Your search keyword '"Peter Igarashi"' showing total 138 results

51. Ksp-cadherin gene promoter. I. Characterization and renal epithelial cell-specific activity

Author

Congyi Li, Peter S. Aronson, Peter Igarashi, Stacey L. Nix, Sharon L. Karp, R. Brent Thomson, Reza Zanjani, and Dilys A. Whyte

Subjects

Transcription, Genetic, Physiology, DNA Mutational Analysis, Molecular Sequence Data, 5' flanking region, CAAT box, Gene Expression, Biology, Kidney, Mice, Gene expression, Animals, Cloning, Molecular, Promoter Regions, Genetic, Transcription factor, Epithelial polarity, Base Sequence, Activator (genetics), Cadherin, Chromosome Mapping, Nuclear Proteins, Epithelial Cells, Promoter, Cadherins, Molecular biology, Gene Deletion

Abstract

Kidney-specific cadherin (Ksp-cadherin, cadherin 16) is a novel, kidney-specific member of the cadherin superfamily that is expressed exclusively in the basolateral membrane of renal tubular epithelial cells. To characterize the Ksp-cadherin gene promoter, a λ bacteriophage clone containing 3.7 kb of the proximal 5′ flanking region of the mouse Ksp-cadherin gene was isolated. The transcription initiation site was mapped by RNase protection assays and 5′ rapid amplification of cDNA ends, and a 709-bp intron was identified within the 5′ untranslated region. The proximal 5′ flanking region was “TATA-less” but contained other consensus promoter elements including an initiator (Inr), GC boxes, and a CAAT box. Potential binding sites were identified for transcription factors that are involved in tissue-specific gene expression including activator protein-2 (AP-2), hepatocyte nuclear factor-3 (HNF-3), basic helix-loop-helix (bHLH) proteins, CCAAT/enhancer-binding protein (C/EBP), and GATA factors. Transfection of luciferase reporter plasmids containing 2.6 kb of the 5′ flanking region markedly increased luciferase activity in renal epithelial cells (MDCK and mIMCD-3) but not in mesenchymal cells (NIH 3T3 and MMR1). Deletion analysis identified an 82-bp region from −31 to −113 that was essential for promoter activity in transfected renal epithelial cells. Electrophoretic mobility-shift assays showed that mIMCD-3 cells contain nuclear proteins that bind to this region of the promoter. Mutational analysis showed that sequences within the HNF-3 consensus site and CAAT box were involved in protein binding and promoter activity. We conclude that the proximal 5′ flanking region of the mouse Ksp-cadherin gene contains an orientation-dependent promoter that is kidney epithelial cell specific. The region of the promoter from −113 to −31 is required for transcriptional activity and contains binding sites for nuclear proteins that are specifically expressed in renal epithelial cells.

Published

1999

52. Sex Steroids Mediate HOXA11 Expression in the Human Peri-Implantation Endometrium1

Author

Aydin Arici, Peter Igarashi, David L. Olive, and Hugh S. Taylor

Subjects

Messenger RNA, medicine.medical_specialty, Pregnancy, medicine.drug_class, Endocrinology, Diabetes and Metabolism, media_common.quotation_subject, Biochemistry (medical), Clinical Biochemistry, Biology, Endometrium, medicine.disease, Biochemistry, Endocrinology, medicine.anatomical_structure, Estrogen, Internal medicine, Gene expression, medicine, Gestation, Hox gene, Menstrual cycle, media_common

Abstract

Under the influence of sex steroids, human endometrium undergoes sequential development in preparation for implantation. Hoxa11 is essential for implantation in the mouse. Here we describe a potential role for HOXA11 in human endometrial development and implantation. Northern analysis demonstrates that HOXA11 is expressed in a menstrual cycle phase-dependent fashion in adult human endometrium. HOXA11 messenger RNA levels dramatically increase at the time of implantation and remain increased in pregnancy. In vitro, HOXA11 expression is increased in response to estrogen or progesterone. There is a dose-responsive increase over the physiologic range of progesterone concentration. Pretreatment with Cyclohexamide does not decrease the response to estrogen. Steroids are novel regulators HOX gene expression. The spatial and temporal pattern of HOXA11 expression in the human endometrium suggests a role in endometrial development, implantation, and maintenance of pregnancy.

Published

1999

53. Gastrointestinal Amyloidosis Associated With Transthyretin Phe64Ser Mutation

Author

Farnas Nematollah Farsian, Amir Said Alizadeh Naderi, and Peter Igarashi

Subjects

Adult, Male, endocrine system, Pathology, medicine.medical_specialty, Gastrointestinal Diseases, Phenylalanine, medicine.disease_cause, GASTROINTESTINAL AMYLOIDOSIS, Polymorphism, Single Nucleotide, Cytosine, Serine, medicine, Humans, Prealbumin, Codon, Gene, Mutation, biology, business.industry, Amyloidosis, nutritional and metabolic diseases, DNA, Exons, General Medicine, medicine.disease, Phenotype, Pedigree, Thyroxine binding prealbumin, Transthyretin, Amino Acid Substitution, biology.protein, Female, business, Amyloidosis, Familial, Polyneuropathy, Thymine

Abstract

Familial amyloidotic polyneuropathy (FAP) is a hereditary generalized amyloidosis that results from mutations in the transthyretin (TTR) gene. More then 100 mutations of TTR have been described. Corresponding to the wide variety of TTR mutations, FAP presents with diverse clinical phenotypes. TTR-Phe64Ser is a rare mutation that has previously only been described once in a Canadian family that presented with oculoleptomeningeal symptoms. We report the clinical and molecular characterization of the first described case of a TTR-Phe64Ser mutation in an African-American family with profound gastrointestinal symptoms.

Published

2007

54. Polycystic Kidney Disease

Author

Stefan Somlo and Peter Igarashi

Subjects

Adult, Pathology, medicine.medical_specialty, TRPP Cation Channels, medicine.medical_treatment, Population, 030232 urology & nephrology, Autosomal dominant polycystic kidney disease, Receptors, Cell Surface, Disease, urologic and male genital diseases, Pathogenesis, Mice, 03 medical and health sciences, Tuberous sclerosis, 0302 clinical medicine, medicine, Polycystic kidney disease, Animals, Humans, Child, education, Dialysis, 030304 developmental biology, Polycystic Kidney Diseases, 0303 health sciences, education.field_of_study, business.industry, General Medicine, medicine.disease, 3. Good health, Transplantation, Nephrology, Disease Progression, business, Signal Transduction

Abstract

Renal cysts are common clinical findings, often incidentally discovered in the course of evaluating other problems. They may be either acquired or seen in association with a number of inherited and congenital disorders. The most common disorder, autosomal dominant polycystic kidney disease (ADPKD), is an important cause of end-stage renal disease (ESRD), accounting for 5–8% of the entire ESRD population. At the time of Dalgaard’ s sentinel description of polycystic kidney disease (PKD), death from renal failure was a frequent outcome for affected individuals. While transplantation and dialysis have improved the prognosis for those suffering from PKD, no therapies have yet been discovered that prevent or inhibit cystogenesis. Hindering their development has been an incomplete knowledge of the pathogenesis of this process. Although most types of renal cysts share some common features (cell proliferation, basement membrane abnormalities, fluid secretion), the broad range of disorders associated with renal cysts suggests that defects in multiple, possibly intersecting, pathways are responsible for cyst formation and expansion. Recent molecular genetic studies have yielded important breakthroughs that are likely to lead to the unraveling of this mystery. In this chapter, we will review these data and how they have improved our understanding of renal cystic disease.

Published

2007

55. HOXA10 is expressed in response to sex steroids at the time of implantation in the human endometrium

Author

David L. Olive, Aydin Arici, Hugh S. Taylor, and Peter Igarashi

Subjects

medicine.drug_class, media_common.quotation_subject, Uterus, Medroxyprogesterone Acetate, In situ hybridization, Biology, Endometrium, Andrology, Tumor Cells, Cultured, medicine, Humans, Embryo Implantation, RNA, Messenger, Northern blot, Cycloheximide, Hox gene, Cells, Cultured, Menstrual cycle, media_common, Homeodomain Proteins, Protein Synthesis Inhibitors, Estradiol, Embryogenesis, Gene Expression Regulation, Developmental, General Medicine, Molecular biology, Menstruation, DNA-Binding Proteins, Homeobox A10 Proteins, medicine.anatomical_structure, Receptors, Estrogen, Estrogen, Female, Receptors, Progesterone, Infertility, Female, Research Article

Abstract

Hox genes are well-known transcriptional regulators that play an essential role in directing embryonic development. Mice that are homozygous for a targeted disruption of the Hoxa10 gene exhibit uterine factor infertility. We have recently demonstrated that HOXA10 is expressed in the adult human uterus. To examine expression of HOXA10 during the menstrual cycle, Northern blot analysis and in situ hybridization were performed. Expression of HOXA10 dramatically increased during the midsecretory phase of the menstrual cycle, corresponding to the time of implantation and increase in circulating progesterone. Expression of HOXA10 in cultured endometrial cells was stimulated by estrogen or progesterone. Stimulation of HOXA10 by progesterone was concentration-dependent within the physiologic range, and the effect of estrogen was inhibited by cycloheximide. These results identify sex steroids as novel regulators of HOX gene expression. HOXA10 may have an important function in regulating endometrial development during the menstrual cycle and in establishing conditions necessary for implantation in the human.

Published

1998

56. Pod-1, a mesoderm-specific basic-helix-loop-helix protein expressed in mesenchymal and glomerular epithelial cells in the developing kidney

Author

Peter Igarashi, Gregory B. Vanden Heuvel, and Susan E. Quaggin

Subjects

Male, Mesoderm, Embryology, DNA, Complementary, Kidney Glomerulus, Molecular Sequence Data, Kidney development, Mice, Inbred Strains, Cell fate determination, Biology, Mice, Organ Culture Techniques, Basic Helix-Loop-Helix Transcription Factors, medicine, Animals, Humans, Amino Acid Sequence, In Situ Hybridization, Kidney, urogenital system, Helix-Loop-Helix Motifs, Mesenchymal stem cell, Embryogenesis, Chromosome Mapping, Epithelial Cells, Oligonucleotides, Antisense, Blotting, Northern, Embryonic stem cell, Molecular biology, Mice, Inbred C57BL, medicine.anatomical_structure, Organ Specificity, Ureteric bud, Female, Transcription Factors, Developmental Biology

Abstract

Basic-helix-loop-helix (bHLH) proteins are transcriptional regulatory proteins that govern cell fate determination and differentiation in a variety of tissues. We have identified a novel bHLH protein, named Pod-1, that belongs to a recently-described subfamily of bHLH proteins that have essential roles in the embryonic development of mesodermal tissues. In the adult human and mouse, Pod-1 was most highly expressed in the kidney, lung and heart. In developing mouse embryos, Pod-1 was selectively expressed in mesenchymal cells at sites of epithelial-mesenchymal interaction in the kidney, lung, intestine and pancreas. Pod-1 was also expressed in visceral glomerular epithelial cells (podocytes) in the kidney, and its expression coincided with the onset of podocyte differentiation. The expression of Pod-1 in embryonic kidney explants was inhibited using antisense oligonucleotides. Inhibition of Pod-1 expression resulted in decreased mesenchymal cell condensation around the ureteric bud and a 40% decrease in ureteric branching. Pod-1 is the first tissue-restricted basic-helix-loop-helix protein that has been identified in the developing kidney where it may play a role in the regulation of morphogenetic events.

Published

1998

57. Overview

Author

Peter Igarashi

Subjects

Organogenesis, Physiology, Kidney development, General Medicine, Anatomy, Disease, Malpighian Tubules, Biology, biology.organism_classification, Disease Models, Animal, Nematode, Species Specificity, Nephrology, Excretory system, Models, Animal, Animals, Humans, Drosophila, Kidney Diseases, Higher animals, Anura, Caenorhabditis elegans, Zebrafish

Abstract

All animals must excrete the waste products of metabolism and maintain a constant body composition despite changes in the external environment. In higher animals, these functions are performed by specialized excretory organs. The excretory organs range from a single excretory cell in the nematode

Published

2005

58. A Unique Variant of a Homeobox Gene Related to Drosophila cut is Expressed in Mouse Testis1

Author

Susan E. Quaggin, Gregory B. Vanden Heuvel, and Peter Igarashi

Subjects

Regulation of gene expression, Mutation, EMX2, Alternative splicing, Homeobox A1, Cell Biology, General Medicine, Biology, medicine.disease_cause, Molecular biology, Homeobox protein Nkx-2.5, Reproductive Medicine, Gene expression, medicine, Homeobox

Abstract

Mammalian homologues of the Drosophila cut homeobox gene encode transcriptional repressors that are involved in tissue-specific and developmental gene regulation. We examined the expression of a murine cut homologue (Cux-1) in the adult mouse. In many somatic tissues, Cux-1 was expressed as a 13-kb transcript. However, the highest expression of Cux-1 was in the testis, where a unique 2.4-kb splice variant was identified. Less abundant transcripts of 5 kb, 6.5 kb, and 8.5 kb were also detected only in the testis. The nucleotide sequence of the 2.4-kb Cux-1 transcript was identical to the 13-kb transcript in the region of overlap, but the testis-specific transcript encoded a truncated protein that contained only one Cut repeat in addition to the Cut-related homeodomain. Studies of mice homozygous for the atrichosis (at/at) mutation suggested that the 2.4-kb transcript was expressed in germ cells in the testis. In situ hybridization verified that Cux-1 was transiently expressed in post-meiotic germ cells at the round spermatid stage. Immunoblot analysis of nuclear extracts showed that the testis-specific Cux-1 transcripts encoded a 55-kDa protein. These results demonstrate that multiple products of a cut-related homeobox gene are expressed in the testis. The highly restricted pattern of expression of Cux-1 in the testis suggests that it may be involved in regulation of postmeiotic gene expression.

Published

1996

59. Primary Structure, Neural-specific Expression, and Chromosomal Localization of , a Second Murine Homeobox Gene Related to

Author

Peter Igarashi, Krista Golden, Gregory B. Vanden Heuvel, Rolf Bodmer, and Susan E. Quaggin

Subjects

DLX3, EMX2, Homeobox A1, Homeobox, Cell Biology, DLX5, Biology, CDX2, Molecular Biology, Biochemistry, Molecular biology, NKX2-3, Homeobox protein Nkx-2.5

Abstract

The cut locus of Drosophila encodes a diverged homeodomain-containing protein that is required for the development of external sensory (es) organs and other tissues. A homologous gene (Cux-1) that encodes a transcriptional repressor has been identified in the mouse and other mammals. We have identified a second murine homeobox-containing gene (designated Cux-2) that is structurally related to Drosophila cut. The murine Cux-2 homeobox was similar to Drosophila cut and encoded a homeodomain that contained a characteristic histidine residue at position 50. The predicted Cux-2 protein contained 1426 amino acids and included three internal 60-amino acid repeats (Cut repeats) that were previously found in Drosophila Cut and murine Cux-1. Unlike Cux-1, expression of Cux-2 was restricted to neural tissue. In the adult brain, Cux-2 was prominently expressed in neurons in the thalamus and limbic system. In embryos, Cux-2 was expressed in the developing central and peripheral nervous systems, including the telencephalon and peripheral ganglia of the trigeminal and glossopharyngeal nerves. A glutathione S-transferase fusion protein containing the carboxyl-terminal Cut repeat and homeodomain of Cux-2 exhibited sequence-specific binding to oligonucleotides derived from the promoter of the Ncam gene. Using an interspecific backcross panel, Cux-1 and Cux-2 were mapped to distinct loci that were genetically linked on distal chromosome 5. These results demonstrate that a family of homeobox genes related to Drosophila cut is located on chromosome 5 in the mouse. Cux-2 is expressed exclusively in the central and peripheral nervous systems, and the Cux-2 gene product binds to DNA in a sequence-specific manner. Cux-2 may encode a transcription factor that is involved in neural specification in mammals.

Published

1996

60. Cloning and Kidney Cell-specific Activity of the Promoter of the Murine Renal Na-K-Cl Cotransporter Gene

Author

Peter Igarashi, Dilys A. Whyte, Kui Li, and Glenn T. Nagami

Subjects

urogenital system, TATA box, Response element, CAAT box, Kidney metabolism, Promoter, Cell Biology, Transfection, Biology, Biochemistry, Molecular biology, Transcription (biology), Molecular Biology, Transcription factor

Abstract

The murine Nkcc2/Slcl2a1 gene encodes a bumetanide-sensitive Na-K-Cl cotransporter that is expressed exclusively in the kidney in the thick ascending limb of the loop of Henle. Nuclear run-off assays demonstrated that kidney-specific expression of Nkcc2 was due, at least in part, to kidney-specific gene transcription. To begin study of the gene promoter, a genomic clone that contained 13.5 kilobases of the 5'-flanking region of Nkcc2 was isolated. A single transcription initiation site was located 1330 base pairs (bp) upstream of the start codon. The sequence of the proximal 5'-flanking region contained typical eukaryotic promoter elements including a TATA box, two CCAAT boxes, and an initiator. A (G-A)28.(C-T)28 microsatellite and consensus binding sites for hepatocyte nuclear factor 1, cAMP-response element binding protein, CCAAT/enhancer-binding proteins, and basic helix-loop-helix proteins, were also identified. To functionally express the promoter, 2255 bp of the proximal 5'-flanking region was ligated to a luciferase reporter gene and transfected into thick ascending limb (TAL) cells, a stable cell line derived from microdissected loops of Henle of the Tg(SV40E)Bri7 mouse. TAL cells exhibited furosemide-sensitive Na-K((NH4)+)-Cl cotransport activity and endogenously expressed the 5.0-kilobase Nkcc2 transcript. Luciferase activity was 130-fold greater following transfection into TAL cells compared with transfection into cells that did not express Nkcc2 (NIH 3T3 fibroblasts). Deletion analysis revealed that promoter activity in TAL cells was similar in constructs extending from the transcription initiation site to -1529 to -469, whereas further deletion to -190 resulted in a 76% decrease in activity. We conclude that the Nkcc2 promoter exhibits kidney cell-specific activity. Regulatory elements required for maximal promoter activity are located in a 280-bp DNA segment that contains consensus binding sites for several transcription factors expressed in the kidney.

Published

1996

61. Kidney-Specific Gene Targeting

Author

Peter Igarashi

Subjects

Genetics, Nephrology, Gene targeting, Cre recombinase, Site-specific recombinase technology, General Medicine, Cre-Lox recombination, Biology, Homologous recombination, Embryonic stem cell, Gene, Floxing, Cell biology

Abstract

Gene targeting in mice is a powerful tool for identifying the in vivo functions of proteins and for producing new animal models of human diseases. In the conventional approach, the gene encoding a protein of interest is disrupted by homologous recombination in embryonic stem (ES) cells. Targeted ES

Published

2004

62. Isolation and cDNA Cloning of Ksp-cadherin, a Novel Kidney-specific Member of the Cadherin Multigene Family

Author

Peter Igarashi, Peter S. Aronson, Manoocher Soleimani, R. B. Thomson, Richard W. Kim, Ali K. Abu-Alfa, and Daniel Biemesderfer

Subjects

Male, DNA, Complementary, Proteolysis, Molecular Sequence Data, Biology, Kidney, Biochemistry, Recognition sequence, medicine, Animals, Amino Acid Sequence, Molecular Biology, chemistry.chemical_classification, Base Sequence, medicine.diagnostic_test, Cadherin, Cell Biology, Cadherins, Trypsin, Molecular biology, Amino acid, chemistry, Cytoplasm, Multigene Family, Rabbits, Sequence motif, Cysteine, medicine.drug

Abstract

Cadherins are recognized as the principal mediators of homotypic cellular recognition and play a demonstrated role in the morphogenic direction of tissue development. We report here the identification of a structurally unique, kidney-specific member of the cadherin multigene family (Ksp-cadherin). cDNA cloning and molecular analysis of the 130-kDa protein confirmed that it was novel and indicated that it most closely resembled members of the LI-cadherin/HPT-1 cadherin subgroup. The predicted protein possesses the definitive cadherin-specific sequence motifs LDRE, DXND, and DXD in well conserved sequential arrangement, and the characteristic cysteine residues found in the last ectodomains of almost all known cadherins. Like LI-cadherin and HPT-1, Ksp-cadherin lacks the prosequence and HAV adhesion recognition sequence typical of most classical cadherins, and possesses a truncated cytoplasmic domain (18-22 amino acids). When expressed in a transient Vaccinia/T7 expression system, Ksp-cadherin displayed the classic calcium sensitivity to trypsin proteolysis that is observed in all cadherins. Immunolocalization studies and Northern analysis indicated that expression of Ksp-cadherin was kidney-specific and limited to the basolateral membranes of renal tubular epithelial cells. In summary, we have identified and cloned a novel, kidney-specific member of the cadherin multigene family that we propose be designated Ksp-cadherin.

Published

1995

63. Searching for Stem/Progenitor Cells in the Adult Mouse Kidney

Author

Peter Igarashi and Fangming Lin

Subjects

Endothelial stem cell, Zygote, Nephrology, Mouse Kidney, General Medicine, Biology, Progenitor cell, Stem cell, Clonogenic assay, Cell biology, Interleukin 3, Adult stem cell

Abstract

Stem cells are generally defined as clonogenic cells that are capable of both self-renewal and multilineage differentiation ([1–3][1][⇓][2][⇓][3]). The fertilized zygote has the highest developmental potential and gives rise to the cells of the entire organism. More than 20 years ago

Published

2003

64. MicroRNAs Regulate Renal Tubule Maturation through Modulation of Pkd1

Author

Sachin Hajarnis, Peter Igarashi, Donovan Huynh, Vishal Patel, Darren Williams, and Ryan Hunter

Subjects

TRPP Cation Channels, biology, PKD1, urogenital system, Kidney development, General Medicine, medicine.disease, urologic and male genital diseases, Brief Communication, Gene dosage, Molecular biology, female genital diseases and pregnancy complications, Cell biology, MicroRNAs, Kidney Tubules, Downregulation and upregulation, Nephrology, microRNA, biology.protein, Polycystic kidney disease, medicine, Animals, Humans, Renal stem cell, Dicer

Abstract

MicroRNAs (miRNAs) contribute to the regulation of early kidney development, but their role during later stages of renal tubule maturation is not well understood. Here, we found that ablation of the miRNA-processing enzyme Dicer from maturing renal tubules produces tubular and glomerular cysts in mice. Inactivation of Dicer is associated with downregulation of miR-200, a kidney-enriched miRNA family, and upregulation of the polycystic kidney disease gene Pkd1. Inhibition of miR-200 in cultured renal epithelial cells disrupted tubulogenesis and led to upregulation of Pkd1. Using bioinformatic and in vitro approaches, we found that miR-200b/c/429 induce post-transcriptional repression of Pkd1 through two conserved binding sites in the 3'-Untranslated regions of Pkd1. Overexpression of PKD1 in renal epithelial cells was sufficient to disrupt tubulogenesis and produce cyst-like structures. In conclusion, miRNAs are essential for the maturation of renal tubules, and Pkd1 is a target of miR-200. These results also suggest that miRNAs may modulate PKD1 gene dosage and play a role in the initiation of cystogenesis.

Published

2012

65. Loss of cilia suppresses cyst growth in genetic models of autosomal dominant polycystic kidney disease

Author

Xin Tian, Stefan Somlo, Ming Ma, Gregory J. Pazour, and Peter Igarashi

Subjects

medicine.medical_specialty, TRPP Cation Channels, Genotype, 030232 urology & nephrology, Autosomal dominant polycystic kidney disease, Biology, urologic and male genital diseases, Article, Pathogenesis, 03 medical and health sciences, Mice, 0302 clinical medicine, Intraflagellar transport, Internal medicine, Genetic model, Genetics, medicine, Polycystic kidney disease, Animals, Involution (medicine), Cyst, Cilia, 030304 developmental biology, Mice, Knockout, 0303 health sciences, urogenital system, Cysts, Cilium, respiratory system, medicine.disease, Polycystic Kidney, Autosomal Dominant, female genital diseases and pregnancy complications, Disease Models, Animal, Endocrinology, Phenotype, Mutation

Abstract

Kidney cysts occur following inactivation of polycystins in otherwise intact cilia or following complete removal of cilia by inactivation of intraflagellar transport-related proteins. We investigated the mechanisms of cyst formation in these two distinct processes by combining conditional inactivation of polycystins with concomitant ablation of cilia in developing and adult kidney and liver. We found that loss of intact cilia suppresses cyst growth following inactivation of polycystins and that the severity of cystic disease was directly related to the length of time between the initial loss of the polycystin proteins and the subsequent involution of cilia. This cilia-dependent cyst growth was not explained by activation of the MAPK/ERK, mTOR or cAMP pathways and is likely to be distinct from the mechanism of cyst growth following complete loss of cilia. The data establish the existence of a novel pathway defined by polycystin-dependent inhibition and cilia-dependent activation that promotes rapid cyst growth.

Published

2012

66. Transcription factors and apoptosis in kidney development

Author

Peter Igarashi

Subjects

Programmed cell death, Base Sequence, Cell Death, Tumor suppressor gene, Molecular Sequence Data, Kidney development, Apoptosis, Biology, Kidney, Cell biology, Nephrology, TAF2, Knockout mouse, Internal Medicine, Transcriptional regulation, Animals, Humans, E2F1, Transcription factor, Transcription Factors

Abstract

The study of kidney development at the cellular and molecular levels remains an active area of nephrologic research. This review highlights recent advances in two specific areas: transcriptional control of nephrogenesis and the role of cell death in normal kidney development. The mesenchymal-epithelial conversion that occurs during kidney development requires alterations in gene expression. Some transcription factors involved in early steps in nephrogenesis have recently been identified from the effects of gene "knockout" or dysregulated expression in transgenic mice. These include the product of the Wilms' tumor suppressor gene (WT-1), a mammalian paired homologue (Pax-2), and the N-myc oncoprotein. Other proteins, including Pax-8, hepatocyte nuclear factor-1, hepatocyte nuclear factor-4, Kid-1, and formins, exhibit spatiotemporally restricted patterns of expression, homology to products of developmental control genes in Drosophila, or mutant phenotypes consistent with possible roles in nephrogenesis. During the past year, another important observation was that apoptosis (programmed cell death) occurs during normal kidney development. Studies of knockout mice suggest that Bcl-2, which protects against death in many contexts, is also involved in kidney development.

Published

1994

67. Inducible expression of kallikrein in renal tubular cells protects mice against spontaneous lupus nephritis

Author

Xinli, Shao, Ru, Yang, Mei, Yan, Yajuan, Li, Yong, Du, Indu, Raman, Bo, Zhang, Edward K, Wakeland, Ward, Wakeland, Peter, Igarashi, Chandra, Mohan, and Quan-Zhen, Li

Subjects

Male, Selective Estrogen Receptor Modulators, medicine.medical_specialty, Immunology, Green Fluorescent Proteins, Lupus nephritis, Mice, Inbred Strains, Mice, Transgenic, urologic and male genital diseases, Nitric Oxide, Gene Expression Regulation, Enzymologic, Nitric oxide, chemistry.chemical_compound, Mice, Mice, Congenic, Rheumatology, Superoxides, Internal medicine, Immunology and Allergy, Medicine, Animals, Pharmacology (medical), Creatinine, Kidney, Proteinuria, Integrases, urogenital system, business.industry, Kallikrein, medicine.disease, Lupus Nephritis, Oxidative Stress, Tamoxifen, Endocrinology, medicine.anatomical_structure, Kidney Tubules, chemistry, Renal pathology, Lac Operon, Female, medicine.symptom, business, Nephritis, Tissue Kallikreins

Abstract

Objective To ascertain whether engineered expression of kallikreins within the kidneys, using an inducible Cre/loxP system, can ameliorate murine lupus nephritis. Methods In mice with a lupus-prone genetic background, we engineered the expression of tamoxifen-inducible Cre recombinase under the control of a kidney-specific promoter whose activation initiates murine kallikrein-1 expression within the kidneys. These transgenic mice were injected with either tamoxifen or vehicle at age 2 months and then were monitored for 8 months for kallikrein expression and disease. Results Elevated expression of kallikrein was detected in the kidney and urine of tamoxifen-injected mice but not in controls. At age 10 months, all vehicle-injected mice developed severe lupus nephritis, as evidenced by increased proteinuria (mean ± SD 13.43 ± 5.65 mg/24 hours), increased blood urea nitrogen (BUN) and serum creatinine levels (39.86 ± 13.45 mg/dl and 15.23 ± 6.89 mg/dl, respectively), and severe renal pathology. In contrast, the tamoxifen-injected mice showed significantly reduced proteinuria (6.6 ± 4.12 mg/24 hours), decreased BUN and serum creatinine levels (15.71 ± 8.17 mg/dl and 6.64 ± 3.39 mg/dl, respectively), and milder renal pathology. Tamoxifen-induced up-regulation of renal kallikrein expression increased nitric oxide production and dampened renal superoxide production and inflammatory cell infiltration, alluding to some of the pathways through which kallikreins may be operating within the kidneys. Conclusion Local expression of kallikreins within the kidney has the capacity to dampen lupus nephritis, possibly by modulating inflammation and oxidative stress.

Published

2011

68. Genetic basis of prune belly syndrome: screening for HNF1β gene

Author

Sachin Hajarnis, Steven M. Harrison, Linda A. Baker, Shaohua Zhang, Daniel DaJusta, Candace F. Granberg, and Peter Igarashi

Subjects

Genetics, Male, Mutation, Candidate gene, Urology, fungi, Chromosome, Single-nucleotide polymorphism, Biology, medicine.disease_cause, medicine.disease, law.invention, nervous system, law, Prune belly syndrome, medicine, SNP, Humans, Prune Belly Syndrome, Female, Prospective Studies, Gene, Polymerase chain reaction, Hepatocyte Nuclear Factor 1-beta

Abstract

Although the cause of prune belly syndrome is unknown, familial evidence suggests a genetic component. Recently 2 nonfamilial cases of prune belly syndrome with chromosome 17q12 deletions encompassing the HNF1β gene have made this a candidate gene for prune belly syndrome. To date, there has been no large-scale screening of patients with prune belly syndrome for HNF1β mutations. We assessed the role of HNF1β in prune belly syndrome by screening for genomic mutations with functional characterization of any detected mutations.We studied patients with prune belly syndrome who were prospectively enrolled in our Pediatric Genitourinary DNA Repository since 2001. DNA from patient samples was amplified by polymerase chain reaction, sequenced for coding and splice regions of the HNF1β gene, and compared to control databases. We performed functional assay testing of the ability of mutant HNF1β to activate a luciferase construct with an HNF1β DNA binding site.From 32 prune belly syndrome probands (30 males, 2 females) HNF1β sequencing detected a missense mutation (V61G) in 1 child with prune belly syndrome. Absent in control databases, V61G was previously reported in 2 patients without prune belly syndrome who had congenital genitourinary anomalies. Functional testing showed similar luciferase activity compared to wild-type HNF1β, suggesting the V61G substitution does not disturb HNF1β function.One genomic HNF1β mutation was detected in 3% of patients with prune belly syndrome but found to be functionally normal. Thus, functionally significant HNF1β mutations are uncommon in prune belly syndrome, despite case reports of HNF1β deletions. Further genetic study is necessary, as identification of the genetic basis of prune belly syndrome may ultimately lead to prevention and improved treatments for this rare but severe syndrome.

Published

2011

69. Polycystin-2 and phosphodiesterase 4C are components of a ciliary A-kinase anchoring protein complex that is disrupted in cystic kidney diseases

Author

Hannah C. Chapin, Peter Igarashi, Sachin Hajarnis, Stefan Somlo, Yun Hee Choi, Akira Suzuki, Michael J. Caplan, Marco Pontoglio, and Zhendong Ma

Subjects

TRPP Cation Channels, A Kinase Anchor Proteins, Biology, Kidney cysts, Immunoenzyme Techniques, Mice, Intraflagellar transport, medicine, Polycystic kidney disease, Cyclic AMP, Animals, KIF3A, Cilia, Protein kinase A, education, Cystic kidney, education.field_of_study, Multidisciplinary, Cilium, Biological Sciences, Kidney Diseases, Cystic, medicine.disease, Cell biology, Cyclic Nucleotide Phosphodiesterases, Type 4, Polycystin 2, Mutation, medicine.symptom, Signal Transduction

Abstract

Polycystic kidney disease (PKD) is a genetic disorder that is characterized by cyst formation in kidney tubules. PKD arises from abnormalities of the primary cilium, a sensory organelle located on the cell surface. Here, we show that the primary cilium of renal epithelial cells contains a protein complex comprising adenylyl cyclase 5/6 (AC5/6), A-kinase anchoring protein 150 (AKAP150), and protein kinase A. Loss of primary cilia caused by deletion of Kif3a results in activation of AC5 and increased cAMP levels. Polycystin-2 (PC2), a ciliary calcium channel that is mutated in human PKD, interacts with AC5/6 through its C terminus. Deletion of PC2 increases cAMP levels, which can be corrected by reexpression of wild-type PC2 but not by a mutant lacking calcium channel activity. Phosphodiesterase 4C (PDE4C), which catabolizes cAMP, is also located in renal primary cilia and interacts with the AKAP150 complex. Expression of PDE4C is regulated by the transcription factor hepatocyte nuclear factor-1β (HNF-1β), mutations of which produce kidney cysts. PDE4C is down-regulated and cAMP levels are increased in HNF-1β mutant kidney cells and mice. Collectively, these findings identify PC2 and PDE4C as unique components of an AKAP complex in primary cilia and reveal a common mechanism for dysregulation of cAMP signaling in cystic kidney diseases arising from different gene mutations.

Published

2011

70. Primary cilia regulate mTORC1 activity and cell size through Lkb1

Author

Gerd Walz, Michael Köttgen, Peter Igarashi, Martin Herbst, Markus Gödel, Christoph Hamann, Miriam Hornung, E. Wolfgang Kuehn, Theresa Beyer, Mara Doerken, Vishal Patel, Klaus Müller, Roland Nitschke, Henriette Voelker, Simone Braeg, Saskia Bredt, Heike Janusch, Christopher Boehlke, and Fruzsina Kotsis

Subjects

Regulator, Kinesins, Mice, Transgenic, mTORC1, AMP-Activated Protein Kinases, Mechanistic Target of Rapamycin Complex 1, Protein Serine-Threonine Kinases, Biology, Article, Cell Line, Mice, Dogs, Animals, Basal body, Cilia, Phosphorylation, PI3K/AKT/mTOR pathway, Cell Size, TOR Serine-Threonine Kinases, Cilium, Proteins, AMPK, Cell Biology, Cell biology, Cell culture, Multiprotein Complexes, Calcium, Signal transduction, Signal Transduction

Abstract

The mTOR pathway is the central regulator of cell size1. External signals from growth factors and nutrients converge on the mTORC1 multi-protein complex to modulate downstream targets, but how the different inputs are integrated and translated into specific cellular responses is incompletely understood2–4. Deregulation of the mTOR pathway occurs in polycystic kidney disease (PKD)5–7, where cilia (filiform sensory organelles) fail to sense urine flow because of inherited mutations in ciliary proteins8. We therefore investigated if cilia have a role in mTOR regulation. Here, we show that ablation of cilia in transgenic mice results in enlarged cells when compared with control animals. In vitro analysis demonstrated that bending of the cilia by flow is required for mTOR downregulation and cell-size control. Surprisingly, regulation of cell size by cilia is independent of flow-induced calcium transients, or Akt. However, the tumour-suppressor protein Lkb1 localises in the cilium, and flow results in increased AMPK phosphorylation at the basal body. Conversely, knockdown of Lkb1 prevents normal cell-size regulation under flow conditions. Our results demonstrate that the cilium regulates mTOR signalling and cell size, and identify the cilium-basal body compartment as a spatially restricted activation site for Lkb1 signalling.

Published

2010

71. Smad2 protects against TGF-beta/Smad3-mediated renal fibrosis

Author

Peter Igarashi, Xiao-Ming Meng, Xinli Shao, Erwin P. Bottinger, Hui Y. Lan, Xiao R. Huang, Arthur C.K. Chung, Wenjun Ju, and Wei Qin

Subjects

Male, medicine.medical_specialty, Smad2 Protein, Biology, Kidney, Collagen Type I, Cell Line, Transforming Growth Factor beta1, Mice, Fibrosis, Internal medicine, medicine, Renal fibrosis, Animals, Smad3 Protein, Gene knockdown, Tissue Inhibitor of Metalloproteinase-1, integumentary system, General Medicine, medicine.disease, Cell biology, Mice, Inbred C57BL, medicine.anatomical_structure, Endocrinology, Kidney Tubules, Basic Research, Nephrology, Cell culture, Phosphorylation, Female, Signal transduction, biological phenomena, cell phenomena, and immunity, Transforming growth factor, Signal Transduction, Ureteral Obstruction

Abstract

Smad2 and Smad3 interact and mediate TGF-beta signaling. Although Smad3 promotes fibrosis, the role of Smad2 in fibrogenesis is largely unknown. In this study, conditional deletion of Smad2 from the kidney tubular epithelial cells markedly enhanced fibrosis in response to unilateral ureteral obstruction. In vitro, Smad2 knockdown in tubular epithelial cells increased expression of collagen I, collagen III, and TIMP-1 and decreased expression of the matrix-degrading enzyme MMP-2 in response to TGF-beta1 compared with similarly treated wild-type cells. We obtained similar results in Smad2-knockout fibroblasts. Mechanistically, Smad2 deletion promoted fibrosis through enhanced TGF-beta/Smad3 signaling, evidenced by greater Smad3 phosphorylation, nuclear translocation, promoter activity, and binding of Smad3 to a collagen promoter (COL1A2). Moreover, deletion of Smad2 increased autoinduction of TGF-beta1. Conversely, overexpression of Smad2 attenuated TGF-beta1-induced Smad3 phosphorylation and collagen I matrix expression in tubular epithelial cells. In conclusion, in contrast to Smad3, Smad2 protects against TGF-beta-mediated fibrosis by counteracting TGF-beta/Smad3 signaling.

Published

2010

72. Kidney-specific inactivation of Ofd1 leads to relal cystic disease associated with upregulation of the mTOR pathway

Author

Giovanbattista Capasso, Alessandra Cantone, Brunella Franco, Daniela Iaconis, Pascal Dollé, Nadia Messaddeq, Peter Igarashi, Adriano Barra, Alessandro Zullo, A., Zullo, D., Iaconi, A., Barra, A., Cantone, N., Messadeq, G., Capasso, P., Dolle’, P., Igarashi, and Franco, Brunella

Subjects

Male, medicine.medical_specialty, 030232 urology & nephrology, Mice, Transgenic, Biology, Protein Serine-Threonine Kinases, Kidney, Nephropathy, 03 medical and health sciences, Mice, 0302 clinical medicine, Dogs, Internal medicine, Genetics, medicine, Animals, Cyst, Cilia, Gene Silencing, Molecular Biology, Genetics (clinical), PI3K/AKT/mTOR pathway, Cells, Cultured, 030304 developmental biology, Cystic kidney, 0303 health sciences, Cilium, TOR Serine-Threonine Kinases, Intracellular Signaling Peptides and Proteins, Kidney metabolism, Proteins, Epithelial Cells, General Medicine, Articles, Kidney Diseases, Cystic, medicine.disease, Up-Regulation, Endocrinology, medicine.anatomical_structure, Organ Specificity, Cancer research, Disease Progression, Female, Kidney disease, Signal Transduction

Abstract

The oral-facial-digital type I syndrome (OFDI; MIM 311200) is a rare syndromic form of inherited renal cystic disease. It is transmitted as an X-linked dominant, male lethal disorder and is caused by mutations in the OFD1 gene. Previous studies demonstrated that OFDI belongs to the growing number of disorders ascribed to dysfunction of primary cilia. We generated a conditional inactivation of the mouse Ofd1 gene using the Ksp-Cre transgenic line, which resulted in a viable model characterized by renal cystic disease and progressive impairment of renal function. The study of this model allowed us to demonstrate that primary cilia initially form and then disappear after the development of cysts, suggesting that the absence of primary cilia is a consequence rather than the primary cause of renal cystic disease. Immunofluorescence and western blotting analysis revealed upregulation of the mTOR pathway in both dilated and non-dilated renal structures. Treatment with rapamycin, a specific inhibitor of the mTOR pathway, resulted in a significant reduction in the number and size of renal cysts and a decrease in the cystic index compared with untreated mutant animals, suggesting that dysregulation of this pathway in our model is mTOR-dependent. The animal model we have generated could thus represent a valuable tool to understand the molecular link between mTOR and cyst development, and eventually to the identification of novel drug targets for renal cystic disease.

Published

2010

73. Loss of oriented cell division does not initiate cyst formation

Author

Peter Igarashi, Stefan Somlo, Zhiheng Yu, Saori Nishio, Xin Tian, Anna Rachel Gallagher, and Vishal Patel

Subjects

Pathology, medicine.medical_specialty, TRPP Cation Channels, Cell division, Mice, Transgenic, Receptors, Cell Surface, Nephron, Biology, urologic and male genital diseases, Kidney cysts, Mice, Cell polarity, medicine, Polycystic kidney disease, Animals, Cyst, Mitosis, Polycystic Kidney Diseases, PKD1, urogenital system, Cell Polarity, General Medicine, medicine.disease, female genital diseases and pregnancy complications, Cell biology, Disease Models, Animal, medicine.anatomical_structure, Basic Research, Kidney Tubules, Nephrology, Mutation, medicine.symptom, Cell Division, Signal Transduction

Abstract

Polycystic kidney disease (PKD) can arise from either developmental or postdevelopmental processes. Recessive PKD, caused by mutations in PKHD1, is a developmental defect, whereas dominant PKD, caused by mutations in PKD1 or PKD2, occurs by a cellular recessive mechanism in mature kidneys. Oriented cell division is a feature of planar cell polarity that describes the orientation of the mitotic axes of dividing cells during development with respect to the luminal vector of the elongating nephron. In polycystic mutant mice, the loss of oriented cell division may also contribute to the pathogenesis of PKD. Here, we examined the role of oriented cell division in mouse models based on mutations in Pkd1, Pkd2, and Pkhd1. Precystic tubules after kidney-selective inactivation of either Pkd1 or Pkd2 did not lose oriented division before cystic dilation but lost oriented division after tubular dilation began. In contrast, Pkhd1(del4/del4) mice lost oriented cell division but did not develop kidney cysts. Increased intercalation of cells into the plane of the tubular epithelium maintained the normal tubular morphology in Pkhd1(del4/del4) mice, which had more cells present in transverse tubular profiles. In conclusion, loss of oriented cell division is a feature of Pkhd1 mutation and cyst formation, but it is neither sufficient to produce kidney cysts nor required to initiate cyst formation after mutation in Pkd1 or Pkd2.

Published

2009

74. Advances in the pathogenesis and treatment of polycystic kidney disease

Author

Peter Igarashi, Vishal Patel, and Renuka Chowdhury

Subjects

medicine.medical_specialty, TRPP Cation Channels, Kinesins, Biology, Octreotide, Kidney cysts, Article, Pathogenesis, chemistry.chemical_compound, Internal medicine, Internal Medicine, medicine, Polycystic kidney disease, Roscovitine, Animals, Humans, Cilia, Sirolimus, Polycystic Kidney Diseases, Cilium, Acute kidney injury, Cell Polarity, Triptolide, medicine.disease, Ciliopathy, Endocrinology, chemistry, Nephrology, Purines, Cancer research, medicine.symptom, Antidiuretic Hormone Receptor Antagonists, Kidney disease

Abstract

Purpose of review—Polycystic kidney disease (PKD) is the most common genetic cause of chronic renal failure. Mouse models of PKD, especially those with mutations in genes that are orthologous to human disease genes, have provided insights into the pathogenesis of cyst formation and advanced the preclinical testing of new drugs. Recent findings—PKD is a ciliopathy that arises from abnormalities in the primary cilium, a sensory organelle present on the surface of most cells. The primary cilium is required for the maintenance of planar cell polarity, which regulates tubular diameter. Acute kidney injury stimulates cell proliferation and promotes cyst formation in a mouse model of PKD. Studies of signaling pathways that are perturbed in PKD have identified new potential therapeutic targets. Drugs that have shown beneficial effects in orthologous animal models of PKD include tolvaptan, octreotide, src inhibitors, CFTR inhibitors, pioglitazone, etanercept, and triptolide. Summary—Abnormalities in the primary cilium perturb signaling pathways that regulate renal epithelial cell growth and differentiation and lead to the formation of kidney cysts. Acute kidney injury promotes cyst formation and may underlie the variability in disease progression that is observed in affected individuals. Several promising new therapeutic agents that have been validated in orthologous animal models have entered clinical trials in humans.

Published

2009

75. Collecting duct‐specific Rh C Glycoprotein deletion alters basal and acidosis‐stimulated renal ammonia metabolism

Author

I. David Weiner, Hyun-Wook Lee, Peter Igarashi, Jill W. Verlander, Jesse M. Bishop, and Mary E. Handlogten

Subjects

chemistry.chemical_classification, medicine.medical_specialty, Chemistry, Metabolism, Biochemistry, Ammonia, chemistry.chemical_compound, medicine.anatomical_structure, Endocrinology, Internal medicine, Genetics, medicine, medicine.symptom, Glycoprotein, Molecular Biology, Duct (anatomy), Biotechnology, Acidosis

Published

2009

76. CXCR4/CXCL12 hyperexpression plays a pivotal role in the pathogenesis of lupus

Author

Katalin Tus, Yang Liu, Xin J. Zhou, Anna-Marie Fairhurst, Frédéric Batteux, Peter Igarashi, Chandra Mohan, Edward K. Wakeland, Donald Wong, Andrew Wang, Srividya Subramanian, and Fangming Lin

Subjects

Male, Receptors, CXCR4, Immunology, Lupus nephritis, Inflammation, Enzyme-Linked Immunosorbent Assay, Biology, Article, Proinflammatory cytokine, Pathogenesis, Mice, immune system diseases, medicine, Leukocytes, Immunology and Allergy, Animals, Lupus Erythematosus, Systemic, skin and connective tissue diseases, B cell, Systemic lupus erythematosus, Lupus erythematosus, Toll-Like Receptors, medicine.disease, Flow Cytometry, Immunohistochemistry, Lupus Nephritis, Chemokine CXCL12, Up-Regulation, Chemotaxis, Leukocyte, medicine.anatomical_structure, Cytokines, Female, medicine.symptom, Nephritis

Abstract

Among various surface molecules screened, CXCR4 was significantly up-regulated on monocytes, neutrophils, B cell subsets, and plasma cells in multiple murine models of lupus with active nephritis, including B6.Sle1Yaa, BXSB, and MRL.lpr. TLR-mediated signaling and inflammatory cytokines accounted in part for this increase. Increased CXCR4 expression was associated with functional consequences, including increased migration and enhanced B cell survival. Simultaneously, the ligand for CXCR4, CXCL12, was significantly up-regulated in the nephritic kidneys. Treatment with a peptide antagonist of CXCR4 prolonged survival and reduced serum autoantibodies, splenomegaly, intrarenal leukocyte trafficking, and end organ disease in a murine model of lupus. These findings underscore the pathogenic role of CXCR4/CXCL12 in lymphoproliferative lupus and lupus nephritis and highlight this axis as a promising therapeutic target in this disease.

Published

2009

77. CONTRIBUTORS

Author

Michael Apkon, Peter S. Aronson, Eugene J. Barrett, Paula Barrett, Henry J. Binder, Walter F. Boron, Emile L. Boulpaep, Lloyd Cantley, Michael J. Caplan, Barry W. Connors, Arthur DuBois, Gerhard Giebisch, Fred S. Gorelick, Peter Igarashi, Ervin E. Jones, W. Jonathan Lederer, Christopher R. Marino, Edward J. Masoro, Edward G. Moczydlowski, Kitt Falk Petersen, Bruce R. Ransom, Adrian Reuben, George B. Richerson, Steven S. Segal, Gerald I. Shulman, John T. Stitt, Frederick J. Suchy, and Erich E. Windhager

Published

2009

78. REGULATION OF GENE EXPRESSION

Author

Peter Igarashi

Subjects

Regulation of gene expression, Biology, Cell biology

Published

2009

79. Renal Dysgenesis

Author

Vishal Patel, Fangming Lin, and Peter Igarashi

Subjects

Kidney, Pathology, medicine.medical_specialty, business.industry, urologic and male genital diseases, medicine.disease, Renal dysplasia, Renal hypoplasia, Frasier syndrome, Nephropathy, medicine.anatomical_structure, Male pseudohermaphroditism, medicine, business, Imperforate anus, Nephrotic syndrome

Abstract

Publisher Summary Renal dysgenesis, comprising a diverse group of disorders that are characterized by defects in the embryonic development, includes abnormalities in the size or position of the kidney and abnormalities in renal differentiation. Renal dysplasia is defined as an abnormality in metanephric differentiation. Kidney size is variable, and normal renal tissue is often minimally present or absent. One of the syndromes associated with renal dysplasia is renal-coloboma syndrome, an autosomal dominant disorder that affects the development of the kidneys and eyes. Affected individuals present with optic disc dysplasia and renal anomalies, especially renal hypoplasia. Another syndrome is Denys-Drash syndrome, an autosomal dominant disorder that is characterized by the triad of diffuse mesangial sclerosis, male pseudohermaphroditism, and Wilms’ tumor. Denys-Drash syndrome usually manifests in early infancy with proteinuria leading to nephrotic syndrome. Edema and proteinuria can present between 2 weeks and 10 months of age. Renal function declines rapidly, and most patients develop end-stage renal disease before 3 years of age. Yet another syndrome is Frasier syndrome that is an autosomal dominant disorder closely related to Denys-Drash syndrome and consists of intersex disorders and nephropathy. WT1gene mutations are associated with male pseudohermaphrodism in Denys-Drash syndrome and intersex in Frasier syndrome. Affected XY males with Frasier syndrome may appear to have a normal female phenotype including normal development of pubic hair and breast tissues. Townes-Brocks syndrome is characterized by renal anomalies (mainly hypoplastic kidneys), deformity of the external ear, deafness, imperforate anus, and limb malformations. TBS is a rare autosomal dominant disorder with an estimated frequency of 1 in 250,000 live births.

Published

2009

80. Cloning of cDNAs encoding a rabbit renal brush border membrane protein immunologically related to band 3. Sequence similarity with microsomal dipeptidase

Author

Peter Igarashi and L P Karniski

Subjects

Male, Signal peptide, Dipeptidases, Kidney Cortex, Swine, Renal cortex, Molecular Sequence Data, Biology, Polymerase Chain Reaction, Biochemistry, Microvillus membrane, Kidney Tubules, Proximal, Anion Exchange Protein 1, Erythrocyte, Microsomes, Sequence Homology, Nucleic Acid, Complementary DNA, Consensus sequence, medicine, Animals, Humans, Amino Acid Sequence, Cloning, Molecular, Molecular Biology, Peptide sequence, Band 3, Gene Library, Base Sequence, Microvilli, cDNA library, Membrane Proteins, DNA, Cell Biology, Molecular biology, medicine.anatomical_structure, Oligodeoxyribonucleotides, biology.protein, Rabbits, Research Article

Abstract

Distinct anion transport processes have been identified in the mammalian renal proximal tubule, but none of the responsible proteins or genes have been isolated. A 43 kDa rabbit microvillus membrane protein that is immunologically related to the erythroid anion exchanger (band 3) was a candidate for a renal anion transporter. To examine the structural relationship with band 3, we cloned cDNAs encoding the 43 kDa protein. The 43 kDa band-3-like protein was purified, and a novel sequence of 24 amino acids was obtained from the N-terminus. Degenerate oligonucleotides were synthesized based on this sequence, and the polymerase chain reaction with single-sided specificity was used to amplify and clone a 1330 bp cDNA from rabbit renal cortex. Additional overlapping 272 bp and 1123 bp cDNAs were obtained by synthesizing and screening a rabbit renal cortical cDNA library. The composite sequence was 1483 bp, terminated with (A)16, and was similar in size to the principal transcript expressed in rabbit renal cortex. The single long open reading frame was predicted to encode a protein composed of 410 amino acids with a molecular mass of 45,193 Da; 15 amino acids predicted to reside at the N-terminus were absent in the mature protein and may constitute a signal peptide. There was only limited sequence similarity with human erythroid band 3. Rather, the sequence was highly similar to microsomal dipeptidase, including the presence of a signal peptide and a consensus sequence for covalent linkage to glycosylphosphatidylinositol. In summary, the 43 kDa protein from rabbit renal cortex that is recognized by a monospecific antibody to erythroid band 3 is most likely a microvillus membrane dipeptidase.

Published

1991

81. HNF-1beta regulates transcription of the PKD modifier gene Kif12

Author

Evelyne Fischer, Vishal Patel, Peter Igarashi, Yimei Gong, Zhendong Ma, Thomas Hiesberger, and Marco Pontoglio

Subjects

Chromatin Immunoprecipitation, Transcription, Genetic, Kinesins, Biology, Cell Line, SOX4, Mice, Gene expression, Polycystic kidney disease, medicine, Animals, Kidney Tubules, Collecting, Promoter Regions, Genetic, Transcription factor, Hepatocyte Nuclear Factor 1-beta, Cystic kidney, Regulation of gene expression, General Medicine, medicine.disease, CREB-Binding Protein, Gene expression profiling, Mice, Inbred C57BL, Basic Research, Gene Expression Regulation, Nephrology, Cancer research, Chromatin immunoprecipitation

Abstract

Hepatocyte nuclear factor-1beta (HNF-1beta) is a transcription factor that regulates gene expression in the kidney, liver, pancreas, and other epithelial organs. Mutations of HNF-1beta lead to a syndrome of inherited renal cysts and diabetes and are also a common cause of sporadic renal dysplasia. The full complement of target genes responsible for the functions of HNF-1beta, however, is incompletely defined. Using a functional genomics approach involving chromatin immunoprecipitation and promoter arrays, combined with gene expression profiling, we found that an HNF-1beta target gene in the kidney is kinesin family member 12 (Kif12), a gene previously identified as a candidate modifier gene in the cpk mouse model of polycystic kidney disease. Mutations of HNF-1beta inhibited Kif12 transcription in both cultured cells and knockout mice by altering co-factor recruitment and histone modification. Because kinesin-12 family members participate in orienting cell division, downregulation of Kif12 may underlie the abnormal planar cell polarity observed in cystic kidney diseases.

Published

2008

82. Triptolide Reduces Cystogenesis in a Model of ADPKD

Author

Stefan Somlo, Craig M. Crews, Stephanie J. Leuenroth, Natasha Bencivenga, and Peter Igarashi

Subjects

Nephrology, medicine.medical_specialty, Autosomal dominant polycystic kidney disease, Mice, Transgenic, urologic and male genital diseases, Brief Communication, chemistry.chemical_compound, Mice, Internal medicine, medicine, Animals, Cyst, Antineoplastic Agents, Alkylating, Kidney, PKD1, Cell growth, business.industry, urogenital system, General Medicine, Triptolide, Phenanthrenes, medicine.disease, Polycystic Kidney, Autosomal Dominant, medicine.anatomical_structure, Endocrinology, chemistry, Animals, Newborn, Epoxy Compounds, Diterpenes, business, Kidney disease

Abstract

Mutations in PKD1 result in autosomal dominant polycystic kidney disease, which is characterized by increased proliferation of tubule cells leading to cyst initiation and subsequent expansion. Given the cell proliferation associated with cyst growth, an attractive therapeutic strategy has been to target the hyperproliferative nature of the disease. We previously demonstrated that the small molecule triptolide induces cellular calcium release through a polycystin-2-dependent pathway, arrests Pkd1(-/-) cell growth, and reduces cystic burden in Pkd1(-/-) embryonic mice. To assess cyst progression in neonates, we used the kidney-specific Pkd1(flox/-);Ksp-Cre mouse model of autosomal dominant polycystic kidney disease, in which the burden of cysts is negligible at birth but then progresses rapidly over days. The number, size, and proliferation rate of cysts were examined. Treatment with triptolide significantly improved renal function at postnatal day 8 by inhibition of the early phases of cyst growth. Because the proliferative index of kidney epithelium in neonates versus adults is significantly different, future studies will need to address whether triptolide delays or reduces cyst progression in the Pkd1 adult model.

Published

2008

83. Wnt9b signaling regulates planar cell polarity and kidney tubule morphogenesis

Author

Thomas L. Carroll, Shigehisa Aoki, Peter Igarashi, Courtney M. Karner, John B. Wallingford, and Rani Chirumamilla

Subjects

Male, Cellular polarity, Morphogenesis, Biology, Kidney, Kidney morphogenesis, Article, 03 medical and health sciences, Cell polarity, Genetics, Polycystic kidney disease, medicine, Animals, 030304 developmental biology, 0303 health sciences, Convergent extension, 030302 biochemistry & molecular biology, Wnt signaling pathway, Cell Polarity, Gene Expression Regulation, Developmental, medicine.disease, Cell biology, Wnt Proteins, Tubule, Kidney Tubules, Female, Signal Transduction

Abstract

Although many vertebrate organs, such as kidneys, lungs and liver, are composed of epithelial tubules, little is known of the mechanisms that establish the length or diameter of these tubules. In the kidney, defects in the establishment or maintenance of tubule diameter are associated with one of the most common inherited human disorders, polycystic kidney disease. Here we show that attenuation of Wnt9b signaling during kidney morphogenesis affects the planar cell polarity of the epithelium and leads to tubules with significantly increased diameter. Although previous studies showed that polarized cell divisions maintain the diameter of postnatal kidney tubules, we find that cell divisions are randomly oriented during embryonic development. Our data suggest that diameter is established during early morphogenetic stages by convergent extension processes and maintained by polarized cell divisions. Wnt9b, signaling through the non-canonical Rho/Jnk branch of the Wnt pathway, is necessary for both of these processes.

Published

2008

84. Impaired sodium excretion and increased blood pressure in mice with targeted deletion of renal epithelial insulin receptor

Author

Pritmohinder S. Gill, C. Ronald Kahn, Swasti Tiwari, Peter Igarashi, James B. Wade, Nikhil Sharma, and Carolyn A. Ecelbarger

Subjects

Male, medicine.medical_specialty, Sodium, Urinary system, medicine.medical_treatment, chemistry.chemical_element, Fluorescent Antibody Technique, Natriuresis, Nitric oxide, Excretion, chemistry.chemical_compound, Mice, Internal medicine, Diabetes mellitus, medicine, Animals, Insulin, RNA, Messenger, Kidney Tubules, Collecting, Nitrites, Mice, Knockout, Kidney Medulla, Multidisciplinary, Nitrates, biology, Integrases, Reproducibility of Results, Epithelial Cells, Biological Sciences, medicine.disease, Receptor, Insulin, Insulin receptor, Endocrinology, chemistry, Gene Expression Regulation, Liver, Organ Specificity, Gene Targeting, biology.protein, Female, Gene Deletion

Abstract

Renal tubule epithelial cells express the insulin receptor (IR); however, their value has not been firmly established. We generated mice with renal epithelial cell-specific knockout of the IR by Cre-recombinase-loxP recombination using a kidney-specific (Ksp) cadherin promoter. KO mice expressed significantly lower levels of IR mRNA and protein in kidney cortex (49–56% of the WT) and medulla (32–47%) homogenates. Immunofluorescence showed the greatest relative reduction in the thick ascending limb and collecting duct cell types. Body weight, kidney weight, and food and water intakes were not different from WT littermates. However, KO mice had significantly increased basal systolic blood pressure (BP, 15 mm Hg higher) as measured by radiotelemetry. In response to a volume load by gavage (20 ml/kg of body weight, 0.9% NaCl, 15% dextrose), KO mice had impaired natriuresis (37 ± 10 versus 99 ± 9 mmol of Na + per 2 h in WT). Furthermore, volume load led to a sustained increase in BP in KO mice only. In contrast, insulin administration i.p. (0.5 units/kg of body weight) resulted in a significant fall in BP in WT, but not in KO mice. To test the role of reduced renal nitric oxide (NO) production in these responses, basal urinary nitrates plus nitrites excretion (UNOx) was measured and found to be 61% lower in KO vs. WT mice. Furthermore, acute insulin increased UNOx by 202% in the WT, relative to a significantly blunted rise (67%) in KO animals. These results illuminate a previously uncharacterized role for renal IR to reduce BP and facilitate sodium and water excretion, possibly via NO production.

Published

2008

85. Acute kidney injury and aberrant planar cell polarity induce cyst formation in mice lacking renal cilia

Author

Xinli Shao, Fangming Lin, Ling Li, Peter Igarashi, Vishal Patel, Stefan Somlo, and Patricia Cobo-Stark

Subjects

medicine.medical_specialty, Pathology, Kinesins, Mice, Transgenic, Biology, Kidney cysts, Mice, Internal medicine, Genetics, medicine, Polycystic kidney disease, Animals, Humans, Cyst, Cilia, Molecular Biology, Genetics (clinical), Renal stem cell, Kidney, Polycystic Kidney Diseases, urogenital system, Cysts, Cilium, Acute kidney injury, Cell Polarity, General Medicine, Articles, medicine.disease, Endocrinology, medicine.anatomical_structure, Acute Disease, Loop of Henle, Kidney Diseases, medicine.symptom, Kidney disease

Abstract

Polycystic kidney disease (PKD) is an inherited disorder that is characterized by the accumulation of cysts in the renal parenchyma and progressive decline in renal function. Recent studies suggest that PKD arises from abnormalities of the primary cilium. We have previously shown that kidney-specific inactivation of the ciliogenic gene Kif3a during embryonic development produces kidney cysts and renal failure. Here, we used tamoxifen-inducible, kidney-specific gene targeting to inactivate Kif3a in the postnatal mouse kidney. Kidney-specific inactivation of Kif3a in newborn mice resulted in the loss of primary cilia and produced kidney cysts primarily in the loops of Henle, whereas inactivation in adult mice did not lead to the rapid development of cysts despite a comparable loss of primary cilia. The age-dependence and locations of the cysts suggested that cyst formation required increased rates of cell proliferation. To test this possibility, we stimulated cell proliferation in the adult kidney by inducing acute kidney injury and tubular regeneration. Acute kidney injury induced cyst formation in adult Kif3a mutant mice. Analysis of pre-cystic tubules in Kif3a mutant mice showed that the loss of cilia did not stimulate cell proliferation but instead resulted in aberrant planar cell polarity as manifested by abnormalities in the orientation of cell division. We conclude that primary cilia are required for the maintenance of planar cell polarity in the mammalian kidney and that acute kidney injury exacerbates cystic disease.

Published

2008

86. Cyst formation and activation of the extracellular regulated kinase pathway after kidney specific inactivation of Pkd1

Author

Angeliki Louvi, Zhiheng Yu, Sekiya Shibazaki, Stefan Somlo, Michihiro Mitobe, Saori Nishio, Shuta Ishibe, Lloyd G. Cantley, Xin Tian, Peter Igarashi, Heino Velazquez, and R. Brent Thomson

Subjects

MAPK/ERK pathway, medicine.medical_specialty, TRPP Cation Channels, MAP Kinase Kinase 2, MAP Kinase Kinase 1, Apoptosis, Biology, urologic and male genital diseases, Kidney, chemistry.chemical_compound, Mice, Internal medicine, Nitriles, Genetics, medicine, Polycystic kidney disease, Butadienes, Animals, Cyst, Molecular Biology, Protein Kinase Inhibitors, Genetics (clinical), Cell Proliferation, Cystic kidney, Mitogen-Activated Protein Kinase 1, Mitogen-Activated Protein Kinase 3, PKD1, Kinase, urogenital system, Cysts, General Medicine, Articles, medicine.disease, Polycystic Kidney, Autosomal Dominant, Mice, Mutant Strains, Enzyme Activation, Disease Models, Animal, medicine.anatomical_structure, Endocrinology, chemistry, Cancer research, Bromodeoxyuridine

Abstract

Polycystic kidney disease (ADPKD) results from failure of the kidney to properly maintain three-dimensional structure after loss of either polycystin-1 or -2. Mice with kidney selective inactivation of Pkd1 during embryogenesis develop profound renal cystic disease and die from renal failure within 3 weeks of birth. In this model, cysts form exclusively from cells in which Cre recombinase is active, but the apparent pace of cyst expansion varies by segment and cell type. Intercalated cells do not participate in cyst expansion despite the presence of cilia up to at least postnatal day 21. Cystic segments show a persistent increase in proliferation as determined by bromodeoxyuridine (BrdU) incorporation; however, the absolute proliferative index is dependent on the underlying proliferative potential of kidney tubule cells. Components of the extracellular regulated kinase (MAPK/ERK) pathway from Ras through MEK1/2 and ERK1/2 to the effector P90(RSK) are activated in both perinatal Pkd1 and adult Pkd2 ortholgous gene disease models. The pattern of MAPK/ERK activation is focal and does not correlate with the pattern of active proliferation identified by BrdU uptake. The possibility of a causal relationship between ERK1/2 activation and cyst cell proliferation was assessed in vivo in the acute perinatal Pkd1 model of ADPKD using MEK1/2 inhibitor U0126. U0126 treatment had no effect on progression of cyst formation in this model at doses sufficient to reduce phospho-ERK1/2 in cystic kidneys. Cysts in ADPKD exhibit both increased proliferation and activation of MAPK/ERK, but cyst growth is not prevented by inhibition of ERK1/2 activation.

Published

2008

87. Kidney-targeted Birt-Hogg-Dubé gene inactivation in a mouse model: Erk1/2 and Akt-mTOR activation, cell hyperproliferation, and polycystic kidneys

Author

Robert M. Leighty, Peter L. Choyke, Peter Igarashi, Diana C. Haines, Laura S. Schmidt, Marcelino Bernardo, Lilia Ileva, Michelle B. Warren, W. Marston Linehan, Vishal Patel, W. Gregory Alvord, Lino Tessarollo, Berton Zbar, Masaya Baba, Eileen Southon, Seung-Beom Hong, Masahiro Yao, and Mutsuo Furihata

Subjects

Cancer Research, Tumor suppressor gene, Genotype, Estrone, Immunoblotting, Fluorescent Antibody Technique, Kaplan-Meier Estimate, Kidney, Birt–Hogg–Dubé syndrome, Article, Mice, Random Allocation, Germline mutation, Proto-Oncogene Proteins, medicine, PTEN, Animals, Gene Silencing, Folliculin, PI3K/AKT/mTOR pathway, Germ-Line Mutation, Cell Proliferation, Cystic kidney, Mice, Knockout, Mitogen-Activated Protein Kinase 1, Sirolimus, Polycystic Kidney Diseases, Antibiotics, Antineoplastic, Mitogen-Activated Protein Kinase 3, biology, Reverse Transcriptase Polymerase Chain Reaction, TOR Serine-Threonine Kinases, Tumor Suppressor Proteins, Syndrome, medicine.disease, Immunohistochemistry, Kidney Neoplasms, Blotting, Southern, Disease Models, Animal, medicine.anatomical_structure, Oncology, biology.protein, Cancer research, Protein Kinases, Signal Transduction

Abstract

Birt-Hogg-Dube (BHD) syndrome is an inherited kidney cancer syndrome that is characterized by benign hair follicle tumors, lung cysts, spontaneous pneumothorax, and an increased risk of renal neoplasia (1-3). We previously identified germline mutations in the BHD gene, which is located at chromosome 17p11.2, in BHD patients (4). Nearly all BHD mutations are frameshift or nonsense mutations that are predicted to prematurely truncate the BHD protein, folliculin (FLCN) (4-7). BHD patients most frequently develop bilateral multifocal chromophobe renal tumors and renal oncocytic hybrid tumors with features of chromophobe renal carcinoma and renal oncocytoma (8-10). Somatic mutations in the remaining wild-type copy of BHD and loss of heterozygosity at chromosome 17p11.2 have been identified in BHD-associated renal tumors, supporting the Knudson “two-hit” hypothesis and a tumor suppressor role for BHD (11). Folliculin is a novel 64-kDa protein with no known functional domains (4). We recently identified FNIP1, the first folliculin-interacting protein, which also interacts with 5′-AMP-activated protein kinase (AMPK (12)), an important energy sensor in cells that negatively regulates mammalian target of rapamycin (mTOR), the master switch for cell growth and proliferation (13). We demonstrated that FLCN and FNIP1 could serve as substrates for AMPK in vitro and in vivo and that inhibition of AMPK activity resulted in reduced phosphorylation and decreased expression of these proteins. Phospho-folliculin levels were reduced by inhibition of mTOR activity. Under serum-starved conditions, the level of mTOR signaling was somewhat higher in BHD-null renal tumor cells than in BHD-restored cells (12). These results suggest that FLCN may play a role in cellular energy and nutrient sensing through interactions with the AMPK-mTOR signaling pathway. Mutations in several other tumor suppressor genes, including LKB1 (14), PTEN (15), and TSC1/2 (16), have been shown to lead to dysregulation of mTOR signaling and to the development of other hamartoma syndromes. Intriguingly, recent studies in yeast have suggested that Bhd activates Tor2 in opposition to the role of Tsc1/2 , which inhibits Tor2 in this model organism (17). Animal models of human cancer provide valuable research tools for dissecting the biochemical pathways responsible for neoplasia and for testing new therapeutic agents. Renal cystadenocarcinoma nodular dermatofibrosis (RCND) in dogs (18,19) and renal tumors in the Nihon rat (20,21) occur in animals that inherit a germline mutation in the corresponding BHD homolog. However, these naturally-occurring animal models may harbor additional genetic changes that could confound studies of the functional consequences of BHD inactivation. A genetically engineered mouse model provides a “clean” system with which to pursue FLCN functional studies. Here we report the generation of a conditionally targeted BHD allele and kidney-directed BHD inactivation in the mouse using the cadherin16 (KSP)-Cre transgene (22). We compared BHD-knockout and control kidneys by histology, cell proliferation measurements, immunostaining to evaluate activation of Raf-Erk1/2 and Akt-mTOR pathways, and evaluated the therapeutic effects of rapamycin treatment, an inhibitor of mTOR, on the BHD-knockout kidney phenotype.

Published

2008

88. Renal and bone marrow cells fuse after renal ischemic injury

Author

Peter Igarashi, Fangming Lin, Ling Li, and Phu Truong

Subjects

Nephrology, Male, medicine.medical_specialty, Pathology, Urinary system, Bone Marrow Cells, Mice, Transgenic, Biology, urologic and male genital diseases, Kidney, Sensitivity and Specificity, Mice, Sex Factors, Ischemia, Internal medicine, medicine, Animals, In Situ Hybridization, Fluorescence, Bone Marrow Transplantation, Recombination, Genetic, Cell fusion, Microscopy, Confocal, Acute kidney injury, Ischemic injury, General Medicine, medicine.disease, Coculture Techniques, medicine.anatomical_structure, Female, Bone marrow

Abstract

After acute kidney injury, bone marrow cells contribute to renal repair by converting into renal cells, but the mechanism of this conversion is not well understood. To determine whether cell fusion between bone marrow cells and injured renal cells plays a role, we subjected female mice expressing

Published

2007

89. Kidney cysts, pancreatic cysts, and biliary disease in a mouse model of autosomal recessive polycystic kidney disease

Author

Patricia Cobo-Stark, Scott S. Williams, Peter Igarashi, Stefan Somlo, and Leighton R. James

Subjects

Nephrology, medicine.medical_specialty, Pathology, Receptors, Cell Surface, Gallbladder Diseases, Biology, urologic and male genital diseases, Kidney, Kidney cysts, Polymerase Chain Reaction, Mice, Internal medicine, medicine, Polycystic kidney disease, Animals, Polycystic Kidney, Autosomal Recessive, Mice, Knockout, PKD1, Cysts, Pancreatic Ducts, Gallbladder, medicine.disease, Autosomal Recessive Polycystic Kidney Disease, Mice, Inbred C57BL, Disease Models, Animal, medicine.anatomical_structure, Endocrinology, Pediatrics, Perinatology and Child Health, Mutation, RNA, Female, Pancreatic cysts, medicine.symptom, Pancreatic Cyst, Pancreas

Abstract

Mutations in PKHD1 cause autosomal recessive polycystic kidney disease (ARPKD). We produced a mouse model of ARPKD by replacing exons 1-3 of Pkhd1 with a lacZ reporter gene utilizing homologous recombination. This approach yielded heterozygous Pkhd1 (lacZ/+) mice, that expressed beta-galactosidase in tissues where Pkhd1 is normally expressed, and homozygous Pkhd1 (lacZ/lacZ) knockout mice. Heterozygous Pkhd1 (lacZ/+) mice expressed beta-galactosidase in the kidney, liver, and pancreas. Homozygous Pkhd1 (lacZ/lacZ) mice lacked Pkhd1 expression and developed progressive renal cystic disease involving the proximal tubules, collecting ducts, and glomeruli. In the liver, inactivation of Pkhd1 resulted in dilatation of the bile ducts and periportal fibrosis. Dilatation of pancreatic exocrine ducts was uniformly seen in Pkhd1 (lacZ/lacZ ) mice, with pancreatic cysts arising less frequently. The expression of beta-galactosidase, Pkd1, and Pkd2 was reduced in the kidneys of Pkhd1 (lacZ/lacZ ) mice compared with wild-type littermates, but no changes in blood urea nitrogen (BUN) or liver function tests were observed. Collectively, these results indicate that deletion of exons 1-3 leads to loss of Pkhd1 expression and results in kidney cysts, pancreatic cysts, and biliary ductal plate malformations. The Pkhd1 (lacZ/lacZ ) mouse represents a new orthologous animal model for studying the pathogenesis of kidney cysts and biliary dysgenesis that characterize human ARPKD.

Published

2007

90. The role for HNF-1beta-targeted collectrin in maintenance of primary cilia and cell polarity in collecting duct cells

Author

Hong Zhang, Haiyan Wang, Peter Igarashi, Hirofumi Makino, Qin Yang, Kazuya Yamagata, Shigeru Akagi, Yanling Zhang, Thomas Hiesberger, Jun Eguchi, Jun Wada, Kenji Fukui, Yashpal S. Kanwar, Akihiro Yasuhara, and Izumi Iseda

Subjects

Cell Biology/Developmental Molecular Mechanisms, Cell Biology/Cell Growth and Division, lcsh:Medicine, Electrophoretic Mobility Shift Assay, Mice, Transgenic, Biology, Cell Line, Mice, 03 medical and health sciences, 0302 clinical medicine, Cell Biology/Membranes and Sorting, Cell polarity, Animals, Immunoprecipitation, Cilia, Kidney Tubules, Collecting, RNA, Small Interfering, lcsh:Science, Integral membrane protein, DNA Primers, Hepatocyte Nuclear Factor 1-beta, 030304 developmental biology, 0303 health sciences, Nephrology/Hereditary, Genetic, and Development Nephrology, Membrane Glycoproteins, Multidisciplinary, Base Sequence, Cilium, lcsh:R, Cell Polarity, Molecular Biology/Transcription Initiation and Activation, Apical membrane, Molecular biology, Transmembrane protein, Cell biology, Membrane protein, 030220 oncology & carcinogenesis, Ureteric bud, Body region, lcsh:Q, Research Article

Abstract

Collectrin, a homologue of angiotensin converting enzyme 2 (ACE2), is a type I transmembrane protein, and we originally reported its localization to the cytoplasm and apical membrane of collecting duct cells. Recently, two independent studies of targeted disruption of collectrin in mice resulted in severe and general defects in renal amino acid uptake. Collectrin has been reported to be under the transcriptional regulation by HNF-1alpha, which is exclusively expressed in proximal tubules and localized at the luminal side of brush border membranes. The deficiency of collectrin was associated with reduction of multiple amino acid transporters on luminal membranes. In the current study, we describe that collectrin is a target of HNF-1beta and heavily expressed in the primary cilium of renal collecting duct cells. Collectrin is also localized in the vesicles near the peri-basal body region and binds to gamma-actin-myosin II-A, SNARE, and polycystin-2-polaris complexes, and all of these are involved in intracellular and ciliary movement of vesicles and membrane proteins. Treatment of mIMCD3 cells with collectrin siRNA resulted in defective cilium formation, increased cell proliferation and apoptosis, and disappearance of polycystin-2 in the primary cilium. Suppression of collectrin mRNA in metanephric culture resulted in the formation of multiple longitudinal cysts in ureteric bud branches. Taken together, the cystic change and formation of defective cilium with the interference in the collectrin functions would suggest that it is necessary for recycling of the primary cilia-specific membrane proteins, the maintenance of the primary cilia and cell polarity of collecting duct cells. The transcriptional hierarchy between HNF-1beta and PKD (polycystic kidney disease) genes expressed in the primary cilia of collecting duct cells has been suggested, and collectrin is one of such HNF-1beta regulated genes.

Published

2007

91. Role of the hepatocyte nuclear factor-1beta (HNF-1beta) C-terminal domain in Pkhd1 (ARPKD) gene transcription and renal cystogenesis

Author

Xinli Shao, Marco Pontoglio, Andreas Reimann, Thomas Hiesberger, Peter Igarashi, Eric Gourley, Department of Internal Medicine, University of Texas Southwestern Medical Center [Dallas], Expression Génétique et Maladies, Institut Pasteur [Paris]-Centre National de la Recherche Scientifique (CNRS), Division of basic sciences, and Institut Pasteur [Paris] (IP)-Centre National de la Recherche Scientifique (CNRS)

Subjects

MESH: Kidney Diseases, Cystic, Transcription, Genetic, Mutant, MESH: Microscopy, Fluorescence, Kidney, medicine.disease_cause, Biochemistry, MESH: Down-Regulation, Mice, MESH: Histone Acetyltransferases, MESH: Protein Structure, Tertiary, MESH: Lectins, Isobutyrates, Genes, Reporter, Lectins, Gene expression, MESH: Animals, Promoter Regions, Genetic, Genes, Dominant, Histone Acetyltransferases, MESH: Receptors, Cell Surface, Mutation, MESH: DNA, MESH: Transcription Factors, Kidney Diseases, Cystic, DNA-Binding Proteins, Butyrates, Hepatocyte nuclear factors, MESH: Promoter Regions (Genetics), Kidney Tubules, MESH: Epithelial Cells, embryonic structures, MESH: Kidney Tubules, Dimerization, Plasmids, Protein Binding, MESH: Mutation, MESH: Mice, Transgenic, Down-Regulation, Mice, Transgenic, Receptors, Cell Surface, MESH: Butyric Acids, [SDV.BC]Life Sciences [q-bio]/Cellular Biology, Biology, Transfection, CREB, digestive system, Acetyltransferases, MESH: Plasmids, MESH: Cell Proliferation, medicine, Animals, Humans, Immunoprecipitation, MESH: Protein Binding, RNA, Messenger, MESH: Hepatocyte Nuclear Factor 1-beta, Molecular Biology, Transcription factor, MESH: Mice, Cell Proliferation, Hepatocyte Nuclear Factor 1-beta, MESH: RNA, Messenger, Binding Sites, MESH: Humans, MESH: Immunoprecipitation, MESH: Transcription, Genetic, MESH: Transfection, MESH: Genes, Reporter, Kidney metabolism, MESH: Acetyltransferases, Epithelial Cells, DNA, Cell Biology, MESH: Kidney, Molecular biology, Protein Structure, Tertiary, MESH: Hela Cells, Microscopy, Fluorescence, MESH: Binding Sites, MESH: Dimerization, MESH: Gene Deletion, biology.protein, Hepatocyte Nuclear Factor 1-Beta, MESH: Genes, Dominant, Gene Deletion, MESH: DNA-Binding Proteins, HeLa Cells, Transcription Factors

Abstract

Hepatocyte nuclear factor-1beta (HNF-1beta) is a homeodomain-containing transcription factor that regulates tissue-specific gene expression in the kidney and other epithelial organs. Mutations of HNF-1beta produce congenital cystic abnormalities of the kidney, and previous studies showed that HNF-1beta regulates the expression of the autosomal recessive polycystic kidney disease (ARPKD) gene, Pkhd1. Here we show that the C-terminal region of HNF-1beta contains an activation domain that is functional when fused to a heterologous DNA-binding domain. An HNF-1beta deletion mutant lacking the C-terminal domain interacts with wild-type HNF-1beta, binds DNA, and functions as a dominant-negative inhibitor of a chromosomally integrated Pkhd1 promoter. The activation of the Pkhd1 promoter by wild-type HNF-1beta is stimulated by sodium butyrate or coactivators CREB (cAMP-response element)-binding protein (CBP) and P/CAF. The interaction with CBP and P/CAF requires the C-terminal domain. Expression of an HNF-1beta C-terminal deletion mutant in transgenic mice produces renal cysts, increased cell proliferation, and dilatation of the ureter similar to mice with kidney-specific inactivation of HNF-1beta. Pkhd1 expression is inhibited in cystic collecting ducts but not in non-cystic proximal tubules, despite transgene expression in this nephron segment. We conclude that the C-terminal domain of HNF-1beta is required for the activation of the Pkhd1 promoter. Deletion mutants lacking the C-terminal domain function as dominant-negative mutants, possibly by preventing the recruitment of histone acetylases to the promoter. Cyst formation correlates with inhibition of Pkhd1 expression, which argues that mutations of HNF-1beta produce kidney cysts by down-regulating the ARPKD gene, Pkhd1. Expression of HNF-1alpha in proximal tubules may protect against cystogenesis.

Published

2005

92. Mechanical stimuli induce cleavage and nuclear translocation of the polycystin-1 C terminus

Author

Veronique, Chauvet, Xin, Tian, Herve, Husson, David H, Grimm, Tong, Wang, Thomas, Hiesberger, Thomas, Hieseberger, Peter, Igarashi, Anton M, Bennett, Oxana, Ibraghimov-Beskrovnaya, Stefan, Somlo, and Michael J, Caplan

Subjects

TRPP Cation Channels, Transgene, Autosomal dominant polycystic kidney disease, Mice, Transgenic, CHO Cells, Biology, Cleavage (embryo), Bioinformatics, urologic and male genital diseases, Cell Line, Mice, Cricetulus, Dogs, Clinical investigation, Cricetinae, Chlorocebus aethiops, medicine, Animals, Amino Acid Sequence, Sequence Deletion, Polycystin-1, Cell Nucleus, COS cells, Chemistry, urogenital system, C-terminus, Membrane Proteins, Proteins, Epithelial Cells, General Medicine, medicine.disease, Embryo, Mammalian, Polycystic Kidney, Autosomal Dominant, Nuclear translocation, female genital diseases and pregnancy complications, Cell biology, Transcription Factor AP-1, Cell nucleus, medicine.anatomical_structure, Kidney Tubules, Biochemistry, embryonic structures, COS Cells, Commentary, Stress, Mechanical, Signal transduction, Corrigendum, Nucleus, Signal Transduction

Abstract

Polycystin-1, the protein encoded by the principal gene involved in autosomal dominant polycystic kidney disease, has been implicated in extracellular sensing as well as in cell-cell and cell-matrix interactions. However, the precise mechanisms involved in polycystin-1 signaling are not well defined. A report in this issue of the JCI demonstrates that the C-terminal tail of polycystin-1 is cleaved from the membrane through regulated intramembrane proteolysis (RIP) and that this domain translocates to the nucleus, where it activates the AP-1 transcription pathway. This translocation appears to be modulated by polycystin-2, with which polycystin-1 is thought to interact. These findings provide what we believe to be the first evidence that polycystin-1 can signal directly to the nucleus and that polycystin-1–polycystin-2 interactions do not require colocalization of these proteins in the same membrane compartment.

Published

2004

93. Hematopoietic stem cells contribute to the regeneration of renal tubules after renal ischemia-reperfusion injury in mice

Author

Linheng Li, Stuart J. Shankland, William G. Couser, Kimberly R. Cordes, Leroy Hood, Peter Igarashi, and Fangming Lin

Subjects

Male, Pathology, medicine.medical_specialty, Indoles, Ischemia, Mice, Inbred Strains, Cell Separation, Biology, Antibodies, Nephropathy, Mice, Y Chromosome, medicine, Myocyte, Animals, Antigens, Ly, Regeneration, Genes, sry, Renal stem cell, In Situ Hybridization, Fluorescence, Cell Death, Staining and Labeling, Regeneration (biology), Hematopoietic Stem Cell Transplantation, Membrane Proteins, Cell Differentiation, Epithelial Cells, Galactosides, General Medicine, medicine.disease, Hematopoietic Stem Cells, beta-Galactosidase, Haematopoiesis, Proto-Oncogene Proteins c-kit, Kidney Tubules, Nephrology, Reperfusion Injury, Female, Stem cell, Biomarkers, Kidney disease

Abstract

Ischemia-reperfusion injury (I/R injury) is a common cause of acute renal failure. Recovery from I/R injury requires renal tubular regeneration. Hematopoietic stem cells (HSC) have been shown to be capable of differentiating into hepatocytes, cardiac myocytes, gastrointestinal epithelial cells, and vascular endothelial cells during tissue repair. The current study tested the hypothesis that murine HSC can contribute to the regeneration of renal tubular epithelial cells after I/R injury. HSC isolated from male Rosa26 mice that express β-galactosidase constitutively were transplanted into female nontransgenic mice after unilateral renal I/R injury. Four weeks after HSC transplantation, β-galactosidase-positive cells were detected in renal tubules of the recipients by X-Gal staining. PCR analysis of the male-specific Sry gene and Y chromosome fluorescence in situ hybridization confirmed the presence of male-derived cells in the kidneys of female recipients. Antibody co-staining showed that β-galactosidase was primarily expressed in renal proximal tubules. This is the first report to show that HSC can differentiate into renal tubular cells after I/R injury. Because of their availability, HSC may be useful for cell replacement therapy of acute renal failure. E-mail: fangming.lin@UTSouthwestern.edu

Published

2003

94. Genetics and pathogenesis of polycystic kidney disease

Author

Peter Igarashi and Stefan Somlo

Subjects

Polycystin-1, Pathology, medicine.medical_specialty, Kidney, Polycystic Kidney Diseases, TRPP Cation Channels, urogenital system, Membrane Proteins, Proteins, Receptors, Cell Surface, General Medicine, Biology, urologic and male genital diseases, medicine.disease, Collection system, Pathogenesis, medicine.anatomical_structure, Nephrology, medicine, Polycystic kidney disease, Chronic renal failure, Humans, Cyst, Kidney disease

Abstract

Eberhard Ritz Polycystic kidney disease (PKD), a common genetic cause of chronic renal failure in children and adults, is characterized by the accumulation of fluid-filled cysts in the kidney and other organs. The renal cysts originate from the epithelia of the nephrons and renal collecting system

Published

2002

95. A minimal Ksp-cadherin promoter linked to a green fluorescent protein reporter gene exhibits tissue-specific expression in the developing kidney and genitourinary tract

Author

Xinli Shao, Jane E. Johnson, James A. Richardson, Peter Igarashi, and Thomas Hiesberger

Subjects

Aging, Genetic Linkage, Transgene, Green Fluorescent Proteins, Urogenital System, Mice, Inbred Strains, Mice, Transgenic, Biology, Kidney, Green fluorescent protein, Mice, Genes, Reporter, medicine, Animals, Transgenes, Promoter Regions, Genetic, Regulation of gene expression, Reporter gene, Mice, Inbred ICR, Cadherin, Mesonephros, Gene Expression Regulation, Developmental, General Medicine, Cadherins, Embryo, Mammalian, Molecular biology, Luminescent Proteins, medicine.anatomical_structure, Kidney Tubules, Animals, Newborn, Nephrology, Ureteric bud

Abstract

Ksp-cadherin is a unique, tissue-specific member of the cadherin family of cell adhesion molecules that is expressed exclusively in tubular epithelial cells in the kidney and developing genitourinary (GU) tract. Transgenic mice carrying 3425 bp of the Ksp-cadherin 5' flanking region linked to a lacZ reporter gene express beta-galactosidase exclusively in the kidney, although the expression pattern is incomplete (Am J Physiol 277: F599-F610, 1999). To further define the region that mediates tissue-specific expression, transgenic mice carrying 1341 bp or 324 bp of the 5' flanking region linked to a green fluorescent protein (GFP) reporter gene were produced. Transgenic mice carrying 1341 bp of the 5' flanking region expressed GFP in all embryonic tissues that endogenously express Ksp-cadherin, including the ureteric bud, Wolffian duct, Mullerian duct, and developing tubules in the mesonephros and metanephros. In the adult kidney, GFP was highly expressed in thick ascending limbs of Henle's loops and collecting ducts and weakly expressed in proximal tubules and Bowman's capsules. Transgenic mice carrying 324 bp of the 5' flanking region exhibited expression exclusively in tubular epithelial cells in the developing kidney and GU tract. Immunoblot analysis showed that the expression of GFP was restricted to the kidney in adult mice. Taken together, these results demonstrate that 324 bp of the Ksp-cadherin 5' flanking region is sufficient to direct epithelial-specific expression in the developing kidney and GU tract. Transgenic mice that express GFP in the mesonephros, metanephros, ureteric bud, and sex ducts may be useful for cell lineage studies.

Published

2002

96. Ksp-cadherin gene promoter. II. Kidney-specific activity in transgenic mice

Author

Shuxian Liu-Chen, Frank H. Ruddle, Dilys A. Whyte, Peter S. Aronson, R. Brent Thomson, Cooduvalli S. Shashikant, and Peter Igarashi

Subjects

Regulation of gene expression, Aging, Physiology, Cadherin, Kidney metabolism, Gene Expression, Promoter, Mice, Inbred Strains, Mice, Transgenic, Biology, Cadherins, Embryo, Mammalian, Kidney, Molecular biology, Epithelium, Mice, medicine.anatomical_structure, Animals, Newborn, Gene expression, medicine, Animals, Transgenes, Promoter Regions, Genetic, Epithelial polarity, Epithelial cell differentiation

Abstract

Kidney-specific cadherin (Ksp-cadherin, cadherin 16) is a tissue-specific member of the cadherin superfamily that is expressed exclusively in the basolateral membrane of tubular epithelial cells in the kidney. To determine the basis for tissue-specific expression of Ksp-cadherin in vivo, we evaluated the activity of the promoter in transgenic mice. Transgenic mice containing 3.3 kb of the mouse Ksp-cadherin promoter and an Escherichia coli lacZ reporter gene were generated by pronuclear microinjection. Assays of β-galactosidase enzyme activity showed that the transgene was expressed exclusively in the kidney in both adult and developing mice. Within the kidney, the transgene was expressed in a subset of renal tubular epithelial cells that endogenously expressed Ksp-cadherin and that were identified as collecting ducts by colabeling with Dolichos biflorus agglutinin. In the developing metanephros, expression of the transgene in the branching ureteric bud correlated with the developmental expression of Ksp-cadherin. Identical patterns of expression were observed in multiple founder mice, indicating that kidney specificity was independent of transgene integration site. However, heterocellular expression was observed consistent with repeat-induced gene silencing. We conclude that the Ksp-cadherin gene promoter directs kidney-specific expression in vivo. Regulatory elements that are sufficient to recapitulate the tissue- and differentiation-specific expression of Ksp-cadherin in the renal collecting duct are located within 3.3 kb upstream to the transcriptional start site.

Published

1999

97. Radioactive Labeling of DNA and RNA Probes

Author

Peter Igarashi

Subjects

chemistry.chemical_compound, chemistry, Biochemistry, Oligonucleotide, Spin column-based nucleic acid purification, Nuclease protection assay, Isoamyl alcohol, DNA sequencing, Primer extension, DNA, Klenow fragment

Abstract

End-labeling is most commonly utilized for synthetic oligodeoxyribo-nucleotides, although double-stranded DNA may also be labeled (particularly if protruding 5′ ends are present). End-labeled oligonucleotides are used for hybridization probes, primer extension analysis, or DNA sequencing using the Maxam-Gilbert chemical cleavage method. End-labeled double- stranded DNA is used in nuclease protection assays and other applications requiring probes of defined length.

Published

1999

98. Immunochemical characterization of Na+/H+ exchanger isoform NHE4

Author

Peter S. Aronson, Markus Exner, Daniel Biemesderfer, Ming-Shiou Wu, Peter Igarashi, Paul Isenring, John H. Pizzonia, and Ali K. Abu-Alfa

Subjects

Sodium-Hydrogen Exchangers, Physiology, Recombinant Fusion Proteins, Blotting, Western, Enzyme-Linked Immunosorbent Assay, Biology, Transfection, Cell Line, Mice, L Cells, Western blot, Antibody Specificity, Gastric glands, medicine, Animals, Epithelial polarity, medicine.diagnostic_test, Antibodies, Monoclonal, Subcellular localization, Molecular biology, Fusion protein, Immunohistochemistry, Transport protein, Rats, Blot, Sodium–hydrogen antiporter, medicine.anatomical_structure, Biochemistry, Gastric Mucosa, Rabbits

Abstract

Mammalian Na+/H+exchangers (NHEs) are a family of transport proteins (NHE1–NHE5). To date, the cellular and subcellular localization of NHE4 has not been characterized using immunochemical techniques. We purified a fusion protein containing a portion of rat NHE4 (amino acids 565–675) to use as immunogen. A monoclonal antibody (11H11) was selected by ELISA. It reacted specifically with both the fusion protein and to a 60- to 65-kDa polypeptide expressed in NHE4-transfected LAP1 cells. By Western blot analysis, NHE4 was identified as a 65- to 70-kDa protein that was expressed most abundantly in stomach and in multiple additional epithelial and nonepithelial rat tissues including skeletal muscle, heart, kidney, uterus, and liver. Subcellular localization of NHE4 in the kidney was evaluated by Western blot analysis of membrane fractions isolated by Percoll gradient centrifugation. NHE4 was found to cofractionate with the basolateral markers NHE1 and Na+-K+-ATPase rather than the luminal marker γ-glutamyl transferase. In stomach, NHE4 was detected by immunoperoxidase labeling on the basolateral membrane of cells at the base of the gastric gland. We conclude that NHE4 is a 65- to 70-kDa protein with a broad tissue distribution. In two types of epithelial cells, kidney and stomach, NHE4 is localized to the basolateral membrane.

Published

1998

99. cDNA cloning and chromosomal localization of the human and mouse isoforms of Ksp-cadherin

Author

Peter Igarashi, David C. Ward, Peter S. Aronson, R. B. Thomson, Z. E. Muckler, and Susan E. Quaggin

Subjects

Gene isoform, Molecular Sequence Data, Mice, Inbred Strains, Biology, Kidney, Homology (biology), Mice, Gene mapping, Complementary DNA, Gene duplication, Genetics, Animals, Humans, Amino Acid Sequence, RNA, Messenger, Cloning, Molecular, Gene, In Situ Hybridization, Fluorescence, Sequence Homology, Amino Acid, Cadherin, Nucleic acid sequence, Chromosome Mapping, Sequence Analysis, DNA, Cadherins, Molecular biology, Multigene Family, Cell Adhesion Molecules, Chromosomes, Human, Pair 16

Abstract

Ksp-cadherin is a novel kidney-specific member of the cadherin superfamily of cell adhesion molecules. We have determined the complete cDNA coding sequences of both the human and the mouse isoforms of Ksp-cadherin. The inferred amino acid sequences of the human and mouse isoforms are 79 and 75% identical to the originally described rabbit isoform of Ksp-cadherin (Thomsonet al.,1995;J. Biol. Chem.270, 17594–17601), respectively. The relative locations of cadherin-specific sequence motifs, putativeN-glycosylation sites, and characteristic protein domains are entirely conserved in all three isoforms. Multiple organ Northern analyses indicate that, as in the rabbit, both the human and the mouse Ksp-cadherin transcripts appear to have distinct kidney-specific distributions. The human Ksp-cadherin gene (CDH16) maps to chromosome 16q21–proximal 16q22. The mouse Ksp-cadherin gene (Cdh16) was localized to a highly syntenic region of distal Chromosome 8. Both the human and the mouse Ksp-cadherin genes were localized to previously identified clusters of cadherin gene sequences, consistent with the hypothesis that most cadherin family members arose by gene duplication from a single ancestral gene at a relatively early stage in the evolution of the mammalian genome.

Published

1998

100. A conserved Hox axis in the mouse and human female reproductive system: late establishment and persistent adult expression of the Hoxa cluster genes

Author

Peter Igarashi, Hugh S. Taylor, and Gregory B. Vanden Heuvel

Subjects

Adult, Aging, Uterus, Gene Expression, Female reproductive system, Biology, Mice, Species Specificity, Pregnancy, Gene expression, medicine, Animals, Humans, Hox gene, Gene, Mullerian Ducts, Fallopian Tubes, In Situ Hybridization, Paramesonephric duct, Genetics, Homeodomain Proteins, Genes, Homeobox, Cell Biology, General Medicine, Genitalia, Female, Embryonic stem cell, Cell biology, medicine.anatomical_structure, Reproductive Medicine, Mesonephros, Vagina, Trans-Activators, Developmental plasticity, Female

Abstract

The mammalian female reproductive system arises from the uniform paramesonephric duct. The molecular mechanisms that establish differential development along this axis are unknown. We determined the pattern and timing of genes of the Hoxa axis in the development of the Mullerian tract. Hoxa-9, Hoxa-10, Hoxa-11, and Hoxa-13 are all expressed along the length of the paramesonephric duct in the embryonic mouse. After birth, a spatial Hox axis is established, corresponding to the postnatal differentiation of this organ system in the mouse. Hoxa-9 is expressed in the fallopian tubes, Hoxa-10 in the uterus, Hoxa-11 in the uterus and uterine cervix, and Hoxa-13 in the upper vagina. This expression pattern follows the paradigm of spatial colinearity but is a novel exception to temporal colinearity that has been considered typical of Hox genes. These genes remain expressed in the adult mouse and are expressed in the same pattern in the human. The female reproductive system undergoes dramatic structural and functional changes during the estrous cycle and in pregnancy, retaining a high degree of developmental plasticity. The late establishment of a Hox axis and persistent expression of Hox genes in the adult may play an important role in preserving this plasticity.

Published

1998