Abolished InsP3R2 function inhibits sweat secretion in both humans and mice
Joakim Klar, … , Katsuhiko Mikoshiba, Niklas Dahl
Joakim Klar, … , Katsuhiko Mikoshiba, Niklas Dahl
Published October 20, 2014
Citation Information: J Clin Invest. 2014;124(11):4773-4780. https://doi.org/10.1172/JCI70720.
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Abolished InsP3R2 function inhibits sweat secretion in both humans and mice

Abstract

There are 3 major sweat-producing glands present in skin; eccrine, apocrine, and apoeccrine glands. Due to the high rate of secretion, eccrine sweating is a vital regulator of body temperature in response to thermal stress in humans; therefore, an inability to sweat (anhidrosis) results in heat intolerance that may cause impaired consciousness and death. Here, we have reported 5 members of a consanguineous family with generalized, isolated anhidrosis, but morphologically normal eccrine sweat glands. Whole-genome analysis identified the presence of a homozygous missense mutation in ITPR2, which encodes the type 2 inositol 1,4,5-trisphosphate receptor (InsP3R2), that was present in all affected family members. We determined that the mutation is localized within the pore forming region of InsP3R2 and abrogates Ca2+ release from the endoplasmic reticulum, which suggests that intracellular Ca2+ release by InsP3R2 in clear cells of the sweat glands is important for eccrine sweat production. Itpr2–/– mice exhibited a marked reduction in sweat secretion, and evaluation of sweat glands from Itpr2–/– animals revealed a decrease in Ca2+ response compared with controls. Together, our data indicate that loss of InsP3R2-mediated Ca2+ release causes isolated anhidrosis in humans and suggest that specific InsP3R inhibitors have the potential to reduce sweat production in hyperhidrosis.

Authors

Joakim Klar, Chihiro Hisatsune, Shahid M. Baig, Muhammad Tariq, Anna C.V. Johansson, Mahmood Rasool, Naveed Altaf Malik, Adam Ameur, Kotomi Sugiura, Lars Feuk, Katsuhiko Mikoshiba, Niklas Dahl

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Figure 3

The p.G2498S mutation abolishes the channel activity of InsP3R2.

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The p.G2498S mutation abolishes the channel activity of InsP3R2. (A) Exp...
(A) Expression of WT and mutant p.G2498S mouse InsP3R2 in 3 independent stable clones. (B) Intracellular Ca2+ signals upon IgM stimulation in R23-11 cells expressing WT and p.G2498S mouse InsP3R2 variants. Arrows denote IgM stimulation (M4) at 0.25 μg/ml. Ca2+ signals from 2 independent p.G2498S InsP3R2 clones and 1 WT InsP3R2 clone were analyzed. Representative data (ratio change of Fura-2) from 4 independent experiments are shown. Cells expressing p.G2498S InsP3R2 exhibited no detectable Ca2+ signal in response to IgM stimulation (0%; n = 50 cells). Of WT InsP3R2 cells, 78% showed Ca2+ oscillation, 14% were Ca2+ transient, and 8% exhibited no response (n = 139 cells).