Fibroblast deletion of ROCK2 attenuates cardiac hypertrophy, fibrosis, and diastolic dysfunction
Toru Shimizu, Nikhil Narang, Phetcharat Chen, Brian Yu, Maura Knapp, Jyothi Janardanan, John Blair, James K. Liao
Toru Shimizu, Nikhil Narang, Phetcharat Chen, Brian Yu, Maura Knapp, Jyothi Janardanan, John Blair, James K. Liao
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Research Article Cardiology

Fibroblast deletion of ROCK2 attenuates cardiac hypertrophy, fibrosis, and diastolic dysfunction

Abstract

Although left ventricular (LV) diastolic dysfunction is often associated with hypertension, little is known regarding its underlying pathophysiological mechanism. Here, we show that the actin cytoskeletal regulator, Rho-associated coiled-coil containing kinase-2 (ROCK2), is a critical mediator of LV diastolic dysfunction. In response to angiotensin II (Ang II), mutant mice with fibroblast-specific deletion of ROCK2 (ROCK2Postn–/–) developed less LV wall thickness and fibrosis, along with improved isovolumetric relaxation. This corresponded with decreased connective tissue growth factor (CTGF) and fibroblast growth factor–2 (FGF2) expression in the hearts of ROCK2Postn–/– mice. Indeed, knockdown of ROCK2 in cardiac fibroblasts leads to decreased expression of CTGF and secretion of FGF2, and cardiomyocytes incubated with conditioned media from ROCK2-knockdown cardiac fibroblasts exhibited less hypertrophic response. In contrast, mutant mice with elevated fibroblast ROCK activity exhibited enhanced Ang II–stimulated cardiac hypertrophy and fibrosis. Clinically, higher leukocyte ROCK2 activity was observed in patients with diastolic dysfunction compared with age- and sex-matched controls, and correlated with higher grades of diastolic dysfunction by echocardiography. These findings indicate that fibroblast ROCK2 is necessary to cause cardiac hypertrophy and fibrosis through the induction CTGF and FGF2, and they suggest that targeting ROCK2 may have therapeutic benefits in patients with LV diastolic dysfunction.

Authors

Toru Shimizu, Nikhil Narang, Phetcharat Chen, Brian Yu, Maura Knapp, Jyothi Janardanan, John Blair, James K. Liao

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Figure 1

Deletion of ROCK2 in angiotensin II–induced (Ang II–induced) activated cardiac fibroblasts from fibroblast-specific ROCK2-deficient (ROCK2Postn–/–) mice.

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Deletion of ROCK2 in angiotensin II–induced (Ang II–induced) activated c...
(A) Representative fluorescent sections from hearts double-stained with ROCK2 (green) and periostin (red) in ROCK2Postn–/– and littermate control (ROCK2flox/flox) mice at 4 wk after saline or Ang II infusion. Nuclei are stained with DAPI (blue). The nuclei of cardiac fibroblasts are elongated in the direction of cardiomyocytes, and their cytoplasms are substantially reduced in volume. Activated cardiac fibroblasts (arrowheads) are identified as periostin-expressing spindle-shaped cells in ROCK2flox/flox mice treated with Ang II (n = 4–5 each). Scale bars: 10 μm. (B–D) Quantitative PCR analysis of Rock2, Rock1, and Acta2 (encoding α-smooth muscle actin) mRNA expression in cardiac fibroblasts isolated from ROCK2Postn–/– and ROCK2flox/flox mice treated with saline or Ang II (n = 4–5 each). **P < 0.01 vs. saline-treated ROCK2flox/flox mice. ##P < 0.01 vs. Ang II-treated ROCK2flox/flox mice. Data are expressed as mean ± SEM. P values were calculated using one-way ANOVA with Tukey’s HSD test.