AJP - Cell Physiology, Vol 253, Issue 6 C872-C882, Copyright © 1987 by American Physiological Society
Interaction of angiotensin II with functional smooth muscle cells in culture
S. Paglin, H. Stukenbrok, N. C. Joyce and J. D. Jamieson
Department of Cell Biology, Yale University School of Medicine, New Haven, Connecticut 06510.
In this study we report on the characterization of a highly enriched
population of cultured vascular smooth muscle cells (SMC) prepared from
collagenase-treated medial layer explant outgrowths of rabbit aortae.
Studies done on cells from first passage explant outgrowths showed that the
cells retain the fine structural features of vascular SMC in situ, can be
immunostained with anti-smooth muscle myosin IgG, and bind
[125I]angiotensin II (ANG II) in a specific and saturable manner with an
apparent Kd of 1 nM. Addition of ANG II (0.1 microM) to the cultures causes
obvious shape changes and retraction of cell processes. Electron
microscopic autoradiography of cells labeled with [125I]ANG II show that
the initial site of interaction of ANG II with the SMC is the plasma
membrane. The distribution of ANG II receptors among cells in the
population was studied using light microscopic autoradiography. The
autoradiographical grain density varied among cells in the population
ranging from cells that were heavily labeled to those that possessed
virtually no label. These data imply that the expression of ANG II
receptors may be limited to a certain progeny within the cell population or
is a function of their stage within the cell cycle.
