Primary antibodies were obtained

Primary antibodies were obtained selleck screening library from Santa Cruz (Santa Cruz, CA, US: COX-2), Millipore (activated caspase-3: Temecula, CA, USA), Peprotech (London, UK: IL-1β), Abcam (Cambridge UK: IBA-1), Invitrogen (NY, USA: IRF3), Promega (TUNEL, Southampton, UK). Biotinylated secondary antibodies, normal sera, and avidin–biotin

complex were from Vector Laboratories (Peterborough, UK). Avidin-horseradish peroxidase was obtained from DAKO (Cambridge, UK). Immunohistochemistry for all antigens was carried out by the Avidin–Biotin-Complex (ABC) method with minor modifications, depending on the antibody used, and has been described in detail in previous publications (Cunningham et al., 2005a). Cell counting was performed for IL-1b, TUNEL and IBA-1. For IL-1b and TUNEL, positive cells were identified and counted throughout the hippocampus and thalamus of all animal groups. For IBA-1, a 0.62 × 0.47 mm section of the centre of the dorsal hippocampus, (containing the CA1 pyramidal layer and stratum oriens and radiatum, but not the dentate gyrus granule layer) was photographed and used for microglial counts in NBH and ME7 animals treated with poly I:C. Positively stained cells were identified and counted using the

analyse particles function in Image J software (rsbweb.nih.gov). Animals challenged intraperitoneally with poly I:C (12 mg/kg) or saline were terminally anaesthetised at 4 and 6 h after poly I:C and then transcardially perfused with heparinised saline. Brains were rapidly removed, hippocampi and hypothalami dissected out, placed in eppendorf tubes, snap frozen on liquid nitrogen and stored at −80 °C until further check details use. Total RNA was extracted from

brain samples using Qiagen RNeasy® Plus mini kits (Qiagen, Crawley, UK) according to the manufacturer’s instructions. Contaminating genomic DNA was eliminated via degradation during extraction using the Qiagen selleck kinase inhibitor RNase-free DNase1 enzyme. Approximate yields were determined by spectrophotometry at 260 and 280 nm. RNA was stored at −80 °C until cDNA synthesis and PCR assay. All equipment and reagents were supplied by Applied Biosystems (Warrington, UK) unless otherwise stated. Assays for IFN-α, IFN-β, IL-10, IP-10, IRF-7, TLR3, RIG-I, PKR, OAS, Mx1, Bax, Fas, IFNγ, and all T cell transcripts were designed using the published sequences for these genes, applied to Primes Express™ software. Where possible, probes were designed to cross an intron such that they were cDNA specific. All primer pairs were checked for specificity by standard reverse transcription (RT)-PCR followed by gel electrophoresis. Each primer pair produced a discrete band of expected amplicon size. We subsequently learned that C57 mice have a non-functional Mx1 protein due to a deletion in exons 9 though 11 in the Mx1 gene ( Staeheli and Sutcliffe, 1988 and Jin et al., 1998). Our primers for this gene were designed such that they are specific to an unaffected region of the gene and span the boundary of exons 2 and 3.

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