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Mutations in the protein kinase A R1α regulatory subunit cause familial cardiac myxomas and Carney complex
Mairead Casey, … , Cynthia C. Morton, Craig T. Basson
Mairead Casey, … , Cynthia C. Morton, Craig T. Basson
Published September 1, 2000
Citation Information: J Clin Invest. 2000;106(5):R31-R38. https://doi.org/10.1172/JCI10841.
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Mutations in the protein kinase A R1α regulatory subunit cause familial cardiac myxomas and Carney complex

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Abstract

Cardiac myxomas are benign mesenchymal tumors that can present as components of the human autosomal dominant disorder Carney complex. Syndromic cardiac myxomas are associated with spotty pigmentation of the skin and endocrinopathy. Our linkage analysis mapped a Carney complex gene defect to chromosome 17q24. We now demonstrate that the PRKAR1α gene encoding the R1α regulatory subunit of cAMP-dependent protein kinase A (PKA) maps to this chromosome 17q24 locus. Furthermore, we show that PRKAR1α frameshift mutations in three unrelated families result in haploinsufficiency of R1α and cause Carney complex. We did not detect any truncated R1α protein encoded by mutant PRKAR1α. Although cardiac tumorigenesis may require a second somatic mutation, DNA and protein analyses of an atrial myxoma resected from a Carney complex patient with a PRKAR1α deletion revealed that the myxoma cells retain both the wild-type and the mutant PRKAR1α alleles and that wild-type R1α protein is stably expressed. However, in this atrial myxoma, we did observe a reversal of the ratio of R1α to R2β regulatory subunit protein, which may contribute to tumorigenesis. Further investigation will elucidate the cell-specific effects of PRKAR1α haploinsufficiency on PKA activity and the role of PKA in cardiac growth and differentiation.

Authors

Mairead Casey, Carl J. Vaughan, Jie He, Cathy J. Hatcher, Jordan M. Winter, Stanislawa Weremowicz, Kate Montgomery, Raju Kucherlapati, Cynthia C. Morton, Craig T. Basson

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Figure 5

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Western blot analysis of R1α and R2β in normal lymphoblasts, Carney comp...
Western blot analysis of R1α and R2β in normal lymphoblasts, Carney complex lymphoblasts, and Carney complex cardiac myxoma. (a) Positive controls for antibodies to R1α and R2β were electrophoresed and Western blotted as described in Methods. (b, c) Protein lysates of lymphoblasts from (b) a normal individual and (c) an individual affected by Carney complex (family YA, IV-1) were electrophoresed and analyzed. Densitometry revealed similar levels of R2β protein in the two samples but a 60% decrease in R1α levels. (d) R1α and R2β were analyzed in lysate from a left atrial myxoma resected from individual IV-1 in family YA. Densitometry was used to determine R1α and R2β expression in all samples, and the ratio of R1α:R2β was calculated. A reversal of the R1α:R2β ratio is observed in the tumor sample compared with affected and unaffected lymphocytes.

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ISSN: 0021-9738 (print), 1558-8238 (online)

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