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Nestin Expression in Adult and Developing Human Kidney

Eugenio Bertelli, Marì Regoli, Luciano Fonzi, Rossella Occhini, Susanna Mannucci, Leonardo Ermini and Paolo Toti

Department of Pharmacology "Giorgio Segre" (EB,MR,LF), Department of Human Pathology and Oncology, Policlinico Le Scotte (RO,SM,PT), and Department of Evolutionary Biology (LE), University of Siena, Siena, Italy

Correspondence to: Eugenio Bertelli, Dept. of Pharmacology "Giorgio Segre", Section of Anatomy, University of Siena, Via Aldo Moro 4, I-53100 Siena, Italy. E-mail: bertelli5{at}unisi.it

	Summary

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Nestin is considered a marker of neurogenic and myogenic precursor cells. Its arrangement is regulated by cyclin-dependent kinase 5 (CDK5), which is expressed in murine podocytes. We investigated nestin expression in human adult and fetal kidney as well as CDK5 presence in adult human podocytes. Confocal microscopy demonstrated that adult glomeruli display nestin immunoreactivity in vimentin-expressing cells with the podocyte morphology and not in cells bearing the endothelial marker CD31. Glomerular nestin-positive cells were CDK5 immunoreactive as well. Western blotting of the intermediate filament-enriched cytoskeletal fraction and coimmunoprecipitation of nestin with anti-CDK5 antibodies confirmed these results. Nestin was also detected in developing glomeruli within immature podocytes and a few other cells. Confocal microscopy of experiments conducted with antibodies against nestin and endothelial markers demonstrated that endothelial cells belonging to capillaries invading the lower cleft of S-shaped bodies and the immature glomeruli were nestin immunoreactive. Similar experiments carried out with antibodies raised against nestin and -smooth muscle actin showed that the first mesangial cells that populate the developing glomeruli expressed nestin. In conclusion, nestin is expressed in the human kidney from the first steps of glomerulogenesis within podocytes, mesangial, and endothelial cells. This expression, restricted to podocytes in mature glomeruli, appears associated with CDK5. (J Histochem Cytochem 55:411–421, 2007)

Key Words: nestin • podocytes • cyclin-dependent kinase 5 • CD31 • -smooth muscle actin • immunohistochemistry • confocal microscopy

	Introduction

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THE RENAL CORPUSCLE consists of a tuft of blood capillaries surrounded by Bowman's capsule, a bowl-shaped double-layered epithelial structure. The two epithelial layers of the capsule, though continuous at the vascular pole of the corpuscle, are separated by an interval, the urinary space, into which the primary urine is ultrafiltrated. The inner layer of the capsule, tightly applied to the blood capillaries, is also referred to as the visceral layer and is formed of highly specialized epithelial cells called podocytes because of their peculiar shape. Along with the basement membrane and the fenestrated endothelial cells, these cells constitute the glomerular filtration barrier, whose integrity is essential for the filtration and proper composition of the primary urine. Several functions have been assigned to podocytes, including key roles in determining the permeability properties of the glomerular filter, in counteracting intraglomerular hydrostatic pressure, and in the synthesis of basement membrane components (Pavenstädt et al. 2003). Even though some of these functions are more supposed than definitely proven (Pavenstädt et al. 2003), the importance of podocytes in maintaining glomerular homeostasis and proper renal function is testified to by the development of proteinuria and progressive glomerulosclerosis upon their injury (Kriz et al. 1994; Ruggenenti et al. 2001; Gubler 2003). Podocytes display a very complex morphology that must be preserved to accomplish their delicate functions (Bariety et al. 1998; Nakahama et al. 1999; Hir et al. 2001; Kerajaschki 2001). The shape of podocytes is sui generis, with a cell body that protrudes into the capsule lumen and long primary processes anchored to the basement membrane by extending secondary processes referred to as foot processes. The foot processes of adjacent podocytes interdigitate on the surface of the basement membrane, leaving a space between them, the filtration slit, which is occupied by a thin diaphragm. The complex and ramified shape of podocytes has led some investigators to compare them with neurons. Indeed, an increasing number of features are described as being shared by the two cell types. First, podocytes and neurons are postmitotic terminally differentiated cells (Nagata et al. 1998; Gubler 2003); second, they express common sets of proteins including synaptopodin (Mundel et al. 1997; Czarnecki et al. 2005), nephrin (Putaala et al. 2001), cyclin-dependent kinase 5 (CDK5) (Griffin et al. 2004), olfactomedin-related glycoprotein (Kondo et al. 2000), a type III receptor protein tyrosine phosphatase (Beltran et al. 2003), and Rab3A and Rabphilin-3a (Rastaldi et al. 2003). Third, some transcription factors such as N-myc (Hirvonen et al. 1989) and Wilms' tumor suppressor protein (Armstrong et al. 1992) are at least transiently expressed either in neurons or podocytes. Finally, if on one hand the mechanism for the formation of podocyte processes is somehow similar to the development of neuronal dendrites (Kobayashi et al. 2004), on the other hand it has recently been shown that podocytes possess neuronal-like functional synaptic vesicles (Rastaldi et al. 2006). In this respect, the fact that CDK5 has been shown to regulate podocyte morphology (Griffin et al. 2004), coupled with the finding that CDK5 in neuronal progenitor ST15A cells and in C2C12 myoblasts is associated with nestin and governs its arrangement (Sahlgren et al. 2003), prompted us to investigate if nestin was expressed by human podocytes as well. Here we report that nestin is present in human podocytes, is associated with CDK5 and vimentin, and represents an early marker of developing glomeruli where it can be detected in the vesicles (the first epithelial structure consisting of polarized cells) and in the podocyte layer of the S-shaped bodies, in endothelial cells of blood capillaries invading the lower cleft of the S-shaped bodies and, finally, in mesangial precursor cells.

	Materials and Methods

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Antibodies
Primary antibodies were purchased as follows: mouse anti-nestin monoclonal antibody (MAb5326) and rabbit anti-nestin polyclonal antibody (Ab5922; Chemicon, Temecula, CA); mouse anti-SMA MAb (clone 1A4; Neomarkers, Fremont, CA); mouse anti-CD31 (clone JC70A) and anti-CD34 MAbs (clone QBEnd-10) from DakoCytomation (Glostrup, Denmark); mouse anti-vimentin MAb (clone V9; Sigma, St Louis, MO); and rabbit anti-CDK5 PAb C-8 and rabbit anti-vimentin (H-84) (Santa Cruz Biotechnology; Santa Cruz, CA).

Secondary antibodies were obtained from the following sources: double-labeling-grade tetramethylrhodamine isothiocyanate (TRITC)-conjugated donkey anti-mouse IgG and TRITC-conjugated donkey anti-rabbit IgG from Chemicon; fluorescein isothiocyanate-conjugated (FITC) goat anti-mouse IgG antibody from Sigma; double-labeling-grade horseradish peroxidase (HRP)-conjugated goat anti-rabbit IgG from Zymed (South San Francisco, CA); and rabbit anti-mouse IgG from DakoCytomation.

Tissues
Cases and controls were taken consecutively and retrospectively from the surgical and autoptic files of the department of Human Pathology and Oncology. Adult kidney samples were obtained from surgical nephrectomy for carcinoma (n=10, age range 24–78 years, median age 60 years). Kidneys were fixed in 4% buffered formalin for 24–48 hr, and normal tissue, far from the neoplasia, was sampled and paraffin embedded.

Fetal kidneys were obtained from autopsies for spontaneous abortion or induced termination of pregnancy (TP) (n=23; gestational age range, 16–37 weeks; median gestational age 22 weeks). Macerated and malformed stillbirths were not included in the study. The cause of spontaneous fetal death was placental in origin and included abruptio placentae, true cord knot, acute massive placenta infarcts, acute chorioamnionitis; and conditions associated with prolonged stress such as fetal growth restriction and other morphological signs of chronic suffering, as well as maternal preeclampsia and eclampsia, were excluded from this study. TP stemmed from either minor malformations unrelated to alterations in the urinary system or maternal (personal) reasons. A complete autopsy was carried out between the second and twelfth hour after fetal expulsion.

Selected samples for biochemical analysis were immediately frozen in liquid nitrogen and stored at –80C. Other fresh tissues (only from adult kidneys) were sampled for immunofluorescence histochemistry, cryoprotected with Killik Frozen Medium (Bio Optica; Milan, Italy), and promptly frozen in liquid nitrogen. Ten-µm-thick sections were cut at –25C, air-dried, fixed in acetone at –20C for 10 min, and stored at –80C.

Immunohistochemistry
Immunohistochemistry to detect nestin was performed as previously described (Toti et al. 2005). Three- to 5-µm sections were cut from each specimen, mounted on electrostatically charged slides, and dried. Sections were dewaxed, rehydrated, and washed in TBS. TBS was used for all subsequent washes and for antibody dilutions. Nestin antigenic sites were unmasked by heating sections in 0.01 M citrate buffer (pH 6.0) with a microwave oven (two 5-min cycles at 750 W) and were subsequently rinsed for 10 min in 3% hydrogen peroxide to block endogenous peroxidase. Slides were then incubated for 1 hr at room temperature with anti-nestin MAb (working dilution 1:200). The ABC system (Vector Laboratories; Burlingame, CA) was applied on sections of fetal samples, and the reaction was developed with 1 mg/ml 3,3'-diaminobenzidine tetrahydrochloride (Sigma) dissolved in TBS containing 0.3% H₂O₂. Sections of adult kidneys were incubated with a bridge antibody anti-mouse IgG for 30 min at room temperature, and the reactions were developed by the alkaline phosphatase–anti-alkaline phosphatase technique (Dakopatts; DakoCytomation) with new fuchsin. Harris hematoxylin was used for nuclear counterstaining. Negative controls were prepared by substituting the primary antibody with the corresponding preimmune serum. Cognate sections were stained with hematoxylin and eosin to check for renal pathologies or malformations.

Confocal Microscopy
A TCS 4D Leica (Wetzlar, Germany) confocal microscope was used to evaluate double-labeling experiments carried out on frozen sections of adult kidney and on formalin-fixed, paraffin-embedded sections of fetal kidney.

Frozen sections were incubated 2 hr at room temperature with anti-vimentin MAb (working dilution 1:50) or anti-CD31 MAb (working dilution 1:100) followed by FITC-conjugated anti-mouse IgG for 1 hr at room temperature; the second primary antibody, anti-nestin PAb (working dilution 1:200), was applied overnight at 4C followed for 1 hr at room temperature by the appropriate TRITC-conjugated secondary antibody (working dilution 1:50). Other experiments were carried out incubating sections with anti-nestin MAb (working dilution 1:100) or anti-CD31 MAb (working dilution 1:100) for 2 hr at room temperature, followed for 1 hr by TRITC-conjugated anti-mouse IgG (working dilution 1:50). Rabbit anti-CDK5 was then applied overnight at 4C, followed by HRP-conjugated anti-rabbit IgG for 1 hr at room temperature. Application of fluorescein-labeled tyramide amplification reagent (Perkin-Elmer; Boston, MA) catalyzed a HRP-driven reaction that resulted in the deposition of a fluorescent precipitate.

Sections of embryonic kidney were dewaxed, rehydrated, and processed as follows: they were incubated with rabbit anti-nestin PAb for 1 hr at room temperature followed by the ABC system according to manufacturer's instructions (Vector Laboratories); the second primary antibody, anti-CD34 MAb (working dilution 1:100) or anti-SMA MAb (working dilution 1:200), was applied overnight at 4C followed for 1 hr at room temperature by TRITC-conjugated anti-mouse IgG (working dilution 1:50). Final application of fluorescein-labeled tyramide amplification reagent (Perkin-Elmer) catalyzed a HRP-driven reaction that resulted in the deposition of a fluorescent precipitate on nestin antigenic sites.

SDS/PAGE Electrophoresis, Coimmunoprecipitation, and Western Blotting
To confirm our immunohistochemical results, Western blotting analysis with anti-nestin antibody was carried out on proteins of the intermediate filament-enriched cytoskeletal fraction (IFCF) of adult and fetal kidney, separated by SDS-PAGE. IFCFs were prepared as previously reported (Achtstaetter et al. 1986; Carapelli et al. 2004; Toti et al. 2005) and stored at –80C until use. Just before use, aliquots of IFCF were thawed and mixed with Laemmli sample buffer.

Immunoprecipitation experiments were carried out on total homogenates of adult renal cortex. Pieces of renal cortex were placed in homogenization buffer (50 mM Tris/HCl, 150 mM NaCl, 1 mM EDTA, 0.25% sodium deoxycholate, 1% NP-40, 1 mM PMSF, 2 µg/ml aprotinin, pH 7.4) and homogenized with a Dounce homogenizer. The suspension was centrifuged at 5000 x g for 10 min at 4C, and the protein content was measured with the microBCA protein assay reagent kit (Pierce; Rockford, IL). Samples were stored at –80C until use. Five hundred µl of homogenate was precleared with protein A–Sepharose (Sigma), centrifuged, and the pellet of Sepharose beads was placed in Laemmli sample buffer. Two µl of anti-CDK5 IgG or 3 µl of anti-vimentin PAb was added to the supernatant and incubated overnight at 4C, followed by 2 hr with the protein A–Sepharose. Immunocomplexes were washed three times with buffer, and the final pellet was resuspended in Laemmli sample buffer.

IFCFs, immunoprecipitates, and proteins released from the Protein A–Sepharose complexes used for the preclearings were separated by electrophoresis through a 6% polyacrylamide gel and transferred to nitrocellulose in a Bio-Rad Transblot apparatus (BioRad; Segrate, Italy). A 5% (w/v) solution of skim milk in TBS was used to quench nonspecific protein binding. Membranes were incubated overnight at room temperature with 1:2000 anti-nestin MAb in 5% (w/v) solution of skim milk in TBS. Specific bands were detected using an electrochemiluminescense kit (Roche Diagnostics; Milan, Italy).

	Results

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Adult Kidney
In adult kidney, nestin staining was restricted to glomeruli, smooth muscle cells of the arterioles, and some endothelial cells (Figures 1A –1C). The highest intensity of staining was referred to podocytes where nestin immunoreactivity was consistent (Figures 1A–1C) and to the tunica media of some arterioles. Even though with a variable degree of intensity, endothelial cells of arterioles and of some blood capillaries were nestin labeled as well (Figure 1A).

View larger version (97K): [in this window] [in a new window]   Figure 1 Nestin expression in adult kidney. (A–C) Nestin staining is located within glomeruli. (A) A glomerulus with an arteriole at the vascular pole (arrow). Staining is observed in the endothelial cells of the arteriole. (B,C) A glomerulus at low (B) and higher magnification (C). Staining is restricted to cells with the morphological features of podocytes. (D–L) Confocal microscopy analysis of nestin/vimentin (D–I) and nestin/CD31 (J–L) double-labeling experiments. (D–F) All nestin+ cells (red) costain with vimentin (green). (G–I) The morphology of nestin/vimentin double-labeled cells is typical of podocytes, with long and branched primary processes. (J–L) Endothelial CD31+ cells do not costain with nestin. Bars: A–C = 100 µm; D–L = 10 µm.

Because it has been reported that CDK5 is expressed in murine podocytes (Griffin et al. 2004), and that it plays a key role in the regulation of nestin organization (Sahlgren et al. 2003), we performed CDK5/nestin double-labeling experiments that showed a certain degree of colocalization of the two proteins (Figures 2A –2F). Moreover, because CDK5 has been previously reported in endothelial cells (Sharma et al. 2004), additional experiments have been carried out to rule out the possibility that CDK5 staining had to be referred in part to the glomerular endothelium. Indeed, confocal microscopy of CDK5/CD31 double-labeled sections showed two different staining patterns with no detectable colocalizations of the two antigens in the renal corpuscles (Figures 2G–2I). Remarkably, CDK5 fluorescence appeared frequently arranged parallel to the glomerular endothelium (Figure 2I).

View larger version (93K): [in this window] [in a new window]   Figure 2 Nestin/CDK5 colocalization. Confocal microscopy of sections from adult human kidney. (A–F) Nestin/CDK5 double labeling. (A–C) Low magnification showing an entire glomerulus. CDK5 appears expressed in nestin+ cells. (D–F) Higher magnification. Apparently, whereas nestin staining is restricted to the cell bodies and primary processes of podocytes, CDK5 labeling is extended throughout their entire cytoplasm, probably involving foot processes that cover capillary loops. (G–I) CDK5/CD31 double labeling. The stainings do not overlap. On the abluminal side of the glomerular endothelium, a thin CDK5+ thread occupying the typical position of pedicels covers the capillary loops. Bar = 10 µm.

View larger version (22K): [in this window] [in a new window]   Figure 3 Western blottings with anti-nestin antibody. (A) Two samples of the intermediate filament-enriched cytoskeletal fraction (IFCF) of cortex from adult kidneys display one or two immunoreactive bands migrating at 240 and 280 kDa. (B) Immunoprecipitates obtained with anti-vimentin (Lane 1) and anti-CDK5 (Lane 5) polyclonal antibodies were run in parallel with the IFCF of cortex from adult kidney as positive control (Lane 3) and with the pellets of protein A–Sepharose used to preclear the homogenates as negative control (Lanes 2 and 4). Nestin-immunoreactive bands are visible only in the immunoprecipitates (Lanes 1 and 5) and in the positive control (Lane 3). The nestin-immunoreactive bands migrate at 240 and 280 kDa and show that nestin coprecipitates with CDK5 and vimentin. A lower band likely represents a product of degradation. (C) One sample of the IFCF of cortex from a fetal kidney. The two immunoreactive bands migrate with the same relative mobility of the adult samples.

View larger version (186K): [in this window] [in a new window]   Figure 4 Nestin expression in developing kidney. (A) Low magnification of the nephrogenic area. Nestin staining is intense in the glomeruli at all the stages of development. (B) Renal vesicles (arrows) display some nestin+ epithelial cells. Endothelial cells of blood capillaries (triangles) are also nestin stained. (C) Two S-shaped bodies intensely stained. One of them displays nestin labeling in the epithelial cells that eventually differentiates into podocytes (lower arrow). The second S-shaped body (higher arrow) is also intensely stained in correspondence to the cells that populate the cleft. (D) At the capillary loop stage (arrows), immature podocytes are strongly labeled. In addition, endothelial cells of some blood capillaries are also nestin+ (triangles). Few endothelial or mesangial cells are labeled even within the developing glomeruli. (E,F) In mature glomeruli, nestin immunoreactivity is restricted to podocytes and to only a few parietal cells of Bowman's capsule (arrowheads). Bar = 100 µm.

View larger version (80K): [in this window] [in a new window]   Figure 5 Nestin expression in glomerular cells at various stages of development. (A–L) Confocal analysis of double-labeling experiments detecting nestin (green) and the mesangial marker smooth muscle actin (SMA) (red). Large round-shaped red spots (arrowheads) are autofluorescent red blood cells. (A–C) S-shaped body: among the nestin+ elements that invade the lower cleft, one cell (triangle) costains with SMA. (D–F) Capillary loop stage: several SMA-containing cells populate the glomeruli. Some of them (triangles) coexpress nestin. (G–I) Immature glomeruli are still provided with cells coexpressing nestin and SMA. (J–L) Mature glomeruli do not display any nestin-expressing mesangial cells. In contrast, the smooth muscle cells of the arteriolar media (arrow) are clearly double labeled. (M–X) Confocal analysis of double-labeling experiments detecting nestin (green) and the endothelial marker CD34 (red). Large round-shaped red and green spots (arrowheads) are autofluorescent red blood cells. (M–O) S-shaped body: apparently, at this stage, all endothelial cells that invade the lower cleft costain with CD34. (P–U) Capillary loop stage. (P–R) Some CD34+ coexpress nestin (triangles), but nestin immunoreactivity is overall less intense. (S–U) At the same stage, but when the glomeruli are a little more mature, double-labeled cells are definitely decreased in number (triangle). (V–X) Mature glomeruli do not display any nestin-expressing endothelial cells. Bars: A–L = 10 µm; M–X = 20 µm.

	Discussion

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Nestin, a high molecular mass intermediate filament (IF), was first described as expressed in central nervous system stem cells (Lendahl et al. 1990). Since then, several other tissues and cells, including skeletal and cardiac myogenic cells (Sejersen and Lendahl 1993; Kachinsky et al. 1995), Leydig cells (Lobo et al. 2004), adrenocortical cells (Bertelli et al. 2002; Toti et al. 2005), adult and embryonic pancreas (Lardon et al. 2002; Klein et al. 2003; Delacour et al. 2004; Street et al. 2004), and many other cell types (for review, see Wiese et al. 2004) have been reported to contain nestin. On the whole, however, stable expression of nestin in cells from adult individuals is considered a rare phenomenon and a marker of stem or progenitor cells (Lendahl et al. 1990; Wiese et al. 2004). The present investigation, demonstrating that nestin is constitutively expressed in adult human podocytes, should change this view. Moreover, as nestin has been recently shown in mouse and rat podocytes as well (Chen et al. 2006; Wagner et al 2006; Zou et al. 2006), its presence in human kidney confirms that it should play a fundamental role in the biology of the renal corpuscle. Because of its frequent species-specific variability, it is important to evaluate the pattern of expression of IF proteins in human samples. Even considering the same animal species, cells can change IF content once they are grown in culture (Franke et al. 1979; Virtanen et al. 1981). To mention a few examples, we recall membranous-epithelial (M-) cells that, in addition to cytokeratins, display vimentin in rabbits but not in other species (Jepson and Clark 1998; Carapelli et al. 2004) and pancreatic duct cells that express cytokeratin 20 in rats and pigs (Bouwens 1998; Bertelli et al. 2001; Bertelli and Bendayan 2005) but not in humans and mice (Bouwens 1998). However, many other cases could be listed and even podocytes differ in IF content from one animal species to another (Yaoita et al. 1999; Zou et al. 2006) showing, accordingly, that the molecular arrangement of the IF network can be quite diverse, depending on the animals. Nestin is expressed in undifferentiated and dividing cells in the central nervous system and in myogenic tissues (Lendahl et al. 1990; Sejersen and Lendahl 1993). Upon differentiation, nestin is downregulated and replaced by other IFs. Nevertheless, it is re-expressed upon injury and in regenerating phenomena (Frisen et al. 1995; Vaittinen et al. 2001). These features have led some investigators to propose nestin as a marker of multilineage progenitor cells (Wiese et al. 2004). Nestin expression has also been correlated to increased motility and tumor invasiveness (Dahlstrand et al. 1992; Thomas et al. 2004). It is evident that podocytes cannot be placed into such a framework. Podocytes are non-motile, postmitotic terminally differentiated cells that re-enter the cell cycle only in a limited set of diseases, namely, HIV glomerulopathy, collapsing glomerulopathy, and the cellular variant of focal segmental glomerulosclerosis (Pavenstädt et al. 2003).

Nestin has been functionally linked to CDK5. CDK5 seems to play a fundamental role in triggering the exit of neurons from the cell cycle and in inducing differentiation (Cicero and Herrup 2005). In addition, CDK5 is important in regulating the differentiation of muscle cells and the rearrangement of the nestin network (Lazaro et al. 1997; Sahlgren et al. 2003). To carry out its kinase activity, CDK5 requires an activator, p35, which has been reported to associate with nestin as well (Sahlgren et al. 2003). When activated, CDK5 phosphorylates nestin and, in this way, probably regulates nestin disassembling because phosphorylated nestin is detected exclusively in the Triton X-100 soluble fraction (Sahlgren et al. 2003). Our results demonstrate for the first time that in vivo nestin and CDK5 are coexpressed and associated in adult human podocytes. Moreover, our data show that, whereas CDK5 is diffuse throughout the entire cytoplasm, pedicels included, the nestin network is located in the cell body and in the primary processes, but not in the foot processes. This is in accordance with the notion that the IF network does not extend into foot processes (Drenckhahn and Franke 1988; Pavenstädt et al. 2003). CDK5 in podocytes likely plays multiple roles because it is probably responsible for the differentiation and exit from the cell cycle (Griffin et al. 2004). However, an additional and pivotal role could be the regulation of IF network extension, preventing it from invading foot processes. In support of this view, nestin disassembling has been reported as regulated by the active complex CDK5/p35 (Sahlgren et al. 2003), which has been spotted mainly gathered at the podocyte cell processes (Griffin et al. 2004).

Nestin, however, is not capable of forming IFs on its own, as it must copolymerize with other type III IF proteins (Sjoberg et al. 1994; Steinert et al. 1999). In accordance with the well-known expression of vimentin in podocytes (Holthöfer et al 1984; Stamenkovic et al. 1986; Moll et al. 1991), our immunocytochemical and biochemical results confirm that the nestin partner in human podocytes is vimentin. The persistence of nestin expression in adult postmitotic terminally differentiated cells, in contrast to the more general rule that would restrict nestin to undifferentiated and dividing cells, implies an involvement of nestin in peculiar roles specific for podocytes. The possibility of a structural strengthening of the podocyte IF network is not convincing because nestin, far from reinforcing vimentin IFs, has been shown to make them less stable (Steinert et al. 1999). Nestin/vimentin heterodimers, however, have been proposed to be located at the periphery of a core of vimentin homodimers with the long nestin carboxyl terminal that sticks out of the filament. The importance of this arrangement would reside in the ability of the carboxyl domain to interact with microfilaments and microtubules cross-linking the three distinct components of the cytoskeleton (Herrmann and Aebi 2000). These interconnections could result, therefore, in a net advantage for the mechanical stability of podocytes. Another possibility is that nestin may serve a regulatory function for the assembly state of vimentin because it has been demonstrated in mitotic cells where vimentin IFs, in spite of their phosphorylated state, disassemble only when nestin is coexpressed (Chou et al. 2003). In this respect, based also on our results, a functional chain linking CDK5, nestin, and vimentin could be envisioned in podocytes: active CDK5/p35 complex within foot processes would phosphorylate nestin which, in turn, could regulate vimentin disassembly, preventing the IF network from extending into the pedicels. This view is supported by the observation that, in puromomycin-induced nephrosis, nestin and vimentin are both overexpressed (Zou et al. 2006) and that foot process effacement is characterized by the presence of IFs within the cytoplasmic sheet that, replacing pedicels, covers the basement membrane (Kubosawa and Kondo 1994). At any rate, the proper architecture of the IF network seems essential to maintain foot process integrity. This is confirmed by experiments of nestin silencing with siRNA where the effect of nestin knock-down resulted in a marked decrease of podocyte processes (Chen et al. 2006).

The present investigation shows that nestin IF is expressed in human podocytes starting from the very beginning of their differentiation. The pattern of nestin expression during human glomerulogenesis shares some resemblances with that which has been observed in rat and mouse (Chen et al. 2006; Wagner et al. 2006; Zou et al. 2006) but also shows significant differences. In contrast to mouse developing kidney where nestin has been detected within podocytes only in mature glomeruli (Chen et al. 2006), in humans nestin appears to be expressed from the first stage of glomerulogenesis (V stage). Throughout the following stages of development, nestin staining becomes more intense, localizing preferentially in the epithelial cells of the visceral layer. This behavior seems closer to what has been reported in rat developing kidney (Zou et al. 2006). On the other hand, whereas nestin expression in human differentiating glomerular endothelial cells is in accordance with mouse glomerulogenesis (Chen et al. 2006), our finding of a further expression in mesangial precursors seems to be unique to human immature glomeruli.

In Western blotting, nestin is usually reported as migrating as a double-immunoreactive band at 220 and 240 kDa (Sultana et al. 1998; Sahlgren et al. 2001; Lobo et al. 2004; Wiese et al. 2004). However, our evaluation gives considerably higher molecular masses, 240 and 280 kDa. Our values, in accordance with other studies (Messam et al. 2000; Chou et al. 2003; Toti et al. 2005; Zou et al. 2006), point toward nestin heavy posttranslational modifications as possibly serving particular functions in podocytes and in a few other particular cell types. Otherwise, considering that the molecular mass predicted by the amino acid sequence should be only 177 kDa and that posttranslational modifications should add 100 kDa to the molecule, the existence of alternative splicings of nestin gene is a possibility that should also be considered. However, more studies are required to clarify this point.

In conclusion, the present investigation has shown, for the first time, that human podocytes express nestin and that this is associated in vivo with CDK5, which is also located within the foot processes where nestin is not detectable. Moreover, we have demonstrated that, during glomerulogenesis, nestin is expressed in differentiating and mature podocytes, in some endothelial cells and, for the first time, in mesangial precursors.

	Acknowledgments

 
This work was supported by PAR2004 (quota servizi) (to EB) and PRIN2004 (to PT).

	Footnotes

 
Received for publication July 13, 2006; accepted December 20, 2006

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