Immuno-Localization of CD44 and Osteopontin in Developing Human Kidney

Crisi, Giovanna M.; Marconi, Sharon; Rockwell, Gary; Braden, Gregory; Campfield, Thomas

doi:10.1203/pdr.0b013e31818912b7

Cited by 10 publications

(6 citation statements)

References 45 publications

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“…WT1 is highly expressed in early metanephrogenic epithelial structures in fetal kidneys, while its expression is absent in the UB of the developing kidney [ 4 ]. Meanwhile, MUC-1 is known to be expressed in the UB of the developing kidney [ 22 , 40 ], which was differentially expressed in the triphasic tumours in our microarray data. We examined whether the WT1-negative and MUC-1 positive (WT1 - /MUC-1 + ) epithelial structures ( Fig 4B , S5A and S5B Fig ) in WTs are equivalent to the UB of the developing kidney.…”

Section: Resultsmentioning

confidence: 99%

The developmental programme for genesis of the entire kidney is recapitulated in Wilms tumour

et al. 2017

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Wilms tumour (WT) is an embryonal tumour that recapitulates kidney development. The normal kidney is formed from two distinct embryological origins: the metanephric mesenchyme (MM) and the ureteric bud (UB). It is generally accepted that WT arises from precursor cells in the MM; however whether UB-equivalent structures participate in tumorigenesis is uncertain. To address the question of the involvement of UB, we assessed 55 Wilms tumours for the molecular features of MM and UB using gene expression profiling, immunohistochemsitry and immunofluorescence. Expression profiling primarily based on the Genitourinary Molecular Anatomy Project data identified molecular signatures of the UB and collecting duct as well as those of the proximal and distal tubules in the triphasic histology group. We performed immunolabeling for fetal kidneys and WTs. We focused on a central epithelial blastema pattern which is the characteristic of triphasic histology characterized by UB-like epithelial structures surrounded by MM and MM-derived epithelial structures, evoking the induction/aggregation phase of the developing kidney. The UB-like epithelial structures and surrounding MM and epithelial structures resembling early glomerular epithelium, proximal and distal tubules showed similar expression patterns to those of the developing kidney. These observations indicate WTs can arise from a precursor cell capable of generating the entire kidney, such as the cells of the intermediate mesoderm from which both the MM and UB are derived. Moreover, this provides an explanation for the variable histological features of mesenchymal to epithelial differentiation seen in WT.

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Section: Resultsmentioning

confidence: 99%

The developmental programme for genesis of the entire kidney is recapitulated in Wilms tumour

et al. 2017

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“…Immunohistochemical staining was performed on a DakoCytomation AutoStainer using the Dako ADVANCE HRP/DAB staining kit protocol in accordance with the Signet Acuity data sheet (Dako, Carpenteria, CA), as previously reported (32). The antibodies used included mouse monoclonal antibody anti-CSR clone 5C10 corresponding to amino acids 214-235 of the human CSR (1:10,000; Novus Biologicals, Littleton, CO) (33), rabbit polyclonal antibody anti-CSR corresponding to amino acids 345-359 of the bovine CSR (1:500, generous gift of Edward M. Brown) (34), monoclonal antihuman EMA clone E29 (1:4,000; Dako) (35), monoclonal CD10 clone 56C6 (1:200; Vector Laboratories, Burlingame, CA) (36), and polyclonal antibody to PAX2 (1:100; Invitrogen, Camarillo, CA) (37).…”

Section: Calcium Receptor In Human Kidneymentioning

confidence: 99%

Immunolocalization of the calcium-sensing receptor in developing human kidney

et al. 2013

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Background:The calcium-sensing receptor (CSR) is a G-protein receptor that plays a critical role in calcium regulation. In the kidney, the CSR regulates calcium reabsorption in the thick ascending limb, where stimulation of the CSR inhibits calcium reabsorption in response to increased calcium in the peritubular fluid. In the collecting duct, apical CSR activation may play a role in osmoregulation, increasing water excretion in response to increased luminal calcium. Methods: We studied the ontogeny of the CSR in developing human kidney using immunohistochemical methods. results: The CSR is first expressed in the S-shaped body in the region destined to form the ascending limb and distal tubule. Other regions of the S-shaped body, as well as ureteric buds, do not express the CSR. The CSR is observed in thick ascending limb as early as 20 wk of development. The CSR is not observed in proximal tubule or collecting duct between 20 and 40 wk of human development. conclusion: During early human renal development, CSR expression is limited to the thick ascending limb and distal tubule, where this receptor may play a role in calcium homeostasis between 20 and 40 wk of human development.

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“…Indeed, our experience suggests long‐term retention of the glomeruli while the renal tubules (especially the distal segments) are progressively lost. This phenomenon is not due to fibrosis or the conversion of the LN into a fibrotic environment, as suggested by staining for Erasmus University Rotterdam‐Thymic Reticulum (ER‐TR7), CD44, and platelet‐derived growth factor receptor beta (PDGFR‐β; Figure S4), which are expressed in kidney during development and/or adult life (Crisi, Marconi, Rockwell, Braden, & Campfield, ; Floege et al, ; Tsujie et al, ), and overexpressed during renal disease (Floege, Eitner, & Alpers, ; Kirimca, Sarioglu, Camsari, & Kavukcu, ; Roy‐Chaudhury et al, ; Wagrowska‐Danilewicz & Danilewicz, ). The precise mechanism of tubular loss in our ectopic human kidney grafts remains unknown.…”

Section: Overviewmentioning

confidence: 93%

Kidney‐in‐a‐lymph node: A novel organogenesis assay to model human renal development and test nephron progenitor cell fates

Francipane

Han

Oxburgh

et al. 2019

J Tissue Eng Regen Med

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Stem cell‐derived organoids are emerging as sophisticated models for studying development and disease and as potential sources for developing organ substitutes. Unfortunately, although organoids containing renal structures have been generated from mouse and human pluripotent stem cells, there are still critical unanswered questions that are difficult to attain via in vitro systems, including whether these nonvascularized organoids have a stable and physiologically relevant phenotype or whether a suitable transplantation site for long‐term in vivo studies can be identified. Even orthotopic engraftment of organoid cultures in the adult does not provide an environment conducive to vascularization and functional differentiation. Previously, we showed that the lymph node offers an alternative transplantation site where mouse metanephroi can differentiate into mature renal structures with excretory, homeostatic, and endocrine functions. Here, we show that the lymph node lends itself well as a niche to also grow human primary kidney rudiments and can additionally be viewed as a platform to interrogate emerging renal organoid cultures. Our study has a wide‐ranging impact for tissue engineering approaches to rebuild functional tissues in vivo including—but not limited to—the kidney.

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Immuno-Localization of CD44 and Osteopontin in Developing Human Kidney

Cited by 10 publications

References 45 publications

The developmental programme for genesis of the entire kidney is recapitulated in Wilms tumour

The developmental programme for genesis of the entire kidney is recapitulated in Wilms tumour

Immunolocalization of the calcium-sensing receptor in developing human kidney

Kidney‐in‐a‐lymph node: A novel organogenesis assay to model human renal development and test nephron progenitor cell fates

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