Background
Podocytes are terminally differentiated and highly specialized cells that reside on the glomerular basement membrane (GBM). As crucial components of the glomerular filtration barrier, podocytes play a key role in the pathogenesis of glomerular diseases [
1]. Due to limited podocytic proliferative capacity, it has been suggested that podocytes that are lost cannot be effectively replaced, causing damage to glomerular filtration barrier, development of proteinuria and progressive loss of renal function [
2-
5].
Angiopoietin-like-3 (Angptl3), a secreted protein, is mainly expressed in hepatocytes and weakly expressed in normal kidney cells [
6]. Our previous study found that the expression of Angptl3 was upregulated in nephrotic syndrome kidney tissue, and altered expression of Angptl3 in the glomerulus was associated with proteinuria and foot process effacement in kidney diseases [
7,
8]. Moreover, it was confirmed that following treatment with adriamycin or puromycin aminonucleoside (PAN), the expression of Angptl3 in podocytes was especially upregulated, and Angptl3 was involved in podocyte injury, Angptl3 increased the motility of podocytes, and ameliorated the PAN-induced detachment of podocytes [
9,
10]. Recently, it was further confirmed that Angptl3 induces F-actin rearrangement [
11]. Podocyte loss is caused by detachment of cells from the GBM and/or by apoptosis (programmed cell death) [
12]. Seminal studies have shown that podocyte cytoskeletal disaggregation preceded, and detachment from the GBM occurred in the PAN model; actin filament played a role in the regulation of cellular apoptosis, and disruption of F-actin could lead to increased levels of apoptosis [
13,
14]. Whether Angptl3 influences podocyte loss by affecting detachment and apoptosis is a crucial question that warrants further study.
Podocytes adhere to the GBM principally via integrin α3β1, which is believed to be a major receptor for extracellular matrix components of the GBM [
15]. Studies have reported that lower expression of integrin α3β1 in podocytes is found in a range of glomerular disorders in humans, and in a variety of experimental animal models of renal disease [
16]. Integrin-linked kinase (ILK) plays a key role in integrin-mediated cell adhesion and signaling [
17]. Overexpression of ILK in podocytes might reduce matrix adhesion and induce detachment of podocytes [
18].
Both the tumor suppressor protein p53 and caspases are involved in the crucial processes of renal and nonrenal cell apoptosis [
19,
20]. The occurrence of podocyte apoptosis directly or indirectly has a correlation with the activation of caspase3, and increased level of p53 induces apoptosis [
21,
22].
In the present study, it was hypothesized that Angptl3 plays a potential role in the PAN-induced podocyte loss by affecting detachment and apoptosis in vitro. Integrin α3β1, ILK, p53 and caspase3 are molecules of interest for further study to know the possible mechanism. However, the partial result obtained in the present study – recombinant Angptl3 protein aggravated the PAN-induced podocyte detachment is contrary to the results of our previous study, i.e. ANGPTL3 gene transfection ameliorates PAN-induced podocyte detachment [
9].
Methods
Antibodies and reagents
The antibodies and reagents used in the present study are listed with their sources in parentheses: mouse monoclonal antibody (mAb) to glyceraldehyde-phosphate dehydrogenase (GAPDH), rabbit polyclonal antibody to Angptl3, integrin alpha 3, total integrin beta 1, phospho-integrin beta 1 (phospho T789) and ILK; anti-active + pro- caspase 3 antibody (Abcam, Cambridge, UK); p53 mouse mAb (Cell Signaling Technology, Beverly, USA); recombinant mouse Angptl3 protein (rm-Angptl3) (R&D Systems, Minneapolis, USA); PE Annexin V Apoptosis Detection Kit I (BD Biosciences, San Diego, USA); In Situ Cell Death Detection kit (Roche, Mannheim, Germany); and fluorescein-labelled phalloidin (Sigma Aldrich, St. Louis, USA).
Cell-lines, culture, and treatment
The mouse podocytes used in this study were a conditionally immortalized cell-line originated by Dr. Peter Mundel (Massachusetts General Hospital, Boston, USA). Culture procedures of the cells were performed according to the standards outlined by Professor Mundel [
23]. Briefly, the podocytes were cultured in RPMI 1640 medium containing 10% fetal bovine serum, 100 U/ml penicillin, and 100 ug/ml streptomycin. Podocytes were cultured in a medium containing 10 U/ml mouse interferon-gamma (IFN-γ) at 33°C with 100% relative humidity and a 5% CO2 in air atmosphere to enhance the expression of a thermosensitive T antigen. To induce differentiation, podocytes were grown under non-permissive conditions at 37°C in the absence of IFN-γ for 14 days. At that time, podocytes became large cells with numerous small branches when well differentiated. All cell culture dishes were coated with type I collagen (Sigma- Aldrich). Podocytes were treated with Angptl3 proteins at various doses (50,100,200,250 and 500 ng/ml) for 24 hours, and with Angptl3 proteins (500 ng/ml) for 0, 3, 6, 9, 12, 24, 36 and 48 hours, either alone or after PAN (50 μg/ml, 10 hours) pretreatment. Doses of Angptl3 proteins and times were determined according to our previously reported data [
11,
24]. All experiments were repeated at least three times.
Treatment of podocytes with siRNA
Podocytes cultured in six-well plates were incubated with 100 pmol siRNA for 30 hours using Lipofectamine® 2000 (lip2000) Transfection Reagent (Invitrogen, Carlsbad, USA) for transient transfection according to the manufacturer’s protocol of lip2000. Podocytes were 30–50% confluent at the time of transfection. Angptl3-specfic siRNA (Angptl3 siRNA) that was used to silence Angptl3 as well as the control siRNA was designed and produced by Invitrogen. The negative control carboxy-fluorescein - labeled siRNA was used in pilot experiments to determine the optimal transfection rates. The sequences of siRNAs are shown in Table
1.
Table 1
Sequences for all the siRNAs
siRNAs | Control siRNA | sense | UUC UCC GAA CGU GUC AVG UTT |
| | antisense | ACG UGA CAC GUU CGG AGA ATT |
| Angptl3 siRNA | sense | GGG UCA UGG ACU UAA AGA UTT |
| | antisense | AUC UUU AAG UCC AUG ACC CTT |
Western blot analysis
Western blotting was performed according to the standard procedures. An equal amount of each protein lysate was loaded onto 8% or 10% sodium dodecyl sulfate-polyacrylamide gel electrophoresis gels and blotted onto polyvinylidene fluoride membranes. Samples were blocked in Tris-buffered saline Tween 20 (20 mM Tris-HCl, pH 7.4 and 0.05% Tween 20) with 5% non-fat dry milk. The membranes were incubated with primary antibodies at appropriate dilutions overnight at 4°C and horseradish peroxidase-linked secondary antibody (at a dilution of 1:2000) (Santa Cruz, USA) for 1 hour at room temperature. The results were visualized by fluorography using the Tanon gel imaging system (Tanon, Shanghai, China).
Enzyme linked-immunosorbent assay
After treatment, cell culture supernatant was collected and centrifuged at 1000 g for 20 min to remove particulates and assayed for Angptl3 protein secreted by podocytes by the ANGPTL3 (mouse) enzyme-linked immunosorbent assay (ELISA) Kit (AdipoGen, Liestal, Switzerland) according to the manufacturer’s protocol.
F-action immunoflurorescence staining
Cells were washed twice with PBS and fixed in 4% paraformaldehyde in PBS for 20 min at room temperature. After the cells were washed three times with PBS, the non-specific binding sites were blocked for 45 min with 3% bovine serum albumin at room temperature before being incubated with fluorescein-labeled phalloidin overnight at 4°C. Nuclei were stained with 4′6′-diamidino-2-phenylindole dihydrochloride (DAPI) for 20 min at room temperature. Images were obtained using an LSM 710 laser scanning confocal microscope (Carl Zeiss, Thornwood, USA). The percentage of stress fibers and mean fluorescence intensity (MFI) of F-actin under confocal microscopy were analyzed as per our previous study by Liu et al. [
25]; lamellopodia was quantified as per our previous study by Lin et al. [
11]; at least 100 randomly chosen cells were analyzed.
Detachment assay
The detachment of podocytes was assayed according to our previous study [
9]. All cells were cultured on six-well plates under nonpermissive conditions for 14 days prior to the experiments, fields of cells were marked, and cell numbers per field were counted to establish a baseline number. The mean numbers of different fields in three independent sets in this experiment were determined.
Detection of apoptosis
Both PE-Annexin-V detection of apoptosis and deoxynucleotidyl transferase-mediated dUTP nick-end labeling (TUNEL) assay were used to detect apoptosis. Methods were performed using PE-Annexin-V Apoptosis Detection Kit (BD Biosciences) and In Situ Cell Death Detection kit (Roche) following the manufacturer’s protocol. Overall, 6000 cells per experiment were resuspended with PE-Annexin-V and 7-aminoactinomycin D and analyzed using flow cytometry. TUNEL staining was examined under fluorescence microscope (Olympus, Japan), for each group in given experiments, at least 300 randomly chosen cells were determined for the quantification.
Statistical analysis
All experiments were repeated at least three times. Data were expressed as mean ± standard deviation. Cell detachment assay was performed by Student’s t-test or one-way analysis of variance followed by the Student Newman-Keuls post hoc test, with P-values <0.05 considered statistically significant.
Discussion
Progressive glomerulosclerosis accounts for the vast majority of chronic kidney disease leading to end-stage renal disease [
26]. Ongoing podocyte loss contributes to the progression of glomerulosclerosis and proteinuria, as podocytes cannot be replaced easily [
2,
27]. PAN model is one of the best described models of podocyte injury, which could induce cytoskeletal disaggregation, detachment and apoptosis in podocytes [
16,
28,
29].
First, the present study indicated that Angptl3 played a vital role in the PAN-induced podocyte loss, both detachment and apoptosis occurred, and F-actin rearrangement was involved in the process of Angptl3-influenced podocyte loss.
It was found that rm-Angptl3 could not induce the detachment of podocytes under normal conditions. Interestingly, in the PAN-induced podocyte injury model, rm-Angptl3 aggravated the detachment, and the knockdown of Angptl3 served to rescue detachment. Curiously, this partial finding in the present study – rm-Angptl3 aggravated the PAN-induced podocyte detachment was in contrast to our previous study by Rao et al. – ANGPTL3 gene transfection ameliorates the PAN-induced podocyte detachment [
9]. The experimental methods and conditions in the two studies were different: in the former study, recombinant Angptl3 protein was used to treat podocytes to mimic the conditions of Angptl3 overexpression, most of the Angptl3 protein found in the culture medium was derived from the exogenous recombinant Angptl3 protein, weakly secreted by podocytes; in the latter study, recombinant plasmid pcDNA3.1-ANGPTL3 was transfected into podocytes with lip2000 reagent to promote the overexpression of Angptl3, the Angptl3 protein presented in culture medium was all secreted by podocytes. Angptl3 is a secreted glycoprotein, Ge et al. performed that Angptl3 can form higher-order structures [
30], and Ryuta, et al. suggested deglycosylation reduces the apparent molecular mass of the secreted recombinant Angptl3 (70kD) to 53 kD [
31]. We detected the podocyte Angptl3 proteins and the exogenous recombinant Angptl3 proteins by western blotting with anti- Angptl3 polyclonal antibody, both protein bands of approximately 70kD and 53kD appeared in the podocytes Angptl3 proteins, while, only protein band of 70kD (no 53kD protein band) appeared in the recombinant Angptl3 proteins (data not shown). We therefore suggest that the podocyte-specific Angptl3 and the exogenous recombinant Angptl3 might have different protein modifications and/or structures. Clement et al. found podocyte-specific Angptl4 and circulating Angptl4 might play different roles in proteinuria [
32,
33]. Angptl3 is a homolog of Angptl4 [
30]. Hence it was speculated that the different experimental methods and conditions might partially influence the contrasting results; moreover, much of the contrasting results is likely due to the differential roles the podocyte-specific Angptl3 and the exogenous Angptl3 proteins played in podocyte detachment, and the differential roles might result from the different protein modifications and/or structures. The contradictory results indicate that exogenous recombinant Angptl3 proteins may be a damaging factor in PAN-induced podocyte detachment, while, podocyte-specific Angptl3 may provide a protective role to some extent under abnormal states. However, direct evidence is lacking, further studies are needed to confirm the present results.
Apoptosis is one of the key factors in determining the number of podocytes in the glomeruli [
3]. And it was found in this study that rm-Angptl3 combined with PAN could induce podocyte apoptosis, while the knockdown of Angptl3 ameliorated apoptosis of podocytes with PAN pretreatment. So we concluded that Angptl3 affected apoptosis almost simultaneously with detachment in PAN-induced podocyte injury model, both detachment and apoptosis occurred in Angptl3-influenced podocyte loss.
Using confocal microscopy to assess the rearrangement of F-actin in podocyte under the same experimental conditions in our present study, it was confirmed that Angptl3 induces the rearrangement of actin filament in podocytes, which is consistent with our previous observation [
13]. Moreover, knockdown of Angptl3 by siRNA failed to change F-actin filament, which may indicate that Angptl3 is not a necessary conditional molecule in maintaining the intricate shape and structure of podocytes. Rm-Angptl3 combined with PAN pretreatment disrupted F-actin filament, knockdown of Angptl3 attenuated the rearrangement of F-actin induced by PAN. It was confirmed that F-actin rearrangement was involved in the process of Angptl3-influenced podocyte loss. The results of the present study indicated that decrease or disruption of podocytes stress fibers may aggravate the loss of podocytes.
Second, the present study pointed to the possible molecular mechanism of the observed effects of Angptl3. Both integrin α3β1 and ILK are key molecules in podocyte detachment, ILK is in its inactive state under normal resting conditions, PAN-induced podocyte damage could activate ILK, and active ILK can phosphorylate the cytoplasmic domain of β1-integrin, which results in a low-affinity binding state and podocytes are detached from the GBM[
15-
18]. It is likely that the combined action of both integrin α3β1 and ILK accounts for the effects of Angptl3 on PAN-induced podocyte detachment, which were partially correlated with Angptl3 could affect the influence of PAN on altering the expression of integrin α3, total integrinβ1, phosphorylation of integrin β1 and ILK. Angptl3 may affect the PAN-induced detachment via ILK/integrin α3β1 pathway, detection of the activity of ILK and observation of the results after inhibiting ILK, which would provide much more information.
Changes in activated caspase 3 and increased levels of p53 are often observed in podocyte apoptosis [
21]. In the present study, it was found that the increased p53 was positively correlated with the increased apoptosis, while activated caspase 3 was rarely observed. Mohr, et al. found that not all apoptosis requires caspase-3 activation [
34], so we speculated that the alterations of p53 protein levels rather than activation of caspase3 contributed to the influence of ANGPTL3 on apoptosis in the present study. Taken together, the effects of Angptl3 may be more complex than currently understood, and the exact mechanism needs to be further studied.
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Competing interests
The authors declare that they have no competing interests.
Authors’ contributions
HX and X-lZ conceptualized the study. R-fD performed the experiment. HX and H-mL obtained funding. R-fD and YL acquired the data. R-fD, YL and JR analyzed the data. HX, X-lZ, R-fD, YL, JR, H-mL, X-yF and Y-hZ contributed to data interpretation and manuscript preparation. All authors read and approved the final manuscript.