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Techniques to Assess Kidney Function in Mouse Models of Glomerular Disease
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Summary
This protocol describes a full kidney work-up that should be carried out in mouse models of glomerular disease. The methods allow for detailed functional, structural, and mechanistic analysis of glomerular function, which can be applied to all mouse models of glomerular disease.
Abstract
The use of murine models to mimic human kidney disease is becoming increasingly common. This protocol describes a full kidney work-up that should be carried out in mouse models of glomerular disease, enabling a vast amount of information regarding kidney and glomerular function to be obtained from a single mouse. In comparison to alternative methods presented in the literature to assess glomerular function, the use of the method outlined in this paper enables the glomerular phenotype to be fully evaluated from multiple aspects. By using this method, the researcher can determine the kidney phenotype of the model and assess the mechanism as to why the phenotype develops. This vital information on the mechanism of disease is required when examining potential therapeutic avenues in these models. The methods allow for detailed functional assessment of the glomerular filtration barrier through measurement of the urinary albumin creatinine ratio and individual glomerular water permeability, as well as both structural and ultra-structural examination using the Periodic Acid Schiff stain and electron microscopy. Furthermore, analysis of the genes dysregulated at the mRNA and protein level enables mechanistic analysis of glomerular function. This protocol outlines the generic but adaptable methods that can be applied to all mouse models of glomerular disease.
Introduction
The use of murine models to mimic human kidney disease is becoming increasingly common. Such murine models include 1) spontaneous models such as spontaneously hypertensive rats (SHR)1, streptozotocin (STZ)-induced diabetic rats and mice2, and the db/db type II diabetic mice3, 2) genetically engineered models such as primary podocyte-specific focal segmental glomerular sclerosis (FSGS) models4, the podocyte-specific vascular endothelial growth factor A (VEGF-A) knock-out (VEGF-A KO) model5, and Alport syndrome models6, and 3) a....
Protocol
All experiments were conducted in accordance with UK legislation and local ethical committee approval. Animal studies were approved by University of Bristol research ethics committee.
Assessment of glomerular phenotype in mouse models of glomerular injury
1. Urinary albumin creatinine ratio (uACR)
- Urine should be collected at baseline and at regular intervals.
- Set up mouse metabolic cages with water and enrichment diet. Place mice in individual c.......
Representative Results
Progressive depletion of podocyte VEGF-A results in albuminuria, which is rescued by the constitutive expression of the human VEGF-A165b splice isoform
Urine was collected using metabolic cages from wild type (WT), inducible podocyte-specific VEGF-A knock out (VEGF-A KO), and VEGF-A KO X Neph-VEGF165b mice (VEGF-A KO mice that over-express the human VEGF-A<.......
Discussion
This protocol describes a full kidney work-up that should be carried out in mouse models of glomerular disease, enabling a vast amount of information regarding kidney and glomerular function to be obtained from a single mouse. The critical steps in each method allow for detailed functional, structural, and mechanistic analysis of glomerular function, including assessment of the permeability of the kidneys as a whole (uACR and plasma creatinine measurements), the permeability of individual glomeruli (glomerular Lp
Acknowledgements
This work was supported by the British Heart Foundation, Richard Bright VEGF Research Trust and the MRC.
....Materials
| Name | Company | Catalog Number | Comments |
| Metabolic Cages | Harvard Apparatus | 52-6731 | |
| Mouse Albumin ELISA Quantitation Set | Bethyl Laboratories | E90-134 | |
| Creatinine Companion | Exocell | 1012 Strip Plate | |
| Glass Capillary Tubes | Harvard Apparatus | EC1 64-0770 | |
| Glomerular Permeability Rig | Built at the Univeristy of Bristol - not comercially available | ||
| 100 μm Stainless Steel Sieve | Cole-Parmer | WZ-59984-18 | |
| 70 μm Stainless Steel Sieve | Cole-Parmer | WZ-59984-21 | |
| Periodic Acid-Schiff (PAS) Staining System | Sigma-Aldrich | 395B-1KT | |
| Hematoxylin | Sigma-Aldrich | H3136 | |
| Poly-Prep Slides | Sigma-Aldrich | P0425-72EA | |
| Nephrin (1243-1256) Antibody | Acris | BP5030 | |
| Anti-Podocin | Sigma-Aldrich | P0372-200UL | |
| Anti-CD31 | BD Biosciences | 550274 | |
| NP40 Cell Lysis Buffer | ThermoFisher Scientific | FNN0021 | |
| Halt Protease and Phosphatase Inhibitor Cocktail | ThermoFisher Scientific | 78437X4 | |
| TRIzol | ThermoFisher Scientific | 15596018 | |
| Dnase I | New England Biolabs | M0303S | |
| M-MLV Reverse Transcriptase | New England Biolabs | M053S | |
| Bovine Serum Albumin | Sigma-Aldrich | A2058 |
References
- Humtstrom, M. Development of structural kidney damage in spontaneously hypertensive rats. J Hypertens. 30 (6), 1087-1091 (2012).
- Kitada, M., Ogura, Y., Koya, D. Rodent models of diabetic nephropathy: their uti....
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