HMGB-1 human clinical studies
Watanabe et al. were the first to test the level of HMGB1 and of the endogenous secretory receptor for advanced glycation end products (esRAGE) in sputum of asthmatic patient. In 2011 they dosed HMGB-1 and esRAGE levels in induced sputum of 44 asthmatic patients (before any asthma treatment) and 15 normal controls (Japanese, non-smokers subjects, with no history of respiratory infection for minimum of 4 weeks before the study). HMGB-1 sputum levels were significantly augmented in asthmatic patients than in controls, and there was an accordance between HMGB-1 level and the severity of disease. esRAGE levels in induced sputum from asthmatic subjects were considerably higher than those in healthy ones, with no significant differences in esRAGE levels between the mild persistent and the severe asthmatic patients [
13].
In 2011 Hou et al. enrolled 61 asthmatic and 47 COPD untreated patients and compared them with controls. HMGB1 levels in induced sputum were higher in patients with all severities of asthma and in those with COPD than healthy subjects. Plasma and sputum HMGB1 levels were higher in patients with severe asthma than in patients with mild one. There were no significant variation in sputum HMGB1 levels between subjects with mild asthma and controls and between mild asthma and moderate asthma. Plasma HMGB1 levels were noticeably higher in patients with moderate asthma than in those with mild asthma. Serum and sputum HMGB1 levels of COPD patients were significantly augmented than levels in asthmatic ones. The differences of plasma and sputum HMGB1 levels were not significant between patients with non eosinophilic asthma and eosinophilic asthma patients. In every patient, HMGB1 levels in plasma and induced sputum pointed out a significant negative correlation with lung function parameters (FEV1, FEV1) and FEV1/FVC ratio [
14].
Sukkar et al. in 2012, enrolled asthmatic subjects (n = 516), COPD ones (n = 537) and healthy controls (n = 518). They rated total sRAGE, neutrophils, endogenous secretory RAGE (esRAGE), HMGB1 and serum amyloid A (SAA) on bronchial lavage fluid. They enrolled subjects using inhaled corticosteroids (ICS) reporting increased HMGB1 in the airways in stable COPD and in asthmatic sputum. Moreover, they dosed systemic levels of soluble RAGE (sRAGE) in a separate group of asthmatic (n = 5101) and COPD (n = 534) patients. Subjects with neutrophilic asthma or COPD had no levels of lung sRAGE, while levels of sRAGE in non-neutrophilic asthma/COPD were almost the same to those in controls. Systemic sRAGE was significantly decreased in patients affected by neutrophilic asthma or COPD compared to those which haven’t airway neutrophilia. sRAGE and esRAGE in the lung and systemically had a significant positive correlation. HMGB1 levels were similar in all subject groups, while SAA was undetectable. Thus, they aimed to report whether reduced sRAGE was associated with augmented levels of HMGB1 and SAA, both mediators of neutrophil inflammatory reaction. They observed similar BL levels of HMGB1 in every group speculating that HMGB-1 levels differences were abrogated by the use of ICS [
15].
Shim et al. in 2012 joined up 50 asthmatics and 15 normal controls. This study confirmed that sputum HMGB1 expression was higher in asthmatics than in healthy controls; sputum HMGB1 expression was significantly higher in subjects with sputum eosinophilia than in subjects without sputum eosinophilia. There was a positive correlations between sputum HMGB1 expressions in sputum eosinophilia and sputum TNF-a, IL-5 and IL-13 levels [
16].
Zhou et al. in 2012 recruited 72 asthmatic patients in treatment and 30 healthy individuals. In induced sputum samples of asthma group was detected an augmented presence of neutrophils, HMGB1 and RAGE levels. In severe asthmatics, the percentage of neutrophils and HMGB1 levels were noticeably higher than in mild and moderate asthmatic patients. The percentage of neutrophils, HMGB1 and RAGE levels were diminished after treatment administration than before treatment administration. It was reported a negative correlations between HMGB1 or RAGE levels and FEV1%, and positive one between HMGB1 or RAGE levels and the percentage of neutrophils [
17].
Liang et al. isolated normal Human bronchial epithelial cells from human lung tissue obtained from four patients undergoing lobectomy. They focused on specific receptor of p38 MAPK, ERK1/2, or PI3-K and showed that HMGB1 increased the expression and secretion of TNF-a, TSLP, MMP-9, and VEGF; this event was dose and time dependent. Elevated expression of RAGE protein was induced by HMGB1. RAGE blockade and p38 MAPK pathway inhibition decreased secretion of TNF-a, VEGF, MMP-9, and TSLP, ERK1/2 inhibition determined a smaller decrease. This study suggested that HMGB1 promotes activities of p38 MAPK and ERK1/2 pathways in bronchial epithelial cells by enhancement of TNF-a, VEGF, MMP-9, and TSLP level [
18].
Cuppari et al. enrolled 50 children or adolescents with mild, moderate and severe asthma and 44 healthy children. They showed that sputum HMGB1 levels were significantly augmented in patients with asthma compared to healthy ones. Particularly, patients with severe asthma presented higher sputum HMGB1 levels than patients with mild asthma and than moderate asthmatic ones. In addition, total serum IgE levels in the asthmatic group were noticeably elevated than those in the control group and positively correlated to sputum HMGB1. Sputum HMGB1 values were positively related to total IgE levels in children with asthma. It emerged an inverse correlation between sputum HMGB1 levels and lung function indices [
7].
Ojo et al. in 2015 treated human bronchial epithelial cell line with various concentrations of HMGB1 and demonstrated the reduction of E-cadherin and an enhanced scratch wound closure. Then they assessed the impact of glycyrrhizin, an inhibitor of extracellular HMGB1, and demonstrated that it is sufficient to block this effect. Also the addiction of TLR4 or RAGE inhibitors block this effect, so this study demonstrated that TLR4 and RAGE may be required to response to HMGB1. For the first time, this study demonstrated HMGB1 promotes bronchial epithelial cell wound repair by enhanced production of integrins and ECM proteins. HMGB1 interacted with TLR4 and/or RAGE, actived downstream signaling MAPKs (ERK1/2 and JNK; 2), induced fibronectin, laminin-5(2 chain), 3-integrin. Also the addiction of TLR4 or RAGE inhibitors blocked the production of laminin-5(2chain) and 3integrin. By ERK1/2 and JNK signaling, (possible through SMAD2) the HMGB1-induced wound repair through TGF-receptor1 [
19].
HMGB-1 experimental animal studies
Shim et al. created an animal model of asthma (mice) to analyse lung tissue and bronchoalveolar lavage (BAL) fluid after an intraperitoneal injection of neutralizing antibodies. They observed that RAGE and TLR2 expression on the CD11b−CD11c+ cells (dendritic cells) augmented importantly in asthmatic animals compared with control ones and these changes were incredibly attenuated by the injection of HMGB1 neutralizing antibodies [
16].
Lee et al. in 2013 created a animal model (mice) of chronic asthma in order to demonstrate that the inhibition of HMGB1 expression decreased airway inflammation, mucus generation, and collagen production in lung tissues. The count of CD4+ T helper (Th) cells in the mediastinal lymph nodes and lungs demonstrated that Th17 had a greater increase than Th2 cells and Th1 cells in OVA-immunized mice; moreover Th1, Th2, and Th17 cells got lower in anti-HMGB1 antibody (Ab)-treated animals. In OVA-immunized mice, TLR-2 and TLR-4 expression, but not RAGE expression, was expressed ex novo in the lungs and diminished after anti-HMGB1 Ab administration [
20].
Ullah et al. in 2014 investigated TLR4 and RAGE interaction in a house dust mite asthma mice model. They demonstrated that the shortage of RAGE reduced the allergic airway inflammation but in absence of both RAGE and TLR4 there was not further reduction in inflammatory response. The release of HMGB1 from the airway epithelium obtained in a biphasic way, lead to the sequential activation of TLR4 then RAGE and was followed by the downstream of IL-1a, and the upstream of IL-25 and IL-33 production. They, also, demonstrated that Immunoneutralization of HMGB1 reduced allergic airway inflammation [
21].
Qiao et al. investigated the consequence of different doses of 1,25-(OH)2D3 on airway remodelling and on the expression of HMGB1 and TLR4 in a mice model. They used groups of 10 mice: a control, an asthmatic and 1,25-(OH)2D3 low, middle, high dose group. There was a higher expression of HMGB1 and TLR4 mRNAs in the lungs of asthmatic group than in control one. The expression of HMGB1 and TLR4 mRNAs in 1,25-(OH)2D3 low and middle dose groups was considerably lower than the asthma group and higher than the control one; the high dose group had an augmented expression of HMGB1 and TLR4 mRNAs compared to the asthmatic group [
22].
Tang et al. in 2014, made a toluene-2,4-diisocyanate (TDI)-induced murine asthma model, dominated by granulocytic inflammation and explored the role of ethyl pyruvate (EP) on this model. Their paper demonstrated the capability of EP in suppressing inflammation in the peribronchial and perivascular lung structure and in reducing the amount of neutrophils in BAL. Levels of HMGB1 were significantly higher in TDI induced murine asthma model and EP treatment down-regulated HMGB1 in a dose-dependent manner [
23].
Zhang et al. thanks to their previous observation in a murine model of neutrophilic asthma of positive correlation between the increase in HMGB1 expression and Th17-mediated airway inflammation, speculated that HMGB1 promoted the production of Th17 polarization-related factors, and that HMGB1 blocking inhibited the Th17 response. They assessed that rHMGB1-stimulated DCs secreted IL-23, in vitro, that act as a Th17 polarization factor. IL-23 antibody, added in the culture, reduced the IL-17A expression level and the percentage of IL-17+ CD4+ T cells, suggesting that the IL-17 expression level was dependent upon rHMGB1 and potentially regulated by the endogenous production of IL-23 by BMDCs. They showed that anti-HMGB1 IgG decreased HMGB1 expression, levels of neutrophilic inflammation in lung tissue, in BALF by decreased levels of Th17-related cytokines (IL-23 and IL-17A) [
24,
25].
Shim et al. considered eosinophils, dendritic, and CD4+ T cells obtained from a mice model of asthma. They demonstrated that HMGB1 levels were higher in the supernatant of the eosinophil culture stimulated with IL-5. On the contrary, anti-HMGB1 antibodies significantly decreased IL-4 and IL-5 levels in the supernatant of CD4+ T cells co-cultured with DCs [
26].
Yao et al. in 2015 investigated the role of HMGB1 in TDI-induced asthma with the IgY anti-HMGB1 antibody. They used a TDI-induced asthmatic murine model, measured levels of IFNg, IL-4, IL-5, IL-13, IL-17A and TNF-a in supernatants of cultured lymphocytes and accomplished pulmonary histopathological examination. They found that IgY could augment cytokine release in asthma [
27].
Liang et al. in 2015, using a TDI-induced murine asthma model, demonstrated that caspase-1 activation and HMGB1 production was mediated by Phosphatidylinositol 3-kinases (PI3Ks); this study also assessed the role of LY294002 a specific inhibitor of PI3K. They considered lymphocytes by cervical lymphonodes, total serum IgE, Bronchoalveolar lavage (BAL), lung histopathology. First, they proved administration of LY294002 abolished the TDI induced elevated p-Akt expression, involved in downstream of PI3K signal pathway. Level serum IgE was significantly increased in TDI-induced murine asthma model, as well as IL-4 in supernatant of cultured lymphocytes, the number of inflammatory cells and the protein level of HMGB1 in BAL fluid and lung tissue. These changes in both BALF and lung tissue were reversed after LY294002 treatment. HMGB1 trans-located from the nuclei to the cytoplasm after TDI challenge; both the higher protein expression and nucleocytoplasmic translocation of HMGB1 were diminished after LY294002 adminstration. In TDI-induced murine asthma model, caspase-1 was activated after TDI exposure; after LY294002 adminstration was found abnormal distribution of cleaved caspase-1 but not procaspase-1, so the role of this specific inhibitor was established in the cleavage process of caspase-1 rather than increasing its protein expression. Also they detected higher level of IL-1b after TDI exposure, and showed that LY294002 administration reduced this TDI induced IL-1b expression in the cytoplasm [
28].
Ma et al. reported that levels of HMGB1 in BALF and lung tissue of asthmatic mice were significantly augmented than controls. HMGB1 injection was correlated to increased mucus production and presence of eosinophils and neutrophils in the airways together with a decreased pulmonary function, to increased levels of IL-4, IL-5, IL-6, IL-8 and IL-17 and reduction of IFN-γ in the BALF and lung tissue, enhanced GATA3 expression of Th2 cells and attenuated T-bet expression of Th1 cells. These effects could be reversed after inhibiting HMGB1 [
29].
Finally in 2015 Hou et al. elaborated a mice model of chronic asthma (which have a considerably high HMGB1 expression) in order to consider the effects of HMGB1 on airway responsiveness and re-modeling. They administered to the mice anti-HMGB1 antibody therapy. The anti-HMGB1 antibody animals exhibited diminished levels of IgE, inflammatory cytokines and inflammatory cell accumulation, airway hyperresponsiveness (AHR), mucus generation, smooth muscle thickness and lung collagen levels [
30].