Archives
br Materials and methods br Results A
Materials and methods
Results
A first series of experiments explored whether the Ampkα1 isoform is involved in the regulation of cardiac Pkcζ. To this end, HL-1 cardiomyocytes were transfected with a construct encoding constitutively active Prkaa1T183D (CAα1) or with the empty vector as control. Pkcζ phosphorylation at Thr410 was measured in Pkcζ-immunoprecipitated samples. In view of the low abundance of Pkcζ, immunoprecipitation was employed to avoid isoform cross-reaction of the phospho-Pkcζ/λ (Thr410/403) antibody. No significant increase of Pkcζ protein abundance was observed after overexpression of CAα1 (Suppl. Fig. 1). As illustrated in Fig. 1A, overexpression of CAα1 resulted in a significant increase of Pkcζ phosphorylation at Thr410 in HL-1 cardiomyocytes. Moreover, immunostaining and confocal microscopy revealed an increased protein abundance of Pkcζ at the cell membrane of HL-1 cardiomyocytes following CAα1 transfection (Fig. 1B).
Subsequently, RNA interference was used to suppress endogenous Pkcζ gene Obeticholic Acid in HL-1 cardiomyocytes (Suppl. Fig. 2). As shown in Fig. 1C, AP-1-dependent transcriptional activity measured by luciferase reporter assay was significantly higher in CAα1-overexpressing HL-1 cardiomyocytes than in empty vector transfected HL-1 cardiomyocytes, a difference significantly blunted by silencing of Pkcζ. Furthermore, the mRNA levels of the AP-1 target genes: c-Fos, Il6 and Ncx1 were significantly up-regulated by overexpression of CAα1 in HL-1 cardiomyocytes, effects virtually abolished by silencing of Pkcζ (Fig. 1D). Thus, Ampkα1 increases AP-1-dependent transcriptional activity in a Pkcζ-dependent manner.
Additional experiments investigated, whether the effects of Ampkα1 can be mimicked by Ampkα2 or by the Ampk activator 5-Aminoimidazole-4-carboxamide 1-β-D-ribofuranoside (AICAR). As a result, overexpression of constitutively active Prkaa2T172D (CAα2; Suppl. Fig. 3) did not increase c-Fos or Il6, but decreased Ncx1 mRNA expression in HL-1 cardiomyocytes (Fig. 2A). Treatment of HL-1 cardiomyocytes with the Ampk activator AICAR increased c-Fos, but decreased Il6 and Ncx1 mRNA expression (Fig. 2B). To further investigate isoform specificity of the Ampkα1 effects on cardiac AP-1-mediated gene expression, endogenous Prkaa1 or Prkaa2 genes were silenced in HL-1 cardiomyocytes with or without a 24h treatment with 100nM angiotensin-II (Suppl. Fig. 4). Angiotensin-II treatment tended to increase Prkaa1 and Prkaa2 mRNA expression in HL-1 cardiomyocytes (Suppl. Fig. 4). More importantly, angiotensin-II treatment significantly increased AP-1-dependent transcriptional activity in negative control silenced HL-1 cardiomyocytes, an effect significantly blunted following silencing of Prkaa1, but not of Prkaa2 (Fig. 3A). Moreover, the angiotensin-II-induced increase of c-Fos, Il6 and Ncx1 mRNA expression in negative control silenced HL-1 cardiomyocytes, was again significantly inhibited in Prkaa1 silenced HL-1 cardiomyocytes, but not in Prkaa2 silenced HL-1 cardiomyocytes (Fig. 3B–D). Thus, AP-1-dependent transcriptional activity and AP-1 target gene expression is specifically sensitive to the Ampkα1 isoform.
To further explore whether Pkcζ participates in the angiotensin-II-induced regulation of cardiac AP-1-dependent transcriptional activity, the Pkcζ gene was silenced in HL-1 cardiomyocytes with or without treatment with 100nM angiotensin-II (Suppl. Fig. 5). As shown in Fig. 4, AP-1-dependent transcriptional activity (Fig. 4A) and c-Fos, Il6 and Ncx1 mRNA expression (Fig. 4B–D) were all significantly increased by angiotensin-II treatment in negative control silenced HL-1 cardiomyocytes, effects significantly blunted following silencing of Pkcζ. Thus, up-regulation of cardiac AP-1 activity by angiotensin-II requires Pkcζ.
Further experiments investigated whether the Ampkα1 isoform is involved in the regulation of cardiac Pkcζ and AP-1 activity in vivo. To this end, Ampkα1−/− mice and corresponding Ampkα1+/+ mice were infused subcutaneously with either saline or with angiotensin-II. Angiotensin-II treatment for 2weeks induced a comparable increase of blood pressure and heart-weight to body-weight ratio in both genotypes (Suppl. Table 1). Ejection fraction was increased in the Ampkα1−/− mice, but was not significantly different from Ampkα1+/+ mice following angiotensin-II treatment (Suppl. Table 1). However, angiotensin-II treatment significantly increased Ampkα1 protein levels in cardiac tissue from Ampkα1+/+ mice as compared to control treated mice (Fig. 5A). The protein abundance of the Ampkα2 isoform tended to be higher in cardiac tissue from Ampkα1−/− mice than from Ampkα1+/+ mice, an effect, however, not reaching statistical significance (p=0.059, Fig. 5B). Ampkα2 protein levels were not significantly modified by angiotensin-II treatment in cardiac tissues of neither, Ampkα1+/+ mice nor Ampkα1−/− mice (Fig. 5B). Angiotensin-II treatment significantly increased the mRNA expression of the AP-1 target genes c-Fos, Il6 and Ncx1 in cardiac tissue of Ampkα1+/+ mice, effects significantly suppressed in Ampkα1−/− mice (Fig. 5C). These effects were paralleled by similar alterations of cardiac Pkcζ expression. As shown by immunostaining, the expression of Pkcζ protein was barely detectable in myocardial tissue from control treated mice (Fig. 5D). Following angiotensin-II treatment, Pkcζ protein expression was increased in cardiac tissue from Ampkα1+/+ mice, and localized mainly to the intercalated discs. This effect was blunted in cardiac tissue from Ampkα1−/− mice (Fig. 5D). Thus, Ampkα1 deficiency similarly suppresses angiotensin-II-induced cardiac Pkcζ expression and AP-1-target gene expression in vivo.