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Force spectroscopy of hepatocytic extracellular matrix components.

作者信息

Yongsunthon R, Baker W A, Bryhan M D, Baker D E, Chang T, Petzold O N, Walczak W J, Liu J, Faris R A, Senaratne W, Seeley L A, Youngman R E

机构信息

Corning Incorporated, SP-FR-01, R1S32D, Corning, NY 14831, USA.

出版信息

Ultramicroscopy. 2009 Jul;109(8):942-7. doi: 10.1016/j.ultramic.2009.03.007. Epub 2009 Mar 19.

Abstract

We present atomic force microscopy and force spectroscopy data of live hepatocytes (HEPG2/C3A liver cell line) grown in Eagle's Minimum Essential Medium, a complex solution of salts and amino acids commonly used for cell culture. Contact-mode imaging and force spectroscopy of this system allowed correlation of cell morphology and extracellular matrix (ECM) properties with substrate properties. Force spectroscopy analysis of cellular "footprints" indicated that the cells secrete large polymers (e.g., 3.5mum contour length and estimated MW 1000kDa) onto their substrate surface. Although definitive identification of the polymers has not yet been achieved, fluorescent-labeled antibody staining has specified the presence of ECM proteins such as collagen and laminin in the cellular footprints. The stretched polymers appear to be much larger than single molecules of known ECM components, such as collagen and heparan sulfate proteoglycan, thus suggesting that the cells create larger entangled, macromolecular structures from smaller components. There is strong evidence which suggests that the composition of the ECM is greatly influenced by the hydrophobicity of the substrate surface, with preferential production and/or adsorption of larger macromolecules on hydrophobic surfaces.

摘要

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