Urinary proteome pattern in children with renal Fanconi syndrome

doi:10.1093/ndt/gfp063

NDT Advance Access originally published online on February 18, 2009
Nephrology Dialysis Transplantation 2009 24(7):2161-2169; doi:10.1093/ndt/gfp063

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Urinary proteome pattern in children with renal Fanconi syndrome

Jens Drube¹^,*, Eric Schiffer²^,*, Harald Mischak², Markus J. Kemper³, Thomas Neuhaus⁴, Lars Pape¹, Ralf Lichtinghagen⁵ and Jochen H. H. Ehrich¹

¹ Department of Paediatric Nephrology, Children's Hospital, Hannover Medical School ² Mosaiques Diagnostics and Therapeutics AG, Hannover ³ Department of Paediatric Nephrology, Hamburg University Hospital, Hamburg, Germany ⁴ Department of Paediatric Nephrology, University Children's Hospital, Zurich, Switzerland ⁵ Department of Clinical Chemistry, Hannover Medical School, Germany

Correspondence and offprint requests to: Jens Drube; E-mail: jens.drube{at}web.de

Abstract

Background. The renal Fanconi syndrome (FS) is characterizedby renal glucosuria, loss of electrolytes, bicarbonate and lactate,generalized hyperaminoaciduria and low-molecular-weight proteinuria.We studied the urinary low-molecular-weight proteome to identifyexcreted peptides indicative of a pathogenetic mechanism leadingto tubular dysfunction.

Methods. We established a urinary proteome pattern using capillaryelectrophoresis mass spectrometry (CE-MS) of 7 paediatric patientswith cystinosis and 6 patients with ifosfamide-induced FS asthe study group, and 54 healthy volunteers and 45 patients sufferingfrom other renal diseases such as lupus nephritis (n = 8), focalsegmental glomerulosclerosis (n = 27), minimal change disease(n = 7) and membranous glomerulonephritis (n = 3) as controls.Consequently, we conducted a blinded study consisting of 11FS patients and 9 patients with renal disease other than FS.Additionally, we applied this pattern to 294 previously measuredsamples of patients with different renal diseases. Amino acidsequences of some marker proteins were obtained.

Results. Specificity for detecting FS was 89% and sensitivitywas 82%. The marker peptides constituting the proteome patternare fragments derived from osteopontin, uromodulin and collagenalpha-1.

Conclusions. CE-MS can be used to diagnose FS in paediatricpatients and might be a future tool for the non-invasive diagnosisof FS. The reduced amount of the marker proteins osteopontinand uromodulin indicates loss of function of tubular excretionin all patients suffering from FS regardless of the underlyingcause. In addition, the six different fragments of the collagenalpha-1 (I) chain were either elevated or reduced in the urine.This indicates a change of proteases in collagen degradationas observed in interstitial fibrosis. These changes were prominentirrespectively of the stages of FS. This indicates fibrosisas an early starting pathogenetic reason for the developmentof renal insufficiency in FS patients.

Keywords: capillary electrophoresis; DeToni-Debré-Fanconi-syndrome; mass spectrometry; pathomechanism; proteomics

^* Both authors contributed equally to this work.

Received for publication: 22. 8.08
Accepted in revised form: 29. 1.09

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