Functional Genomic Analysis Identifies Indoxyl Sulfate as a Major, Poorly Dialyzable Uremic Toxin in End-Stage Renal Disease

BACKGROUND: Chronic renal failure is characterized by progressive renal scarring and accelerated arteriosclerotic cardiovascular disease despite what is considered to be adequate hemodialysis or peritoneal dialysis. In rodents with reduced renal mass, renal scarring has been attributed to poorly fil...

Descripción completa

Detalles Bibliográficos
Autores principales: Jhawar, Sachin, Singh, Prabhjot, Torres, Daniel, Ramirez-Valle, Francisco, Kassem, Hania, Banerjee, Trina, Dolgalev, Igor, Heguy, Adriana, Zavadil, Jiri, Lowenstein, Jerome
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2015
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4374671/
https://www.ncbi.nlm.nih.gov/pubmed/25811877
http://dx.doi.org/10.1371/journal.pone.0118703
_version_ 1782363522998468608
author Jhawar, Sachin
Singh, Prabhjot
Torres, Daniel
Ramirez-Valle, Francisco
Kassem, Hania
Banerjee, Trina
Dolgalev, Igor
Heguy, Adriana
Zavadil, Jiri
Lowenstein, Jerome
author_facet Jhawar, Sachin
Singh, Prabhjot
Torres, Daniel
Ramirez-Valle, Francisco
Kassem, Hania
Banerjee, Trina
Dolgalev, Igor
Heguy, Adriana
Zavadil, Jiri
Lowenstein, Jerome
author_sort Jhawar, Sachin
collection PubMed
description BACKGROUND: Chronic renal failure is characterized by progressive renal scarring and accelerated arteriosclerotic cardiovascular disease despite what is considered to be adequate hemodialysis or peritoneal dialysis. In rodents with reduced renal mass, renal scarring has been attributed to poorly filtered, small protein-bound molecules. The best studied of these is indoxyl sulfate (IS). METHODS: We have attempted to establish whether there are uremic toxins that are not effectively removed by hemodialysis. We examined plasma from patients undergoing hemodialysis, employing global gene expression in normal human renal cortical cells incubated in pre- and post- dialysis plasma as a reporter system. Responses in cells incubated with pre- and post-dialysis uremic plasma (n = 10) were compared with responses elicited by plasma from control subjects (n = 5). The effects of adding IS to control plasma and of adding probenecid to uremic plasma were examined. Plasma concentrations of IS were measured by HPLC (high pressure liquid chromatography). RESULTS: Gene expression in our reporter system revealed dysregulation of 1912 genes in cells incubated with pre-dialysis uremic plasma. In cells incubated in post-dialysis plasma, the expression of 537 of those genes returned to baseline but the majority of them (1375) remained dysregulated. IS concentration was markedly elevated in pre- and post-dialysis plasma. Addition of IS to control plasma simulated more than 80% of the effects of uremic plasma on gene expression; the addition of probenecid, an organic anion transport (OAT) inhibitor, to uremic plasma reversed the changes in gene expression. CONCLUSION: These findings provide evidence that hemodialysis fails to effectively clear one or more solutes that effect gene expression, in our reporter system, from the plasma of patients with uremia. The finding that gene dysregulation was simulated by the addition of IS to control plasma and inhibited by addition of an OAT inhibitor to uremic plasma identifies IS as a major, poorly dialyzable, uremic toxin. The signaling pathways initiated by IS and possibly other solutes not effectively removed by dialysis may participate in the pathogenesis of renal scarring and uremic vasculopathy.
format Online
Article
Text
id pubmed-4374671
institution National Center for Biotechnology Information
language English
publishDate 2015
publisher Public Library of Science
record_format MEDLINE/PubMed
spelling pubmed-43746712015-04-04 Functional Genomic Analysis Identifies Indoxyl Sulfate as a Major, Poorly Dialyzable Uremic Toxin in End-Stage Renal Disease Jhawar, Sachin Singh, Prabhjot Torres, Daniel Ramirez-Valle, Francisco Kassem, Hania Banerjee, Trina Dolgalev, Igor Heguy, Adriana Zavadil, Jiri Lowenstein, Jerome PLoS One Research Article BACKGROUND: Chronic renal failure is characterized by progressive renal scarring and accelerated arteriosclerotic cardiovascular disease despite what is considered to be adequate hemodialysis or peritoneal dialysis. In rodents with reduced renal mass, renal scarring has been attributed to poorly filtered, small protein-bound molecules. The best studied of these is indoxyl sulfate (IS). METHODS: We have attempted to establish whether there are uremic toxins that are not effectively removed by hemodialysis. We examined plasma from patients undergoing hemodialysis, employing global gene expression in normal human renal cortical cells incubated in pre- and post- dialysis plasma as a reporter system. Responses in cells incubated with pre- and post-dialysis uremic plasma (n = 10) were compared with responses elicited by plasma from control subjects (n = 5). The effects of adding IS to control plasma and of adding probenecid to uremic plasma were examined. Plasma concentrations of IS were measured by HPLC (high pressure liquid chromatography). RESULTS: Gene expression in our reporter system revealed dysregulation of 1912 genes in cells incubated with pre-dialysis uremic plasma. In cells incubated in post-dialysis plasma, the expression of 537 of those genes returned to baseline but the majority of them (1375) remained dysregulated. IS concentration was markedly elevated in pre- and post-dialysis plasma. Addition of IS to control plasma simulated more than 80% of the effects of uremic plasma on gene expression; the addition of probenecid, an organic anion transport (OAT) inhibitor, to uremic plasma reversed the changes in gene expression. CONCLUSION: These findings provide evidence that hemodialysis fails to effectively clear one or more solutes that effect gene expression, in our reporter system, from the plasma of patients with uremia. The finding that gene dysregulation was simulated by the addition of IS to control plasma and inhibited by addition of an OAT inhibitor to uremic plasma identifies IS as a major, poorly dialyzable, uremic toxin. The signaling pathways initiated by IS and possibly other solutes not effectively removed by dialysis may participate in the pathogenesis of renal scarring and uremic vasculopathy. Public Library of Science 2015-03-26 /pmc/articles/PMC4374671/ /pubmed/25811877 http://dx.doi.org/10.1371/journal.pone.0118703 Text en © 2015 Jhawar et al http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Jhawar, Sachin
Singh, Prabhjot
Torres, Daniel
Ramirez-Valle, Francisco
Kassem, Hania
Banerjee, Trina
Dolgalev, Igor
Heguy, Adriana
Zavadil, Jiri
Lowenstein, Jerome
Functional Genomic Analysis Identifies Indoxyl Sulfate as a Major, Poorly Dialyzable Uremic Toxin in End-Stage Renal Disease
title Functional Genomic Analysis Identifies Indoxyl Sulfate as a Major, Poorly Dialyzable Uremic Toxin in End-Stage Renal Disease
title_full Functional Genomic Analysis Identifies Indoxyl Sulfate as a Major, Poorly Dialyzable Uremic Toxin in End-Stage Renal Disease
title_fullStr Functional Genomic Analysis Identifies Indoxyl Sulfate as a Major, Poorly Dialyzable Uremic Toxin in End-Stage Renal Disease
title_full_unstemmed Functional Genomic Analysis Identifies Indoxyl Sulfate as a Major, Poorly Dialyzable Uremic Toxin in End-Stage Renal Disease
title_short Functional Genomic Analysis Identifies Indoxyl Sulfate as a Major, Poorly Dialyzable Uremic Toxin in End-Stage Renal Disease
title_sort functional genomic analysis identifies indoxyl sulfate as a major, poorly dialyzable uremic toxin in end-stage renal disease
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4374671/
https://www.ncbi.nlm.nih.gov/pubmed/25811877
http://dx.doi.org/10.1371/journal.pone.0118703
work_keys_str_mv AT jhawarsachin functionalgenomicanalysisidentifiesindoxylsulfateasamajorpoorlydialyzableuremictoxininendstagerenaldisease
AT singhprabhjot functionalgenomicanalysisidentifiesindoxylsulfateasamajorpoorlydialyzableuremictoxininendstagerenaldisease
AT torresdaniel functionalgenomicanalysisidentifiesindoxylsulfateasamajorpoorlydialyzableuremictoxininendstagerenaldisease
AT ramirezvallefrancisco functionalgenomicanalysisidentifiesindoxylsulfateasamajorpoorlydialyzableuremictoxininendstagerenaldisease
AT kassemhania functionalgenomicanalysisidentifiesindoxylsulfateasamajorpoorlydialyzableuremictoxininendstagerenaldisease
AT banerjeetrina functionalgenomicanalysisidentifiesindoxylsulfateasamajorpoorlydialyzableuremictoxininendstagerenaldisease
AT dolgalevigor functionalgenomicanalysisidentifiesindoxylsulfateasamajorpoorlydialyzableuremictoxininendstagerenaldisease
AT heguyadriana functionalgenomicanalysisidentifiesindoxylsulfateasamajorpoorlydialyzableuremictoxininendstagerenaldisease
AT zavadiljiri functionalgenomicanalysisidentifiesindoxylsulfateasamajorpoorlydialyzableuremictoxininendstagerenaldisease
AT lowensteinjerome functionalgenomicanalysisidentifiesindoxylsulfateasamajorpoorlydialyzableuremictoxininendstagerenaldisease

Ejemplares similares