Calcium sensitivity of dicarboxylate transport in cultured proximal tubule cells.

Am J Physiol Renal Physiol

Southeastern Louisiana Veterans Health Care System, Research Service, New Orleans, LA, USA.

Published: February 2011

AI Article Synopsis

  • Researchers investigated how varying levels of extracellular calcium impact citrate and succinate transport in opossum kidney cells, finding that lower calcium significantly enhances transport efficiency without affecting glucose transport.
  • The study concludes that extracellular calcium affects citrate and succinate transport in these cells through a novel mechanism distinct from NaDC1, as demonstrated by differing transport responses in cultured kidney cells and Xenopus oocytes.

Article Abstract

Urinary citrate is an important inhibitor of calcium nephrolithiasis and is primarily determined by proximal tubule reabsorption. The major transporter to reabsorb citrate is Na(+)-dicarboxylate cotransporter (NaDC1), which transports dicarboxylates, including the divalent form of citrate. We previously found that opossum kidney (OK) proximal tubule cells variably express either divalent or trivalent citrate transport, depending on extracellular calcium. The present studies were performed to delineate the mechanism of the effect of calcium on citrate and succinate transport in these cells. Transport was measured using isotope uptake assays. In some studies, NaDC1 transport was studied in Xenopus oocytes, expressing either the rabbit or opossum ortholog. In the OK cell culture model, lowering extracellular calcium increased both citrate and succinate transport by more than twofold; the effect was specific in that glucose transport was not altered. Citrate and succinate were found to reciprocally inhibit transport at low extracellular calcium (<60 μM), but not at normal calcium (1.2 mM); this mutual inhibition is consistent with dicarboxylate transport. The inhibition varied progressively at intermediate levels of extracellular calcium. In addition to changing the relative magnitude and interaction of citrate and succinate transport, decreasing calcium also increased the affinity of the transport process for various other dicarboxylates. Also, the affinity for succinate, at low concentrations of substrate, was increased by calcium removal. In contrast, in oocytes expressing NaDC1, calcium did not have a similar effect on transport, indicating that NaDC1 could not likely account for the findings in OK cells. In summary, extracellular calcium regulates constitutive citrate and succinate transport in OK proximal tubule cells, probably via a novel transport process that is not NaDC1. The calcium effect on citrate transport parallels in vivo studies that demonstrate the regulation of urinary citrate excretion with urinary calcium excretion, a process that may be important in decreasing urinary calcium stone formation.

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http://www.ncbi.nlm.nih.gov/pmc/articles/PMC3043994PMC
http://dx.doi.org/10.1152/ajprenal.00036.2010DOI Listing

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