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80% of chronic kidney diseases are caused by the loss and the damage of a differentiated and postmitotic cell type, the podocytes. The size-selectivity of the blood filtration barrier is highly dependent on the complex interdigitation of the podocyte foot processes as well as of the slit membrane which is spanned in between. Changes of this specific morphology as well as a detachment of podocytes lead to the clinical hallmark of a nephrotic syndrome e.g. proteinuria and oedema formation.
Since specific drugs or therapies are usually not available, patients are often dependent on dialysis and transplantation. Therefore, intensive studies are necessary to understand the pathogenesis of glomerulopathies as well as to identify specific drugs. In the past, it was already demonstrated that the zebrafish is an ideal model to study kidney function and to screen for drugs, since the larvae quickly develop a simple glomerulus that is comparable to the glomeruli of mice, rat and human.
In the present work, a zebrafish model was established to study a specific glomerulopathy named focal segmental glomerulosclerosis (FSGS). FSGS is mainly characterized by histology of the glomeruli which shows segmental scar formation and matrix deposition due to an activation of parietal epithelial cells (PEC) lining the Bowman’s capsule. For this purpose, we used the nitroreductase/metronidazole (NTR/MTZ) system, in which a cytotoxic agent is exclusively generated in podocytes by the enzyme NTR resulting in apoptosis of cells. Firstly, the parameters for development of an FSGS-like disease were evaluated and the glomerular response to podocyte depletion was examined during three days after the induction of podocyte damage. Using classic histological techniques, immunofluorescence staining and transmission electron microscopy, it was possible to demonstrate that zebrafish larvae phenocopy human FSGS in important characteristics after partial podocyte depletion. Secondly, by intravascular injection of fluorescence-labeled high molecular weight dextran, we found that the filtration barrier became leaky. Moreover, we identified a severe podocyte foot process effacement, formation of subpodocyte space pseudocysts and loss of the slit membrane protein podocin. Morphometrical, histological and ultrastructural analysis revealed an enlargement of the glomerulus, proliferation of cuboidal PECs and intraglomerular deposition of extracellular matrix components, all typical hallmarks of FSGS. Further, we observed adhesions between the parietal and the visceral glomerular cell layer forming sclerotic lesions. However, it remains still unclear whether an inflammatory response is involved in the development of sclerotic lesions. Our microscopic analysis provided some evidence for immigration of immunocompetent cells like neutrophils, presumably due to induction of apoptosis in our model.
Taken together, in the present work a zebrafish model was established with characteristics of mammals FSGS which will be useful for pathomechanism studies as well as for drug screening.
Until today, more than 17% of the population in Mecklenburg Western-Pomerania suffer from chronic kidney disease (CKD) which was revealed by the SHIP study (Study of Health in Pomerania). 20% of CKD cases can be traced back to glomerulopathies. One common characteristic of glomerulopathies is the morphologic change of the glomerular filtration barrier which consists of endothelial cells, the glomerular basement membrane and podocytes. Under healthy conditions, the foot processes of the podocytes interdigitate with the foot processes of the neighboring podocytes with a filtration slit in between. Apart from the slit membrane protein nephrin, typical adherens junction proteins like occludin or JAM-A are also expressed at this cell-cell junction. This junction is therefore considered to be a specialized type of adherens junction, necessary to maintain the size-selectivity of the filtration barrier. During podocyte injury, podocyte foot processes lose their characteristic morphology and the typical meandering filtration slit becomes linearized, a process which is described as foot process effacement.
Since morphological change is directly linked to change or loss of function, ultrastructural analysis of the foot processes is necessary for diagnostics and research. By using 3D-structured illumination microscopy (3D-SIM), we quantified these morphological changes as well as studied a possible biomarker, the tight junction protein claudin 5 (CLDN5). Our study showed a spatially restricted up-regulation of CLDN5 in effaced filtration slit areas in biopsies of patients suffering from minimal change disease (MCD), focal and segmental glomerulosclerosis (FSGS) as well as in mice after NTS injection and in the uninephrectomy DOCA-salt mouse model. CLDN5/nephrin ratios of biopsies from patients with glomerulopathies and of tissue received from NTS-treated mice were significantly higher compared to controls. We found that in patients the CLDN5/nephrin ratios were negatively correlated with the filtration slit density. Since CLDN5 up-regulation was observed in several areas of high filtration slit density, we hypothesized that CDLN5 upregulation preceded visible foot process effacement. Taken together, we suggest that CLDN5 could be a helpful biomarker to identify an early change of the foot process morphology in addition to filtration slit density measurement. Additionally, correlation analysis of foot process effacement with patient data showed a significant negative correlation of the filtration slit density with proteinuria in MCD patients.
Podocytes are highly specialized kidney cells that are attached to the outer aspect of the glomerular capillaries and are damaged in more than 75% of patients with an impaired renal function. This specific cell type is characterized by a complex 3D morphology which is essential for proper filtration of the blood. Any changes of this unique morphology are directly associated with a deterioration of the size-selectivity of the filtration barrier. Since podocytes are postmitotic, there is no regenerative potential and the loss of these cells is permanent. Therefore, identification of small molecules that are able to protect podocytes is highly important. The aim of this work was to establish an in vivo high-content drug screening in zebrafish larvae. At first, we looked for a reliable podocyte injury model which is fast, reproducible and easy to induce. Since adriamycin is commonly used in rodents to damage podocytes, we administered it to the larvae and analyzed the phenotype by in vivo microscopy, (immuno-) histology and RT-(q)PCR. However, adriamycin did not result in a podocyte-specific injury in zebrafish larvae. Subsequently, we decided to use a genetic ablation model which specifically damages podocytes in zebrafish larvae. Treatment of transgenic zebrafish larvae with 80 µM metronidazole for 48 hours generated an injury resembling focal and segmental glomerulosclerosis which is characterized by podocyte foot process effacement, cell depletion and proteinuria. Following this, we established an in vivo high-content screening system by the use of a specific screening zebrafish strain. This screening strain expresses a circulating 78 kDa eGFP-labeled Vitamin D-binding fusion protein, which passes the filtration barrier only after glomerular injury. Therefore, we had an excellent readout to follow podocyte injury in vivo. We generated a custom image analysis software that measures the fluorescence intensity of podocytes and the vasculature automatically on a large scale. Furthermore, we screened a specific drug library consisting of 138 compounds for protective effects on larval podocytes using this in vivo high-content system. The analysis identified several initial hits and the subsequent validation experiments identified belinostat as a reliable and significant protective agent for podocytes. These results led to a patent request and belinostat is a promising candidate for a clinical use and will be tested in mammalian podocyte injury models.
Study of the effect of the podocyte-specific palladin knockout in mice with a 129 genetic background
(2023)
Worldwide, chronic kidney disease is one of the leading public health problems. Podocytes, highly specialized postmitotic cells in the filtration unit of the kidney glomerulus, are essential for the size selectivity of the filtration barrier. Loss of the complex 3D morphology of their interdigitating foot processes, effacement and detachment of the cells from the capillaries lead to proteinuria and often loss of kidney function.
Since the morphology of podocyte foot processes is highly dependent on an intact actin cytoskeleton and actin-binding proteins, we investigated the role of the actin-binding protein palladin in podocytes from mice with a 129 genetic background, that is more susceptible to kidney injury. PodoPalld129-/- mice were examined at 6 and 12 months of age using immunofluorescence staining, electron and 3D super-resolution microscopy as well as qRT-PCR.
Our analysis of PodoPalld129-/- mice at 6 and 12 months of age showed that podocyte- specific knockout of palladin results in dilation of the capillary tuft accompanied by loss of mesangial cells, indicating the influence of palladin on glomerular tuft formation. Besides, we observed morphological abnormalities such as an enlarged sub-podocyte space, cyst formations and an increased number of cell-cell contacts between podocytes and parietal epithelial cells in PodoPalld129-/- mice compared to controls. Moreover, palladin knockout resulted in downregulation of the slit diaphragm protein nephrin as well as an age-dependent significant increase in podocyte foot process effacement. Although there was a significant change in foot process morphology, we did not detect albuminuria in PodoPalld129-/- mice of both age groups. However, we found an increase of trefoil factor 1 (Tff1) in the urine of the mice, indicating an altered, more permeable filtration barrier.
Considering that palladin has several binding sites for important actin-binding and regulatory proteins, we studied the expression of Lasp-1, Pdlim2, VASP and Klotho in dependence on palladin. We found a remarkable reduction in, for example, phosphorylated Lasp-1 as well as Klotho, which could influence the morphology of podocyte foot processes.
Compared with PodoPalldBL/6-/- mice, PodoPalld129-/- mice showed stronger glomerular tuft dilation and developed podocytes with increased morphological abnormalities, underlining the importance of the genetic background.
In conclusion, these results demonstrate the essential role of palladin for podocyte morphology in mice with a 129 genetic background.