Physiological studies have shown that the Na+-H+ exchanger (NHE) is a major
carrier protein regulating the intracellular pH in the cells of the cochle
a. The presence of multiple forms of the exchanger has been demonstrated by
the recent cloning of four mammalian NHEs, NHE-1 to NHE-4. Despite the str
uctural similarity, these NHE isoforms differ in their tissue distribution,
kinetic characteristics, and responses to external stimuli. The present st
udy was undertaken to examine the expression and distribution of four NHE i
soforms in the guinea pig cochlea. We used reverse transcription-polymerase
chain reaction to assess the expression of NHE-1-4 isoforms and non-radioa
ctive in situ hybridization to examine their localization. Although NHE-2,
-3 and -4 isoform mRNAs could be detected in the cochlear tissue, the NHE-1
message was predominant. Cloned guinea pig NHE-1-4 partial cDNA fragments
were highly homologous to the corresponding rat NHE isoforms. NHE-1 isoform
mRNA was distributed in the hair cells. marginal cells, spiral ligament fi
brocytes, spiral prominence cells and spiral ganglion cells. NHE-1 localize
d in a variety of cochlear cells would contribute to their differential fun
ction. (C) 1999 Elsevier Science B.V. All rights reserved.