OrganIn VitroCulture: What Have We Learned about Early Kidney Development?

When Clifford Grobstein set out to study the inductive interaction between tissues in the developing embryo, he developed a method that remained important for the study of renal development until now. From the late 1950s on,in vitrocultivation of the metanephric kidney became a standard method. It provided an artificial environment that served as an open platform to study organogenesis. This review provides an introduction to the technique of organ culture, describes how the Grobstein assay and its variants have been used to study aspects of mesenchymal induction, and describes the search for natural and chemical inducers of the metanephric mesenchyme. The review also focuses on renal development, starting with ectopic budding of the ureteric bud, ureteric bud branching, and the generation of the nephron and presents the search for stem cells and renal progenitor cells that contribute to specific structures and tissues during renal development. It also presents the current use of Grobstein assay and its modifications in regenerative medicine and tissue engineering today. Together, this review highlights the importance ofex vivokidney studies as a way to acquire new knowledge, which in the future can and will be implemented for developmental biology and regenerative medicine applications.

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Genetic Dissection of Cadherin Function during Nephrogenesis

Molecular and Cellular Biology ◽

10.1128/mcb.22.5.1474-1487.2002 ◽

2002 ◽

Vol 22 (5) ◽

pp. 1474-1487 ◽

Cited By ~ 58

Author(s):

Ulf Dahl ◽

Anders Sjödin ◽

Lionel Larue ◽

Glenn L. Radice ◽

Stefan Cajander ◽

...

Keyword(s):

Kidney Development ◽

Morphological Changes ◽

Genetic Dissection ◽

Metanephric Mesenchyme ◽

Ureteric Bud ◽

Metanephric Kidney ◽

The Individual ◽

Deficient Mice

ABSTRACT The distinct expression of R-cadherin in the induced aggregating metanephric mesenchyme suggests that it may regulate the mesenchymal-epithelial transition during kidney development. To address whether R-cadherin is required for kidney ontogeny, R-cadherin-deficient mice were generated. These mice appeared to be healthy and were fertile, demonstrating that R-cadherin is not essential for embryogenesis. The only kidney phenotype of adult mutant animals was the appearance of dilated proximal tubules, which was associated with an accumulation of large intracellular vacuoles. Morphological analysis of nephrogenesis in R-cadherin −/− mice in vivo and in vitro revealed defects in the development of both ureteric bud-derived cells and metanephric mesenchyme-derived cells. First, the morphology and organization of the proximal parts of the ureteric bud epithelium were altered. Interestingly, these morphological changes correlated with an increased rate of apoptosis and were further supported by perturbed branching and patterning of the ureteric bud epithelium during in vitro differentiation. Second, during in vitro studies of mesenchymal-epithelial conversion, significantly fewer epithelial structures developed from R-cadherin −/− kidneys than from wild-type kidneys. These data suggest that R-cadherin is functionally involved in the differentiation of both mesenchymal and epithelial components during metanephric kidney development. Finally, to investigate whether the redundant expression of other classic cadherins expressed in the kidney could explain the rather mild kidney defects in R-cadherin-deficient mice, we intercrossed R-cadherin −/− mice with cadherin-6−/− , P-cadherin −/−, and N-cadherin +/− mice. Surprisingly, however, in none of the compound knockout strains was kidney development affected to a greater extent than within the individual cadherin knockout strains.

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Matrix metalloproteinases and their inhibitors regulate in vitro ureteric bud branching morphogenesis

AJP Renal Physiology ◽

10.1152/ajprenal.2000.279.5.f891 ◽

2000 ◽

Vol 279 (5) ◽

pp. F891-F900 ◽

Cited By ~ 35

Author(s):

Martin Pohl ◽

Hiroyuki Sakurai ◽

Kevin T. Bush ◽

Sanjay K. Nigam

Keyword(s):

Conditioned Medium ◽

Kidney Development ◽

Gelatin Zymography ◽

Branching Morphogenesis ◽

Complex Model ◽

Northern Analysis ◽

Metanephric Mesenchyme ◽

Ureteric Bud ◽

Direct Role

Mammalian kidney development is initiated by the mutual interaction between embryonic metanephric mesenchyme (MM) and the ureteric bud (UB), leading to tightly controlled UB branching morphogenesis. In a three-dimensional cell culture model, which employs MM cell-derived conditioned medium (BSN-CM) to induce UB cell branching morphogenesis in extracellular matrix (ECM) gels (Sakurai H, Barros EJ, Tsukamoto T, Barasch J, and Nigam SK. Proc Natl Acad Sci USA 94: 6279–6284, 1997), branching morphogenesis was inhibited by both chemical agents (ilomastat and 1,10-orthophenanthroline) and a physiological protein factor [tissue inhibitor of metalloproteinases (TIMP)-2], known to act as matrix metalloproteinase (MMP) inhibitors. In addition, UB branching was inhibited in isolated UB culture (Qiao J, Sakurai H, and Nigam SK. Proc Natl Acad Sci USA96: 7330–7335, 1999) by TIMP-2 and ilomastat, suggesting a direct role for MMPs in UB branching. Gelatin zymography and enzymatic measurement of MMP activity revealed that MMPs could originate from at least three different sources: the conditioned medium, the ECM, and the UB cells themselves. In the UB cells, transcription of several MMPs [gelatinase A (MMP2) and B (MMP9), stromelysin (MMP3), MT1-MMP] and TIMPs was altered by BSN-CM and changed as more complex branching structures formed. The ECM appeared to serve as both a reservoir for MMPs and modulated their expression because different ECM compositions altered the total MMP activity as well as specific subsets of MMPs expressed by the UB cells (as determined by zymography and Northern analysis). In the context of UB branching morphogenesis during kidney development, our data suggest a complex model in which soluble factors produced by the MM, in the context of specific ECM components, modulate the expression of specific subsets of MMPs and TIMPs in the UB, which alter as structures develop and the matrix environment changes. This suggests distinct roles for different subsets of MMPs and their inhibitors during different phases of branching morphogenesis.

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Dominant effects of RET receptor misexpression and ligand-independent RET signaling on ureteric bud development

Development ◽

10.1242/dev.126.7.1375 ◽

1999 ◽

Vol 126 (7) ◽

pp. 1375-1386 ◽

Cited By ~ 7

Author(s):

S. Srinivas ◽

Z. Wu ◽

C.M. Chen ◽

V. D'Agati ◽

F. Costantini

Keyword(s):

Kidney Development ◽

Collecting Duct ◽

Target Cells ◽

Metanephric Mesenchyme ◽

Ureteric Bud ◽

Independent Form ◽

Normal Expression ◽

Bud Growth

During kidney development, factors from the metanephric mesenchyme induce the growth and repeated branching of the ureteric bud, which gives rise to the collecting duct system and also induces nephrogenesis. One signaling pathway known to be required for this process includes the receptor tyrosine kinase RET and co-receptor GFR(α)-1, which are expressed in the ureteric bud, and the secreted ligand GDNF produced in the mesenchyme. To examine the role of RET signaling in ureteric bud morphogenesis, we produced transgenic mice in which the pattern of RET expression was altered, or in which a ligand-independent form of RET kinase was expressed. The Hoxb7 promoter was used to express RET throughout the ureteric bud branches, in contrast to its normal expression only at the bud tips. This caused a variable inhibition of ureteric bud growth and branching reminiscent of, but less severe than, the RET knockout phenotype. Manipulation of the level of GDNF, in vitro or in vivo, suggested that this defect was due to insufficient rather than excessive RET signaling. We propose that RET receptors expressed ectopically on ureteric bud trunk cells sequester GDNF, reducing its availability to the normal target cells at the bud tips. When crossed to RET knockout mice, the Hoxb7/RET transgene, which encoded the RET9 isoform, supported normal kidney development in some RET−/− animals, indicating that the other major isoform, RET51, is not required in this organ. Expression of a Hoxb7/RET-PTC2 transgene, encoding a ligand-independent form of RET kinase, caused the development of abnormal nodules, outside the kidney or at its periphery, containing branched epithelial tubules apparently formed by deregulated growth of the ureteric bud. This suggests that RET signaling is not only necessary but is sufficient to induce ureteric bud growth, and that the orderly, centripetal growth of the bud tips is controlled by the spatially and temporally regulated expression of GDNF and RET.

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FGF-7 modulates ureteric bud growth and nephron number in the developing kidney

Development ◽

10.1242/dev.126.3.547 ◽

1999 ◽

Vol 126 (3) ◽

pp. 547-554 ◽

Cited By ~ 11

Author(s):

J. Qiao ◽

R. Uzzo ◽

T. Obara-Ishihara ◽

L. Degenstein ◽

E. Fuchs ◽

...

Keyword(s):

Expression Patterns ◽

Body Volume ◽

Metanephric Mesenchyme ◽

Nephron Number ◽

Wild Type ◽

Ureteric Bud ◽

Kidney Size ◽

Bud Growth ◽

Collecting System

The importance of proportioning kidney size to body volume was established by clinical studies which demonstrated that in-born defecits of nephron number predispose the kidney to disease. As the kidney develops, the expanding ureteric bud or renal collecting system induces surrounding metanephric mesenchyme to proliferate and differentiate into nephrons. Thus, it is likely that nephron number is related to ureteric bud growth. The expression patterns of mRNAs encoding Fibroblast Growth Factor-7 (FGF-7) and its high affinity receptor suggested that FGF-7 signaling may play a role in regulating ureteric bud growth. To test this hypothesis we examined kidneys from FGF-7-null and wild-type mice. Results of these studies demonstrate that the developing ureteric bud and mature collecting system of FGF-7-null kidneys is markedly smaller than wild type. Furthermore, morphometric analyses indicate that mature FGF-7-null kidneys have 30+/−6% fewer nephrons than wild-type kidneys. In vitro experiments demonstrate that elevated levels of FGF-7 augment ureteric bud growth and increase the number of nephrons that form in rodent metanephric kidney organ cultures. Collectively, these results demonstrate that FGF-7 levels modulate the extent of ureteric bud growth during development and the number of nephrons that eventually form in the kidney.

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Abstract 15751: A New Role of Sox6 in Renin Regulation

Circulation ◽

10.1161/circ.130.suppl_2.15751 ◽

2014 ◽

Vol 130 (suppl_2) ◽

Author(s):

Jose Gomez ◽

Eric Sum ◽

Anna Keyte ◽

Conrad Hodgkinson ◽

Mary Hutson ◽

...

Keyword(s):

Blood Pressure ◽

Cell Fate ◽

Kidney Development ◽

Ex Vivo ◽

Expression Profiles ◽

Gene Expression Profiles ◽

Renin Angiotensin System ◽

Adult Kidney ◽

Fold Reduction

Introduction: The renin-angiotensin system (RAS) is an important component of blood pressure regulation in mammals. Renin catalyzes the rate limiting step of RAS, is produced and stored by Juxtaglomerular (JG) cells in the kidney. However, the transcriptional mechanisms that govern the specification of renin expressing cells under normal or pathophysiological conditions remain poorly understood. During blood pressure changes the number of adult renal cells expressing renin increase through a process termed JG recruitment. We found that this process involves differentiation mesenchymal stromal-like cells (MSC) to renin expressing cells. Our aim in this study was to determine new regulators of renin cell fate during kidney development and JG recruitment. Methods: Gene expression profiles of MSC and JG cells were performed with Affymetrix Mouse 430 2.0 array. In vitro assays were performed in adult renal MSCs isolated from C57BL6 Ren1c YFP mice. Renin expression in vitro was induced by treatment with IBMX and Forskolin. MSC were transduced with lentivirus carrying vectors for Sox6, Sox6 shRNA or controls. Ex vivo analysis was performed in embryonic kidneys (14.5 dpc) isolated and transduced with Sox6 or scrambled shRNA, kidneys were then cultured for 4 days and the expression of Sox6 and Renin analyzed by IHC. Results: Data showed that the transcription factor Sox6 is expressed in renin producing cells in the developing kidney (n=4) and in the adult kidney after stimulation that promotes JG recruitment (n=3). Overexpression of Sox6 (n=3, P<0.05) enhanced differentiation of renal MSCs to renin producing cells in vitro , and Sox6 knockdown reduced differentiation of renal MSC to renin producing cells in vitro (6-fold, n=4, P<0.01). Furthermore, knockdown of Sox6 in an ex vivo model of kidney development resulted in a 5-fold reduction in renin expressing cells (n=4, P<0.05). Conclusion: These results support a novel role for Sox6 in the development of renin expressing cells. This may have implications for renal development and physiology, opening new possibilities of addressing questions regarding both developmental and physiological regulation of renin.

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Endothelial cell targeting during renal development: use of monoclonal antibodies

AJP Renal Physiology ◽

10.1152/ajprenal.1997.272.2.f153 ◽

1997 ◽

Vol 272 (2) ◽

pp. F153-F159 ◽

Cited By ~ 4

Author(s):

J. A. Oliver ◽

M. R. Goldberg ◽

Q. Al-Awqati

Keyword(s):

Monoclonal Antibody ◽

Endothelial Cells ◽

Endothelial Cell ◽

Close Association ◽

Renal Development ◽

Cell Targeting ◽

Ureteric Bud ◽

Nephron Segments ◽

And Migration

Development of the different renal capillary beds requires that the transformation of the metanephrogenic mesenchyme and ureteric bud into the different nephron segments be temporally and spatially coordinated with the migration and growth of the endothelial cells present in the renal anlage. This suggests that ureteric bud and/or metanephrogenic mesenchymal cells provide molecules which guide endothelial cells to their appropriate locations. We found that monoclonal antibody (MAb) 5B6-E4, obtained with mechanically dispersed cells of embryonic day 15 (E15) rat renal anlage, identifies an antigen that is temporally and spatially associated with endothelial cell location and migration during renal development. Furthermore, 5B6-E4 disrupts the close association between ureteric bud ampullae and endothelial cells in E14 renal anlages grown in vitro: whereas 43% of the ureteric bud ampullae were in contact with endothelial cells in control conditions, the presence of 20 microg/ml 5B6-E4 reduced this number to 22% (P < 0.02). These results suggest that the antigen recognized by 5B6-E4 is involved in endothelial cell targeting during renal development.

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Murine homolog of SALL1 is essential for ureteric bud invasion in kidney development

Development ◽

10.1242/dev.128.16.3105 ◽

2001 ◽

Vol 128 (16) ◽

pp. 3105-3115 ◽

Cited By ~ 9

Author(s):

Ryuichi Nishinakamura ◽

Yuko Matsumoto ◽

Kazuki Nakao ◽

Kenji Nakamura ◽

Akira Sato ◽

...

Keyword(s):

Kidney Development ◽

Perinatal Period ◽

Homozygous Deletion ◽

Homeotic Gene ◽

Metanephric Mesenchyme ◽

Ureteric Bud ◽

Mouse Homolog ◽

Tubule Formation ◽

Murine Homolog ◽

Inductive Signal

SALL1 is a mammalian homolog of the Drosophilaregion-specific homeotic gene spalt (sal); heterozygous mutations in SALL1 in humans lead to Townes-Brocks syndrome. We have isolated a mouse homolog of SALL1 (Sall1) and found that mice deficient in Sall1 die in the perinatal period and that kidney agenesis or severe dysgenesis are present. Sall1 is expressed in the metanephric mesenchyme surrounding ureteric bud; homozygous deletion ofSall1 results in an incomplete ureteric bud outgrowth, a failure of tubule formation in the mesenchyme and an apoptosis of the mesenchyme. This phenotype is likely to be primarily caused by the absence of the inductive signal from the ureter, as the Sall1-deficient mesenchyme is competent with respect to epithelial differentiation. Sall1 is therefore essential for ureteric bud invasion, the initial key step for metanephros development.

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Conditioned medium from a rat ureteric bud cell line in combination with bFGF induces complete differentiation of isolated metanephric mesenchyme

Development ◽

10.1242/dev.122.12.4159 ◽

1996 ◽

Vol 122 (12) ◽

pp. 4159-4167 ◽

Cited By ~ 5

Author(s):

I.D. Karavanova ◽

L.F. Dove ◽

J.H. Resau ◽

A.O. Perantoni

Keyword(s):

Cell Line ◽

Conditioned Medium ◽

Culture System ◽

Expression Patterns ◽

Blot Hybridization ◽

Northern Blot Hybridization ◽

Metanephric Mesenchyme ◽

Ureteric Bud ◽

Nephron Differentiation

Differentiation of metanephric mesenchyme is triggered by an inductive signal(s) from the epithelial ureteric bud. As a result of this induction, most of the metanephric mesenchyme converts into epithelium of a nephron. We have developed and characterized an explant culture system, in which metanephric mesenchyme can grow and completely differentiate in vitro in the absence of an inductive tissue. When separated 13 dpc rat metanephric mesenchymes were cultured in serum-free conditioned medium from a rat ureteric bud cell line (RUB1) in the presence of bFGF and TGFalpha, they were induced to differentiate into nephron epithelia and glomeruli-like structures. The nephric type of differentiation was confirmed by both morphological and molecular criteria and paralleled the developmental changes of nephron differentiation in vivo. Expression patterns of brush-border antigen as well as molecular markers of kidney differentiation Wt1, Lim1, Hgf and c-met, c-ret, Shh, Wnt4, Wnt7b, and Wnt11 were analyzed in explants by whole mount and tissue section in situ hybridization following 1–9 days in culture. The expression of secreted patterning molecules Bmp7 and Wnt7b, but not Shh or Wnt11, were demonstrated by RT-PCR and northern blot hybridization with RNA from the RUB1 cells. Our culture system lends itself to examining the relevance of these and other signaling molecules required for nephron differentiation.

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Regulation of BMP7 expression during kidney development

Development ◽

10.1242/dev.125.17.3473 ◽

1998 ◽

Vol 125 (17) ◽

pp. 3473-3482 ◽

Cited By ~ 8

Author(s):

R.E. Godin ◽

N.T. Takaesu ◽

E.J. Robertson ◽

A.T. Dudley

Keyword(s):

Wnt Signaling ◽

Kidney Development ◽

Tooth Development ◽

Expression Patterns ◽

Wnt Signaling Pathway ◽

Sodium Chlorate ◽

Bmp Signaling ◽

Proteoglycan Synthesis ◽

Metanephric Mesenchyme ◽

Ureteric Bud

Members of the Bone Morphogenetic Protein (BMP) family exhibit overlapping and dynamic expression patterns throughout embryogenesis. However, little is known about the upstream regulators of these important signaling molecules. There is some evidence that BMP signaling may be autoregulative as demonstrated for BMP4 during tooth development. Analysis of BMP7 expression during kidney development, in conjunction with studies analyzing the effect of recombinant BMP7 on isolated kidney mesenchyme, suggest that a similar mechanism may operate for BMP7. We have generated a beta-gal-expressing reporter allele at the BMP7 locus to closely monitor expression of BMP7 during embryonic kidney development. In contrast to other studies, our analysis of BMP7/lacZ homozygous mutant embryos, shows that BMP7 expression is not subject to autoregulation in any tissue. In addition, we have used this reporter allele to analyze the expression of BMP7 in response to several known survival factors (EGF, bFGF) and inducers of metanephric mesenchyme, including the ureteric bud, spinal cord and LiCl. These studies show that treatment of isolated mesenchyme with EGF or bFGF allows survival of the mesenchyme but neither factor is sufficient to maintain BMP7 expression in this population of cells. Rather, BMP7 expression in the mesenchyme is contingent on an inductive signal. Thus, the reporter allele provides a convenient marker for the induced mesenchyme. Interestingly LiCl has been shown to activate the Wnt signaling pathway, suggesting that BMP7 expression in the mesenchyme is regulated by a Wnt signal. Treatment of whole kidneys with sodium chlorate to disrupt proteoglycan synthesis results in the loss of BMP7 expression in the mesenchyme whereas expression in the epithelial components of the kidney are unaffected. Heterologous recombinations of ureteric bud with either limb or lung mesenchyme demonstrate that expression of BMP7 is maintained in this epithelial structure. Taken together, these data indicate that BMP7 expression in the epithelial components of the kidney is not dependent on cell-cell or cell-ECM interactions with the metanephric mesenchyme. By contrast, BMP7 expression in the metanephric mesenchyme is dependent on proteoglycans and possibly Wnt signaling.

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