Seeding selectivity and ultrasensitive detection of tau aggregate conformers of Alzheimer disease

Kraus, Allison; Saijo, Eri; Metrick, Michael A.; Newell, Kathy L.; Sigurdson, Christina J.; Zanusso, Gianluigi; Ghetti, Bernardino; Caughey, Byron

doi:10.1007/s00401-018-1947-3

Cited by 104 publications

(143 citation statements)

References 47 publications

Supporting

Mentioning

122

Contrasting

Order By: Relevance

“…To our knowledge, no studies have been reported to selectively detect misfolded tau seeds from AD brains using recombinant full-length tau isoforms as substrates. Our study complements a recent investigation describing ultrasensitive detection of tau aggregate conformer of AD with a mixture of two significantly shortened tau fragments as dual substrates (Kraus et al, 2019). The successful seeding activities of AD brain homogenates with individual tau isoforms as a substrate further validated the predicted presence of all six misfolded tau isoforms in AD brains (Goedert et al, 1992;Lee et al, 1999).…”

Section: Discussionsupporting

confidence: 73%

“…RT-QuIC assay has been used for detection of seeding activities of misfolded proteins, first for prions and then for aSyn and tau in vitro (Atarashi et al, 2008;Orru et al, 2017;Groveman et al, 2018;Sano et al, 2018;Saijo et al, 2017;Kraus et al, 2019). To determine whether various recombinant wild-type human tau isoforms can be converted by the tau aggregate seeds from AD brain samples, we detected autopsied AD and non-AD brain samples from neuropathologically confirmed cadavers (Table 1).…”

Section: Full-length Tau Isoform Based Rt-quic Assay Selectively Detementioning

confidence: 99%

“…RT-QuIC Analysis. Tau RT-QuIC assays were conducted as previously described with minor modifications (Orru et al, 2017;Saijo et al, 2017;Kraus et al, 2019;Wang et al, 2019). In brief, each recombinant tau isoform was thawed at room temperature and filtered with a 100 kDa spin column filter (Millipore) to remove unwanted tau aggregates.…”

Section: Thioflavin-t Fluorescence Aggregationmentioning

confidence: 99%

“…Two methods to amplify misfolded proteins in vitro, the real-time quaking-induced conversion (RT-QuIC) assay and the protein misfolding cyclic amplification protocol (PMCA) are used for ultrasensitive detection in a number of neurodegenerative diseases, such as prion disease (Moda et al, 2014;Orru et al, 2017;Wang et al, 2019), Ab oligomers in AD (Salvadores et al, 2014), and a-synuclein in Parkinson's disease (Fairfoul et al, 2016;Shahnawaz et al, 2017;Groveman et al, 2018). Specifically for misfolded tau detection in AD and other tauopathies such as Pick's disease, detection of the prion-like tau seeding activities by RT-QuIC assays was successfully developed using engineered short fragments of tau or a mixture of tau fragments with mutations as a substrate (Saijo et al, 2017;Kraus et al, 2019). However, detection of AD and related tauopathies with recombinant full-length human tau isoforms that match tau isoforms in vivo has not been reported.…”

Section: Introductionmentioning

confidence: 99%

See 3 more Smart Citations

Human Tau Isoform Aggregation and Selective Detection of Misfolded Tau from Post-Mortem Alzheimer’s Disease Brains

Wang

Lad

et al. 2020

Preprint

View full text Add to dashboard Cite

Tau aggregates are present in a large number of neurodegenerative diseases known as "tauopathies", including Alzheimer's disease (AD). As there are six human tau isoforms in brain tissues and both 3R and 4R isoforms have been observed in the neuronal inclusions, we tested whether tau isoforms behave differently in aggregation. We discovered that all six tau isoforms are capable of forming PHF-tau like filaments and the 3R tau isoforms aggregate significantly faster than their 4R counterparts. We further mapped key segments of tau isoforms that contribute to their aggregation kinetics, where it was determined that microtubule binding domains R2 and R3 were the major contributors to tau aggregation. To evaluate the feasibility of using the six recombinant tau isoforms as substrates to amplify misfolded tau, we demonstrated that full-length human tau isoforms can seed and detect misfolded tau from the post-mortem AD brain tissues with high specificity by an ultrasensitive technology termed real-time quaking-induced conversion (RT-QuIC). Mass spectrometric analysis of PHF-tau samples extracted from AD brains identified peptides corresponding to all major forms of human brain tau isoforms along with a consensus hyperphosphorylated peptide near the C-terminus.Together, our findings not only reveal new aggregation kinetic properties of human tau isoforms, support the development of methods to quantitatively measure misfolded human tau isoforms in AD brains, but also uncover the capability of full-length human tau isoforms as substrates for "prion-like" tau seeding by RT-QuIC assays that may be used for new biomarker development for AD and other tauopathy diagnosis.

show abstract

Section: Discussionsupporting

confidence: 73%

Section: Full-length Tau Isoform Based Rt-quic Assay Selectively Detementioning

confidence: 99%

Section: Thioflavin-t Fluorescence Aggregationmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

Human Tau Isoform Aggregation and Selective Detection of Misfolded Tau from Post-Mortem Alzheimer’s Disease Brains

Wang

Lad

et al. 2020

Preprint

View full text Add to dashboard Cite

show abstract

“…A recently described technique called real-time quaking-induced conversion, which exploits the ability of prion protein to induce self-aggregation, has been used to develop a diagnostic CSF test for Creutzfeldt-Jakob disease (145). This method has now also been developed into a test to detect pathological forms of tau in CSF from patients with AD or other tauopathies (146,147). Seedcompetent high-molecular-weight tau species have been detected in human CSF (78), but there is yet no established method in clinical laboratory practice.…”

Section: Measures Of Tau In Body Fluidsmentioning

confidence: 99%

Propagation of Tau Pathology: Integrating Insights From Postmortem and In Vivo Studies

Vogels

Leuzy

Cicognola

et al. 2020

Biological Psychiatry

View full text Add to dashboard Cite

Cellular accumulation of aggregated forms of the protein tau is a defining feature of so-called tauopathies such as Alzheimer's disease, progressive supranuclear palsy, and chronic traumatic encephalopathy. A growing body of literature suggests that conformational characteristics of tau filaments, along with regional vulnerability to tau pathology, account for the distinct histopathological morphologies, biochemical composition, and affected cell types seen across these disorders. In this review, we describe and discuss recent evidence from human postmortem and clinical biomarker studies addressing the differential vulnerability of brain areas to tau pathology, its cell-to-cell transmission, and characteristics of the different strains that tau aggregates can adopt. Cellular biosensor assays are increasingly used in human tissue to detect the earliest forms of tau pathology, before overt histopathological lesions (i.e., neurofibrillary tangles) are apparent. Animal models with localized tau expression are used to uncover the mechanisms that influence spreading of tau aggregates. Further, studies of human postmortem-derived tau filaments from different tauopathies injected in rodents have led to striking findings that recapitulate neuropathology-based staging of tau. Furthermore, the recent advent of tau positron emission tomography and novel fluid-based biomarkers render it possible to study the temporal progression of tau pathology in vivo. Ultimately, evidence from these approaches must be integrated to better understand the onset and progression of tau pathology across tauopathies. This will lead to improved methods for the detection and monitoring of disease progression and, hopefully, to the development and refinement of tau-based therapeutics.

show abstract

Preclinical characterization and IND‐enabling safety studies for PNT001, an antibody that recognizes cis‐pT231 tau

Foster¹,

Manca

McClure³

et al. 2023

Alzheimer's & Dementia

View full text Add to dashboard Cite

BACKGROUNDThe cis‐conformer of tau phosphorylated at threonine‐231 (cis‐pT231 tau) is hypothesized to contribute to tauopathies. PNT001 is a humanized, monoclonal antibody that recognizes cis‐pT231 tau. PNT001 was characterized to assess clinical development readiness.METHODSAffinity and selectivity were assessed by surface plasmon resonance and enzyme‐linked immunosorbent assay. Immunohistochemistry (IHC) was performed with brain sections from human tauopathy patients and controls. Real‐time quaking‐induced conversion (RT‐QuIC) was used to assess whether PNT001 reduced tau seeds from Tg4510 transgenic mouse brain. Murine PNT001 was evaluated in vivo in the Tg4510 mouse.RESULTSThe affinity of PNT001 for a cis‐pT231 peptide was 0.3 to 3 nM. IHC revealed neurofibrillary tangle‐like structures in tauopathy patients with no detectable staining in controls. Incubation of Tg4510 brain homogenates with PNT001 lowered seeding in RT‐QuIC. Multiple endpoints were improved in the Tg4510 mouse. No adverse findings attributable to PNT001 were detected in Good Laboratory Practice safety studies.DISCUSSIONThe data support clinical development of PNT001 in human tauopathies.

show abstract

Seeding selectivity and ultrasensitive detection of tau aggregate conformers of Alzheimer disease

Cited by 104 publications

References 47 publications

Human Tau Isoform Aggregation and Selective Detection of Misfolded Tau from Post-Mortem Alzheimer’s Disease Brains

Human Tau Isoform Aggregation and Selective Detection of Misfolded Tau from Post-Mortem Alzheimer’s Disease Brains

Propagation of Tau Pathology: Integrating Insights From Postmortem and In Vivo Studies

Preclinical characterization and IND‐enabling safety studies for PNT001, an antibody that recognizes cis‐pT231 tau

Contact Info

Product

Resources

About