Collagen hydrogels were prepared with either different tau proteins in a final concentration of 10 ng/μL or empty PBS load as described above. Three collagen hydrogels were placed on small rectangular pieces of Parafilm, which were then placed face down in 500 μL of sterile culture medium in 4-well plates (Nunc, Thermo Fisher Scientific, Vienna, Austria, 144444). Medium was collected in a time-dependent manner until 8 weeks. The total amount of tau protein released into the medium was measured using the automated Lumipulse Technology (Fujirebio, Ghent, Belgium, G600II).
Lumipulse technology
Manufactured by Fujirebio
Sourced in Belgium
Lumipulse technology is a chemiluminescent immunoassay platform developed by Fujirebio. It utilizes luminescent chemical reactions to measure the presence and concentration of specific analytes in biological samples. The core function of Lumipulse technology is to provide quantitative analytical results for various clinical and diagnostic applications.
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6 protocols using lumipulse technology
1
Collagen Hydrogel Tau Protein Release
2
Automated Analysis of Tau and Aβ42
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Total tau and Aβ42) and (40) levels were measured using automated Lumipulse technology (Fujirebio G600II); In brief, the Lumipulse G600II is started and prepared with all sufficient reagents (wash solution, substrate, tips, dilution, a.d.) and the single cartridges for each marker are loaded to the system. The G600II is an automated robotor system and designed to perform all steps itself. Samples (500 µl) are pipetted into Hitachi cups, and added to the racks, the system is started and values can be read after 35 min. Standard curves and quality controls verify the correct values. The system works on basis of an immunologcal reaction and is a 2-step chemicluminescence assay.
3
Biomarker Analysis of Cerebrospinal Fluid
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The CSF samples were analyzed at the Clinical Neurochemistry Laboratory, Sahlgrenska University Hospital, Mölndal, Sweden. CSF concentrations of Aβ40, Aβ42, total tau (T-tau) and phosphorylated tau (P-tau) were measured with Lumipulse technology (Fujirebio, Ghent, Belgium), as previously described [34 (link)]. CSF neurofilament light (NfL) concentration was measured using an in-house enzyme-linked immunosorbent assay as previously described [35 (link)]. S100B was analyzed with a Sangtec 100 ELISA kit (Diasorim, MN, USA). All biomarker measurements were performed using the same batch of reagents by board-certified laboratory technicians blinded to the clinical information. Lumbar and ventricular samples from each patient were run on the same plate to avoid plate-to-plate variance.
4
Cerebrospinal Fluid Biomarker Analysis
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Eight ml of ventricular CSF was collected during the surgical intervention, immediately after shunt insertion and a discard of the first 2 ml. All CSF analyses were performed at the Neurochemistry Laboratory at Sahlgrenska University Hospital, by board-certified laboratory technicians who were blinded to clinical data. Aβ-related biomarkers (Aβ40, Aβ42, sAPPα and sAPPβ) and MCP1 were analyzed by electrochemiluminescence assays (Meso Scale Discovery, Rockville, MD, USA). Validated in-house ELISA methodology was used to analyze NfL [19 (link)), neurogranin [15 (link)), GAP43 [20 (link)) and GFAP [21 (link)), whereas CSF levels of T-tau, and P-tau were measured using commercially available Lumipulse technology (Fujirebio, Ghent, Belgium), as previously described [22 (link)]. YKL-40 was measured using Human Chitinase 3-like 1 Quantikine ELISA Kit (R&D Systems, Minneapolis, MN) [22 (link)]. All concentrations are given in ng/L. All samples were analyzed in one round of experiments using one batch of reagents by board-certified laboratory technicians who were blinded to clinical data. Intra-assay coefficients of variation, monitored using internal quality control samples in the beginning and end of each run, were below 10%.
5
Biomarker Quantification in CSF and Plasma
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In CSF, T‐tau was measured using the Lumipulse technology (Fujirebio), while NfL was measured using an in‐house enzyme‐linked immunosorbent assay (ELISA) method [31 (link)]. NfL and T‐tau measurements in plasma were performed using the NF‐Light and Tau 2.0 kits on a Simoa HD‐X Analyzer (Quanterix) according to the manufacturer's instructions.
6
Quantification of Platelet Tau Proteins
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Platelet tau was characterized using our novel WAN-GEL (Western Blot-native Agarose gel elution) model developed by us recently (Humpel, 2022 submitted) . Native Western Blots were performed as described above but directly after the gel run, different molecular weight bands were dissected with a scalpel with a size between 80 and 0 kDa related to the color molecular weight marker. For the elution, 2.5 mL sample vials (PE, 14 mm, Roth 5863.1) were used and 1 mL 4% agarose was pipetted at the bottom of the tubes and cooled. Then, the cut Western Blot bands were carefully placed on top of the hardened agarose. Next 1 mL 1% handwarm agarose was pipetted onto the extracted bands and cooled to harden. In the next step, the bottom of the vial was cut, and the tube closed with a Millicell culture insert (3 µm, 12 mm, PITP01250, Merck). Next 1 mL of a MES/histidine puffer was carefully pipetted into the tube using a syringe and 10 µL bromphenobuffer was pipetted to follow up the elution. These tubes were placed into the agarose gel chamber and proteins eluted for 20-60 min to the cathode. After the run, the buffer with the eluted proteins was collected and analyzed by Lumipulse assay or mass spectometry. Total tau levels were measured using automated Lumipulse technology (Fujirebio G600II); see https://www.fujirebio.com/en/productssolutions/lumipulse-g600ii.
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