AJP - Cell Physiology, Vol 263, Issue 6 C1241-C1249, Copyright © 1992 by American Physiological Society
Expression of the Na-Ca exchanger in diverse tissues: a study using the cloned human cardiac Na-Ca exchanger
P. Kofuji, R. W. Hadley, R. S. Kieval, W. J. Lederer and D. H. Schulze
Department of Pharmacology and Experimental Therapeutics, School of Medicine, University of Maryland, Baltimore 21201.
In many cells including cardiac myocytes, cytoplasmic Ca is importantly
controlled by the plasmalemmal Na-Ca exchanger (3, 8). The tissue diversity
and differences in cellular environment raise the question whether the same
exchanger is found in all tissues. Recent experiments using rod cells have
demonstrated that at least two forms of Na-dependent Ca transport exist. We
have examined this issue in various rat and human tissues using the cloned
human cardiac Na-Ca exchanger cDNA. Northern blot analysis in these two
species show that the major transcript of the Na-Ca exchanger is 7.2
kilobases in heart, brain, kidney, liver, pancreas, skeletal muscle,
placenta, and lung. Furthermore, ribonuclease protection analysis in rats
shows conservation of the 348-base pair segment tested in heart, brain,
kidney, skeletal muscle, and liver. Additionally, Southern blot analysis
suggests that a single gene encodes this Na-Ca exchanger. Finally, we show
that the clone used to generate our probes encodes a completely functional
Na-Ca exchanger. With the use of COS cells and 293 cells transfected with
the cloned human cardiac Na-Ca exchanger, we tested the Ca transport
properties of the Na-Ca exchanger, the voltage dependence of the Na-Ca
exchanger, as well as the Na dependence of the transport function of the
Na-Ca exchanger. We conclude that the cardiac form of the Na-Ca exchanger
is completely functional when the cDNA is expressed in mammalian cell
lines, and, furthermore, this "cardiac" form of the Na-Ca exchanger is
naturally expressed in all human and rat tissues tested (but at varying
levels).
