Integrin shedding as a mechanism of cellular adaptation during cardiac growth

Edie C. Goldsmith; Wayne Carver; Alex McFadden; Jack G. Goldsmith; Robert L. Price; Mark Sussman; Beverly H. Lorell; Garth Cooper; Thomas K. Borg

doi:10.1152/ajpheart.00920.2002

Integrin shedding as a mechanism of cellular adaptation during cardiac growth

Edie C. Goldsmith, Wayne Carver, Alex McFadden, Jack G. Goldsmith, Robert L. Price, Mark Sussman, Beverly H. Lorell, Garth Cooper, Thomas K. Borg

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

Abstract

Integrin-mediated cell-extracellular matrix (ECM) interactions are essential for multiple cellular processes; however, little is known regarding integrin turnover during these events. Recent studies have demonstrated shedding of cell surface molecules and suggested this as a potential mechanism for integrin turnover. Confocal microscopy of mouse hearts under different physiological conditions demonstrated the presence of β1-integrin-immunbreactive material in the interstitium. Culture media from neonatal rat cardiac myocytes and fibroblasts contained a 55-kDa fragment of β1-integrin. Attachment to ECM components, response to phorbol 12-myristate 13-acetate stimulation, and matrix metalloproteinase inhibition assays demonstrated that fibroblasts responded differently to the fragment compared with myocytes. The β1-integrin fragment stimulated myocyte attachment to collagen and the fragment itself bound a variety of ECM proteins. These studies indicate that as myocytes and fibroblasts change size and shape, cellular contacts with the ECM are altered, resulting in the liberation of a β1-integrin fragment from the cell surface. Integrin shedding may represent a novel mechanism of rapidly modifying cell-ECM contacts during various cellular processes.

Original language	English
Pages (from-to)	H2227-H2234
Journal	American Journal of Physiology: Heart and Circulatory Physiology
Volume	284
Issue number	6
DOIs	https://doi.org/10.1152/ajpheart.00920.2002
Publication status	Published - 1 Jun 2003

Keywords

Extracellular matrix
Hypertrophy
Integrins
Metalloproteinases

Access to Document

10.1152/ajpheart.00920.2002

Cite this

@article{955ebab5567f43c5b99f40b158a19c4c,

title = "Integrin shedding as a mechanism of cellular adaptation during cardiac growth",

abstract = "Integrin-mediated cell-extracellular matrix (ECM) interactions are essential for multiple cellular processes; however, little is known regarding integrin turnover during these events. Recent studies have demonstrated shedding of cell surface molecules and suggested this as a potential mechanism for integrin turnover. Confocal microscopy of mouse hearts under different physiological conditions demonstrated the presence of β1-integrin-immunbreactive material in the interstitium. Culture media from neonatal rat cardiac myocytes and fibroblasts contained a 55-kDa fragment of β1-integrin. Attachment to ECM components, response to phorbol 12-myristate 13-acetate stimulation, and matrix metalloproteinase inhibition assays demonstrated that fibroblasts responded differently to the fragment compared with myocytes. The β1-integrin fragment stimulated myocyte attachment to collagen and the fragment itself bound a variety of ECM proteins. These studies indicate that as myocytes and fibroblasts change size and shape, cellular contacts with the ECM are altered, resulting in the liberation of a β1-integrin fragment from the cell surface. Integrin shedding may represent a novel mechanism of rapidly modifying cell-ECM contacts during various cellular processes.",

keywords = "Extracellular matrix, Hypertrophy, Integrins, Metalloproteinases",

author = "Goldsmith, {Edie C.} and Wayne Carver and Alex McFadden and Goldsmith, {Jack G.} and Price, {Robert L.} and Mark Sussman and Lorell, {Beverly H.} and Garth Cooper and Borg, {Thomas K.}",

note = "HL-37669, NHLBI NIH HHS, United StatesHL-38189, NHLBI NIH HHS, United StatesHL-58224-02, NHLBI NIH HHS, United StatesHL-66035-01, NHLBI NIH HHS, United StatesHL-67245, NHLBI NIH HHS, United StatesP20-RR-16434, NCRR NIH HHS, United States",

year = "2003",

month = jun,

day = "1",

doi = "10.1152/ajpheart.00920.2002",

language = "English",

volume = "284",

pages = "H2227--H2234",

journal = "American Journal of Physiology: Heart and Circulatory Physiology",

issn = "0363-6135",

publisher = "American Physiological Society",

number = "6",

}

TY - JOUR

T1 - Integrin shedding as a mechanism of cellular adaptation during cardiac growth

AU - Goldsmith, Edie C.

AU - Carver, Wayne

AU - McFadden, Alex

AU - Goldsmith, Jack G.

AU - Price, Robert L.

AU - Sussman, Mark

AU - Lorell, Beverly H.

AU - Cooper, Garth

AU - Borg, Thomas K.

N1 - HL-37669, NHLBI NIH HHS, United StatesHL-38189, NHLBI NIH HHS, United StatesHL-58224-02, NHLBI NIH HHS, United StatesHL-66035-01, NHLBI NIH HHS, United StatesHL-67245, NHLBI NIH HHS, United StatesP20-RR-16434, NCRR NIH HHS, United States

PY - 2003/6/1

Y1 - 2003/6/1

N2 - Integrin-mediated cell-extracellular matrix (ECM) interactions are essential for multiple cellular processes; however, little is known regarding integrin turnover during these events. Recent studies have demonstrated shedding of cell surface molecules and suggested this as a potential mechanism for integrin turnover. Confocal microscopy of mouse hearts under different physiological conditions demonstrated the presence of β1-integrin-immunbreactive material in the interstitium. Culture media from neonatal rat cardiac myocytes and fibroblasts contained a 55-kDa fragment of β1-integrin. Attachment to ECM components, response to phorbol 12-myristate 13-acetate stimulation, and matrix metalloproteinase inhibition assays demonstrated that fibroblasts responded differently to the fragment compared with myocytes. The β1-integrin fragment stimulated myocyte attachment to collagen and the fragment itself bound a variety of ECM proteins. These studies indicate that as myocytes and fibroblasts change size and shape, cellular contacts with the ECM are altered, resulting in the liberation of a β1-integrin fragment from the cell surface. Integrin shedding may represent a novel mechanism of rapidly modifying cell-ECM contacts during various cellular processes.

AB - Integrin-mediated cell-extracellular matrix (ECM) interactions are essential for multiple cellular processes; however, little is known regarding integrin turnover during these events. Recent studies have demonstrated shedding of cell surface molecules and suggested this as a potential mechanism for integrin turnover. Confocal microscopy of mouse hearts under different physiological conditions demonstrated the presence of β1-integrin-immunbreactive material in the interstitium. Culture media from neonatal rat cardiac myocytes and fibroblasts contained a 55-kDa fragment of β1-integrin. Attachment to ECM components, response to phorbol 12-myristate 13-acetate stimulation, and matrix metalloproteinase inhibition assays demonstrated that fibroblasts responded differently to the fragment compared with myocytes. The β1-integrin fragment stimulated myocyte attachment to collagen and the fragment itself bound a variety of ECM proteins. These studies indicate that as myocytes and fibroblasts change size and shape, cellular contacts with the ECM are altered, resulting in the liberation of a β1-integrin fragment from the cell surface. Integrin shedding may represent a novel mechanism of rapidly modifying cell-ECM contacts during various cellular processes.

KW - Extracellular matrix

KW - Hypertrophy

KW - Integrins

KW - Metalloproteinases

U2 - 10.1152/ajpheart.00920.2002

DO - 10.1152/ajpheart.00920.2002

M3 - Article

C2 - 12573995

SN - 0363-6135

VL - 284

SP - H2227-H2234

JO - American Journal of Physiology: Heart and Circulatory Physiology

JF - American Journal of Physiology: Heart and Circulatory Physiology

IS - 6

ER -

Integrin shedding as a mechanism of cellular adaptation during cardiac growth

Abstract

Keywords

Access to Document

Fingerprint

Cite this