concentrated in endosomes. From the endosomes, LPL was further routed to the lysosomes, which resulted in a degradation of newly synthesized LPL. Consequently, an 80% reduction of LPL activity was observed in cells that expressed SorLA. By analogy, SorLA regulated the vesicle-like localization of LPL in primary neuronal cells. Thus, LPL binds to SorLA in the biosynthetic pathway and is subsequently transported to endosomes. As a result of this SorLA mediated-transport, newly synthesized LPL can be routed into specialized vesicles and eventually sent to degradation, and its activity thereby regulated.

Originalsprog	Engelsk
Tidsskrift	Journal of Cell Science
Vol/bind	124
Sider (fra-til)	1095-105
Antal sider	11
ISSN	0021-9533
DOI	https://doi.org/10.1242/jcs.072538
Status	Udgivet - 2011
Udgivet eksternt	Ja

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10.1242/jcs.072538

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Citationsformater

Klinger, S. C., Glerup, S., Raarup, M. K., Mari, M. C., Nyegaard, M., Koster, G., Prabakaran, T., Nilsson, B. S., Kjaergaard, M. M., Bakke, O., Nykjær, A., Olivecrona, G., Petersen, C. M., & Nielsen, M. S. (2011). SorLA regulates the activity of lipoprotein lipase by intracellular trafficking. Journal of Cell Science, 124, 1095-105. https://doi.org/10.1242/jcs.072538

@article{0a12607954ec4348aa93804aad768a97,

title = "SorLA regulates the activity of lipoprotein lipase by intracellular trafficking",

abstract = "Many different tissues and cell types exhibit regulated secretion of lipoprotein lipase (LPL). However, the sorting of LPL in the trans Golgi network has not, hitherto, been understood in detail. Here, we characterize the role of SorLA (officially known as SorLA-1 or sortilin-related receptor) in the intracellular trafficking of LPL. We found that LPL bound to SorLA under neutral and acidic conditions, and in cells this binding mainly occurred in vesicular structures. SorLA expression changed the subcellular distribution of LPL so it became more concentrated in endosomes. From the endosomes, LPL was further routed to the lysosomes, which resulted in a degradation of newly synthesized LPL. Consequently, an 80% reduction of LPL activity was observed in cells that expressed SorLA. By analogy, SorLA regulated the vesicle-like localization of LPL in primary neuronal cells. Thus, LPL binds to SorLA in the biosynthetic pathway and is subsequently transported to endosomes. As a result of this SorLA mediated-transport, newly synthesized LPL can be routed into specialized vesicles and eventually sent to degradation, and its activity thereby regulated.",

keywords = "Animals, Cattle, Cell Line, Cricetinae, Humans, Intracellular Space, LDL-Receptor Related Proteins, Lipoprotein Lipase, Membrane Transport Proteins, Protein Binding, Protein Structure, Tertiary, Protein Transport",

author = "Klinger, {Stine C} and Simon Glerup and Raarup, {Merete K} and Mari, {Muriel C} and Mette Nyegaard and Gerbrand Koster and Thaneas Prabakaran and Nilsson, {Bj{\"o}rn Stefan} and Kjaergaard, {Maj M} and Oddmund Bakke and Anders Nykj{\ae}r and Gunilla Olivecrona and Petersen, {Claus Munck} and Nielsen, {Morten Schallburg}",

year = "2011",

doi = "10.1242/jcs.072538",

language = "English",

volume = "124",

pages = "1095--105",

journal = "Journal of Cell Science",

issn = "0021-9533",

publisher = "The/Company of Biologists Ltd.",

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TY - JOUR

T1 - SorLA regulates the activity of lipoprotein lipase by intracellular trafficking

AU - Klinger, Stine C

AU - Glerup, Simon

AU - Raarup, Merete K

AU - Mari, Muriel C

AU - Nyegaard, Mette

AU - Koster, Gerbrand

AU - Prabakaran, Thaneas

AU - Nilsson, Björn Stefan

AU - Kjaergaard, Maj M

AU - Bakke, Oddmund

AU - Nykjær, Anders

AU - Olivecrona, Gunilla

AU - Petersen, Claus Munck

AU - Nielsen, Morten Schallburg

PY - 2011

Y1 - 2011

N2 - Many different tissues and cell types exhibit regulated secretion of lipoprotein lipase (LPL). However, the sorting of LPL in the trans Golgi network has not, hitherto, been understood in detail. Here, we characterize the role of SorLA (officially known as SorLA-1 or sortilin-related receptor) in the intracellular trafficking of LPL. We found that LPL bound to SorLA under neutral and acidic conditions, and in cells this binding mainly occurred in vesicular structures. SorLA expression changed the subcellular distribution of LPL so it became more concentrated in endosomes. From the endosomes, LPL was further routed to the lysosomes, which resulted in a degradation of newly synthesized LPL. Consequently, an 80% reduction of LPL activity was observed in cells that expressed SorLA. By analogy, SorLA regulated the vesicle-like localization of LPL in primary neuronal cells. Thus, LPL binds to SorLA in the biosynthetic pathway and is subsequently transported to endosomes. As a result of this SorLA mediated-transport, newly synthesized LPL can be routed into specialized vesicles and eventually sent to degradation, and its activity thereby regulated.

AB - Many different tissues and cell types exhibit regulated secretion of lipoprotein lipase (LPL). However, the sorting of LPL in the trans Golgi network has not, hitherto, been understood in detail. Here, we characterize the role of SorLA (officially known as SorLA-1 or sortilin-related receptor) in the intracellular trafficking of LPL. We found that LPL bound to SorLA under neutral and acidic conditions, and in cells this binding mainly occurred in vesicular structures. SorLA expression changed the subcellular distribution of LPL so it became more concentrated in endosomes. From the endosomes, LPL was further routed to the lysosomes, which resulted in a degradation of newly synthesized LPL. Consequently, an 80% reduction of LPL activity was observed in cells that expressed SorLA. By analogy, SorLA regulated the vesicle-like localization of LPL in primary neuronal cells. Thus, LPL binds to SorLA in the biosynthetic pathway and is subsequently transported to endosomes. As a result of this SorLA mediated-transport, newly synthesized LPL can be routed into specialized vesicles and eventually sent to degradation, and its activity thereby regulated.

KW - Animals

KW - Cattle

KW - Cell Line

KW - Cricetinae

KW - Humans

KW - Intracellular Space

KW - LDL-Receptor Related Proteins

KW - Lipoprotein Lipase

KW - Membrane Transport Proteins

KW - Protein Binding

KW - Protein Structure, Tertiary

KW - Protein Transport

U2 - 10.1242/jcs.072538

DO - 10.1242/jcs.072538

M3 - Journal article

SN - 0021-9533

VL - 124

SP - 1095

EP - 1105

JO - Journal of Cell Science

JF - Journal of Cell Science

ER -

SorLA regulates the activity of lipoprotein lipase by intracellular trafficking

Abstract

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