{"id":36824,"date":"2020-11-26T17:42:00","date_gmt":"2020-11-26T16:42:00","guid":{"rendered":"https:\/\/supazena.ovh\/c\/etap\/?post_type=ressource&#038;p=36642"},"modified":"2026-04-15T22:48:58","modified_gmt":"2026-04-15T20:48:58","slug":"tau-oligomers-a-new-tool-for-drug-discovery-in-ad","status":"publish","type":"ressource","link":"https:\/\/www.etap-lab.com\/en\/ressource\/tau-oligomers-a-new-tool-for-drug-discovery-in-ad\/","title":{"rendered":"Tau oligomers: a new tool for drug discovery in AD"},"content":{"rendered":"\n<p>One common pathological hallmark of neurodegenerative disease (ND) is the aggregation and accumulation of misfolding proteins, resulting in neuronal dysfunction and brain damage. A growing body of literature suggests that amyloid oligomers (including tau) are the root cause of ND.&nbsp; Significant investment has been made in drug development. However, no curative molecule is currently available on the market. This may be due to several factors \u2013 most notably to flawed preclinical research in which the use and outcome of animals models is crucial to bridging the translational gap to the clinic. The selection of a predictive preclinical model is therefore pivotal to addressing the clinical question. We report a newly-developed in vitro AD model, induced by the highly reproducible human tau oligomer (TauO) preparations for drug screening. This model allows testing for neuroprotective compounds and\/or oligomer-specific antibodies. Compound efficacy can be assessed before, concomitantly or after a TauO challenge in rodent primary cortical neuron cultures.<\/p>\n\n\n\n<hr class=\"wp-block-separator has-alpha-channel-opacity\"\/>\n\n\n\n<p><strong>Contents<\/strong><\/p>\n\n\n\n<ol class=\"wp-block-list\">\n<li>Characterization of TauO preparation<\/li>\n\n\n\n<li>Neurotoxicity of TauO preparation<\/li>\n\n\n\n<li>TauO induce neurotoxicity in a dose-dependent manner<\/li>\n<\/ol>\n\n\n\n<hr class=\"wp-block-separator has-alpha-channel-opacity\"\/>\n\n\n\n<h2 class=\"wp-block-heading\">1. Characterization of TauO preparation<\/h2>\n\n\n\n<p>ETAP-Lab has developed a method of producing stable misfolded TauO from recombinant full-length human tau protein (2N4R, 441 aa) without chemical modification or helper proteins.&nbsp;This preparation contains a mixture of trimers and low-molecular-weight oligomers, as well as remaining monomeric forms of the protein (Fig. 1).<\/p>\n\n\n\n<figure class=\"wp-block-image aligncenter\"><img decoding=\"async\" src=\"https:\/\/www.etap-lab.com\/wp-content\/uploads\/2020\/12\/Tau-SDS-page-2.png\" alt=\"\" class=\"wp-image-12289\"\/><\/figure>\n\n\n\n<p><strong>Fig.1: Characterization of TauO preparation by SDS-PAGE\/Coomassie staining:&nbsp;<\/strong><em>SDS-page gel profile, revealed by Coomassie blue staining, demonstrating that the produced oligomers are a mixture of trimers and low-molecular-weight oligomers.<\/em><\/p>\n\n\n\n<h2 class=\"wp-block-heading\">2. Neurotoxicity of TauO preparation<\/h2>\n\n\n\n<p>TauO-induced neurotoxicity was evaluated in primary rat cortical neurons. Incubation of cortical neurons with TauO decreases cell viability quite significantly (*; p&lt;0.0001), while neuron incubation with the same concentration of monomers showed no neurotoxic effect (Fig. 2). Moreover, neuron treatment with Brain Derived Neurotrophic Factor (BDNF) significantly reversed TauO-induced neurotoxicity (#; p&lt;0.0001).<\/p>\n\n\n\n<figure class=\"wp-block-image aligncenter\"><img decoding=\"async\" src=\"https:\/\/www.etap-lab.com\/wp-content\/uploads\/2020\/12\/Cortical-neurons-Tau-monomers-oligomers-BDNF-2.png\" alt=\"\" class=\"wp-image-12286\"\/><\/figure>\n\n\n\n<p><strong>Fig.2: <\/strong><strong>Neuron incubation with Tau monomers, TauO and TauO+BDNF:&nbsp;<\/strong><em>Incubation of neurons with TauO quite significantly decreases cell viability, while monomers showed no neurotoxic effect. TauO-induced neurotoxicity is reduced by BDNF, used as a positive control. Data are expressed as percent of vehicle (set at 100%) and represent the mean\u2009\u00b1\u2009SD (n=12, N=3). * P&lt;0.0001 vs. vehicle-treated cells, # P&lt;0.0001 vs. TauO-treated cells (Scheffe\u2019s test)<\/em><\/p>\n\n\n\n<h2 class=\"wp-block-heading\">3. Dose-dependant neurotoxicity induced by TauO preparation <\/h2>\n\n\n\n<p>Primary cortical neurons, challenged with TauO over the concentration range of 0.5 to 10 \u03bcM, showed clear and biphasic dose-dependent neurotoxicity, with a clear cut-off around 9 \u00b5M (Fig. 3).<\/p>\n\n\n\n<figure class=\"wp-block-image aligncenter\"><img decoding=\"async\" src=\"https:\/\/www.etap-lab.com\/wp-content\/uploads\/2020\/12\/Cortical-neurons-Tau-oligomers-dose-response-2.png\" alt=\"\" class=\"wp-image-12288\"\/><\/figure>\n\n\n\n<p><strong>Fig.3: <\/strong><strong>TauO induce dose-dependent neurotoxicity in primary cortical neurons: <\/strong><em>Neuron incubation with increasing doses of TauO showed dose-dependent neurotoxicity. Data are expressed as percent of vehicle (set at 100%) and represent the mean\u2009\u00b1\u2009SD (n=12, N=3). * P&lt;0.0001 vs. vehicle-treated cells (Scheffe\u2019s test).<\/em><\/p>\n\n\n\n<p>Primary cortical neurons were challenged with 4 independent batches of TauO to evaluate the reproducibility of the pharmacological assay. Results of cell viability showed very low batch-to-batch variabilities (Fig. 4).<\/p>\n\n\n\n<figure class=\"wp-block-image aligncenter\"><img decoding=\"async\" src=\"https:\/\/www.etap-lab.com\/wp-content\/uploads\/2020\/12\/Cortical-neurons-Tau-oligomers-Batch-reproduicibility-2.png\" alt=\"\" class=\"wp-image-12287\"\/><\/figure>\n\n\n\n<p><strong>Fig.4: Alzheimer\u2019s disease model reproducibility<\/strong><\/p>\n\n\n\n<p><em>Neuron incubation with different TauO batches induced a highly reproducible and significant neurotoxicity. Data are expressed as percent of vehicle (set at 100%) and represent the mean\u2009\u00b1\u2009SD (n=3, N=1). * P&lt;0.0001 vs. vehicle-treated cells (Scheffe\u2019s test)<\/em><\/p>\n\n\n\n<div class=\"wp-block-buttons is-content-justification-center is-layout-flex wp-container-core-buttons-is-layout-a89b3969 wp-block-buttons-is-layout-flex\">\n<div class=\"wp-block-button\"><a class=\"wp-block-button__link wp-element-button\" href=\"https:\/\/www.etap-lab.com\/contact-us\/\">Contact us<\/a><\/div>\n<\/div>\n\n\n\n<p>More information about our neurodegenerative diseases models<\/p>\n\n\n\n<p><a href=\"https:\/\/www.etap-lab.com\/neurodegenerative-diseases\">https:\/\/www.etap-lab.com\/neurodegenerative-diseases<\/a><\/p>\n\n\n\n<p><strong>&nbsp;Complementary articles about tau and Tau oligomers<\/strong><\/p>\n\n\n\n<figure class=\"wp-block-embed is-type-wp-embed is-provider-etap-blog wp-block-embed-etap-blog\"><div class=\"wp-block-embed__wrapper\">\nhttps:\/\/www.etap-lab.com\/old-etaplab\/newsletter-etaptemp\/tau-clinical-trials-what-can-be-learned-from-failure\/embed\/#?secret=A2ldi1t1Za#?secret=yuk6w17h7v\n<\/div><\/figure>\n\n\n\n<figure class=\"wp-block-embed is-type-wp-embed is-provider-etap-blog wp-block-embed-etap-blog\"><div class=\"wp-block-embed__wrapper\">\nhttps:\/\/www.etap-lab.com\/old-etaplab\/newsletter-etaptemp\/new-hope-for-alzheimers-disease-whats-combining-therapeutic-strategies-all-about\n<\/div><\/figure>\n","protected":false},"excerpt":{"rendered":"<p>Discover Tau oligomers: a new tool for drug discovery in AD: One common pathological hallmark of neurodegenerative disease (ND) is the aggregation and accumulation of misfolding\u2026<\/p>\n","protected":false},"featured_media":0,"template":"","meta":{"_acf_changed":false},"categorie-de-ressource":[238],"marque-de-ressource":[],"class_list":["post-36824","ressource","type-ressource","status-publish","hentry","categorie-de-ressource-technical-notes"],"acf":[],"yoast_head":"<!-- This site is optimized with the Yoast SEO plugin v27.5 - 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