4.6 Article

Differential expression of claudin tight junction proteins in the human cortical nephron

期刊

NEPHROLOGY DIALYSIS TRANSPLANTATION
卷 25, 期 7, 页码 2107-2119

出版社

OXFORD UNIV PRESS
DOI: 10.1093/ndt/gfq006

关键词

claudins; glycolmethacrylate; paracellular permeability; renal tubule; tight junctions

资金

  1. Wessex Renal Research and Transplant Unit
  2. Queen Alexandra Hospital
  3. Cosham
  4. Portsmouth UK

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Methods. A survey of claudin staining was performed on human kidney cortex embedded in glycolmethacrylate resin to enhance tissue morphology and facilitate the cutting of 2 mu m serial sections. Results. Claudin-2, -10 and -11 antibodies labelled renal tubular epithelial cells, correlating with Lotus tetragonolobus and N-cadherin positive proximal tubules. Claudin-3, -10, -11 and -16 antibodies strongly stained a population of tubules that were positive for Tamm Horsfall protein on adjacent sections, confirming expression in the thick ascending limb of the Loop of Henle. Claudin-3, -4 and -8 antibodies reacted with tubules that correlated with the distal nephron markers, E-cadherin, epithelial membrane antigen and Dolichos biflorus and claudin-3, -4, -7 and -8 with the distal tubule marker, calbindin, and the collecting duct marker, aquaporin-2. Claudin-14 was localized in distal convoluted tubules, correlating positively with calbindin but negatively with aquaporin-2, whereas claudin-1 staining was identified in the parietal epithelium of Bowman's capsule, distal convoluted tubule and collecting duct. Cellular and tight junction localization of claudin staining in renal tubules was heterogeneous and is discussed. Conclusions. Complex variation in the expression of human claudins likely determines paracellular permeability in the kidney. Altered claudin expression may influence pathologies involving abnormalities of absorption.

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