In order to analyse the expression of platelet APP, Western blot analysis was performed. Five µg acidic platelet extracts (neutralized with PBS pH 9.5) were denatured (10 min 70 °C) and loaded onto 4–12 % Bis–Tris polyacrylamide gel (Invitrogen Life Tech, Darmstadt, Germany) and separated by electrophoresis for 60 min at 200 V. Consecutively, samples were electrotransferred to nylon PVDF Immobilon-PSQ membranes (Millipore, Vienna, Austria) at 30 V for 90 min with 20 % methanol transfer buffer (Invitrogen). Protein detection was performed with Western Breeze Chemiluminescent System (Invitrogen). Thus, membranes were blocked for 30 min with blocking solution at RT on the shaker, then incubated with the primary antibody (Anti-Amyloid beta precursor protein antibody [Y188], abcam, Cambridge, UK, ab32136) overnight at 4 °C. Following, blots were washed and incubated with anti-rabbit antibodies for 30 min at RT, again washed and incubated with CDP-Star chemiluminescent substrate solution (Invitrogen). Imaging was performed with a cooled CCD camera SearchLight camera. In order to quantify the protein amounts in each lane and ensure that there has been an even transfer from gel to membrane, a loading control with αMouse IgG was performed.
Pvdf immobilon psq membranes
Manufactured by Merck Group
PVDF Immobilon-PSQ membranes are a type of laboratory equipment used for protein immobilization and detection. They are made from polyvinylidene fluoride (PVDF), a chemically and mechanically stable material. The membranes provide a high-binding capacity for proteins and facilitate effective protein transfer and detection in various analytical techniques.
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2 protocols using pvdf immobilon psq membranes
1
Western Blot Analysis of Platelet APP
2
Quantitative Western Blot Analysis of Tau Phosphorylation
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Western blot analysis was performed for tau and phospho-tau396 as described by us in detail [35] . Platelet extracts (80 µg per lane total protein) were denatured (70 °C for 10 min) and loaded onto 4-12% Bis-Tris polyacrylamide gels (Invitrogen Life Tech, Darmstadt, Germany) and separated by electrophoresis for 60 min at 200 V. Consecutively, samples were electrotransferred to nylon PVDF Immobilon-PSQ membranes (Millipore, Vienna, Austria) at 30 V for 90 min with 20% methanol transfer buffer (Invitrogen). Protein detection was performed with Western Breeze Chemiluminescent System (Invitrogen). Thus, membranes were blocked for 30 min with blocking solution at RT on the shaker, then incubated with the primary antibody tau-5 (Thermo AHB0042, 1:1000) or phospho-tau-396 (pTau396, BioLegend 807401, 1:10,000) or HT7 antibody (1:500, Thermo MN1000) overnight at 4 °C. Subsequently, blots were washed and incubated with anti-mouse (tau-5, HT7) or anti-rabbit (pTau396) antibodies for 30 min at room temperature (RT), again washed and incubated with CDP-Star chemiluminescent substrate solution (Invitrogen). Imaging was performed with a cooled CCD camera (SearchLight, ThermoScientific, Austria).
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