IL-33 and its decoy sST2 in patients with Alzheimer’s disease and mild cognitive impairment

Ninety elderly Italian individuals were enrolled in the study by the Neurology Department of the IRCCS Ca’ Granda Ospedale Maggiore Policlinico, Italy. Thirty patients had a diagnosis of AD, 30 patients had a diagnosis of mild cognitive impairment (MCI), and 30 individuals were age and sex matched healthy controls (HC). The clinical diagnosis of AD was performed according to NINCDS-ADRDA work group criteria [28] and further revisions [37], the clinical diagnosis of MCI fulfilled Petersen’s operational criteria [29]. Neuropsychological evaluation was performed with a Mini-Mental State Examination (MMSE) [38] and Clinical Dementia Rating Scale (CDR) [39].

All patients underwent a clinical interview, neurological and neuropsychological examination, routine blood tests, brain MRI, and lumbar puncture (LP). The mean age of AD patients (13 males and 17 females) was 74.3 years (age range 54–88 years) and that of MCI patients (8 males and 22 females) was 75.3 years (age range 63–84 years). All the AD patients were enrolled in a Multidimensional Stimulation Rehabilitation program designed for this pathology. Finally, the thirty age- and sex-matched elderly subjects (HC) who were included in the study were selected according to the SENIEUR protocol for immuno-gerontological studies of European Community’s Control Action Programme on Aging [40]; their MMSE score was > 28.

The study was approved by the Ethics Committee of Don Gnocchi Foundation and informed written consent was obtained from all the included subjects before study initiation.

Serum was collected in vacutainer tubes containing serum separator (Becton Dickinson and Co., Rutherford, NJ, USA) and were centrifuged at 3,000 rpm for 10 min to separate sera; CSF samples were collected by lumbar puncture. Serum and CSF were used immediately or stored at − 80 °C.

Whole blood of a subset of individuals (5 AD, 5 MCI, and 5 HC) was collected in vacutainer tubes containing ethylenediaminetetraacetic acid (EDTA) (Becton Dickinson). Peripheral blood mononuclear cells (PBMC) were separated on lympholyte separation medium (Cedarlane, Hornby, Ontario, CA, USA) and washed twice in PBS at 1500 rpm for 10 min; viable leukocytes were determined using a TC20 Automated Cell Counter (Biorad, Hercules, CA, USA).

PBMC (1 × 10⁶/ml) were cultured in RPMI 1640 supplemented with 10% human serum, 2 mM l-glutamine, and 1% penicillin (Invitrogen Ltd, Paisley, UK) and incubated at 37 °C in a humidified 5% CO₂ atmosphere for 2 h in a 12-well plate for monocyte adhesion. After 2 h, non-adhering PBMC were harvested and discarded and monocytes grown on plate were either culture in medium alone (unstimulated) or were or primed with 2 μg/ml lipopolysaccharide (LPS) for 2 h (Sigma-Aldrich, St. Louis, MO, USA) before stimulation with 10 μg/ml of 1-42 amyloid-beta peptide (Aβ₄₂) (Sigma-Aldrich) in the absence/presence of 10 ng/ml of Human Recombinant IL-33 (Biolegend, San Diego, CA, USA) for 24 h at 37 °C in a humidified 5% CO₂ atmosphere. After 24 h, supernatants were collected and stored at − 20 °C; adhering cells (monocytes) were collected and prepared for FlowSight analysis.

IL-33 (catalog number D3300B, sensitivity 1.51 pg/mL, assay range 3.1–200 pg/ml, minimum detectable dose (MDD) ranged from 0.069 to 1.51 pg/mL), sST2 (catalog number DST200, sensitivity 13.5 pg/mL, assay range 31.3–2000 pg/mL, MDD ranged from 2.45 to 13.5 pg/mL), IL-1β (catalog number DLB50, sensitivity 1 pg/mL, assay range 3.9–250 pg/ml, MDD less than 1 pg/mL), IL-6 (catalog number D6050, sensitivity 0.70 pg/mL, assay range 3.1–300 pg/ml, MDD less than 0.70 pg/mL), and IL-10 (catalog number D1000B, sensitivity 3.90 pg/mL, assay range 7.8–500 pg/ml, MDD less than 3.90 pg/mL) concentration was analyzed in serum and CSF by commercially-available ELISA according to the manufacturer’s recommendations (Quantikine Immunoassay; R&D Systems, Minneapolis, MN, USA, or Thermo Fisher Scientific, Waltham, MA, USA). Serum and CSF samples were not diluted prior to being utilized. A plate reader (Sunrise, Tecan, Mannedorf, Switzerland) was used and optical densities (OD) were determined at 450/620 nm. All samples were performed in duplicates. The same methods were used to measure IL-1β, IL-6, and IL-10 in unstimulated and in LPS-primed and Aβ₄₂-stimulated PBMC supernatants in the presence/absence of recombinant IL-33 (see above).

A Qubit Protein Assay Kit was used for protein extraction; total protein amount was measured using a Qubit 3.0 Fluorometer (Thermo Fisher Scientific). Equal amounts of protein (15 μg) from each sample, or 2 ng of artificial truncated IL-33 (amino acids 112–270, 20 kDa) (Recombinant Human IL33 carrier-free, Biolegend, San Diego, CA, USA) used as positive control to confirm that the bands correspond to IL-33 full length (amino acids 1–270, 34–30 kDa), to the cleaved inactive forms (amino acids 1–178, 22–20 kDa; amino acids 179–270, 13–12 kDa) [2, 3] or, finally, to the cleaved active forms (amino acids 95–270, amino acids 99–270, and amino acids 109–270; 19–15 kDa) [4], were separated by 10% SDS-PAGE and transferred to PVDF membranes (Genscript). A pre-stained marker, broad range 11–190 KDa (Cell signaling, Danvers, MA, USA), was also used, PVDF membrane were treated by ONE-HOUR Western detection kit (Genscript) and proteins were visualized using a Chromosensor TMB substrate (Genscript). After protein transfer, PVDF membranes were incubated with a pretreatment solution for 5 min RT and then with the WB solution and an α-human IL-33 Ab (Nessy-1) (Abcam, Cambridge, UK) for 40 min. After three washes, membranes were developed with a TMB substrate.

Monocytes that were either unstimulated or LPS-primed and Aβ₄₂-stimulated in the presence/absence of 10 ng/ml of recombinant IL-33 were analyzed to evaluate nuclear translocation of NF-kB; the Amnis® NF-kB Translocation Kit was used according to the manufacturer’s recommendations (Merck KGaA, Darmstadt, Germany). Briefly, cells were fixed, permeabilized, and stained with Anti-Hu NF-κB (p50) Alexa Fluor® 488 for 30 min RT. After incubation, monocytes were washed and fixed and 10 μl of 7AAD were added.

The FlowSight (Amnis Corporation, Seattle, WA, USA) is equipped with two lasers operating at 488 and 642 nm, two camera, and twelve standard detection channels. It simultaneously produces side scatter (darkfield) images, one or two transmitted light (brightfield) images, and up to ten channels of fluorescence imagery of every cell. FlowSight acquires 2000 cells/s and operates with a 1-μm pixel size (× ~ 20 magnification) allowing visualization of fluorescence from the membrane, cytoplasm, or nucleus. The IDEAS image analysis software allows quantification of cellular morphology and fluorescence at different cellular localizations by defining specific cellular regions (masks) and mathematical expressions that uses image pixel data or masks (feature) by different wizards. Analysis of NF-kB translocation was performed by Nuclear Localization Wizard using the Similarity Feature. Briefly, nuclear translocation has occurred if the NF-κB and nuclear fluorescence signals overlap with similar shapes. The Bright Detail Similarity is designed specifically to compare the small bright image detail of two images and can be used to quantify the co-localization of two probes (NF-kB and 7AAD) in a defined region. The similarity score is the log transformed Pearson’s correlation coefficient and it is a measure of the degree to which two images are linearly correlated within a masked region and is calculated on a double-positive region (NF-kB+7AAD+).

Analysis of the different isoforms of IL-33 (full-length; cleaved inactive; cleaved active) was performed by Western blotting in serum and CSF of AD, MCI and HC individuals. Results showed that the full-length IL-33 protein (30–kDa band) was present in all analyzed serum and CSF samples. Notably, in two cases an additional 20-kDa band, corresponding to the cleaved (c), inactive form of IL-33 [3] was observed. These results are shown in Fig. 1.

IL-33 concentration was decreased in serum and CSF of both AD and MCI individuals compared to HC (p value vs. HC: serum, AD p = 0.02; MCI p = 0.04; CSF, AD p = 0.01; MCI p = 0.009). In contrast with these results, serum concentration of the IL-33 decoy receptor sST2 was significantly increased in AD and MCI compared to HC (p value vs. HC: p = 0.02 and p = 0.01, respectively) (Fig. 2). CSF sST2 concentration was below the limit of detection of the assay (33 pg/ml) in all the analyzed samples (data not shown).

IL-1β serum concentration was significantly increased in AD and MCI sera compared to HC (p = 0.01 in both cases), whereas that of IL-10 was significantly reduced in both groups of patients compared to HC (p = 0.04 in both cases). No significant differences were detected when IL-6 serum concentration was compared between the three groups. These results are shown in Fig 3.

In CSF, IL-1β concentration was significantly augmented in AD and MCI compared to HC (p = 0.02 and p = 0.01, respectively). IL-6 concentration was slightly augmented and IL-10 concentration was marginally reduced in AD and MCI compared to what was seen in HC but these differences did not reach statistical significance (Fig. 3).

Monocytes of AD, MCI, and HC individuals (n = 8 in all cases) were LPS-primed and Aβ₄₂-stimulated and IL-1β, IL-6, and IL-10 production was measured by ELISA. Whereas the production of these cytokines was minimal (< 20 pg/ml in all cases) and comparable between the three groups of individuals analyzed when monocytes were unstimulated (medium alone) or when IL-33 was added to the culture medium, LPS-primed, and Aβ₄₂-stimulated monocytes of AD and MCI patients produce significantly augmented quantities of IL-1β (median, AD = 230 ng/ml; MCI = 140 ng/ml ) compared to HC (median, 62 ng/ml; AD vs. HC p = 0.006; MCI vs. HC p = 0.03). Notably, IL-10 production by cells stimulated in the same conditions was significantly reduced in AD (median, 129 ng/ml) compared to HC individuals (median, 245 ng/ml) (p = 0.01).

Addition of IL-33 to cell cultures resulted in a significant reduction of the production of both IL-1β (median, 36 pg/ml; p = 0.04) and IL-6 (median, 616 pg/ml; p = 0.01) in HC, and of IL-1β alone in MCI (median, 23 pg/ml; p = 0.02). Finally, LPS+Aβ₄₂-stimulated IL-10 production was not modified by IL-33 in AD and MCI, but was significantly increased in HC (median, 585 pg/ml; p = 0.02) (Fig. 4).

These results support the idea that IL-33 reduces the generation of proinflammatory cytokines and stimulates that of anti-inflammatory cytokines, favoring the establishment of an anti-inflammatory milieu, and suggest that IL-10-mediated anti-inflammatory mechanisms are impaired/exhausted in AD and MCI.

Unstimulated as well as LPS-primed and Aβ₄₂-stimulated monocyte of AD (n = 5), MCI (n = 5), and HC individuals (n = 5) were analyzed to verify the effect of IL-33 on NF-kB nuclear translocation using the FlowSight technology. No differences in NF-kB nuclear translocation were detected in unstimulated cells (data not shown); upon antigenic stimulation, the IL-33 was observed to significantly reduce NF-kB nuclear translocation (p = 0.01) in HC alone (Fig. 5). These results suggest that this is a pivotal IL-33 anti-inflammatory mechanism that is possibly lost in MCI and AD.