RNA-seq analysis of glycosylation related gene expression in STZ-induced diabetic rat kidney inner medulla

The UT-A1 urea transporter is crucial to the kidney's ability to generate concentrated urine. Native UT-A1 from kidney inner medulla (IM) is a heavily glycosylated protein with two glycosylation forms of 97 and 117 kDa. In diabetes, UT-A1 protein abundance, particularly the 117 kD isoform, is s...

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Autores principales: Qian, Xiaoqian, Li, Xuechen, Ilori, Titilayo O., Klein, Janet D., Hughey, Rebecca P., Li, Cong-jun, Alli, Abdel A., Guo, Zhengyu, Yu, Peng, Song, Xiang, Chen, Guangping
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Frontiers Media S.A. 2015
Materias:
Physiology
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4590316/
https://www.ncbi.nlm.nih.gov/pubmed/26483702
http://dx.doi.org/10.3389/fphys.2015.00274
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author Qian, Xiaoqian
Li, Xuechen
Ilori, Titilayo O.
Klein, Janet D.
Hughey, Rebecca P.
Li, Cong-jun
Alli, Abdel A.
Guo, Zhengyu
Yu, Peng
Song, Xiang
Chen, Guangping
author_facet Qian, Xiaoqian
Li, Xuechen
Ilori, Titilayo O.
Klein, Janet D.
Hughey, Rebecca P.
Li, Cong-jun
Alli, Abdel A.
Guo, Zhengyu
Yu, Peng
Song, Xiang
Chen, Guangping
author_sort Qian, Xiaoqian
collection PubMed
description The UT-A1 urea transporter is crucial to the kidney's ability to generate concentrated urine. Native UT-A1 from kidney inner medulla (IM) is a heavily glycosylated protein with two glycosylation forms of 97 and 117 kDa. In diabetes, UT-A1 protein abundance, particularly the 117 kD isoform, is significantly increased corresponding to an increased urea permeability in perfused IM collecting ducts, which plays an important role in preventing the osmotic diuresis caused by glucosuria. However, how the glycan carbohydrate structure change and the glycan related enzymes regulate kidney urea transport activity, particularly under diabetic condition, is largely unknown. In this study, using sugar-specific binding lectins, we found that the carbohydrate structure of UT-A1 is changed with increased amounts of sialic acid, fucose, and increased glycan branching under diabetic conditions. These changes were accompanied by altered UT-A1 association with the galectin proteins, β-galactoside glycan binding proteins. To explore the molecular basis of the alterations of glycan structures, the highly sensitive next generation sequencing (NGS) technology, Illumina RNA-seq, was employed to analyze genes involved in the process of UT-A1 glycosylation using streptozotocin (STZ)—induced diabetic rat kidney. Differential gene expression analysis combining with quantitative PCR revealed that expression of a number of important glycosylation related genes were changed under diabetic conditions. These genes include the glycosyltransferase genes Mgat4a, the sialylation enzymes St3gal1 and St3gal4 and glycan binding protein galectin-3, -5, -8, and -9. In contrast, although highly expressed in kidney IM, the glycosyltransferase genes Mgat1, Mgat2, and fucosyltransferase Fut8, did not show any changes. Conclusions: In diabetes, not only is UT-A1 protein abundance increased but the protein's glycan structure is also significantly changed. UT-A1 protein becomes highly sialylated, fucosylated and branched. Consistently, a number of crucial glycosylation related genes are changed under diabetic conditions. The alteration of these genes may contribute to changes in the UT-A1 glycan structure and therefore modulate kidney urea transport activity and alleviate osmotic diuresis caused by glucosuria in diabetes.
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spelling pubmed-45903162015-10-19 RNA-seq analysis of glycosylation related gene expression in STZ-induced diabetic rat kidney inner medulla Qian, Xiaoqian Li, Xuechen Ilori, Titilayo O. Klein, Janet D. Hughey, Rebecca P. Li, Cong-jun Alli, Abdel A. Guo, Zhengyu Yu, Peng Song, Xiang Chen, Guangping Front Physiol Physiology The UT-A1 urea transporter is crucial to the kidney's ability to generate concentrated urine. Native UT-A1 from kidney inner medulla (IM) is a heavily glycosylated protein with two glycosylation forms of 97 and 117 kDa. In diabetes, UT-A1 protein abundance, particularly the 117 kD isoform, is significantly increased corresponding to an increased urea permeability in perfused IM collecting ducts, which plays an important role in preventing the osmotic diuresis caused by glucosuria. However, how the glycan carbohydrate structure change and the glycan related enzymes regulate kidney urea transport activity, particularly under diabetic condition, is largely unknown. In this study, using sugar-specific binding lectins, we found that the carbohydrate structure of UT-A1 is changed with increased amounts of sialic acid, fucose, and increased glycan branching under diabetic conditions. These changes were accompanied by altered UT-A1 association with the galectin proteins, β-galactoside glycan binding proteins. To explore the molecular basis of the alterations of glycan structures, the highly sensitive next generation sequencing (NGS) technology, Illumina RNA-seq, was employed to analyze genes involved in the process of UT-A1 glycosylation using streptozotocin (STZ)—induced diabetic rat kidney. Differential gene expression analysis combining with quantitative PCR revealed that expression of a number of important glycosylation related genes were changed under diabetic conditions. These genes include the glycosyltransferase genes Mgat4a, the sialylation enzymes St3gal1 and St3gal4 and glycan binding protein galectin-3, -5, -8, and -9. In contrast, although highly expressed in kidney IM, the glycosyltransferase genes Mgat1, Mgat2, and fucosyltransferase Fut8, did not show any changes. Conclusions: In diabetes, not only is UT-A1 protein abundance increased but the protein's glycan structure is also significantly changed. UT-A1 protein becomes highly sialylated, fucosylated and branched. Consistently, a number of crucial glycosylation related genes are changed under diabetic conditions. The alteration of these genes may contribute to changes in the UT-A1 glycan structure and therefore modulate kidney urea transport activity and alleviate osmotic diuresis caused by glucosuria in diabetes. Frontiers Media S.A. 2015-10-01 /pmc/articles/PMC4590316/ /pubmed/26483702 http://dx.doi.org/10.3389/fphys.2015.00274 Text en Copyright © 2015 Qian, Li, Ilori, Klein, Hughey, Li, Alli, Guo, Yu, Song and Chen. http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) or licensor are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.
spellingShingle Physiology
Qian, Xiaoqian
Li, Xuechen
Ilori, Titilayo O.
Klein, Janet D.
Hughey, Rebecca P.
Li, Cong-jun
Alli, Abdel A.
Guo, Zhengyu
Yu, Peng
Song, Xiang
Chen, Guangping
RNA-seq analysis of glycosylation related gene expression in STZ-induced diabetic rat kidney inner medulla
title RNA-seq analysis of glycosylation related gene expression in STZ-induced diabetic rat kidney inner medulla
title_full RNA-seq analysis of glycosylation related gene expression in STZ-induced diabetic rat kidney inner medulla
title_fullStr RNA-seq analysis of glycosylation related gene expression in STZ-induced diabetic rat kidney inner medulla
title_full_unstemmed RNA-seq analysis of glycosylation related gene expression in STZ-induced diabetic rat kidney inner medulla
title_short RNA-seq analysis of glycosylation related gene expression in STZ-induced diabetic rat kidney inner medulla
title_sort rna-seq analysis of glycosylation related gene expression in stz-induced diabetic rat kidney inner medulla
topic Physiology
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4590316/
https://www.ncbi.nlm.nih.gov/pubmed/26483702
http://dx.doi.org/10.3389/fphys.2015.00274
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