Modulation of TGF‐β type 1 receptor: Flow cytometric detection with biotinylated TGF‐β
- 1 October 1989
- journal article
- research article
- Published by Wiley in Journal of Cellular Physiology
- Vol. 141 (1) , 170-180
- https://doi.org/10.1002/jcp.1041410125
Abstract
Transforming growth factor β‐ type 1 (TGF‐β) was reacted with NHS‐biotin to yield a derivative of TGF‐β1 which was biotinylated on lysine residues. The biotinylated form of TGF‐β1 was separated from the unreacted material by reverse phase chromatography. In three separate bioassays, the derivatized peptide was as active as the starting material. The use of FITC‐avidin in conjunction with flow cytometry demonstrated that the binding of biotinylated TGF‐β to its receptor is saturable, competable, and specific. A 100‐fold molar excess of unde‐rivatized TGF‐β1 gave 85% inhibition of binding of the biotinylated peptide to the mink lung cell line CCL‐64, while TGF‐β2 showed no inhibition of binding, nor did insulin, calcitonin, or TGF‐α. Both CCL‐64 cells and human umbilical vein endothelial cells showed a density‐dependent down‐regulation of receptor expression in culture. Several factors were examined that might mediate this effect. The down‐regulation was shown not to be due to the secretion of an active form of TGF‐β1. The extracellular matrix from high‐density cells did not decrease expression of the receptor. Fibronectin, collagen, and gelatin were also unable to signal changes in receptor expression, even though in other systems such matrix components can regulate the responsiveness of cells to TGF‐β1. Lastly, staining simultaneously for DNA content and TGF‐β1receptor expression showed that there was no correlation between cell cycle and receptor levels.This publication has 28 references indexed in Scilit:
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