The liver and kidney expression of sulfate anion transporter sat-1 in rats exhibits male-dominant gender differences

被引:22
作者
Brzica, Hrvoje [1 ]
Breljak, Davorka [1 ]
Krick, Wolfgang [3 ]
Lovric, Mila [2 ]
Burckhardt, Gerhard [3 ]
Burckhardt, Birgitta C. [3 ]
Sabolic, Ivan [1 ]
机构
[1] Inst Med Res & Occupat Hlth, Unit Mol Toxicol, Zagreb 10001, Croatia
[2] Univ Zagreb, Ctr Hosp, Clin Inst Lab Diag, Zagreb 10000, Croatia
[3] Univ Med Gottingen, Abt Vegetat Physiol & Pathophysiol, Zentrum Physiol & Pathophysiol, D-37073 Gottingen, Germany
来源
PFLUGERS ARCHIV-EUROPEAN JOURNAL OF PHYSIOLOGY | 2009年 / 457卷 / 06期
关键词
Estrogen; Oxalate; Proximal tubules; Sex hormones; Sulfate; Urolithiasis; Progesterone; Testosterone; Sex differences; Sexual dimorphism; OXALATE TRANSPORT; ESTROGEN SULFOTRANSFERASE; BASOLATERAL MEMBRANE; TISSUE DISTRIBUTION; PROXIMAL TUBULE; STONE FORMATION; SEX-HORMONES; GENE SAT1; EXCHANGE; CLONING;
D O I
10.1007/s00424-008-0611-5
中图分类号
Q4 [生理学];
学科分类号
071003 ;
摘要
The sulfate anion transporter (sat-1, Slc26a1) has been cloned from rat liver, functionally characterized, and localized to the sinusoidal membrane in hepatocytes and basolateral membrane (BLM) in proximal tubules (PT). Here, we confirm previously described localization of sat-1 protein in rat liver and kidneys and report on gender differences (GD) in its expression by immunochemical, transport, and excretion studies in rats. The similar to 85-kDa sat-1 protein was localized to the sinusoidal membrane in hepatocytes and BLM in renal cortical PT, with the male-dominant expression. However, the real-time reverse-transcription polymerase chain reaction data indicated no GD at the level of sat-1 mRNA. In agreement with the protein data, isolated membranes from both organs exhibited the male-dominant exchange of radiolabeled sulfate for oxalate, whereas higher oxalate in plasma and 24-h urine indicated higher oxalate production and excretion in male rats. Furthermore, the expression of liver, but not renal, sat-1 protein was: unaffected by castration, upregulated by ovariectomy, and downregulated by estrogen or progesterone treatment in males. Therefore, GD (males > females) in the expression of sat-1 protein in rat liver (and, possibly, kidneys) are caused by the female sex-hormone-driven inhibition at the posttranscriptional level. The male-dominant abundance of sat-1 protein in liver may conform to elevated uptake of sulfate and extrusion of oxalate, causing higher plasma oxalate in males. Oxalate is then excreted by the kidneys via the basolateral sat-1 (males > females) and the apical CFEX (Slc26a6; GD unknown) in PT and eliminated in the urine (males > females), where it may contribute to the male-prevailing development of oxalate urolithiasis.
引用
收藏
页码:1381 / 1392
页数:12
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