Candida Administration Worsens Neutrophil Extracellular Traps in Renal Ischemia Reperfusion Injury Mice: An Impact of Gut Fungi on Acute Kidney Injury

Abstract

Because of gut-barrier defect (gut-leakage) after acute kidney injury (AKI) and higher abundance of Candida albicans in human intestines compared with mouse guts, Candida administration in renal ischemia reperfusion injury (I/R) mice possibly more closely resemble patients with AKI than non-Candida model. Fungi in feces were detectable only in mice with Candida administration. Candida renal-I/R mice, when compared with non-Candida I/R, demonstrated more profound injuries, including (i) gut-leakage; FITC-dextran assay and serum (1→3)-β-D-glucan (BG), (ii) systemic inflammation (serum cytokines), and (iii) neutrophil extracellular traps (NETs); gene expression of peptidyl arginase 4 (PAD4) and IL-1β, nuclear morphology staining by 4′,6-diamidino-2-phenylindole (DAPI) and co-staining of myeloperoxidase (MPO) with neutrophil elastase (NE) in peripheral blood neutrophils. Although renal excretory function (serum creatinine) and renal histology score were nondifferent between renal-I/R mice with and without Candida, prominent renal NETs (PAD4 and IL-1β expression with MPO and NE co-staining) was demonstrated in Candida renal-I/R mice. Additionally, neutrophil activation by lipopolysaccharide (LPS) plus BG (LPS + BG), when compared with LPS alone, caused (i) NETs formation; dsDNA, DAPI-stained nuclear morphology and MPO with NE co-staining, (ii) inflammatory responses; Spleen tyrosine kinase (Syk) and NFκB expression, and (iii) reduced cell energy status (maximal respiratory capacity using extracellular flux analysis). Also, LPS + BG-activated NETs formation was inhibited by a dectin-1 inhibitor, supporting an impact of BG signaling. In conclusion, Candida-renal I/R demonstrated more prominent serum BG and LPS from gut translocation that increased systemic inflammation and NETs through TLR-4 and dectin-1 activation. The influence of gut fungi in AKI should be concerned.

© 2022 The Author(s). Published by S. Karger AG, Basel

Introduction

The cross talk between gastrointestinal (GI) tract and other systems, partly through gut microbiota and immune responses [1], referred to as gut-renal axis [2] is well-known. One of the intestinal influences against other organs is through the translocation of pathogen-associated molecular patterns (PAMPs) from Gram-negative bacteria and fungi, the most and second-highest abundant organisms in feces, respectively [2]. Although gram-negative bacteria are an important source of lipopolysaccharide (LPS), an endogenous toxin, in gut of both human and mice, the abundance of fungi, particularly Candida albicans which are the source of (1→3)-β-D-glucan (BG) in gut, of mouse GI tract, is less than in human [3, 4]. As such, fungi in mouse feces could not be detectable by culture different from human stool [3, 4]. Due to the difference, several mouse models, especially the models with possible GI cross talk, might not appropriately represent the human conditions and Candida administration in mice might make the models resemble more that of human conditions [5-7]. In parallel, acute kidney injury (AKI), a common health care problem worldwide, is mainly caused by ischemia and renal ischemia reperfusion injury (I/R) model is a common representative model of AKI [8, 9]. Because of the well-established gut-renal axis [2], uremia in regular mice might be different from uremia in mice with the presence of Candida in gut. Accordingly, Candida administration worsens uremia-induced gut permeability defect in bilateral nephrectomy mice [10], partly through an impact of BG on macrophages [7]. However, macrophages are not only the immune cells responsible for uremia-induced inflammation and uremia from bilateral nephrectomy, without an influence of the injured kidney, might be different from the patients with AKI.

As such, renal ischemia induces neutrophil accumulation, as a response to the injury [11-13], and renal cell apoptosis (and necrosis) causes the distance impact on several organs [14, 15]. Interestingly, neutrophil extracellular traps (NETs) the networks of extracellular DNA fibers, of accumulated neutrophils in kidney is one of the important innate immune responses against renal-I/R injury [16]. The program cell death (apoptosis and necrosis) in renal parenchymal cells also induces NETs in other nonrenal organs [16]. Additionally, NETosis (cell death after NETs formation) is inducible by either infection or noninfectious conditions [17] through peptidylarginine deiminase 4 (PAD4) activation [18]. The NETosis pathways, both by NADPH oxidase 2 (NOX2)-dependent and NOX2-independent pathways, enhance exposure of nuclear contents [19], including dsDNA (free dsDNA), that is recognized as DAMPs by innate immune cells and increase pro-inflammatory status [20]. Not only apoptosis and necrosis of renal cells, but also cell death of the accumulated neutrophils also further enhance severity of renal I/R [16]. In AKI, NETosis is not only caused by DAMPs from renal cells [17] but also inducible by several PAMPs (LPS and BG) from uremia-induced gut permeability defect [21]. However, gut translocation of BG might be more prominent in humans than mice because of the prominent presence of Candida in human gut [3, 4]. Interestingly, both LPS and BG activate NETosis through TLR-4 and dectin-1, respectively [21], with a possible additive effect by the co-stimulation of LPS and BG through TLR-4 and dectin-1 cross-link [22, 23] with some important downstream signals, including spleen tyrosine kinase (Syk) and nuclear factor kappa-B (NFκB) [24, 25]. Because of (i) the presence of LPS and BG in serum from uremia-induced gut permeability defect [10], (ii) NETs induction by both LPS and BG [21], and (iii) less fungal abundance in mouse guts than human intestines [3, 4], NETs formation was explored in renal I/R mice with Candida administration and the stimulations by LPS and BG in peripheral blood neutrophils from healthy volunteers.

Materials and Methods Renal I/R Model

The animal study protocol, following the National Institutes of Health (NIH, Bethesda, MD, USA), was approved by the Faculty of Medicine, Chulalongkorn University, Bangkok, Thailand, and 8-week-old male mice were purchased from Nomura Siam International (Pathumwan, Bangkok, Thailand). To explore impact of gut fungi in acute uremia, Candida albicans from the American Type Culture Collection (ATCC; 90028) (Fisher Scientific, Waltham, MA, USA) were administered. As such, C. albicans was cultured overnight on Sabouraud dextrose broth (Oxoid, Hampshire, UK) at 35°C for 48 h before enumeration using a hemocytometer, and C. albicans at 1 × 106 CFU in a 0.5 mL phosphate buffer solution (PBS) or PBS alone was orally administered daily for 3 days before surgery. Then, renal I/R was performed at 6 h after the last dose of fungi by abdominal incision according to a previous publication [9]. In brief, bilateral renal arteries were clamped for 35 min through abdominal incision under ketamine anesthesia on a 37°C heated operation table. In sham surgery, both renal arteries were only identified before closing the abdominal wall. Tramadol, 20 mg/kg diluted in 0.5 mL normal saline (NSS) was administered subcutaneously after surgery and at 6 h post-I/R. Mice were sacrificed at 24 h after I/R under isoflurane anesthesia for sample collection. Serum was kept at −80°C until analysis and organs were processed in 10% formalin or Tissue-Tek O.C.T. Compound (Sakura Finetek, Torrance, CA, USA) or snap frozen and separately stored at −80°C.

Mouse Serum and Fecal Sample Analysis

To explore fungi in feces, mouse feces were collected using metabolic cages (Hatteras Instruments, Cary, NC, USA). Then, fecal samples were suspended with PBS at a ratio of 100 mg feces per 1 mL PBS, serially diluted onto SDA (Oxoid), and incubated at 35°C for 72 h before colony enumeration of fungi. Renal injury was determined by blood urea nitrogen and serum creatinine (Scr) using QuantiChrom Urea-assay (DIUR-500) and Creatinine-Assay (DICT-500) (BioAssay, Hayward, CA, USA), respectively. Proteinuria was calculated by spot urine protein creatinine index with the equation; urine protein creatinine index = urine protein (mg)/urine creatinine (mg/dL). Urine protein and creatinine were measured by Bradford Bio-Rad Protein Assay (Bio-Rad, Hercules, CA, USA) and QuantiChrom Creatinine-Assay (DICT-500) (BioAssay), respectively. Serum pro-inflammatory cytokines (TNF-α, IL-6, IL-10, and IL-1β) and liver enzyme (alanine transaminase) were measured by enzyme-linked immunosorbent assay (Invitrogen, Waltham, MA, USA) and EnzyChrom alanine transaminase assay (EALT-100; BioAssay), respectively. For detection of NETs in peripheral blood neutrophils [21], mouse neutrophils were isolated using Polymorph-prep (Alere Technologies AS, Oslo, Norway), according to the manufacturer’s instructions and neutrophils were resuspended in RPMI 1640 media. Only the samples with >95% neutrophils purity by Wright’s stains were further used. Then, NETs formation was determined by (i) serum dsDNA using Quant-iTTM PicoGreen dsDNA Assay Kit (Thermo Scientific, Waltham, MA, USA), (ii) nuclear morphology of neutrophils (branching of the nuclei) using a blue-fluorescent DNA stain 4′,6-diamidino-2-phenylindole (DAPI ) (Sigma-Aldrich, St. Louis, MO, USA) and (iii) the co-staining of myeloperoxidase (MPO) and neutrophil elastase (NE) (Abcam, Cambridge, MA, USA) according to the previous publication [21]. The fluorescent intensities were analyzed with ZEISS LSM 800 (Carl Zeiss, Jena, Germany).

Gut Integrity Determination

Gut permeability defect (gut leakage) was determined by the detection of nonabsorbable carbohydrate (fluorescein isothiocyanate-dextran; FITC-dextran) in serum after an oral administration and the spontaneous serum elevation of gut microbial molecules, including LPS (endotoxin) and BG, as previously published [10]. Accordingly, FITC-dextran (molecular weight 4.4 kDa; Sigma-Aldrich) at 25 mg/mL in 0.25 mL PBS was orally administered at 3 h before detecting FITC-dextran in serum by fluorospectrometry (Thermo Scientific, Wilmington, DE, USA). In parallel, serum LPS and BG were measured using HEK-blue LPS detection assay (InvivoGen, San Diego, CA, USA) and Fungitell (Associates of Cape Cod, Falmouth, MA, USA). The values of LPS <0.01 EU/mL and BG <7.8 pg/mL were recorded as 0 due to the limitation of the standard curves.

Polymerase Chain Reaction

PAD4 and interleukin-1 beta (IL-1β), the NETs formation associated genes, were determined from mouse samples using real-time polymerase chain reaction by a standard protocol [21] with the following primers (for mouse genes); PAD4 forward 5′-ACAGGTGAAAGCAGCCAGC-3′, reverse 5′-AGTGATGTAGATCAG­GGCTTGG-3′; IL-1β forward 5′-GAAATGCCACCTTTTGACAGTG-3′, reverse 5′-TGGATGCTCTCATCAGGACAG-3′; Beta-actin (β-actin, an endogenous housekeeping gene) forward 5′-CGGTTCCGATGCCCTGAGGCTCTT-3′, reverse 5′-CGTCACACTTCATGATGGAATTGA-3′. Also, other primers were used for detection of human genes as follows: Syk forward 5′-TGGGAAGCATTCTCCTATGG-3′, reverse 5′-CCACATCGTATGTCCAGCAC-3′; nuclear factor kappa B (NFκB) forward 5′-GCGAGAGGAGCACAGATACC-3′, reverse 5′-CTGATA­GC­CTGCTCCAGGTC-3; and β-actin forward 5′-GGACTTCGAGCAAGAGATGG-3′, reverse 5′-AGCACTGTGTTGGCGTACAG-3′. The samples were prepared by an RNA-easy mini kit (Qiagen, Hilden, Germany), nanodrop 100 spectrophotometer, high-capacity cDNA reverse transcription, and SYBR Green PCR Master Mix for quantitative real-time polymerase chain reaction with QuantStudio6 Flex Real-time PCR System (Thermo Scientific). The results were demonstrated in relative quantitation of the comparative threshold method (2−ΔΔCt) as normalized by β-actin.

Histological Analysis and Immunofluorescent Imaging

The semi-quantitative evaluation of renal histology on paraffin-embedded slides was performed after 10% neutral buffered formalin fixation, followed by hematoxylin and eosin and periodic acid-schiff staining at ×200 magnification in 10 randomly selected fields for each animal [26-28]. Renal injury was defined as tubular epithelial swelling, loss of brush border, vacuolar degeneration, necrotic tubules, cast formation, and desquamation using the following scoring method: 0, area of damage <5%; 1, area of damage 5–10%; 2, area of damage 10–25%; 3, area of damage 25–50%; and 4, area of damage >50%. In parallel, immunofluorescent histological analysis and in peripheral blood neutrophils were performed following previous publications [29-31]. In brief, the internal organs were prepared in Tissue-Tek O.C.T. Compound (Sakura Finetek) and stained for NETs using the co-staining of MPO and NE (Abcam) with DAPI color (Sigma-Aldrich). The fluorescent intensities were analyzed with ZEISS LSM 800 (Carl Zeiss).

The in vitro Experiments on Neutrophils and Dectin-1 Inhibitor

An impact of BG, a main cell wall component of fungi on NETosis was tested in human neutrophils. As such, heparinized blood was collected from healthy donors under an approved protocol by the Ethical Institutional Review Board, Faculty of Medicine, Chulalongkorn University, according to the Declaration of Helsinki, with written informed consent. Neutrophils were isolated by density centrifugation with PolymorphprepTM (Axis-Shield, Oslo, Norway) and were resuspended in RPMI 1640 supplemented with 10% fetal bovine serum. Human neutrophils (at 1 × 104 cells) were placed onto Poly-L-Lysine (Sigma-Aldrich) coated glass coverslips, incubated at 37°C, 5% CO2 for 1 h with BG using whole glucan particle (WGP) (the purified BG from Saccharomyces cerevisiae) (Biothera, Eagan, MN, USA), at 10 μg/mL with or without LPS (Escherichia coli 026: B6) (Sigma-Aldrich) at 10 μg/mL [10, 21, 29, 32-36]. After 2 h of incubation, the coverslips were fixed with 4% formaldehyde, blocked with tris buffered saline in 2% bovine serum albumin (Sigma-Aldrich) and permeabilized by tris buffered saline with 0.05% Tween 20 (Sigma-Aldrich). Then, NETs formation was detected by nuclear morphology DAPI staining, the co-staining of MPO and NE fluorescent colors as previously described and free dsDNA in supernatant. For the detection of free dsDNA, stimulated neutrophils were incubated with 0.1 M CaCl2 and 0.5 unit (U) of micrococcal nuclease (Sigma-Aldrich) at 37°C, 5% CO2 for 10 min before stopping the nuclease reaction by 0.5 M ethylenediaminetetraacetic acid. Then, the supernatant was collected and Quant-iTTM PicoGreen reagent (Thermo Fisher Scientific) was added to measure dsDNA by incubating aqueous working solution in the sample for 5 min at room temperature (protected from light). The amount of dsDNA in the mixture was measured at 480 nm excitation (520 nm emission) on a fluorescent microplate reader. Furthermore, dectin-1 inhibitor (soluble glucan, a competitive dectin-1 binding agent) (InvivoGen) was used to explore the mechanistic pathway of LPS with BG in FcgRIIb−/− neutrophils. Then, LPS (LPS Escherichia coli 026: B6) (Sigma-Aldrich) at 10 μg/mL plus BG (WGP) (Biothera) at 10 μg/mL was incubated with human neutrophils (at 1 × 104 cells) for 2 h together with dectin-1 inhibitor at 25 mg/mL or PBS (as a control) before determination of NETs using supernatant dsDNA, PAD4 expression, and NETs formation by MPO plus NE co-staining as previously mentioned.

Extracellular Flux Analysis

Because the enhanced cell energy might be responsible for the increased cell activity, the stimulated human neutrophils by LPS with or without BG and control media were analyzed by Seahorse XF Analyzers (Agilent, Santa Clara, CA, USA) as previously published [28, 37]. The energy metabolism profiles are estimated by glycolysis and mitochondrial oxidative phosphorylation based on extracellular acidification rate and oxygen consumption rate, respectively, on neutrophils. Due to the short life span of neutrophils, LPS (Escherichia coli 026: B6) (Sigma-Aldrich) at 100 μg/mL with or without BG (WGP) (Biothera) at 100 μg/mL were added in neutrophils (1 × 104 cells per well) right before incubation with the standard reagents of Seahorse XF analysis. For mitochondrial stress test, assays were performed in Seahorse XF DMEM medium (Agilent Technologies) supplemented with 2 mM Seahorse XF L-glutamine, 1 mM pyruvate, and 10 mM XF glucose. Then, cells were sequentially incubated by oligomycin, carbonyl cyanide 4-(trifluoromethoxy) phenylhydrazone, and rotenone/antimycin A (final concentration of 1.5 μM, 1 μM, and 0.5 μM, respectively). In parallel, glycolysis stress tests were calculated from the mitochondrial stress test using the wave program of Seahorse XF Analyzers (Agilent). Notably, the results in Seahorse analysis were normalized by applying the total protein abundance in the wave program to measure all parameters.

Statistical Analysis

Statistical differences among groups were examined using the unpaired Student’s t test or one-way analysis of variance with Tukey’s comparison test for the analysis of experiments with two groups or more than two groups, respectively. The data are presented as the mean ± SE. SPSS 11.5 software (SPSS, Chicago, IL, USA) was used for all statistical analyses.

Results

Candida administration enhanced gut leakage, gut translocation of BG and systemic inflammation in renal I/R, partly through the reduced cell energy status that facilitated NETs.

Candida Administration Enhanced Systemic Inflammation and Neutrophil Extracellular Traps in Renal I/R Mice

Culture for fecal fungi was negative in all group without Candida administration and the abundance of fungi in feces was similar between sham and renal I/R with fecal gavage (Fig. 1a). Because the peak of injury in renal I/R injury was at 24 h of the model as previously published [8], several parameters were determined at 24 h post-I/R. Accordingly, renal function (blood urea nitrogen and Scr), renal histology, and liver enzyme were not different between renal I/R with or without fungal gavage but proteinuria and gut permeability defect (FITC-dextran assay and serum BG but not endotoxemia) were more prominent in renal I/R with Candida compared with I/R injury alone (Fig. 1b–j). Notably, proteinuria at 24 h after I/R demonstrates an initial consequence of renal ischemia-induced podocyte damage, despite normal renal excretory function (blood urea nitrogen and Scr) [38, 39]. Despite the increase in serum BG, renal I/R with Candida had similar serum LPS compared to I/R alone (Fig. 1i, j). To demonstrate an impact of neutrophil accumulation in kidneys at 24 h post renal-I/R using the hematoxylin and eosin-stained renal sections, neutrophils in sediments (online suppl. Fig. 1, left; for all online suppl. material, see www.karger.com/doi/10.1159/000521633), tubulointerstitial area and glomeruli (online suppl. Fig. 1 right) of I/R with PBS (which were not different from Candida-administered I/R) were demonstrated. However, gut translocation of LPS and BG in renal I/R mice with or without Candida were severe enough to enhance systemic inflammation (serum cytokines; TNF-α, IL-6, IL-10, and IL-1β) (Fig. 2a–c) and NETosis (cell death from NETs formation); serum dsDNA, PAD4 expression and neutrophils staining (nuclear morphology by DAPI, co-staining of MPO with NE) (Fig. 2a–i). Nevertheless, the systemic inflammation and NETs formation in blood neutrophils were more prominent in Candida-administered I/R mice (Fig. 2a–i). Likewise, NETs formation in kidneys, as determined by expression of PAD4 and IL-1β with immunofluorescent of MPO and NE co-staining, were detectable in both renal I/R mice with and without Candida but more prominent in Candida I/R group (Fig. 3a–e). Notably, NETs formation could not be demonstrated in several internal organs (liver, kidney, and lung) at 6 h post-I/R (online suppl. Fig. 2) nor in the liver at 24 h post-I/R (online suppl. Fig. 3).

Fig. 1.

Characteristics of renal I/R with Candida administration (I/R fungi) or I/R PBS or sham with Candida administration (Sham fungi) at 24 h after surgery as determined by abundance of fecal fungi (a), renal injury; BUN and Scr (b, c), the representative pictures in H&E and PAS (original magnification, ×200) with the histological score (d, e), proteinuria (protein creatinine index; UPCI) (f), liver injury (serum ALT) (g), and gut leakage, serum FITC-dextran assay, endotoxemia, and serum BG (h–j), are demonstrated (n = 6–7/time-point). Notably, the sham group without Candida administration is not demonstrated due to the similarity to sham with Candida (normal values in all parameters). BUN, blood urea nitrogen; H&E, hematoxylin and eosin.

/WebMaterial/ShowPic/1401282 Fig. 2.

Characteristics of renal I/R with Candida administration (I/R fungi) or I/R PBS or sham with Candida administration (Sham fungi) at 24 h after surgery as determined by systemic inflammatory responses as indicated by serum cytokines (TNF-α, IL-6, IL-10, and IL-1β) (a–d) and NETs formation as evaluated by serum dsDNA (e) and in peripheral blood neutrophils using gene expression of PAD4 (f), cell morphology in DAPI staining (blue color) (g), co-staining of MPO and NE (h), with the representative pictures of DAPI staining (original magnification, ×200) (i, upper part) and immunofluorescence of MPO/NE (original magnification, ×630) (i, lower part) are demonstrated (n = 6–7/group). Notably, the sham group without Candida administration is not demonstrated due to the similarity to sham with Candida (normal values in all parameters).

/WebMaterial/ShowPic/1401280 Fig. 3.

Characteristics of renal I/R with Candida administration (I/R fungi) or (I/R PBS) or sham with Candida administration (Sham fungi) at 24 h after surgery as indicated by NETs in renal tissue as determined by expression of IL-1β and PAD4 (a, b) and the co-staining of MPO and NE at 24 h post-I/R with the representative immunofluorescent pictures of MPO (red), NE (green), and DAPI ( blue nuclear staining) (original magnification, ×630) (c–e) are demonstrated (n = 6–7/group). Notably, the sham group without Candida administration is not demonstrated due to the similarity to sham with Candida (normal values in all parameters).

/WebMaterial/ShowPic/1401278 The Additive Effect of BG on LPS-Induced NETs Possibly through Spleen Tyrosine Kinase Signaling and Cell Energy Alteration

Although DAMPs from necrotic renal cells could induce NETosis [40], PAMPs (both LPS and BG from uremia-induced gut translocation) could also induce NETs formation and the presence of both LPS and BG might have an additive effect on NETs. Indeed, LPS or BG, alone or in combination, facilitated NETs formation of human neutrophils but NETosis from LPS + BG was more prominent than the activation by either LPS or BG alone as indicated by dsDNA, DAPI, and MPO-NE co-staining (Fig. 4a–d). Notably, NETs formation after LPS induction was higher than BG activation as demonstrated by DAPI and MPO-NE co-staining, but not dsDNA (Fig. 4a–d). Because (i), respectively, and Syk and NFκB are common downstream mediators of TLR4 and dectin-1, the receptors of LPS and BG, respectively [24, 41], and (ii) LPS and BG induce energy alteration in several cells [25, 34, 42] that might be associated with NETosis [43], these factors are evaluated. Indeed, LPS + BG up-regulated Syk and NFκB expression when compared with the activation by LPS or BG alone (nondifference between the stimulation by LPS vs. BG) (Fig. 5a, b). Despite a limited number of mitochondria in neutrophils [43], LPS + BG reduced mitochondrial function (oxygen consumption rate) as indicated by a reduction of maximal respiration in extracellular flux analysis (Fig. 5c–e). Meanwhile, there was no effect of LPS and/or BG on glycolysis activity of neutrophils (Fig. 5c–e).

Fig. 4.

Characteristics human neutrophils after activation by LPS with or without (1→3)-β-D-glucan (BG) or control PBS at 2 h of the stimulation as evaluated by supernatant dsDNA (a), nuclear morphology after DAPI (blue nuclear staining) (b) and the co-staining of MPO and NE (c) with the representative immunofluorescent pictures of DAPI staining (d) and the staining of MPO and NE (e) are demonstrated (independent triplicated experiments were performed).

/WebMaterial/ShowPic/1401276 Fig. 5.

Characteristics human neutrophils after activation by LPS with or without BG or control PBS at 2 h of the stimulation as evaluated by gene expression of Syk and NFκB (a, b) and the extracellular flux analysis as indicated by OCR (mitochondrial function), ECAR (glycolysis activity) and maximal respiration (from OCR curve) (c–e) are demonstrated (independent triplicated experiments were performed).

/WebMaterial/ShowPic/1401274

Additionally, the importance of dectin-1 for the additive effect of BG on LPS activation was demonstrated through the inhibitory activity of dectin-1 inhibitor on NETs formation as indicated by the reduction of dsDNA, PAD4 expression, and NETs formation using DAPI and co-staining of MPO and NE (Fig. 6a–e). Hence, the enhanced severity of systemic inflammation in Candida-administered renal I/R mice over non-Candida mice (Fig. 1-3) might be due to uremia-induced gut translocation of LPS and BG (Fig. 1h–j) with an additive effect of LPS plus BG on TLR4 and dectin-1 through Syk and NFκB signaling as demonstrated in a picture of working hypothesis (Fig. 7). The previously known crosstalk between TLR4 and dectin-1 [22, 44, 45] might be responsible for the additive effect of BG on LPS-induced NETosis. The different abundance of gut fungi between humans and mice in several mouse models should be concerned. More studies on the influence of gut fungi in AKI are interesting.

Fig. 6.

Characteristics human neutrophils after activation by control PBS or LPS + BG with or without dectin-1 inhibitor at 2 h of the stimulation as evaluated by supernatant dsDNA (a), PAD4 expression (b), nuclear morphology after DAPI (blue nuclear staining) (c) and the co-staining of MPO and NE (d) with the representative immunofluorescent pictures of DAPI staining (e) and the co-staining of MPO and NE (f) are demonstrated (independent triplicated experiments were performed).

/WebMaterial/ShowPic/1401272 Fig. 7.

A picture of the working hypothesis demonstrates NETs formation, nuclear membrane disruption, chromatin release and the activation of MPO and NE, from the possible cross talk between dectin-1 and TLR-4 through the common downstream signaling; Syk and NFκB, with PAD4 activation are demonstrated. While dectin-1 is activated by (1→3)-BG of fungal cell wall, TLR-4 could be stimulated by LPS from Gram-negative bacterial cell wall, DAMPs or free histone DNA (from NETosis of other neutrophils).

/WebMaterial/ShowPic/1401270 Discussion

In comparison with non-Candida, 24 h renal-I/R in Candida-administered mice caused prominent NETs (in peripheral blood neutrophils and in glomeruli) with systemic inflammation through the profound gut translocation of LPS and BG.

Gut Translocation of Pathogen Molecules and NETosis in Candida-Administered Renal I/R Mice

The increased serum BG (beta-glucanemia) in uremic patients which is associated with the severity of uremia (uremia-induced inflammation) [46] and beta-glucanemia-induced inflammation might partly be responsible for systemic inflammation. Because BG is a major molecule of fungal cell wall, beta-glucanemia in patients with uremia might be due to gut translocation of BG from fungi in fecal contents. Here, the impact of gut fungi on renal I/R is examined using Candida gavage mice because (i) there is a lower abundance of fungi in mouse guts than the human intestines [3, 4]; (ii) the presence of Candida in gut enhances BG level in serum [7, 10, 34, 47, 48]; and (iii) serum BG might facilitate NETosis [21]. Accordingly, oral Candida administration was required to raise the quantity of fungi to the level that fungal culture in mouse feces could be detected. On the other hand, the restoration of renal blood flow after an acute ischemic insult inevitably worsens renal injury from inflammatory processes and several program cell deaths [49]. Although apoptosis, necrosis, and necroptosis in renal parenchymal cells following ischemia are well-known [14, 15], the program cell death of many immune cells in the kidneys during the reactions against renal cell death [11-13] is also significant as an early step in the wound healing process [50]. Likewise, TLR-4 activation by DAMPs after renal-I/R causes significant apoptosis in renal cells and accumulated immune cells, especially neutrophils and macrophages [51-54]. Among innate immune cells, neutrophils are the most prominent cells in blood circulation and rapidly transmigrate into the injured organs, especially at the acute phase of the injury [55]. Indeed, neutrophil accumulation in renal interstitial area, glomeruli, and in urine sediments was demonstrated at 24 h post renal-I/R, regardless of Candida administration, that might be responsible for excessive acute inflammation, vascular permeability defect, and further loss of kidney function, referred to as “neutrophil-induced organ damage” [55]. Neutrophils in these extremely stress microenvironments from renal I/R with a high level of DAMPs, are further processed onto NETosis (cell death after NETs formation) through DAMPs-activated TLR-4 [56-58]. Although NETs are one of the important neutrophilic responses against DAMPs (either from infection or noninfection) that could induce beneficial or harmful inflammation [59], too profound NETosis worsen renal injury after I/R as indicated by increased proteinuria in Candida I/R mice when compared with non-Candida I/R mice.

Despite a well-known neutrophil-accumulation after renal I/R injury [60], NETs formation was limited only in glomeruli (causing proteinuria) but not at tubulointerstitial area. Because the renal injury score depends not only on glomerular lesion but also tubulointerstitial damage, there was nondifference renal injury score between renal I/R mice with versus without Candida administration. Likewise, the lack of difference in Scr between Candida versus non-Candida I/R mice might be due to the limitations of Scr as a kidney injury biomarker, which takes time to accumulate in serum [61, 62]. Additionally, NETs could not be found in kidneys and extra-renal organs (liver and lung) at 6 h post-I/R, the time point with the most prominent lung injury [63, 64]. Extra-renal NETs could be detected after the time-point of maximal kidney damage following renal I/R injury since the transfer of DAMPs from the necrotic kidney to other organs for NETs activation could take time [40], and NETosis is only evident in the lung at 24 h after renal I/R [65]. Furthermore, NETs are demonstrated in the lung but not in the liver at 24 h post renal I/R [65] implying the different reaction between hepatocytes and lung parenchymal cells (possibly be associated with hepatocyte detoxification property) [66, 67]. The prominent cell deaths of neutrophils, especially NETosis, facilitate further renal injury and also induce injury in several remote organs, partly through thrombosis induction from free extracellular DNA and inflammation from NETs formation [68, 69]. Likewise, NETosis enhances renal tubular necrosis [16, 70, 71] and pretreatment of renal-I/R with NETs inhibitors improves kidney injury [40]. On the other hand, NETs formation is also inducible by LPS and BG which are major cell wall components of Gram-negative bacteria and fungi, the most and second most abundant organisms in intestine, respectively [2]. Although fecal fungi could not be directly detected by culture, BG could be detected in mouse feces because of (i) some nonprominent fungi, which could be detectable by the more sensitive detection methods (gene expression or fecal microbiome analysis) [72], and (ii) BG from the mouse chow components (callose; plant BG) [73].

Due to the well-known translocation of LPS and BG from the gut into the bloodstream as a result of uremia (or renal I/R)-induced gut permeability defect (gut leakage) [10, 74], both LPS and BG might promote NETs formation from renal-I/R. The serum level of BG was elevated only in Candida-administered renal I/R mice but not in Candida sham mice, suggesting a role for the healthy intestinal barrier to prevent gut translocation of BG. On the other hand, serum BG in Candida-administered renal I/R mice was higher than non-Candida renal-I/R mice, implying an influence of gut fungi in renal I/R mouse model. Furthermore, NETosis, both in peripheral blood neutrophils and in kidneys, of Candida-administered renal-I/R mice was more prominent in non-Candida I/R mice supporting an influence of the increased serum BG from the escalated BG in gut contents due to Candida gavage. Although Candida gavage did not increase endotoxin level in intestines, Candida administration enhanced serum LPS, indicating the role of gut fungi in gut leakage facilitation. The increase in both LPS and BG in serum amplified NETosis and systemic inflammation which are well-known worsening factors of AKI and chronic kidney disease progression [32].

An Additive Effect of BG on LPS-Induced NETs Formation, a Possible Impact of Syk Signaling and the Cell Energy Status

Because of the simultaneous presence of LPS and BG in serum of renal I/R mice and the property of NETs induction through TLR-4 and dectin-1 activation [75, 76], an additive effect of LPS plus BG (LPS + BG) on NETosis is possible. As such, LPS + BG more prominently induced NETs than LPS or BG alone that was possibly mediated through Syk and NFκB, the shared downstream signaling of both TLR-4 and dectin-1 [24, 25], potentially with the TLR-4 and dectin-1 cross link [22, 23]. Here, the activity of neutrophil mitochondria (maximal respiratory capacity) was lower in LPS + BG activated neutrophils than in LPS or BG activated neutrophils; however, the mitochondrial activity of LPS or BG activated neutrophils was not different from the control. Interestingly, only LPS + BG activation, but not each molecule alone, was powerful enough to exhaust the cell’s energy reserve that was used for NETs formation, resulting in a reduced ability to raise maximal respiration. On the other hand, LPS and/or BG did not alter glycolysis capacity of neutrophils. Additionally, the simultaneously activation of TLR-4 and dectin-1 and the cross link between these receptors might be necessary for the enhanced NETs formation as a dectin-1 inhibitor blocked NETs formation after LPS + BG activation.

Hence, the working hypothesis from all experiments is presented in Figure 7 which demonstrates the activation on several important processes of NETosis activation pathways, including TLR-4 stimulation by LPS (from uremia-induced gut translocation), DAMPs (from renal-I/R) and free histone DNA (from NETosis of other neutrophils) [77] together with dectin-1 activation by BG (from gut leakage), with the cross link of both receptors (TLR-4 and dectin-1) [22, 23]. After that, the descending signaling through Syk and NFκB (the shared downstream signals of TLR-4 and dectin-1) activate NOX2 dependent NETs by the activation on PAD4, MPO, and NE as previously published [78-80]. Because (i) Syk is a common downstream of several NETs inducible pathways, including dectin-1 and TLR-4 [78, 81-83], and (ii) Syk inhibitors are clinically available [84-88] with NETosis blocking activity [89]. Syk inhibitor might be a useful drug for the prevention of renal injury in patients. Future studies are of interest.

In conclusion, there was a more prominent NETs in Candida-administered renal I/R mice compared with non-Candida group due to gut permeability defect-induced gut translocation of pathogen molecules that facilitated TLR-4/dectin-1 cross link. The higher NETs in Candida-administered renal I/R mice might be more resemblance to patients with AKI, at least in term of the presence of fungi in feces, that caused more severe renal NETs and systemic inflammation then the non-Candida renal I/R model.

Acknowledgments

A.L. is under Translational Research in Inflammation and Immunology Research Unit (TRIRU), Department of Microbiology, Chulalongkorn University, Bangkok, Thailand.

Statement of Ethics

The animal study protocol, following the National Institutes of Health (NIH), was approved by the Faculty of Medicine, Chulalongkorn University, Bangkok, Thailand, approval number [SST 022/2563]. Heparinized blood was collected from healthy donors under an approved protocol by the Ethical Institutional Review Board, Faculty of Medicine, Chulalongkorn University, approval number [IRB No. 130/63], according to the Declaration of Helsinki, with written informed consent from the participants.

Conflict of Interest Statement

The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.

Funding Sources

This research is supported by CU_FRB65_hea(33)_040_30_21, and National Research Council of Thailand (Grant No. NRCT5-RGJ63001) and (NRCT-N41A640076) with NSRF via the Program Management Unit for Human Resources & Institutional Development, Research and Innovation.

Author Contributions

The followings are the authors’ contribution: conceptualization, A.L. and S.S.; methodology, A.L., S.S. and W.S.; software, A.L., S.S., W.S., and C.P.D.; validation, S.S., A.L., P.V., and D.C.; formal analysis, S.S., W.S., and A.L.; investigation, S.S., W.S., C.P.D., P.V., D.C., and A.L.; resources, A.L. and D.C.; data curation, A.L. and S.S.; writing – original draft preparation, A.L.; writing – review and editing, S.S., D.C., and A.L.; visualization, S.S. and A.L.; supervision, A.L.; project administration, S.S. and A.L.; funding acquisition, D.C. and A.L. All authors have read and agreed to the published version of the manuscript.

Data Availability Statement

Some datasets presented in this study can be found in online repositories at the article/online supplementary material. Other raw data supporting the conclusions of this article will be made available by the authors, without undue reservation, to any qualified researcher.

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