A novel human cell culture model to study visceral smooth muscle phenotypic modulation in health and disease

Rianne D. W. Vaes; Linda van den Berk; Bas Boonen; David P. J. van Dijk; Steven W. M. Olde Damink; Sander S. Rensen

doi:10.1152/ajpcell.00167.2017

A novel human cell culture model to study visceral smooth muscle phenotypic modulation in health and disease

Rianne D. W. Vaes^*, Linda van den Berk, Bas Boonen, David P. J. van Dijk, Steven W. M. Olde Damink, Sander S. Rensen

^*Corresponding author for this work

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

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Abstract

Adaptation of the smooth muscle cell (SMC) phenotype is essential for homeostasis and is often involved in pathologies of visceral organs (e.g., uterus, bladder, gastrointestinal tract). In vitro studies of the behavior of visceral SMCs under (patho)-physiological conditions are hampered by a spontaneous, uncontrolled phenotypic modulation of visceral SMCs under regular tissue culture conditions. We aimed to develop a new visceral SMC culture model that allows controlled phenotypic modulation. Human uterine SMCs [ULTR and telomerase-immortalized human myometrial cells (hTERT-HM)] were grown to confluency and kept for up to 6 days on regular tissue culture surfaces or basement membrane (BM) matrix-coated surfaces in the presence of 0-10% serum. mRNA and protein expression and localization of SMC-specific phenotype markers and their transcriptional regulators were investigated by quantitative PCR, Western blotting, and immunofluorescence. Maintaining visceral SMCs confluent for 6 days increased alpha-smooth muscle actin (1.9-fold) and smooth muscle protein 22-alpha (3.1-fold), whereas smooth muscle myosin heavy chain was only slightly upregulated (1.3-fold). Culturing on a BM matrix-coated surface further increased these proteins and also markedly promoted mRNA expression of gamma-smooth muscle actin (15.0-fold), smoothelin (3.5-fold), h-caldesmon (5.2-fold), serum response factor (7.6-fold), and myocardin (8.1-fold). Whereas additional serum deprivation only minimally affected contractile markers, platelet-derived growth factor- BB and transforming growth factor beta 1 consistently reduced versus increased their expression. In conclusion, we present a simple and reproducible visceral SMC culture system that allows controlled phenotypic modulation toward both the synthetic and the contractile phenotype. This may greatly facilitate the identification of factors that drive visceral SMC phenotypic changes in health and disease.

Original language	English
Pages (from-to)	C598-C607
Number of pages	10
Journal	American Journal of Physiology-Cell Physiology
Volume	315
Issue number	4
DOIs	https://doi.org/10.1152/ajpcell.00167.2017
Publication status	Published - Oct 2018

Keywords

basal membrane matrix
differentiation
phenotypic modulation
visceral smooth muscle
EXTRACELLULAR-MATRIX PROTEINS
GENE-EXPRESSION
OUTLET OBSTRUCTION
GROWTH
MYOCARDIN
ALPHA
DIFFERENTIATION
FIBRONECTIN
CONTRACTILE
COLLAGEN

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10.1152/ajpcell.00167.2017

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Cite this

@article{b79106281de344438adf3afa929a127c,

title = "A novel human cell culture model to study visceral smooth muscle phenotypic modulation in health and disease",

abstract = "Adaptation of the smooth muscle cell (SMC) phenotype is essential for homeostasis and is often involved in pathologies of visceral organs (e.g., uterus, bladder, gastrointestinal tract). In vitro studies of the behavior of visceral SMCs under (patho)-physiological conditions are hampered by a spontaneous, uncontrolled phenotypic modulation of visceral SMCs under regular tissue culture conditions. We aimed to develop a new visceral SMC culture model that allows controlled phenotypic modulation. Human uterine SMCs [ULTR and telomerase-immortalized human myometrial cells (hTERT-HM)] were grown to confluency and kept for up to 6 days on regular tissue culture surfaces or basement membrane (BM) matrix-coated surfaces in the presence of 0-10% serum. mRNA and protein expression and localization of SMC-specific phenotype markers and their transcriptional regulators were investigated by quantitative PCR, Western blotting, and immunofluorescence. Maintaining visceral SMCs confluent for 6 days increased alpha-smooth muscle actin (1.9-fold) and smooth muscle protein 22-alpha (3.1-fold), whereas smooth muscle myosin heavy chain was only slightly upregulated (1.3-fold). Culturing on a BM matrix-coated surface further increased these proteins and also markedly promoted mRNA expression of gamma-smooth muscle actin (15.0-fold), smoothelin (3.5-fold), h-caldesmon (5.2-fold), serum response factor (7.6-fold), and myocardin (8.1-fold). Whereas additional serum deprivation only minimally affected contractile markers, platelet-derived growth factor- BB and transforming growth factor beta 1 consistently reduced versus increased their expression. In conclusion, we present a simple and reproducible visceral SMC culture system that allows controlled phenotypic modulation toward both the synthetic and the contractile phenotype. This may greatly facilitate the identification of factors that drive visceral SMC phenotypic changes in health and disease.",

keywords = "basal membrane matrix, differentiation, phenotypic modulation, visceral smooth muscle, EXTRACELLULAR-MATRIX PROTEINS, GENE-EXPRESSION, OUTLET OBSTRUCTION, GROWTH, MYOCARDIN, ALPHA, DIFFERENTIATION, FIBRONECTIN, CONTRACTILE, COLLAGEN",

author = "Vaes, {Rianne D. W.} and {van den Berk}, Linda and Bas Boonen and {van Dijk}, {David P. J.} and Damink, {Steven W. M. Olde} and Rensen, {Sander S.}",

year = "2018",

month = oct,

doi = "10.1152/ajpcell.00167.2017",

language = "English",

volume = "315",

pages = "C598--C607",

journal = "American Journal of Physiology-Cell Physiology",

issn = "0363-6143",

publisher = "American Physiological Society",

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TY - JOUR

T1 - A novel human cell culture model to study visceral smooth muscle phenotypic modulation in health and disease

AU - Vaes, Rianne D. W.

AU - van den Berk, Linda

AU - Boonen, Bas

AU - van Dijk, David P. J.

AU - Damink, Steven W. M. Olde

AU - Rensen, Sander S.

PY - 2018/10

Y1 - 2018/10

N2 - Adaptation of the smooth muscle cell (SMC) phenotype is essential for homeostasis and is often involved in pathologies of visceral organs (e.g., uterus, bladder, gastrointestinal tract). In vitro studies of the behavior of visceral SMCs under (patho)-physiological conditions are hampered by a spontaneous, uncontrolled phenotypic modulation of visceral SMCs under regular tissue culture conditions. We aimed to develop a new visceral SMC culture model that allows controlled phenotypic modulation. Human uterine SMCs [ULTR and telomerase-immortalized human myometrial cells (hTERT-HM)] were grown to confluency and kept for up to 6 days on regular tissue culture surfaces or basement membrane (BM) matrix-coated surfaces in the presence of 0-10% serum. mRNA and protein expression and localization of SMC-specific phenotype markers and their transcriptional regulators were investigated by quantitative PCR, Western blotting, and immunofluorescence. Maintaining visceral SMCs confluent for 6 days increased alpha-smooth muscle actin (1.9-fold) and smooth muscle protein 22-alpha (3.1-fold), whereas smooth muscle myosin heavy chain was only slightly upregulated (1.3-fold). Culturing on a BM matrix-coated surface further increased these proteins and also markedly promoted mRNA expression of gamma-smooth muscle actin (15.0-fold), smoothelin (3.5-fold), h-caldesmon (5.2-fold), serum response factor (7.6-fold), and myocardin (8.1-fold). Whereas additional serum deprivation only minimally affected contractile markers, platelet-derived growth factor- BB and transforming growth factor beta 1 consistently reduced versus increased their expression. In conclusion, we present a simple and reproducible visceral SMC culture system that allows controlled phenotypic modulation toward both the synthetic and the contractile phenotype. This may greatly facilitate the identification of factors that drive visceral SMC phenotypic changes in health and disease.

AB - Adaptation of the smooth muscle cell (SMC) phenotype is essential for homeostasis and is often involved in pathologies of visceral organs (e.g., uterus, bladder, gastrointestinal tract). In vitro studies of the behavior of visceral SMCs under (patho)-physiological conditions are hampered by a spontaneous, uncontrolled phenotypic modulation of visceral SMCs under regular tissue culture conditions. We aimed to develop a new visceral SMC culture model that allows controlled phenotypic modulation. Human uterine SMCs [ULTR and telomerase-immortalized human myometrial cells (hTERT-HM)] were grown to confluency and kept for up to 6 days on regular tissue culture surfaces or basement membrane (BM) matrix-coated surfaces in the presence of 0-10% serum. mRNA and protein expression and localization of SMC-specific phenotype markers and their transcriptional regulators were investigated by quantitative PCR, Western blotting, and immunofluorescence. Maintaining visceral SMCs confluent for 6 days increased alpha-smooth muscle actin (1.9-fold) and smooth muscle protein 22-alpha (3.1-fold), whereas smooth muscle myosin heavy chain was only slightly upregulated (1.3-fold). Culturing on a BM matrix-coated surface further increased these proteins and also markedly promoted mRNA expression of gamma-smooth muscle actin (15.0-fold), smoothelin (3.5-fold), h-caldesmon (5.2-fold), serum response factor (7.6-fold), and myocardin (8.1-fold). Whereas additional serum deprivation only minimally affected contractile markers, platelet-derived growth factor- BB and transforming growth factor beta 1 consistently reduced versus increased their expression. In conclusion, we present a simple and reproducible visceral SMC culture system that allows controlled phenotypic modulation toward both the synthetic and the contractile phenotype. This may greatly facilitate the identification of factors that drive visceral SMC phenotypic changes in health and disease.

KW - basal membrane matrix

KW - differentiation

KW - phenotypic modulation

KW - visceral smooth muscle

KW - EXTRACELLULAR-MATRIX PROTEINS

KW - GENE-EXPRESSION

KW - OUTLET OBSTRUCTION

KW - GROWTH

KW - MYOCARDIN

KW - ALPHA

KW - DIFFERENTIATION

KW - FIBRONECTIN

KW - CONTRACTILE

KW - COLLAGEN

U2 - 10.1152/ajpcell.00167.2017

DO - 10.1152/ajpcell.00167.2017

M3 - Article

C2 - 30044660

SN - 0363-6143

VL - 315

SP - C598-C607

JO - American Journal of Physiology-Cell Physiology

JF - American Journal of Physiology-Cell Physiology

IS - 4

ER -