Tyrosyl phosphorylation of PZR promotes hypertrophic cardiomyopathy in PTPN11-associated Noonan syndrome with multiple lentigines
Jae-Sung Yi, Sravan Perla, Liz Enyenihi, Anton M. Bennett
Jae-Sung Yi, Sravan Perla, Liz Enyenihi, Anton M. Bennett
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Research Article Cardiology

Tyrosyl phosphorylation of PZR promotes hypertrophic cardiomyopathy in PTPN11-associated Noonan syndrome with multiple lentigines

Abstract

Noonan syndrome with multiple lentigines (NSML) is a rare autosomal dominant disorder that presents with cardio-cutaneous-craniofacial defects. Hypertrophic cardiomyopathy (HCM) represents the major life-threatening presentation in NSML. Mutations in the PTPN11 gene that encodes for the protein tyrosine phosphatase (PTP), SHP2, represents the predominant cause of HCM in NSML. NSML-associated PTPN11 mutations render SHP2 catalytically inactive with an “open” conformation. NSML-associated PTPN11 mutations cause hypertyrosyl phosphorylation of the transmembrane glycoprotein, protein zero-related (PZR), resulting in increased SHP2 binding. Here we show that NSML mice harboring a tyrosyl phosphorylation–defective mutant of PZR (NSML/PZRY242F) that is defective for SHP2 binding fail to develop HCM. Enhanced AKT/S6 kinase signaling in heart lysates of NSML mice was reversed in NSML/PZRY242F mice, demonstrating that PZR/SHP2 interactions promote aberrant AKT/S6 kinase activity in NSML. Enhanced PZR tyrosyl phosphorylation in the hearts of NSML mice was found to drive myocardial fibrosis by engaging an Src/NF-κB pathway, resulting in increased activation of IL-6. Increased expression of IL-6 in the hearts of NSML mice was reversed in NSML/PZRY242F mice, and PZRY242F mutant fibroblasts were defective for IL-6 secretion and STAT3-mediated fibrogenesis. These results demonstrate that NSML-associated PTPN11 mutations that induce PZR hypertyrosyl phosphorylation trigger pathophysiological signaling that promotes HCM and cardiac fibrosis.

Authors

Jae-Sung Yi, Sravan Perla, Liz Enyenihi, Anton M. Bennett

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Figure 6

PZR tyrosyl phosphorylation promotes myocardial fibrosis and positively regulates IL-6 expression.

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PZR tyrosyl phosphorylation promotes myocardial fibrosis and positively ...
(AC) Picrosirius red stains of left ventricles from 16-week-old WT (Ptpn11+/+ Mpzl1+/Y242F), NSML (Ptpn11Y279C/+ Mpzl1+/Y242F), PZRY242F (Ptpn11+/+ Mpzl1Y242F/Y242F), and NSML/PZRY242F (Ptpn11Y279C/+ Mpzl1Y242F/Y242F) mice (A) (scale bar: 50 μm). Sirius red–positive areas were quantified (n = 9 for each group; 3 images per mouse, 3 mice per group) (B). The relative mRNA expression levels of Col1a and Col3a in the heart were measured by qRT-PCR (C) (n = 7 for each group). (D) The relative mRNA expression levels of Il1b, Il4, Il6, Il6r, Il10, Il13, Tnf, Ifng, and Crp in the hearts of 16-week-old WT (Ptpn11+/+) and NSML (Ptpn11Y279C/+) mice were measured by qRT-PCR (n = 8 for each group). (EG) Mouse embryonic fibroblasts (MEFs) from WT (Mpzl1+/+) and PZRY242F (Mpzl1Y242F/Y242F+) mice were serum-starved and stimulated with 5 μg/mL of concanavalin A (ConA) for 2 hours. Whole-cell lysates were immunoblotted with anti–p-PZR (Y242), –p-PZR (Y264), and -PZR antibodies (E). The relative mRNA expression of Il6 and Tnf was measured by qRT-PCR (F) (n = 3). (G) MEFs were serum-starved and stimulated with 5 μg/mL of Con A for 1, 2, and 4 hours. Secreted IL-6 protein levels were measured by ELISA (n = 3 for each group). (H) Low-dose dasatinib (0.1 mg/kg/d, i.p.) was administered to 12-week-old WT (Ptpn11+/+) and NSML (Ptpn11Y279C/+) mice for 4 weeks. The relative mRNA expression of Il6 in the heart was measured by qRT-PCR (n = 5 for vehicle-treated WT, n = 7 for vehicle-treated NSML, n = 6 for dasatinib-treated WT, and n = 9 for dasatinib-treated NSML). (I) The relative mRNA expression level of Il6 in the hearts of 16-week-old WT (Ptpn11+/+ Mpzl1+/Y242F), NSML (Ptpn11Y279C/+ Mpzl1+/Y242F), PZRY242F (Ptpn11+/+ Mpzl1Y242F/Y242F), and NSML/PZRY242F (Ptpn11Y279C/+ Mpzl1Y242F/Y242F) mice were measured by quantitative RT-PCR (n = 7 for WT, NSML, and PZRY242F, and n = 8 for NSML/PZRY242F). Serum was collected from 16-week-old mice, and IL-6 protein levels were measured by ELISA (n = 8 for WT and PZRY242F, n = 7 for NSML and NSML/PZRY242F). All data represent mean ± SEM. Statistical significance was analyzed with 2-tailed Student’s t test (D) or 2-way ANOVA (FH) or 1-way ANOVA (B, C, and I) with 2-stage linear step-up procedure of Benjamini, Krieger, and Yekutieli correction for multiple comparisons.