Targeted inhibition of p38 MAPK promotes hypertrophic cardiomyopathy through upregulation of calcineurin-NFAT signaling
Julian C. Braz, Orlando F. Bueno, Qiangrong Liang, Benjamin J. Wilkins, Yan-Shan Dai, Stephanie Parsons, Joseph Braunwart, Betty J. Glascock, Raisa Klevitsky, Thomas F. Kimball, Timothy E. Hewett, Jeffery D. Molkentin
Julian C. Braz, Orlando F. Bueno, Qiangrong Liang, Benjamin J. Wilkins, Yan-Shan Dai, Stephanie Parsons, Joseph Braunwart, Betty J. Glascock, Raisa Klevitsky, Thomas F. Kimball, Timothy E. Hewett, Jeffery D. Molkentin
View: Text | PDF
Article Cardiology

Targeted inhibition of p38 MAPK promotes hypertrophic cardiomyopathy through upregulation of calcineurin-NFAT signaling

Abstract

The MAPKs are important transducers of growth and stress stimuli in virtually all eukaryotic cell types. In the mammalian heart, MAPK signaling pathways have been hypothesized to regulate myocyte growth in response to developmental signals or physiologic and pathologic stimuli. Here we generated cardiac-specific transgenic mice expressing dominant-negative mutants of p38α, MKK3, or MKK6. Remarkably, attenuation of cardiac p38 activity produced a progressive growth response and myopathy in the heart that correlated with the degree of enzymatic inhibition. Moreover, dominant-negative p38α, MKK3, and MKK6 transgenic mice each showed enhanced cardiac hypertrophy following aortic banding, Ang II infusion, isoproterenol infusion, or phenylephrine infusion for 14 days. A mechanism underlying this enhanced-growth profile was suggested by the observation that dominant-negative p38α directly augmented nuclear factor of activated T cells (NFAT) transcriptional activity and its nuclear translocation. In vivo, NFAT-dependent luciferase reporter transgenic mice showed enhanced activation in the presence of the dominant-negative p38α transgene before and after the onset of cardiac hypertrophy. More significantly, genetic disruption of the calcineurin Aβ gene rescued hypertrophic cardiomyopathy and depressed functional capacity observed in p38-inhibited mice. Collectively, these observations indicate that reduced p38 signaling in the heart promotes myocyte growth through a mechanism involving enhanced calcineurin-NFAT signaling.

Authors

Julian C. Braz, Orlando F. Bueno, Qiangrong Liang, Benjamin J. Wilkins, Yan-Shan Dai, Stephanie Parsons, Joseph Braunwart, Betty J. Glascock, Raisa Klevitsky, Thomas F. Kimball, Timothy E. Hewett, Jeffery D. Molkentin

×

Figure 5

Options: View larger image (or click on image) Download as PowerPoint
p38 signaling regulates NFAT transcriptional responses. (a) Transient tr...
p38 signaling regulates NFAT transcriptional responses. (a) Transient transfections in neonatal cardiomyocytes using an NFAT-dependent luciferase reporter plasmid with vectors encoding either NFATc4, activated CnA, dnMKK3, or dnp38α and combinations thereof. The data demonstrate that p38 inhibition activates the NFAT reporter in cardiomyocytes (*P < 0.05 versus vector alone). (b) This p38 inhibitory effect was surveyed against all four NFAT factors in 10T1/2 cells (NFATc1-c4). The data demonstrate that dnp38α cotransfection activates NFATc1, NFATc2, and NFATc4 transcription nearly as well as activated calcineurin. Similar results were observed in two additional, independent experiments (*P < 0.05 versus NFAT alone). (c) Recombinant adenovirus encoding NFATc1-GFP was used to evaluate nuclear translocation in cultured cardiomyocytes. Control coinfection with adenovirus-encoding β-galactosidase (Adβgal) did not induce NFATc1-GFP nuclear translocation, distinct from the effect of CnA adenovirus (AdCnA; activated). The dnp38α-encoding adenovirus (Ad-dnp38α) induced significant NFATc1 nuclear translocation. These results were quantified in approximately 250 infected cardiomyocytes. Arrows, cells with cytoplasmic NFAT-GFP; arrowheads, cells with nuclear NFAT-GFP. Similar results were observed in three independent experiments (*P < 0.05 versus Adβgal).