Junb regulates arterial contraction capacity, cellular contractility, and motility via its target Myl9 in mice
Alexander H. Licht, … , Thomas Korff, Marina Schorpp-Kistner
Alexander H. Licht, … , Thomas Korff, Marina Schorpp-Kistner
Published June 14, 2010
Citation Information: J Clin Invest. 2010;120(7):2307-2318. https://doi.org/10.1172/JCI41749.
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Research Article Vascular biology

Junb regulates arterial contraction capacity, cellular contractility, and motility via its target Myl9 in mice

Abstract

Cellular contractility and, thus, the ability to alter cell shape are prerequisites for a number of important biological processes such as cytokinesis, movement, differentiation, and substrate adherence. The contractile capacity of vascular smooth muscle cells (VSMCs) is pivotal for the regulation of vascular tone and thus blood pressure and flow. Here, we report that conditional ablation of the transcriptional regulator Junb results in impaired arterial contractility in vivo and in vitro. This was exemplified by resistance of Junb-deficient mice to DOCA-salt–induced volume-dependent hypertension as well as by a decreased contractile capacity of isolated arteries. Detailed analyses of Junb-deficient VSMCs, mouse embryonic fibroblasts, and endothelial cells revealed a general failure in stress fiber formation and impaired cellular motility. Concomitantly, we identified myosin regulatory light chain 9 (Myl9), which is critically involved in actomyosin contractility and stress fiber assembly, as a Junb target. Consistent with these findings, reexpression of either Junb or Myl9 in Junb-deficient cells restored stress fiber formation, cellular motility, and contractile capacity. Our data establish a molecular link between the activator protein–1 transcription factor subunit Junb and actomyosin-based cellular motility as well as cellular and vascular contractility by governing Myl9 transcription.

Authors

Alexander H. Licht, Tobias Nübel, Anja Feldner, Nathalie Jurisch-Yaksi, Marco Marcello, Elena Demicheva, Jun-Hao Hu, Bettina Hartenstein, Hellmut G. Augustin, Markus Hecker, Peter Angel, Thomas Korff, Marina Schorpp-Kistner

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Figure 2

Contraction failure of second-order mesenteric artery branches derived from Junb-deficient mice.

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Contraction failure of second-order mesenteric artery branches derived f...
(A) Relative increase in diameter of mesenteric artery segments from control and JunbΔ/– mice challenged with increasing intraluminal pressure. Diameter of unchallenged arteries was set to 100 %. ΔP, pressure difference at which segments were perfused. Results were obtained from 6 independent segments from 3 individual mice of each genotype. (B) Concentration-dependent decrease in luminal arterial diameter of mesenteric artery branches derived from control and JunbΔ/– mice upon treatment with the vasoconstrictive agent norepinephrine is shown. Mesenteric artery branches were denuded by perfusion with an incompatible culture medium (right) or left intact (left) prior to norepinephrine exposure. Vessel integrity or EC removal was confirmed by immunofluorescence costaining for CD31 and α-SMA. Nuclei were counterstained with Hoechst 33342 (blue). Scale bars: 200 μm. In each case, one representative staining of sections of at least 3 different mice is shown. Data are presented as mean ± SEM (n = 6). **P < 0.01, *P < 0.05.