1 research outputs found
A Quantitative LC-MS/MS Method for Distinguishing the Tau Protein Forms Phosphorylated and Nonphosphorylated at Serine-396
Hyperphosphorylated
tau protein is well-known to be involved in
the formation of neurofibrillary tangles and the progression of age-related
neurodegenerative diseases (tauopathies), including Alzheimer’s
Disease (AD). Tau protein phosphorylated at serine-396 (pS396-tau)
is often linked to disease progression, and we therefore developed
an analytical method to measure pS396-tau in cerebrospinal fluid (CSF)
in humans and animal models of AD. In the S396-region, multiple phosphorylation
sites are present, causing structural complexity and sensitivity challenges
for conventional bottom-up mass spectrometry approaches. Here, we
present an indirect LC-MS/MS method for quantification of pS396-tau.
We take advantage of the reproducible miscleavage caused by S396 being
preceded by a lysine (K395) and the proteolytic enzyme trypsin not
cleaving when the following amino acid is phosphorylated. Therefore,
treatment with trypsin discriminates between the forms of tau with
and without phosphorylation at S396 and pS396-tau can be quantified
as the difference between total S396-tau and nonphosphorylated S396-tau.
To qualify the method, it was successfully applied for quantification
of pS396-tau in human CSF from healthy controls and patients with
Mild Cognitive Impairment and AD. In addition, the method was applied
for rTg4510 mice where a clear dose dependent decrease in pS396-tau
was observed in CSF following intravenous administration of a monoclonal
antibody (Lu AF87908, hC10.2) targeting the tau epitope containing
pS396. Finally, a formal validation of the method was conducted. In
conclusion, this sensitive LC-MS/MS-based method for measurement of
pS396-tau in CSF allows for quantitative translational biomarker applications
for tauopathies including investigations of potential drug induced
effects