Fig 1: Brucella melitensis infectious foci in liver. At 3 weeks post-infection, pathogenic B. melitensis-infected cells developed multiple granulomas (A,D; H&E staining). Immunohistochemical analysis of bacterial foci was performed using biotinylated primary antibodies (1.0 μg/ml, #TC-7011, Tetracore Inc.), endogenous biotin blocking, and streptavidin-conjugated to horseradish peroxidase (St∼HRP) using 3,3′-diaminobenzidine (DAB) as the final chromogen (B,E; brown precipitate). Staining of normal liver of healthy non-infected mice produced no signal (not shown). Staining of liver tissue at 3 weeks post-infection using the same protocol but substituting biotinylated anti-Brucella antibodies with normal serum produced no signal (F). Immunohistochemical analysis of macrophage lineage cells using antibodies to IBA-1 (dilution 1:500, #019-19741, Wako Chemicals USA, Inc.) followed by HRP rabbit polymer conjugate (#87-9263, Invitrogen Life Technologies) revealed positive staining of cells at the granuloma periphery (C). Residential macrophages – Kupffer cells were also positive for IBA-1 staining (C). Although Brucella was found in the granuloma core, these core cells were basically negative for IBA-1 staining (compare B versus C). Sections were counterstained with hematoxylin (B,C,E,F). Scale bars: 20 μm (A,B,C,E), 50 μm (F) and 200 μm (D).
Fig 2: Coexpression of Iba1 and CD68. Human brain biopsy samples from the superior frontal gyrus after TBI were stained with the primary antibodies: rabbit anti-Iba1 (1:1000, Wako, Cat No. 019-19741) and mouse anti-CD68 (1:500, Invitrogen, Cat No. 14-0688-82) followed by rabbit anti-Alexa Fluor 488 and mouse anti-Alexa Fluor 594, respectively. Iba1+ microglia co-expressed with CD68 can be observed in various activated states, ranging from the most ramified state (A–C) through increasing states of activation (D–F and G–I) to the most amoeboid morphology (J–L) in the non-contused brain tissue. In contrast, predominantly amoeboid microglia stained with Iba1 and CD68 were observed in contused brain tissue (M–O). Clotted blood from a neurosurgical (brain) operative field was used to identify peripherally-derived macrophages that strongly stained for both Iba1 and CD68 (P–R). Scale bars are 25 μm. Unpublished data.
Fig 3: Coexpression of Iba1 and HLA-DR. Human brain biopsy samples from the superior frontal gyrus after TBI were stained with the primary antibodies: rabbit anti-Iba1 (1:1000, Wako, Cat No. 019-19741) and mouse anti-HLA-DR (1:500, Invitrogen, Cat No. MA5-11966) followed by rabbit anti-Alexa Fluor 488 and mouse anti-Alexa Fluor 594, respectively. Limited HLA-DR expression was observed in Iba1+ microglia with a ramified morphology (A–C), but strong HLA-DR expression in Iba1+ microglia in the activated state (D–L) in the non-contused brain tissue. Predominantly amoeboid microglia stained with Iba1 and HLA-DR were observed in contused brain tissue (M–O). Clotted blood from a neurosurgical (brain) operative field was used to identify a few peripherally-derived macrophages that strongly stained for both Iba1 and HLA-DR (P–R). Scale bars are 25 μm. Unpublished data.
Fig 4: Coexpression of Iba1 and galectin-3. Human brain biopsy samples from the superior frontal gyrus after TBI were stained with the primary antibodies: rabbit anti-Iba1 (1:1000, Wako, Cat No. 019-19741) and goat anti-galectin-3 (1:500, BioLegend, Cat No. 126701) followed by rabbit anti-Alexa Fluor 488 and goat anti-Alexa Fluor 594, respectively. Limited galectin-3 expression was observed in Iba1+ microglia with a ramified morphology (A–C), but there was a strong galectin-3 expression in Iba1+ microglia in the activated state (D–L) in the non-contused brain tissue. Predominantly amoeboid microglia stained with Iba1 and galectin-3 were observed in contused brain tissue (M–O). Clotted blood from a neurosurgical (brain) operative field was used to identify peripherally-derived macrophages that strongly stained for both Iba1 and galectin-3 (P–R). Scale bars are 25 μm. Unpublished data.
Fig 5: Concerns with CD11b (Clone OX42) immunostaining for microglia in human tissue. Human brain biopsy samples from the superior frontal gyrus after TBI were stained with the primary antibodies: mouse anti-rat OX42 (1:100, Bio_Rad, Cat. No. MCA275R) (A–I), or mouse anti-human CD11b (1:400, Novus Biologicals, Cat. No. MAB16991) (J–R); then with rabbit anti-Iba1 (1:1000, Wako, Cat No. 019-19741) (J), or rabbit anti-P2Y12 (1:200, AnaSpec, ANA55043A) (M), or rabbit anti-GFAP (1:1000, Dako, Cat No. Z0334) (P), followed by rabbit anti-Alexa Fluor 488 and mouse anti-Alexa Fluor 594 or tyramide amplification with ExtrAvidin FITC for the mouse anti-human CD11b (K,N,Q). Limited anti-rat OX42 expression was observed in Iba1+ microglia with a ramified state morphology (A–C), but some anti-rat OX42 expression in Iba1+ microglia in the more activated state (D–F) or contused brain tissue (G–I). Anti-human CD11b staining was absent in Iba1 (J–L) and P2Y12 (M–O) immunopositive cells, but coexpressed with the GFAP astrocytic marker (P–R). Scale bars are 25 μm. Unpublished data.
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