Abstract
Our work suggests an important new link between the RCAN1 gene and Huntington disease. Huntington disease is caused by expansion of glutamine repeats in the huntingtin protein. How the huntingtin protein with expanded polyglutamines (mutant huntingtin) causes the disease is still unclear, but phosphorylation of huntingtin appears to be protective. Increased huntingtin phosphorylation can be produced either by inhibition of the phosphatase calcineurin or by activation of the Akt kinase. The RCAN1 gene encodes regulators of calcineurin, and we now demonstrate, for the first time, that RCAN1-1L is depressed in Huntington disease. We also show that RCAN1-1L overexpression can protect against mutant huntingtin toxicity in an ST14A cell culture model of Huntington disease and that increased phosphorylation of huntingtin via calcineurin inhibition, rather than via Akt induction or activation, is the likely mechanism by which RCAN1-1L may be protective against mutant huntingtin. These findings suggest that RCAN1-1L "deficiency" may actually play a role in the etiology of Huntington disease. In addition, our results allow for the possibility that controlled overexpression of RCAN1-1L in the striatal region of the brain might be a viable avenue for therapeutic intervention in Huntington disease patients (and perhaps other polyglutamine expansion disorders).
Highlights
MAY 1, 2009 VOLUME 284 NUMBER 18 and spinobulbar muscular atrophy are associated with polyglutamine expansion
We have demonstrated that at least two RCAN1 mRNA isoforms are expressed in adult human brain and that the mRNA levels of isoform 1 are much higher than those of isoform 4 [11]
We have tested whether the various potential RCAN1 proteins are expressed in adult human brain, and we found at least three isoforms transcribed in adults: RCAN1-1L, RCAN1–1S, and RCAN1– 4 [5, 12]
Summary
MAY 1, 2009 VOLUME 284 NUMBER 18 and spinobulbar muscular atrophy are associated with polyglutamine expansion. We analyzed the effect of RCAN1-1L on calcineurin activity in dividing ST14A cells as well as in cells induced to differentiate either by hormonal factors or by raising the incubation temperature to 39 °C.
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