key: cord-0783299-z6vzi0ut authors: Ozturk, Mumin; Chia, Julius E.; Hazra, Rudranil; Saqib, Mohd; Maine, Rebeng A.; Guler, Reto; Suzuki, Harukazu; Mishra, Bibhuti B.; Brombacher, Frank; Parihar, Suraj P. title: Evaluation of Berberine as an Adjunct to TB Treatment date: 2021-10-20 journal: Front Immunol DOI: 10.3389/fimmu.2021.656419 sha: f59f9354beb4f1cbab475623f578b94708c90ffb doc_id: 783299 cord_uid: z6vzi0ut Tuberculosis (TB) is the global health problem with the second highest number of deaths from a communicable disease after COVID-19. Although TB is curable, poor health infrastructure, long and grueling TB treatments have led to the spread of TB pandemic with alarmingly increasing multidrug-resistant (MDR)-TB prevalence. Alternative host modulating therapies can be employed to improve TB drug efficacies or dampen the exaggerated inflammatory responses to improve lung function. Here, we investigated the adjunct therapy of natural immune-modulatory compound berberine in C57BL/6 mouse model of pulmonary TB. Berberine treatment did not affect Mtb growth in axenic cultures; however, it showed increased bacterial killing in primary murine bone marrow-derived macrophages and human monocyte-derived macrophages. Ad libitum berberine administration was beneficial to the host in combination with rifampicin and isoniazid. Berberine adjunctive treatment resulted in decreased lung pathology with no additive or synergistic effects on bacterial burdens in mice. Lung immune cell flow cytometry analysis showed that adjunctive berberine treatment decreased neutrophil, CD11b(+) dendritic cell and recruited interstitial macrophage numbers. Late onset of adjunctive berberine treatment resulted in a similar phenotype with consistently reduced numbers of neutrophils both in lungs and the spleen. Together, our results suggest that berberine can be supplemented as an immunomodulatory agent depending on the disease stage and inflammatory status of the host. Tuberculosis (TB) is the global health problem with the second highest number of deaths from a communicable disease after COVID-19. Although TB is curable, poor health infrastructure, long and grueling TB treatments have led to the spread of TB pandemic with alarmingly increasing multidrug-resistant (MDR)-TB prevalence. Alternative host modulating therapies can be employed to improve TB drug efficacies or dampen the exaggerated inflammatory responses to improve lung function. Here, we investigated the adjunct therapy of natural immune-modulatory compound berberine in C57BL/6 mouse model of pulmonary TB. Berberine treatment did not affect Mtb growth in axenic cultures; however, it showed increased bacterial killing in primary murine bone marrow-derived macrophages and human monocyte-derived macrophages. Ad libitum berberine administration was beneficial to the host in combination with rifampicin and isoniazid. Berberine adjunctive treatment resulted in decreased lung pathology with no additive or synergistic effects on bacterial burdens in mice. Lung immune cell flow cytometry analysis showed that adjunctive berberine treatment decreased neutrophil, CD11b + dendritic cell and recruited interstitial macrophage numbers. Late onset of adjunctive berberine treatment resulted in a similar phenotype with consistently reduced numbers of neutrophils both in lungs and the spleen. Together, our results suggest that berberine can be supplemented as an immunomodulatory agent depending on the disease stage and inflammatory status of the host. Tuberculosis (TB) is currently the second deadliest infectious disease worldwide caused by a single pathogen with an estimated 10 million cases and 1.4 million deaths reported in 2019 (1) . Although it has been previously stated that between one-third to one-fourth of the world population has latent tuberculosis infection (LTBI) according to the epidemiological modeling studies, this notion has been challenged recently (2, 3) . There is still an alarmingly large reservoir of active TB cases due to a 5-10% risk of LTBI progression (4) . In addition to ongoing transmission in communities, the treatment for TB is long and complex with considerable side effects. Poor compliance, inadequate health infrastructure for drug monitoring has resulted in the increasing prevalence of multidrug (MDR) and extensively drug-resistant (XDR) TB. A recent study forecasted that by 2040, 32.5% of incident TB cases in Russia and 12.4% in India will be MDR-TB even though acquired drug resistance rates have been dropping (5) . TB also impinges on adults during their economically productive life period furthermore, it customarily affects impoverished and socially disadvantaged communities to a greater extent. It is estimated that TB will cost the global economy $983 billion between 2015-2030 (6). Therefore, the development of novel treatment options with a lower toxicity profile that can synergize with the existing firstline and second-line antibiotics to decrease treatment duration is the focus of attention. There has been substantial progress in the anti-mycobacterial field with the recent approvals of bedaquiline, delamanid and pretomanid. Besides antimycobacterials; adjunct host-directed therapies (HDT) are also in the spotlight as alternative approaches to exploit host-pathogen interplay. Improving bacterial killing mechanisms, reinforcing immune and memory responses, disrupting TB granuloma structure and balancing inflammatory responses can be targeted for HDT (7, 8) . One of the hallmarks of pulmonary TB is inadequately regulated inflammatory responses which exacerbate tissue damage, necrosis and eventual lung cavitation (9) . An immunomodulatory HDT that fine-balances the host inflammatory pathway can dampen excess host inflammatory response and long term lung damage. Berberine is the bioactive ingredient extracted from roots, barks, rhizomes of medicinal plant families Berberidaceae (barberry), Ranunculaceae (goldenseal), Rutaceae (cork tree) and Annonaceae (African whitewood). Berberine is an isoquinoline alkaloid with antimicrobial, antidiabetic, anti-tumor and antiinflammatory properties (10) (11) (12) (13) (14) . As a Chinese and Native American traditional medicine, it has been used for the treatment of gastroenteritis and dysentery (15) . The diverse pleiotropic actions of berberine are mainly ascribed to its immunomodulatory properties through inhibition of nuclear factor kappa B (NF-kB), mitogen-activated protein kinase (MAPK) signaling pathways and inhibition of pro-inflammatory cytokine production (16) . Berberine can also affect cell proliferation, cell death and inhibit prolonged activation of immune cells. In the experimental autoimmune neuritis model, berberine treatment ameliorated the development of the autoimmune disease by inhibiting CD4 + T cell proliferation (17) . In the collagen-induced arthritis model, berberine treatment induced apoptosis of IL-12 producing mature dendritic cells in spleen and lymph nodes of mice that can result in subsequent restriction of chronic activation of T cells (18) . In dextran sulfate sodium (DSS)-induced colitis model, berberine induced apoptosis of colonic macrophages and decreased proinflammatory cytokine production from colonic macrophages and colon epithelial cells (19) . In trinitrobenzene sulfonic acid (TNBS)-induced colitis model, berberine treatment shifted macrophages into tissue repair and remodelling associated M2 phenotype rather than tissue destructive, pro-inflammatory M1 phenotype (20) . The immunomodulatory mechanisms of berberine in diverse inflammatory disease models prompted us to investigate the potential of berberine as an adjunct therapy in C57BL/6 murine model of tuberculosis. In the present study, we sought out synergistic effects of berberine with first-line antimycobacterials rifampicin and isoniazid in well-established murine models. Our results suggest that berberine treatment decreases tissue pathology without any additive or synergistic effects on the bacterial burden. The decrease in tissue pathology correlates with a decreasing number of inflammatory neutrophils, recruited macrophages and CD11b + dendritic cells in the C57BL/6 model when the treatment started at earlier stages of infection. However; the effect on decreased inflammatory cells was not observed once berberine treatment started at later stages of C57BL/6 Mtb infection. Our results suggest that berberine adjunctive treatment can exert its beneficial effects depending on the inflammatory stage of the host during tuberculosis. Mice 8-10 weeks old C57BL/6 mice were kept under specificpathogen-free conditions in a biosafety level 3 containment facility individually ventilated cages (5 mice per cage) with filter tops (type 2 long), as well as dried wood shavings and shredded filter paper as floor coverings. The temperature range was set at 22-24°C and 12h dark-12h light cycles. All experiments were performed in accordance with the South African National Guidelines and the University of Cape Town of practice for laboratory animal procedures. The protocol was approved by the Animal Ethics Committee (AEC Permit Number: 015/040), Faculty of Health Sciences, University of Cape Town, Cape Town, South Africa. Similarly, C3HeB/FeJ (Kramnik) mice were kept under specific-pathogen-free conditions in individually ventilated cages at the animal resource facility at Albany Medical College, Albany, New York. All experiments were performed in accordance with the IACUC guidelines at the Albany Medical College, New York. Two-fold diluted concentrations of berberine (Sigma Aldrich, B3251) were screened for their anti-mycobacterial activity in 96-well, black, clear-bottom microplates (Greiner Bio-One, Germany), as previously reported (21) . Single-cell suspension of constitutively GFP expressing H37Rv Mtb strain from frozen glycerol (15%) stock with a working concentration of 1x10 6 colony-forming unit (CFU)/mL was prepared in Middlebrook 7H9 (Difco ™ , BD Biosciences) supplemented with 25 µg/mL kanamycin (Sigma Aldrich), 10% Middlebrook Oleic Acid-Albumin-Dextrose-Catalase (OADC) (v/v), 0.05% Tween 80 (w/v) and 0.2% glycerol (v/v). 100 µl of H37Rv-GFP was added to each experimental well followed by 100 µl 2X concentrated of berberine prepared in 7H9 broth as described above to test the 3.9 µM to 250 µM concentration range. Fluorescence (485ex/ 520em nm) was measured at days 0, 4, 6, 8, 10 and 12, with a BMG Labtech Omega Plate Reader (Germany). Bone marrow-derived macrophages were generated from 8-12 weeks old C57BL/6 mice. Generation of BMDM was performed as described previously (22) . BMDM were seeded in tissue culture-treated 96-well flat-bottom plates (Costar ® , Corning) at a concentration of 1x10 6 cells/ml. The cells were treated with 30µM berberine overnight, followed by H37Rv infection. In other sets of experiments, BMDM were rested overnight and infected with H37Rv. After 4 hours of infection, media was supplemented with berberine or vehicle (DMSO final concentration 0.1%). Monocyte-derived macrophages were generated from Leukopak obtained from Western Province Blood Service. Briefly, Leukopak was diluted 1:1 with phosphate buffered saline (PBS) containing 2% fetal bovine serum (Gibco, ThermoFisher) and centrifuged at 500g for 25 minutes with brakes off in Leucosep (Greiner Bio-one) tubes with Histopaque 1077 (Sigma Aldrich). The buffy coat is removed by Pasteur pipette and washed twice with PBS+2%FBS at 120g to remove platelets. Peripheral blood mononuclear cells were counted and subjected to CD14 + positive selection (Miltenyi) according to the manufacturer's instructions. Isolated monocytes were seeded in 60 mm Nunc cell culture dishes (ThermoFisher) at a concentration of 1x10 6 cells/ml in RPMI 1640 media (Gibco, ThermoFisher) supplemented with 10% human AB serum (Sigma-Aldrich), 50 U/ml penicillin G (ThermoFisher), 50 µg/ ml streptomycin (ThermoFisher) and 50 ng/ml recombinant human M-CSF (Peprotech) for 7 days. MDM were harvested by 20 minutes of incubation in Accutase ® (Sigma-Aldrich) solution. MDM were seeded in tissue culture-treated 96-well flat-bottom plates (Costar ® , Corning) at a concentration of 1x10 6 cells/ml without the antibiotics. The cells were then treated with 30µM berberine overnight, followed by H37Rv infection. BMDM and MDM were infected with a multiplicity of infection (MOI) 1. At 4 hours, 2 days and 5 days postinfection, the cells were washed once with sterile PBS and lysed in 0.1% Triton X-100. The cell lysates were diluted 10-and 100-fold and plated in Middlebrook 7H10 (Difco ™ , BD Biosciences). 7H10 plates incubated at 37°C for 14 days and colonies are counted under Nikon SMZ800N stereomicroscope. BMDM Activation and Reactive Oxygen Species (ROS) Assay 1x10 6 BMDM were infected with H37Rv for 2 days in 12 well plates. The media was removed, and cells were washed once with PBS and incubated for 10 min in 0.5 mg/ml lidocaine and 10 mM EDTA in PBS at 37°C. Cells were lifted by pipetting and washed with PBS. The flow cytometry staining protocol mentioned below was followed. 575V Viability Dye, CD11b-PerCPCy5.5 (Clone M1/70), F4/80-PeCy7 (Clone BM8), MHCII-AlexaFluor700 (Clone M5/114.15.2), CD80-BV421 (Clone 16-10A1) were used for staining. BMDM were seeded on 96 well black/clear bottom plates (ThermoFisher) and infected with H37Rv for two days. Infected BMDM were incubated with 5 µM CellROX Green Reagent (ThermoFisher) according to manufacturer's instruction. Uninfected BMDM were used as blank wells. The fluorescence was measured (485 nm excitation/525 nm emission) on Spectramax iD3 multi-mode reader (Molecular Devices). Western Blot Analysis 3x10 6 BMDM were seeded in 6-well plates and pretreated with berberine (30 µM) or vehicle (DMSO 0.1%) overnight. BMDM were infected H37Rv for 30, 60 and 120 minutes and washed with cold PBS before lysing with RIPA buffer (150 mM NaCl, 50 mM Tris-HCl, 1% Nonidet P-40, 0.5% sodium deoxycholate, 0.1% SDS) including cOmplete Protease inhibitor and PhosSTOP phosphatase inhibitor cocktail (Roche). Cell lysate protein content was determined using the BCA Protein Assay Kit (ThermoFisher). 30 µg of protein was loaded to 10% resolving acrylamide gel and wet WB was performed onto a nitrocellulose membrane. The membrane was probed with either SAPK/JNK Antibody, Phospho-SAPK/JNK (Thr183/Tyr185) (G9), NFkB p65 (D14E12), Phospho-NFkB p65 (Ser536) (93H1) (Cell Signaling Technology) or GAPDH (Santa Cruz Biotechnology) primary antibodies and either with goat anti-rabbit IgG H&L (HRP) pre-absorbed or goat anti-mouse IgG H&L (HRP) pre-absorbed (Abcam) secondary antibodies. Immunoblots were developed using the KPL LumiGLO ® Reserve Chemiluminescent Substrate Kit (SeraCare) on the iBright FL1000 Imaging System (Thermo Fisher). Mycobacterium tuberculosis H37Rv was grown in Middlebrook 7H9 broth as described previously (23) . For infection of the C3HeB/FeJ mice, Mtb Erdman strain was used. Prior to infection, stock solutions of Mtb were thawed, washed once with phosphate-buffered saline and inoculum was prepared in sterile saline containing 0.05% Tween 80. Aerosol infection was performed using an inhalation exposure system (model A4224, Glas-Col). To infect mice with a low dose of 100 CFU/lung, animals were exposed for 40 min to an aerosol generated by nebulizing approximately 6 ml of a suspension containing 2.4x10 7 live bacteria. The infection dose was checked at one day post-infection by determining the bacterial load in the lungs of four infected mice. One-week post-infection, four groups of mice were left untreated, treated with berberine (1 mg/ml), isoniazid/rifampicin (both 0.1 mg/ml), isoniazid/rifampicin/ berberine (both 0.1mg/ml and 1 mg/ml, respectively) in drinking water. Berberine concentration was determined according to previously published reports (24) . Drinking water was supplemented with 1% glucose in all four groups due to decreased water intake in the isoniazid/rifampicin/berberine triple-drug group. Glucose supplemented drug treatment groups showed similar water intake. Drinking water was changed twice a week and volume was measured to estimate the average drug intake. On average, berberine-treated groups received 5.5 mg berberine per day and isoniazid/rifampicin groups received 0.6 mg rifampicin/isoniazid (RIF/INH). At the experimental endpoint, mice were euthanized with halothane and cardiac puncture was performed for confirmation of death by exsanguination. The blood was left at room temperature for 30 min to clot and centrifuged at 1500g for 10 min at 4°C. The serum was collected to measure liver ALT and AST enzyme levels at National Health Laboratory Services (NHLS) diagnostic laboratory. Mycobacterial loads in the lungs and spleen of Mtb-infected mice were determined as previously described (25) . The right superior lobes were fixed with 10% neutral-buffered formalin, and tissue was processed with the Leica TP 1020 benchtop processor for 24 h and embedded in paraffin wax. Four 3 µm thick sections with 30 µm distance apart were cut in Leica Sliding Microtome 2000R, deparaffinized and subsequently stained with the hematoxylin & eosin (H&E) stain. The lung images were acquired in Nikon 90i Eclipse widefield microscope and free alveolar space was quantified using NIS elements (Nikon Corporation, Japan). Briefly, the images were converted to binary, and H&E positive area was measured. Fill holes function of NIS elements was employed to measure the complete lung area including the alveolar spaces. Free alveolar spaces were calculated by subtracting H&E positive area from the complete lung area and presented as a percentage to the complete lung area. Single-cell suspensions of the left lobes of the lung were prepared as previously described (26) . For late-onset berberine treatment experiments, half of the spleen was mechanically digested sequentially through 100 µm and 70 µm cell strainers (SPL Life Sciences). The cells were washed once with media (DMEM+10% FCS) and red blood cells were lysed by ACK lysis buffer (150 mM NaCl, 10 mM KHCO 3 and 0.1mM Na 2 EDTA) for 5 min incubation at room temperature. The cells were washed once with media again and counted with CytoSMART (Corning) automated cell counter. Briefly, 1x10 6 cells were washed once with PBS and stained with dead cell marker (575V Viability Dye, BD Biosciences) for 15 min at room temperature. The staining was later quenched and washed with 0.5%BSA in PBS and cells were then subjected to staining for B cells (CD3 -CD19 + ), CD4 T cells (CD19 -CD3 + CD4 + ), CD8 T cells (CD19 -CD3 + CD8 + ), alveolar macrophages (SiglecF + CD11c + CD64 + ), neutrophils (CD11b + Ly6G + ), CD11b + dendritic cells (CD64 -CD11b + CD11c + MHCII + ) and inflammatory macrophages (CD64 + CD11c -CD11b + SiglecF -) and monocyte-derived DCs (CD64 + CD11c + CD11b + ) in the presence of 10% heat-inactivated rat serum and 10% FcgR blocker for 30min on ice. Similarly, neutrophils (CD11b + Ly6C + Ly6G + ), inflammatory monocytes (CD11b + Ly6C + Ly6G -) and T cells (CD11b -CD3e + Ly6C -Ly6G -) were identified in the lungs of C3HeB/FeJ mice. Spleen myeloid populations were identified as neutrophils (CD11b + Ly6G + ), monocytes (CD11b + Gr-1 + CD11c -Ly6G -), CD169 + macrophages (CD11b + CD169 + CD11c -), red pulp macrophages (F4/80 + CD11b low CD169 -CD11c -), CD11b DC (CD11c + MHCII + CD11b + CD8 -) and CD8 DC(CD11c + MHCII + CD8 + CD11b -). Antibodies used for flow cytometry analysis were as follows: CD3-A700 (Clone 500A2), CD19-PerCPCy5.5 (Clone 1D3) and CD8-APC (Clone 53-6.7), Gr-1 Biotin (Clone RB6-8C5), CD169 APC-eFluor780 (Clone Ser-4) and Streptavidin-PECF594 purchased from BD Biosciences and eBioscience. Cells were washed then fixed in 2% paraformaldehyde overnight and acquired by BD LSRII (BD Pharmingen) and analysed by FlowJo V9 (TreeStar, US). Marker positive stained cells are calculated as a percentage of live cells and later these percentages are backcalculated to cell counts obtained from Trypan Blue exclusion method and finally back-calculated by multiplying the ratio of total lung weight to the left lobe weight. The cell-free lung and spleen homogenate was spun at 3000g for 5 min and stored at -80⁰C until ELISA analysis, samples were thawed and double filtration (0.2 µM) was performed before transporting the supernatant from biosafety level 3 facility. Lung homogenates were analysed for the IFNg, IL-12p40, GM-CSF (BD Biosciences), IFN-b, IL-10 (BioLegend), IL-1b, CXCL10, and CCL3 (R&D Systems) by ELISA according to manufacturers' instructions. Similarly, supernatants from Mtb-infected macrophages were collected and stored at -80°C until further analysis. After thawing, the supernatants were filtered through Corning FiltrEX 96-well low protein binding filter plates and the supernatant was transported out of BSL3. Nitrite concentrations were measured by Griess assay. IL-1a (R&D Systems), IL-6 (BD Biosciences) and TNF (Biolegend) ELISA were performed according to the manufacturers' instructions. Lung middle lobes were washed with cold PBS and immersed in RNAprotect Tissue reagent (Qiagen) overnight at 4°C and the Data are represented as mean values ± SEM. Statistical analysis was performed using one-way ANOVA with Tukey post-hoc test if the data points are normally distributed. The normality is checked through the Shapiro-Wilk normality test and the Anderson Darling test. If the data did not fit into Gaussian distribution Kruskal-Wallis test was performed. Statistical differences in all groups are shown as significant *, P ≤ 0.05; **, P ≤ 0.01; ***, P ≤ 0.001. All the data were plotted using the GraphPad Prism 8 software. We investigated whether berberine has an impact on the survival of Mycobacterium tuberculosis (Mtb) in liquid broth and macrophages. First, we assessed whether berberine has a direct anti-mycobacterial effect in a liquid culture medium supplemented with a range of concentrations for 12 days. We found that berberine had no mycobactericidal effect on the axenic growth of Mtb in a concentration range from 3.9-250 µM ( Figure 1A) . We then determine the cytotoxic effect of berberine on primary murine macrophages by Cell Titer Blue assay. BMDM were pre-treated with 2-fold concentrations of berberine from 0 to 2000 µM for 6 days. Macrophages treated with berberine at 62.5 µM and above displayed a significant cytotoxic effect. The highest concentration which had no cytotoxic effect was 31.25 µM and we used 30 µM used for subsequent intracellular assays ( Figure 1B) . Mouse BMDM were pre-treated with 30 µM overnight to determine the intracellular growth of Mtb in a time-kinetic manner. We found that berberine treatment had no effect on the uptake of Mtb (day 0) and showed a significant decrease in Mtb growth at 2 and 5 days post-infection ( Figure 1C ). The increased mycobacterial killing ability of macrophages was similar in macrophages treated with berberine after phagocytosis of Mtb (Supplementary Figure 1A) . To further probe Mtb infected macrophage modulation upon berberine treatment, interestingly resulted in a higher percentage of MHCII and CD80 ( Figure 1D ) and higher expression of CD80 (Supplementary Figure 1B) . Furthermore, berberine treatment resulted in decreased levels of nitric oxide (NO) ( Figure 1E ), pro-inflammatory cytokines IL-1a ( Figure 1F ), IL-6 ( Figure 2A) ; while it did not effect TNFa ( Figure 2B ) levels in vitro. Berberine can exert its antibacterial effects through the increase of reactive oxygen species (ROS), although there are studies also reporting antioxidant activities of berberine (27) (28) (29) . We have measured intracellular ROS levels of berberine-treated murine macrophages which showed no change in ROS accumulation ( Figure 2C ). In line with the previous reports, we observed decreased phosphorylation of p65 subunit of NF-kB and c-Jun N terminal kinase (JNK) ( Figure 2D ). Furthermore, we assessed the influence of berberine on the intracellular growth of Mtb in human monocyte-derived macrophages (MDM). Considering the sex differences in monocyte or MDM response (30), we measured the bacterial killing effect of berberine supplementation in female and male donor-derived MDM. Similar to mouse macrophages, both female and male MDM significantly decreased intracellular Mtb growth upon berberine treatment ( Figure 2E) . These results show that berberine treatment decreased Mtb growth in mouse and human macrophages possibly by modulating the antimicrobial capacity of the host; while paradoxically downregulating proinflammatory responses. Berberine as an Adjunctive Therapy Decreased the Lung Pathology During Mtb Infection in Mice To investigate the biological relevance of our findings in macrophages, we determined whether berberine as an adjunctive therapy will have a host-protective effect in vivo. Oral administration of berberine is deemed safe since no mortality was observed in mice administered with as high as 20.8 g/kg of body weight due to extremely poor absorption in the gut, rapid and extensive metabolism (31, 32) . Owing to low oral bioavailability, short-term and chronic berberine administration have not resulted in concerning adverse effects in the clinic (33) . To evaluate the potential of berberine in TB therapy, mice were infected with a low dose (100CFU, Mtb H37Rv) by aerosol inhalation. One week after infection, mice were treated with berberine and rifampicin/isoniazid alone or in combination for 4 weeks ad libitum ( Figure 3A) . Berberine treatment groups consumed slightly less water; however, had no differences in body weight change (Supplementary Figure 2A) . Moreover, serum alanine transaminase (ALT) and aspartate transaminase (AST) were similar between the groups after 4 weeks of treatment, indicating that berberine had no liver toxicity though there was a reduced trend of AST and ALT levels in the Rif/Inh/Ber group (Supplementary Figure 2B) . After 4 weeks of treatment, mice were euthanized to determine mycobacterial burdens and lung pathology. We found that berberine alone or as an adjunctive to rifampicin/isoniazid had no effect on the lung and spleen mycobacterial burdens ( Figure 3B ). However, lung sections revealed that berberine used as an adjunct to first-line anti-TB drugs, INH and RIF, significantly decreased the lung tissue pathology ( Figure 3C ). Furthermore, we quantified the free alveolar spaces in these sections indeed revealed that berberine as an adjunct significantly increased the non-inflamed alveolar spaces in the lungs when compared to mice treated with INH/RIF alone or untreated mice ( Figure 3D ). These results demonstrate that berberine as an adjunct to first-line drugs decreased lung pathology during tuberculosis. Berberine as an Adjunctive Therapy Modulates Immune Cell Recruitment in the Lungs During Mtb Infection in Mice We then assessed whether berberine as an adjunct treatment influences lung immune cell recruitment during Mtb infection. A single-cell suspension of lungs was prepared to analyse immune cell recruitment by flow cytometry. We found that mice treated with Rif/Inh or Rif/Inh/Ber showed decreased lung cell numbers ( Figure 4A ). The cell suspension was subjected to flow antibody staining using markers for phenotyping of lymphocytes and myeloid cell compartments. Berberine as an adjunct therapy decreased CD4 + and CD8 + T cells (Figures 4B, C) to the same level as Rif/Inh group. Similar to T cells, B cells ( Figure 4D ) were also decreased in mice treated with Rif/Inh/Ber to a similar extent of Rif/Inh group. Amongst myeloid cells, berberine as an adjunct decreased alveolar macrophages when compared to untreated, similar to rifampicin/isoniazid treated mice ( Figure 4E ). Neutrophils are a major contributor to lung pathology in tuberculosis (34, 35) . Mice treated with rifampicin/ isoniazid decreased neutrophils in the lungs ( Figure 4F ), most probably due to reduced lung burdens. Berberine combined with rifampicin/isoniazid further significantly decreased the neutrophils when compared to mice treated with berberine alone ( Figure 4F ). This may explain the observed reduced lung pathology in this group of mice. Furthermore, mice treated with rifampicin/isoniazid alone and antibiotics with berberine displayed reduced conventional CD11b + dendritic cells ( Figure 4G ) and inflammatory macrophages ( Figure 4H ) when compared to untreated or berberine alone animals. These results suggested that berberine as an adjunct to antibiotic therapy decreased lymphoid and myeloid cell recruitment in the lungs during tuberculosis. We next assessed the cytokine levels in lung homogenates by ELISA at 4 weeks post-treatment. The analysis revealed that mice treated with berberine as an adjunct significantly reduced CXCL-10 ( Figure 5A) , while there was a decreasing trend towards IL-1b ( Figure 5B ) and CCL3 levels ( Figure 5C ) when compared to antibiotics alone. CXCL10 is an inflammatory chemokine that activates cells to increase inflammatory lung damage and is highly expressed in patients with active TB (36) . Rif/Inh treatment decreased IL-12p40 levels drastically; however adjunct berberine treatment did not promote the reduction of IL-12p40 levels ( Figure 5D ). Moreover, adjunct berberine treatment did not affect IFNg, GM-CSF, IFN-b and IL-10 levels in the lung ( Figures 5E-H) . Interestingly, CCL3 and IFNg levels showed a bimodal distribution similar to lung CFU ( Figure 3B ), indicating that lung bacterial burdens are the major driver in the production of these cytokines/chemokines. Together, these results suggest that berberine as an adjunct decreases certain chemokine/cytokine production in the lungs during Mtb infection. H37Rv Mtb strain grows exponentially during the first three-four weeks of infection in the lungs of C57BL/6 mice and bacterial burden stabilizes after this stage which coincides with the arrival of antigen-specific T cells in the lungs (37, 38) . We, therefore, were prompted to adapt adjunct berberine treatment at peak bacterial burdens levels in the lung i.e. 3 weeks after infection ( Figure 6A ). Berberine alone treatment or adjunct berberine treatment did not affect lung and spleen bacterial burdens ( Figure 6B) ; however, the adjunctive treatment resulted in decreased tissue involvement ( Figures 6C, D) similar to berberine treatment started at 1 week after infection. However, adjunctive treatment resulted in increased lung and spleen total cell numbers ( Figure 7A ) which are driven mainly by increased CD4 T cells ( Figure 7B) and B cell numbers ( Figure 7C ). There were also expanded CD4 T cell and CD8 T cell and B cell numbers in the spleens of the adjunctive treatment group and a similar trend was observed in the berberine alone treatment group (Figures 7B, D) . Similar to earlier adjunct treatment, we observed decreased neutrophil numbers in the spleens and lungs of the adjunctive group ( Figure 7E) ; however, conventional CD11b + dendritic cells ( Figure 7F ) remain unaffected. To recapitulate in vitro macrophage activation results, we investigated MHCII expression levels in lung and spleen myeloid subsets. In the lungs, lower percentages of recruited interstitial macrophages in the adjunct group were MHCII positive, but CD169 + macrophages, red pulp macrophages and monocytes of berberine alone and adjunctive treatment groups co ns is te ntl y sh o w ed i nc re a se d MH C II e x p r es si on (Supplementary Figure 2C) . It is shown that berberine influences caspase 3 activation and downstream apoptosis events in a cell-specific manner (39); we sought out in vivo activated caspase-3 levels in lung and spleen cells. The adjunctive treatment group showed decreased caspase-3 positive cells in the spleen, but this effect was not observed in the lungs (Supplementary Figure 2D) . CXCR3 is the receptor for CXCL-10 and regulates the migration of antigen-specific Th1 cells into the lung (40) . CXCR3 + CD4 T cells are efficient in localizing lung parenchyma around the lymphocytic cuff of TB granulomas and rarely in the myeloid core (41) . We found that lung CD4 T cells in the antibiotic-treated groups have increased frequencies of CXCR3 + subsets and the adjunctive berberine treatment decreased the frequency of CXCR3 + CD4 T cells in the spleen compared to Rif/Inh group (Supplementary Figures 3A, E) . Late onset of berberine adjunctive treatment did not change lung alveolar macrophage, recruited interstitial macrophage, lung monocyte-derived DC, spleen CD169 + macrophage, spleen red pulp macrophage or spleen CD8a + DC cell numbers ( Supplementary Figures 3B-D, F-H) . In terms of lung and spleen cytokine/chemokine levels; lung IFNg, lung and spleen CXCL10, lung GM-CSF, lung and spleen IFNb levels remain unchanged (Supplementary Figures 4A, D-F) . Antibiotic treatment groups showed reduced spleen IFNg, spleen IL-1b and lung IL-12p40 levels ( Supplementary Figures 4A-C) . Interestingly, the berberine alone group increased lung and spleen IL-1b levels (Supplementary Figure 4B) ; a similar trend was also observed in the early treatment onset of berberine ( Figure 5B ). Aside from CXCL10 signaling, we also investigated whether IFNg and GM-CSF signaling was affected by gene expression levels of IFNg (Ifngr1) and GM-CSF receptors (Csf2ra) in total lung tissue by qPCR. Berberine alone suppressed Ifngr1 expression levels while Csf2ra expression did not change among different groups (Supplementary Figure 4G) . Our data suggest that late-onset of berberine treatment still reduced neutrophil recruitment and beneficial against lung pathological responses, while spleen tissue was more affected by adjunctive berberine treatment. We further investigated the host protective role of berberine in a more relevant model of tuberculosis. We used C3HeB/FeJ (Kramnik) mice, which recapitulates the progressive lung pathology of patients with TB. Mice were infected with Mtb Erdman via aerosol inhalation to deposit 100CFU in the lungs. After 3 weeks of infection, cohorts of mice were treated with either berberine or antibiotics or berberine combined with antibiotics (Supplementary Figure 5A) . Four weeks following treatment, mice were euthanized to analyze the lung mycobacterial burden as CFU, the extent of inflammation as measured by immune cell recruitment and histopathological lung damage. The bacterial burden was similar between antibiotics and berberine as an adjunctive (Supplementary Figure 5B) . Interestingly, berberine alone also significantly decreased lung mycobacterial burdens in Kramnik mice as opposed to C57BL/6 mice (Supplementary Figure 5B) . Furthermore, H&E staining revealed that lung pathology is decreased in cohorts treated with berberine alone or in combination with antibiotics (Supplementary Figure 5C) . Lung alveolar space quantification revealed that berberine alone did not effect lung pathology to a significant extent, however, berberine as adjunctive therapy increased the lung alveolar free space when compared to berberine alone or untreated group (Supplementary Figure 5D) . We then assess the recruitment of immune cells in the lungs of these mice. In line with late onset in C57BL/6 mice, berberine as an adjunct significantly increased total cells harvest when compared to mice treated with antibiotics alone (Supplementary Figure 5E) . Similarly, T cells (Supplementary Figure 5F ), polymorphonuclear cells (Supplementary Figure 5G ) and recruited monocytes (Supplementary Figure 5H) were significantly increased in mice treated with berberine as an adjunct when compared to animals treated with antibiotics alone. This may explain increased total lung cells harvested. Berberine, alone had no effect on neutrophil influx to the lung suggesting that this compound modulates inflammation without perturbing these innate cell recruitment. In contrast to C57BL/6 model, berberine treatment combined with antibiotics significantly increased neutrophil recruitment to the lung when compared to animals treated with antibiotics alone (Supplementary Figure 5G) . Collectively, these results indicate that berberine as adjunctive therapy may offer enhanced protection against tuberculosis infection in an experimental model of progressive pulmonary TB. Our findings demonstrate that berberine as an adjunct to rifampicin/isoniazid against tuberculosis decreased lung pathology in an experimental murine model of TB. The pleiotropic actions of berberine are mainly associated with its immunomodulatory properties through inhibition of NF-kB, MAPK and inhibition of pro-inflammatory cytokine production (16) . We have also observed similar effects of berberine in Mtb-infected mouse macrophages in vitro. Intriguingly, berberine treatment pre-or post-Mtb infection increased the bactericidal activity of macrophages despite they released decreased levels of nitric oxide, IL-6, and IL-1a. Similar to murine macrophages, human macrophages also reduced mycobacterial growth following berberine treatment. The limitation is macrophages were not generated from CD16negative selected monocytes which may result in mixed M1 and M2 macrophages, however, markers of classical and alternative activation are not very clear in human macrophages. Increased ROS levels contribute to the bacterial killing, we confirmed that decreased bacterial growth in macrophages was independent of ROS. In contrast, berberine had no direct inhibitory effect on Mtb but modulates host responses to mediate antimycobacterial effects. Our findings are in line with the report showed enhanced macrophage antibacterial activity even though berberine inhibits mRNA expression of iNOS, COX-2, IL-1b, TNF and IL-6 in LPSstimulated inner medullary collecting duct-3 cells by reducing NF-kB activity (42) . In atherosclerosis, berberine treatment inhibits inflammation in mouse macrophages (J774A.1) by inducing autophagy through AMPK/mTOR pathway (43) and uncoupling protein 2 in mice (44) . Moreover, berberine inhibits the formation of foamy macrophages by enhancing LXRalpha-ABCA1dependent cholesterol efflux in macrophages (45) . Additionally, a berberine derivative is shown to induce lysosomal acidification through activation of transcription factor EB in methicillinresistant Staphylococcus aureus and enteroinvasive Escherichia coli infected BMDM (46) . Therefore, it is feasible that berberine treatment decreases the intracellular survival of Mtb in macrophages. Activation of macrophages by increased CD80 expression and increased frequencies of MHCII + BMDM or splenic macrophages in vivo can be context-specific to Mtb infection. It has been previously reported that berberine pretreatment did not change cell surface expression of CD80 and MHCII in naïve macrophages (47) or decreased CD80 expression in lipopolysaccharide (LPS) stimulated bone marrow-derived dendritic cells (18) . Increased macrophage activation and macrophage Mtb killing mechanisms, while decreased proinflammatory gene expression and NF-kB and JNK kinase activation shows that berberine has pleiotropic and contextspecific functions in macrophages. Augmenting macrophage activation and bacterial killing mechanisms while reducing inflammation could increase the immunomodulatory potential of berberine during TB disease. Moreover, berberine immunotherapy as an adjunct had a beneficial effect for the host by decreasing lung pathology in the treated C57BL/6 after 4 weeks of therapy. However, berberine alone or in combination did not affect lung mycobacterial burdens. Within 2 weeks Mtb disseminates from the lungs to other organs for example spleen and liver (48) . Considering this berberine may target dissemination to other organs during treatment. Similar to lungs, berberine had no effect on mycobacterial burdens in the spleen. Interestingly, we found that berberine showed stronger effects on macrophage activation and B lymphocyte numbers in the spleen. Increased B cell numbers in the spleen were also reported in the mouse leukemia model before (49) . It will be interesting to study whether berberine affects B-cell development in the bone marrow or reduces B-cell turnover. Overall, this study revealed that berberine treatment reduced deleterious lung pathological consequences during TB. Berberine also has anti-parasitic (50) , -viral (51), -fungal (52) and -helminth activity (53) . Previously, administration of berberine with isoniazid protects against liver injury caused by oxidative stress and inflammation in rats by suppressing NF-kB, iNOS, the proinflammatory cytokines and upregulating PPAR-g (54) . We found that berberine has an adjunctive effect on rifampicin/isoniazidinduced control of lung inflammation in Mtb-infected mice. The synergistic effects of berberine have also been reported with commonly used antibiotics against Methicillin-Resistant Streptococcus aureus (MRSA) (55) and fluconazole-resistant Candida albicans (56) . Berberine has been proven for its antibacterial activity against a broad spectrum of microbial pathogens (57) and exhibited sub-MICs on conventional antimicrobial agents such as ampicillin, azithromycin, cefazolin, and levofloxacin (58) . The primary antibacterial mechanism of berberine is due to inhibition of the cell division protein FtsZ (59) . Berberine has a synergistic effect with some common antibiotics especially with linezolid, cefoxitin, and erythromycin (60) . The direct microbicidal effect of berberine appears to inhibit biofilm formation (61) and synthesis of DNA (57) . In our study, we could not detect ROS levels in vivo due to the short half-life of ROS; however, in vitro BMDM showed that berberine does not show antioxidant properties during Mtb infection. Berberine increases the antibacterial properties of macrophages and we observed a similar trend in the susceptible Kramnik mouse model when the bacterial burdens were high in the lung. We ruled out the possibility of hepatotoxic effects of berberine by probing serum ALT and AST levels. The stronger effects of berberine were seen in the lung pathology in C57BL/6 mice. The decreased lung pathology was associated with fewer neutrophil recruitment both in the lungs and spleen. Additionally, berberine showed immunomodulatory properties in vivo by increased macrophage activation and B cell numbers. Overall, the data suggest that the effects of adjunctive berberine treatment are pleiotropic during Mtb infection. We then further validated our findings in a susceptible and highly inflammatory Kramnik (C3HeB/FeJ) mice, a highly relevant model, which recapitulates human lung lesions and a comprehensive model to study tuberculosis immunopathology (62) . Remarkably in these animals, berberine alone was able to significantly reduce lung mycobacterial burden, which might be attributed to higher susceptibility of this animal model in comparison to C57BL/6 mice. However, no adjunct effect on bacterial load was observed in mice treated with a combination of berberine and antibiotics; the latter was consistent with the C57BL/6 model. Moreover, rifampicin/isoniazid alone significantly increased lung alveolar air spaces compared to mice treated with berberine alone. However, mice treated with rifampicin/isoniazid in combination with berberine did not further increase lung alveolar spaces when compared to antibiotic only group. Furthermore, mice treated with rifampicin/isoniazid in combination with berberine showed increased lung cell numbers, T cells, polymorphonuclear cells and recruited monocytes in the lungs. These findings mirrored our observations with C57BL/6 mice when treated 3 weeks post Mtb infection except for the effect on neutrophils. This indicated that berberine had an adjunct but not additive or synergistic effect on lung inflammation in C57BL/6 mice but not susceptible Kramnik mice. The absence of the adjunctive effect of berberine in Kramnik mice points out that preventing neutrophilic inflammation is the main driver of anti-inflammatory effects of berberine in C57BL/6 mice. Previously, forward genetics analyses revealed that Kramnik mice have a susceptible allele of super susceptibility to tuberculosis (sst1) locus on mouse chromosome 1, unlike C57BL/6 counterparts which harbor the resistant allele (63) Sp140 gene was recently identified to confer resistance to C57BL/6 mouse and it is found to negatively regulate Type I IFN responses (64) . Type I IFNs are shown to drive pathological inflammation in tuberculosis especially in Kramnik mice through neutrophilia (35, 65) . In our experiments, we have seen that the early or late onset of adjunctive berberine treatment did not effect IFNb levels in C57BL/6 mice, hence Type-1 IFN dominated neutrophilia was probably not inhibited in Kramnik mice. Targeting Type I IFN network by neutralizing antibodies with berberine adjunctive therapy would be a future study to understand the extent of berberine immunomodulation and anti-inflammatory effects in adjuvant therapy in Kramnik mice. In summary, we report here that berberine as an adjunctive therapy decreased lung inflammation by targeting immune cell recruitment and reducing inflammatory cytokines. The lack of the development of granulomatous lung pathology with caseous necrosis resembling the human TB disease in the C57BL/6 model and Kramnik experiment further warrants studies starting treatment in much later time points in Kramnik mice or nonhuman primates (NHP) before testing in patients. Another important drawback of berberine adjunctive therapy can be attributed to its low absorption rates in the gut (66) . Therefore, future studies with hyperinflammatory clinical Mtb strains in Kramnik mouse and NHP models are warranted to consider berberine or its derivatives with increased oral bioavailability as a potential adjunct therapy to current first-line anti-TB drugs in the clinic. Data represented as mean ± SEM of four replicates and representative of two experiments, analysed by a two-tailed unpaired Student's t-test defining differences in all groups as significant *P ≤ 0.05; **P ≤ 0.01, ***P ≤ 0.001. Figure 2 | Immunomodulatory effects of berberine as an adjunctive therapy during Mtb infection in C57BL/6 mice (A) Water consumption was measured after every water change to estimate drug uptake per mouse per day. (B) Serum ALT and AST levels were measured 4 weeks post TB treatment to infer liver cytotoxicity and hepatoprotective effects of berberine. (C) MHCII expressing lung alveolar macrophages, interstitial macrophages and monocytederived DCs; spleen CD169 + macrophages, red pulp macrophages and monocytes after 4 weeks treatment in late-onset of berberine adjunctive therapy. The data is presented as the percentage of the parent population. (D) Activated caspase 3 flow cytometry as a marker of apoptosis. Data is shown as Caspase-3 + total live cells in the lungs and spleen of mice 4 weeks post TB treatment in the lateonset adjunctive berberine treatment. Data is shown representative of two experiments (n = 5 per group) and the line denotes mean value, analysed by Kruskal-Wallis test with Dunn's multiple comparisons correction (A, B) and one-way ANOVA with Tukey post-hoc test (C, D) defining differences in all groups as significant *P ≤ 0.05; **P ≤ 0.01. Asterisks without the line below show the significance compared to the untreated group. Supplementary Figure 3 | Effect of late-onset berberine adjunctive therapy on lung and spleen immune cells populations during Mtb infection in C57BL/6 mice. (A) Lung CXCR3 + CD4 and CD8 T cell frequencies, (B) lung alveolar macrophage (SiglecF + CD11c + CD64 + ), (C) lung interstitial macrophages (CD64 + CD11b + CD11c -SiglecF -), (D) lung monocyte-derived DC counts (CD64 + CD11b + CD11c + ), (E) spleen CXCR3 + CD4 and CD8 T cell frequencies, (F) spleen CD169 + macrophage (CD11b + CD169 + CD11c -) (G) spleen red pulp macrophage (F4/80 + CD11b low CD169 -CD11c -), (H) spleen CD8 DC counts (CD11c + MHCII + CD8 + CD11b -). Data is shown representative of two experiments (n = 5 per group) and the line denotes mean value, analysed by one-way ANOVA with Tukey post-hoc test (A-C, E-F) and Kruskal-Wallis test with Dunn's multiple comparisons correction (D, G) defining differences in all groups as significant *P ≤ 0.05; **P ≤ 0.01; ***P ≤ 0.001. Asterisks without the line below show the significance compared to the untreated group. (G) Total RNA was extracted from lung tissue and qPCR was performed to measure Ifngr1 and Csf2ra levels. Hprt housekeeping gene was used for normalization and fold change differences were calculated by using untreated as the reference sample. Data is shown representative of two experiments (n = 5 per group) and the line denotes mean value, analysed by one-way ANOVA with Tukey post-hoc test (A-F) and Kruskal-Wallis test with Dunn's multiple comparisons correction (G) defining differences in all groups as significant *P ≤ 0.05; **P ≤ 0.01; ***P ≤ 0.001. Asterisks without the line below show the significance compared to the untreated group. polymorphonuclear cells (CD11b + Ly6G + Ly6C + ) and (H) inflammatory monocytes (CD11b + Ly6G -Ly6C + ) in the lungs at 4 weeks post-treatment. Data represented as mean ± SEM of n = 3-4 mice per group from one experiment, analysed by one-way ANOVA with Tukey post-hoc test defining differences in all groups as significant *P ≤ 0.05; **P ≤ 0.01; ***P ≤ 0.001. Global Tuberculosis Programme The Global Burden of Latent Tuberculosis Infection: A Re-Estimation Using Mathematical Modelling Revisiting the Timetable of Tuberculosis Latent Tuberculosis Infection -Revisiting and Revising Concepts Estimating the Future Burden of Multidrug-Resistant and Extensively Drug-Resistant Tuberculosis in India, the Philippines, Russia, and South Africa: A Mathematical Modelling Study Host-Directed Drug Therapy for Tuberculosis Du Plessis N. Therapeutic Host-Directed Strategies to Improve Outcome in Tuberculosis Pathology and Immune Reactivity: Understanding Multidimensionality in Pulmonary Tuberculosis The Anti-Inflammatory Potential of Berberine In Vitro and In Vivo Extracts: Antimicrobial Properties and Interaction With Ciprofloxacin Berberine Differentially Modulates the Activities of ERK, P38 MAPK, and JNK to Suppress Th17 and Th1 T Cell Differentiation in Type 1 Diabetic Mice Regulatory Effects of Berberine on Micrornome in Cancer and Other Conditions Current Knowledge and Pharmacological Profile of Berberine: An Update Berberine: A Potential Phytochemical With Multispectrum Therapeutic Activities Anti-Inflammatory and Immune-Modulatory Impacts of Berberine on Activation of Autoreactive T Cells in Autoimmune Inflammation Berberine Ameliorates Experimental Autoimmune Neuritis by Suppressing Both Cellular and Humoral Immunity Berberine Induces Dendritic Cell Apoptosis and has Therapeutic Potential for Rheumatoid Arthritis Berberine Promotes Recovery of Colitis and Inhibits Inflammatory Responses in Colonic Macrophages and Epithelial Cells in DSS-Treated Mice Berberine Ameliorates TNBS Induced Colitis by Inhibiting Inflammatory Responses and Th1/Th17 Differentiation Evaluation of Minor Groove Binders (MGBs) as Novel Anti-Mycobacterial Agents and the Effect of Using non-Ionic Surfactant Vesicles as a Delivery System to Improve Their Efficacy Differential Targeting of C-Maf, Bach-1, and Elmo-1 by microRNA-143 and microRNA-365 Promotes the Intracellular Growth of Mycobacterium Tuberculosis in Alternatively IL-4/IL-13 Activated Macrophages Statin Therapy Reduces the Mycobacterium Tuberculosis Burden in Human Macrophages and in Mice by Enhancing Autophagy and Phagosome Maturation Chemopreventive Effects of Berberine on Intestinal Tumor Development in Apcmin/+ Mice Protein Kinase C-Delta (Pkcd), a Marker of Inflammation and Tuberculosis Disease Progression in Humans, is Important for Optimal Macrophage Killing Effector Functions and Survival in Mice Omega-3 Fatty Acid and Iron Supplementation Alone, But Not in Combination, Lower Inflammation and Anemia of Infection in Mycobacterium Tuberculosis-Infected Mice Proteomic Investigation Into the Action Mechanism of Berberine Against Streptococcus Pyogenes The Effects of Berberine on Reactive Oxygen Species Production in Human Neutrophils and in Cell-Free Assays Berberine Exhibits Antioxidative Effects and Reduces Apoptosis of the Vaginal Epithelium in Bacterial Vaginosis Men Have a Stronger Monocyte-Derived Cytokine Production Response Upon Stimulation With the Gram-Negative Stimulus Lipopolysaccharide Than Women: A Pooled Analysis Including 15 Study Populations Acute Toxicity of Berberine and its Correlation With the Blood Concentration in Mice The Metabolism of Berberine and Its Contribution to the Pharmacological Effects Nitric Oxide Prevents a Pathogen-Permissive Granulocytic Inflammation During Tuberculosis Type I IFN Exacerbates Disease in Tuberculosis-Susceptible Mice by Inducing Neutrophil-Mediated Lung Inflammation and NETosis CXCL10 is Overexpressed in Active Tuberculosis Patients Compared to M. Tuberculosis-Exposed Household Contacts Virulence-Dependent Alterations in the Kinetics of Immune Cells During Pulmonary Infection by Mycobacterium Tuberculosis Initiation of the Adaptive Immune Response to Mycobacterium Tuberculosis Depends on Antigen Production in the Local Lymph Node, Not the Lungs CXCR3 in T Cell Function Defective Positioning in Granulomas But Not Lung-Homing Limits CD4 T-Cell Interactions With Mycobacterium Tuberculosis-Infected Macrophages in Rhesus Macaques Berberine Ameliorates Lipopolysaccharide−Induced Inflammatory Responses in Mouse Inner Medullary Collecting Duct−3 Cells by Downregulation of NF−kb Pathway Berberine Alleviates Ox-LDL Induced Inflammatory Factors by Up-Regulation of Berberine as an Adjunct to TB Therapy Autophagy via AMPK/mTOR Signaling Pathway Activation of AMP-Activated Protein Kinase Is Required for Berberine-Induced Reduction of Atherosclerosis in Mice: The Role of Uncoupling Protein 2 Anti-Atherogenic Effect of Berberine on Lxra-ABCA1-Dependent Cholesterol Efflux in Macrophages Novel Berberine Derivative, Enhances Lysosomal and Bactericidal Properties via TGF-b-Activated Kinase 1-Dependent Activation of the Transcription Factor EB Induction of Interleukin-12 Production in Mouse Macrophages by Berberine, a Benzodioxoloquinolizine Alkaloid, Deviates CD4+ T Cells From a Th2 to a Th1 Response Dissemination of Mycobacterium Tuberculosis is Influenced by Host Factors and Precedes the Initiation of T-Cell Immunity Berberine Chloride Mediates Its Anti-Leishmanial Activity via Differential Regulation of the Mitogen Activated Protein Kinase Pathway in Macrophages Antiviral Activity of Berberine Antileishmanial, and Cytotoxicity Activities of Various Extracts of Berberis Vulgaris (Berberidaceae) and Its Active Principle Berberine Role of Berberine in Ameliorating Schistosoma Mansoni-Induced Hepatic Injury in Mice Berberine Attenuates Isoniazid-Induced Hepatotoxicity by Modulating Peroxisome Proliferator-Activated Receptor ?, Oxidative Stress and Inflammation Potent In Vitro Synergism of Fusidic Acid (FA) and Berberine Chloride (BBR) Against Clinical Isolates of Methicillin-Resistant Staphylococcus Aureus (MRSA) Fluconazole Assists Berberine To Kill Fluconazole-Resistant Candida Albicans Antibacterial Activity and Mechanism of Berberine Against Streptococcus Agalactiae Antibacterial and Synergy of Berberines With Antibacterial Agents Against Clinical Multi-Drug Resistant Isolates of Methicillin-Resistant Staphylococcus Aureus (MRSA) Genetic Evidence for Inhibition of Bacterial Division Protein FtsZ by Berberine Berberine Enhances the Antibacterial Activity of Selected Antibiotics Against Coagulase-Negative Staphylococcus Strains In Vitro Role of Berberine in the Treatment of Methicillin-Resistant Staphylococcus Aureus Infections Mouse Models of Human TB Pathology: Roles in the Analysis of Necrosis and the Development of Host-Directed Therapies Genetic Control of Resistance to Experimental Infection With Virulent Mycobacterium Tuberculosis Role of the Transcriptional Regulator SP140 in Resistance to Bacterial Infections via Repression of Type I Interferons Type I Interferon-Driven Susceptibility to Mycobacterium Tuberculosis is Mediated by IL-1ra Approaches to Improve the Oral Bioavailability and Effects of Novel Anticancer Drugs Berberine and Betulinic Acid 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.