Therefore, the following monoclonal mouse antibodies were applied: IC16 ([30], raised against Aβ1–16; 1:2000), AT8; Thermofisher, Bonn, Germany; 1:1000), MC-1 ([31]; 1:50), CP13 ([32]; 1:500), β-actin (Sigma; 1:5000) IDH inhibitor and β3-tubulin (Millipore, Schwalbach, Germany; 1:2000). In addition, we applied rabbit antisera directed against human tau (Dakocytomation, Hamburg; 1:1000), anti-pS199

(BioSource, 1: 500), anti-pS422 ( [33]; 1:500) and anti-glial fibrillary acidic protein (GFAP; Synaptic Systems, Göttingen, Germany; 1:4000). Following overnight incubation, membranes were washed in TBST two times for 10 min. Secondary anti-rabbit or anti-mouse conjugates of horseradish peroxidase (Dianova, Hamburg, Germany) were applied for 2 h. Membranes were Ibrutinib molecular weight rinsed two times in TBST, and blots were developed using enhanced chemiluminescence,

followed by scanning of X-ray films (Hyperfilm EC, Amersham Biosciences, Freiburg, Germany). For quantification of relative protein amounts, protein levels were determined via ImageJ software (1.46r, National Institutes of Health, USA) by measuring band intensity in densitometric analyses normalized to β-actin or β3-tubulin levels, respectively. Sections containing hippocampi from several animals of all animal groups were pre-treated for 10 min with concentrated formic acid (98–100%, Merck) and routinely used for sensitive 4G8 staining Glycogen branching enzyme (see below). These and all other free-floating sections were extensively rinsed with TBS followed by blocking of non-specific binding sites for subsequently applied immunoreagents with 5% normal donkey serum in TBS containing

0.3% Triton X-100 (NDS-TBS-T). For the analysis of cholinergic markers, forebrain sections were either applied to affinity-purified goat-anti-ChAT (AB144P, Millipore; 1:50 in NDS-TBS-T) or rabbit-anti-p75 (G323A, Promega, Mannheim, Germany; 1:100 in NDS-TBS-T), followed by several rinses with TBS and incubation for 1 h with Cy3-conjugated donkey antibodies recognizing goat or rabbit (both from Dianova, 20 μg/ml TBS containing 2% bovine serum albumin = TBS-BSA), respectively. Markers applied for double labelling of β-amyloidosis and tauopathy in hippocampal sections are summarized in Table 1. For triple fluorescence labelling of Aβ deposits, astrocytes and microglia, sections were first incubated overnight in a mixture of biotinylated mouse antibody 4G8 ([34]; Covance, 1:500 in NDS-TBS-T), Cy3-conjugated-mouse-anti-GFAP IgG (Sigma; 1:250) and rabbit-anti-ionized calcium binding adapter molecule 1 (Iba; Wako, Neuss, Germany; 1:200). Following several rinses with TBS, immunoreactivities were visualized by incubating sections for 1 h in a mixture of Cy3-streptavidin and Cy5-tagged donkey-anti-rabbit IgG (both at 20 μg/ml TBS-BSA and from Dianova).