Development and Validation of a High Sensitivity Assay for Measuring p217 + tau in Cerebrospinal Fluid

Triana‐Baltzer, Gallen; Kolen, Kristof Van; Theunis, Clara; Moughadam, Setareh; Slemmon, Randy; Mercken, Marc; Galpern, Wendy R.; Sun, Hong; Kolb, Hartmuth C.

doi:10.3233/jad-200463

Cited by 18 publications

(31 citation statements)

References 29 publications

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“…The assay relies on the high affinity and specificity of the PT3 mAb, which recognizes tau phosphorylated at threonine residues 212 and 217 22 . Phosphorylation of amino acid 217 is the minimally required epitope, yet phosphorylation of amino acid 212 enhances binding, and thus the recognition is termed “p217+tau.” As described for the CSF p217+tau assay, measurement of species containing both p212 and p217 may yield additional diagnostic relevance than measurement of just one of these residues 19 . Indeed, while liquid chromatography/mass spectrometry (LC/MS) studies of paired helical filament (PHF) tau revealed monophosphorylated peptides containing pT217 alone, pT212 was only found in peptides that also contained phosphorylation of S214 or T217 14 .…”

Section: Discussionmentioning

confidence: 99%

“…Predominantly observed species are comprised of N‐terminal, mid‐region, and select microtubule binding region (MTBR) epitopes, and additional major cleavage sites are likely in the region from aa 70‐120 and at ~aa 224 15,26,34,35,36 . Fractionation of CSF prior to assay has shown that CSF p217+tau is also entirely of fragmented nature, lacking C‐terminus and potentially also cleaved between aa7‐119 19 . Here we show, by comparing the p217+tau “short” and p217+tau “long” assay results, that plasma p217+tau may present a similar level of fragmentation in the aa 7‐119 region as in CSF.…”

Section: Discussionmentioning

confidence: 99%

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Development and validation of a high‐sensitivity assay for measuring p217+tau in plasma

Triana‐Baltzer

Moughadam

Slemmon

et al. 2021

Alz & Dem Diag Ass & Dis Mo

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Introduction Diagnosis of Alzheimer's disease (AD) based on amyloid beta (A), pathologic tau (T), and neurodegeneration (N) biomarkers in peripheral fluids promises to accelerate clinical trials and intercept disease earlier. Methods Qualification of a Simoa plasma p217+tau assay was performed, followed by clinical utility evaluation in a cohort of 227 subjects with broad A and T spectrum. Results The p217+tau plasma assay was accurate, precise, dilution linear, and highly sensitive. All measured samples were within linear range of the assay, presented higher concentration in AD versus healthy controls ( P < .0001), and plasma and cerebrospinal fluid levels correlated (r 2 = 0.35). The plasma p217+tau results were predictive of central T and A status (area under the curve = 0.90 and 0.90, respectively) with low false +/– rates. Discussion The assay described here exhibits good technical performance and shows potential as a highly accurate peripheral biomarker for A or T status in AD and cognitively normal subjects.

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Development and validation of a high‐sensitivity assay for measuring p217+tau in plasma

Triana‐Baltzer

Moughadam

Slemmon

et al. 2021

Alz & Dem Diag Ass & Dis Mo

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“…More recently a high sensitivity Simoa assay has been developed using a capture antibody (pT3) that was raised against tau in paired helical filaments (PHF) of AD brain [12,13]. The core requirement for this antibody binding is phosphorylation at aa217 (p217) with enhanced binding when other nearby phosphorylated sites are present, predominantly at aa212 [12].…”

Section: Introductionmentioning

confidence: 99%

Plasma p217+tau vs NAV4694 amyloid and MK6240 tau PET across the Alzheimer continuum

Doré

Doecke

Saad

et al. 2022

Preprint

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INTRODUCTION: We evaluated a new Simoa plasma assay for phosphorylated tau at aa217 enhanced by additional ptau sites (p217+tau). METHODS: Plasma p217+tau levels were compared to 18F-NAV4694 amyloid-beta (Aβ PET and 18F-MK6240 tau PET in 174 cognitively impaired (CI) and 223 cognitively unimpaired (CU) participants. RESULTS: Compared to Aβ- CU, the plasma levels of p217+tau increased two-fold in Aβ+ CU and 3.5-fold in Aβ+ CI. In Aβ- the p217+tau levels did not significantly differ between CU, MCI or dementia. P217+tau correlated with Aβ centiloids ρ=0.67 (CI 0.64; CU 0.45) and tau SUVRMT ρ=0.63 (CI 0.69; CU 0.34). Area under curve (AUC) for AD vs Aβ- CU was 0.94, for AD vs other dementia was 0.93, for Aβ+ vs Aβ PET was 0.89 and for tau+ vs tau- PET was 0.89. DISCUSSION: Plasma p217+tau levels elevate early in the AD continuum and correlate well with Aβ and tau PET.

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“…We then used an immunoassay which allows the quantification of tau phosphorylated at threonine 217 with or without adjacent phospho-epitopes (“p217 + tau” [ 12 ] (see also Supplementary Methods, online resource). P217 + tau also showed an age-dependent increase and reached a plateau, although at 14- to 16-fold higher levels compared to 1.5-month-old APPPS1 tg animals (Fig.…”

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CSF p-tau increase in response to Aβ-type and Danish-type cerebral amyloidosis and in the absence of neurofibrillary tangles

et al. 2021

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Development and Validation of a High Sensitivity Assay for Measuring p217 + tau in Cerebrospinal Fluid

Cited by 18 publications

References 29 publications

Development and validation of a high‐sensitivity assay for measuring p217+tau in plasma

Development and validation of a high‐sensitivity assay for measuring p217+tau in plasma

Plasma p217+tau vs NAV4694 amyloid and MK6240 tau PET across the Alzheimer continuum

CSF p-tau increase in response to Aβ-type and Danish-type cerebral amyloidosis and in the absence of neurofibrillary tangles

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