TY - JOUR
T1 - Cloning of rodent megsin revealed its up-regulation in mesangioproliferative nephritis
AU - Nangaku, Masaomi
AU - Miyata, Toshio
AU - Suzuki, Daisuke
AU - Umezono, Tomoya
AU - Hashimoto, Tsutomu
AU - Wada, Takehiko
AU - Yagi, Mikio
AU - Nagano, Nobuo
AU - Inagi, Reiko
AU - Kurokawa, Kiyoshi
N1 - Funding Information:
This study was supported by grants from the Research for the Future Program of the Japan Society for the Promotion of Science (96L00303), the Ministry of Education, Science and Culture of Japan (11307016 and 11671503), the Millennium Project of the Ministry of Science and Technology Agency of Japan (12210), the Research on Human Genome and Tissue Engineering of the Japanese Ministry of Health and Welfare (H12-genome-22), the Takeda Medical Research Foundation, and the Novartis Foundation. We are grateful to Y. Kishida for her technical assistance.
PY - 2001
Y1 - 2001
N2 - Background. We recently cloned a new human mesangium-predominant gene, megsin. Megsin is a novel member of the serine protease inhibitor (serpin) superfamily. To elucidate functional roles of this gene, we cloned megsin in rodents and investigated its role in a rat nephritis model. Methods. Megsin homologues were cloned from cultured rat and mouse mesangial cDNAs utilizing polymerase chain reaction (PCR) with degenerative primers. Expression of megsin in three different types of resident glomerular cells was investigated by PCR. Levels of megsin mRNA expression at various time points in the anti-Thy1 rat nephritis model were studied by semiquantitative PCR and Northern blotting analysis. In order to investigate megsin protein expression in anti-Thy1 nephritis rats, we raised antibody against rat megsin specific synthetic peptide, with which immunohistochemical studies were performed. Results. Rat and mouse megsins were composed of 380 amino acids, which revealed 75.3 and 73.9% identity, respectively, with human megsin at the amino acid level. Characteristic features as an inhibitory serpin were conserved in both rat and megsin megsins. PCR analysis revealed expression of megsin in cultured mesangial cells but not in glomerular epithelial or endothelial cells. In anti-Thy1 nephritis rats, semiquantitative PCR and Northern blotting showed that expression of megsin mRNA was up-regulated in glomeruli at day 8. Immunohistochemical studies demonstrated the prominent accumulation of megsin in glomeruli at the same time point. Megsin was mainly localized in mesangial area. The megsin expression level returned to the basal level at day 28. Conclusion. Sequences of megsin were well conserved among different species. Rat megsin was also predominantly expressed in mesangial cells. Expression of megsin was up-regulated at the peak of hypercellularity and matrix accumulation in the mesangioproliferative glomerulonephritis model, suggesting that megsin may participate in the process of glomerulosclerosis by modulating extracellular matrix deposition or cell survival.
AB - Background. We recently cloned a new human mesangium-predominant gene, megsin. Megsin is a novel member of the serine protease inhibitor (serpin) superfamily. To elucidate functional roles of this gene, we cloned megsin in rodents and investigated its role in a rat nephritis model. Methods. Megsin homologues were cloned from cultured rat and mouse mesangial cDNAs utilizing polymerase chain reaction (PCR) with degenerative primers. Expression of megsin in three different types of resident glomerular cells was investigated by PCR. Levels of megsin mRNA expression at various time points in the anti-Thy1 rat nephritis model were studied by semiquantitative PCR and Northern blotting analysis. In order to investigate megsin protein expression in anti-Thy1 nephritis rats, we raised antibody against rat megsin specific synthetic peptide, with which immunohistochemical studies were performed. Results. Rat and mouse megsins were composed of 380 amino acids, which revealed 75.3 and 73.9% identity, respectively, with human megsin at the amino acid level. Characteristic features as an inhibitory serpin were conserved in both rat and megsin megsins. PCR analysis revealed expression of megsin in cultured mesangial cells but not in glomerular epithelial or endothelial cells. In anti-Thy1 nephritis rats, semiquantitative PCR and Northern blotting showed that expression of megsin mRNA was up-regulated in glomeruli at day 8. Immunohistochemical studies demonstrated the prominent accumulation of megsin in glomeruli at the same time point. Megsin was mainly localized in mesangial area. The megsin expression level returned to the basal level at day 28. Conclusion. Sequences of megsin were well conserved among different species. Rat megsin was also predominantly expressed in mesangial cells. Expression of megsin was up-regulated at the peak of hypercellularity and matrix accumulation in the mesangioproliferative glomerulonephritis model, suggesting that megsin may participate in the process of glomerulosclerosis by modulating extracellular matrix deposition or cell survival.
KW - Anti-Thy 1 nephritis
KW - Cell survival
KW - Extracellular matrix
KW - Glomerulonephritis
KW - Glomerulosclerosis
KW - Mesangial cells
KW - Mesangial hypercellularity
KW - Serpin
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U2 - 10.1046/j.1523-1755.2001.060002641.x
DO - 10.1046/j.1523-1755.2001.060002641.x
M3 - Article
C2 - 11473647
AN - SCOPUS:0034912684
SN - 0085-2538
VL - 60
SP - 641
EP - 652
JO - Kidney International
JF - Kidney International
IS - 2
ER -