Aberrant lymphatic endothelial progenitors in lymphatic malformation development.

Aberrant lymphatic endothelial progenitors in lymphatic malformation development.

Lymphatic malformations (LMs) are vascular anomalies thought to arise from dysregulated lymphangiogenesis. These lesions impose a significant burden of disease on affected individuals. LM pathobiology is poorly understood, hindering the development of effective treatments. In the present studies, im...

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Main Authors: June K Wu, Christopher Kitajewski, Maia Reiley, Connie H Keung, Julie Monteagudo, John P Andrews, Peter Liou, Arul Thirumoorthi, Alvin Wong, Jessica J Kandel, Carrie J Shawber
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2015-01-01
Series:PLoS ONE
Online Access:http://europepmc.org/articles/PMC4342011?pdf=render
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spelling doaj-96d0107311c2447ab11616db4e347c772020-11-25T02:29:57ZengPublic Library of Science (PLoS)PLoS ONE1932-62032015-01-01102e011735210.1371/journal.pone.0117352Aberrant lymphatic endothelial progenitors in lymphatic malformation development.June K WuChristopher KitajewskiMaia ReileyConnie H KeungJulie MonteagudoJohn P AndrewsPeter LiouArul ThirumoorthiAlvin WongJessica J KandelCarrie J ShawberLymphatic malformations (LMs) are vascular anomalies thought to arise from dysregulated lymphangiogenesis. These lesions impose a significant burden of disease on affected individuals. LM pathobiology is poorly understood, hindering the development of effective treatments. In the present studies, immunostaining of LM tissues revealed that endothelial cells lining aberrant lymphatic vessels and cells in the surrounding stroma expressed the stem cell marker, CD133, and the lymphatic endothelial protein, podoplanin. Isolated patient-derived CD133+ LM cells expressed stem cell genes (NANOG, Oct4), circulating endothelial cell precursor proteins (CD90, CD146, c-Kit, VEGFR-2), and lymphatic endothelial proteins (podoplanin, VEGFR-3). Consistent with a progenitor cell identity, CD133+ LM cells were multipotent and could be differentiated into fat, bone, smooth muscle, and lymphatic endothelial cells in vitro. CD133+ cells were compared to CD133- cells isolated from LM fluids. CD133- LM cells had lower expression of stem cell genes, but expressed circulating endothelial precursor proteins and high levels of lymphatic endothelial proteins, VE-cadherin, CD31, podoplanin, VEGFR-3 and Prox1. CD133- LM cells were not multipotent, consistent with a differentiated lymphatic endothelial cell phenotype. In a mouse xenograft model, CD133+ LM cells differentiated into lymphatic endothelial cells that formed irregularly dilated lymphatic channels, phenocopying human LMs. In vivo, CD133+ LM cells acquired expression of differentiated lymphatic endothelial cell proteins, podoplanin, LYVE1, Prox1, and VEGFR-3, comparable to expression found in LM patient tissues. Taken together, these data identify a novel LM progenitor cell population that differentiates to form the abnormal lymphatic structures characteristic of these lesions, recapitulating the human LM phenotype. This LM progenitor cell population may contribute to the clinically refractory behavior of LMs.http://europepmc.org/articles/PMC4342011?pdf=render
collection DOAJ
language English
format Article
sources DOAJ
author June K Wu
Christopher Kitajewski
Maia Reiley
Connie H Keung
Julie Monteagudo
John P Andrews
Peter Liou
Arul Thirumoorthi
Alvin Wong
Jessica J Kandel
Carrie J Shawber
spellingShingle June K Wu
Christopher Kitajewski
Maia Reiley
Connie H Keung
Julie Monteagudo
John P Andrews
Peter Liou
Arul Thirumoorthi
Alvin Wong
Jessica J Kandel
Carrie J Shawber
Aberrant lymphatic endothelial progenitors in lymphatic malformation development.
PLoS ONE
author_facet June K Wu
Christopher Kitajewski
Maia Reiley
Connie H Keung
Julie Monteagudo
John P Andrews
Peter Liou
Arul Thirumoorthi
Alvin Wong
Jessica J Kandel
Carrie J Shawber
author_sort June K Wu
title Aberrant lymphatic endothelial progenitors in lymphatic malformation development.
title_short Aberrant lymphatic endothelial progenitors in lymphatic malformation development.
title_full Aberrant lymphatic endothelial progenitors in lymphatic malformation development.
title_fullStr Aberrant lymphatic endothelial progenitors in lymphatic malformation development.
title_full_unstemmed Aberrant lymphatic endothelial progenitors in lymphatic malformation development.
title_sort aberrant lymphatic endothelial progenitors in lymphatic malformation development.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2015-01-01
description Lymphatic malformations (LMs) are vascular anomalies thought to arise from dysregulated lymphangiogenesis. These lesions impose a significant burden of disease on affected individuals. LM pathobiology is poorly understood, hindering the development of effective treatments. In the present studies, immunostaining of LM tissues revealed that endothelial cells lining aberrant lymphatic vessels and cells in the surrounding stroma expressed the stem cell marker, CD133, and the lymphatic endothelial protein, podoplanin. Isolated patient-derived CD133+ LM cells expressed stem cell genes (NANOG, Oct4), circulating endothelial cell precursor proteins (CD90, CD146, c-Kit, VEGFR-2), and lymphatic endothelial proteins (podoplanin, VEGFR-3). Consistent with a progenitor cell identity, CD133+ LM cells were multipotent and could be differentiated into fat, bone, smooth muscle, and lymphatic endothelial cells in vitro. CD133+ cells were compared to CD133- cells isolated from LM fluids. CD133- LM cells had lower expression of stem cell genes, but expressed circulating endothelial precursor proteins and high levels of lymphatic endothelial proteins, VE-cadherin, CD31, podoplanin, VEGFR-3 and Prox1. CD133- LM cells were not multipotent, consistent with a differentiated lymphatic endothelial cell phenotype. In a mouse xenograft model, CD133+ LM cells differentiated into lymphatic endothelial cells that formed irregularly dilated lymphatic channels, phenocopying human LMs. In vivo, CD133+ LM cells acquired expression of differentiated lymphatic endothelial cell proteins, podoplanin, LYVE1, Prox1, and VEGFR-3, comparable to expression found in LM patient tissues. Taken together, these data identify a novel LM progenitor cell population that differentiates to form the abnormal lymphatic structures characteristic of these lesions, recapitulating the human LM phenotype. This LM progenitor cell population may contribute to the clinically refractory behavior of LMs.
url http://europepmc.org/articles/PMC4342011?pdf=render
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