US2021096139A1PendingUtilityA1

Tau kinetic measurements

Assignee: UNIV WASHINGTONPriority: Sep 30, 2014Filed: Sep 25, 2020Published: Apr 1, 2021
Est. expirySep 30, 2034(~8.2 yrs left)· nominal 20-yr term from priority
G01N 33/58G01N 2458/15G01N 33/6896A61K 51/08A61K 2039/505G01N 2560/00
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Claims

Abstract

The invention relates to in vitro methods for measuring the in vivo metabolism of tau in a subject.

Claims

exact text as granted — not AI-modified
What is claimed is: 
     
         1 . An in vitro method for measuring the metabolism of soluble cerebral spinal fluid (CSF) tau in a subject, the method comprising:
 (a) administering at least one labeled amino acid to the subject on one or more days;   (b) collecting at least one blood sample from the subject between day 5 and about day 20, about day 20 and about day 40, about day 40 and about day 100, or a combination thereof;   (c) separating a tau fragment from at least one blood sample collected in step (b) using an antibody that has affinity within tau's N-terminus or mid-domain;   (d) detecting and measuring by mass spectrometry the amount of labeled tau fragment, or the amount of labeled and unlabeled tau fragment, in at least one sample from step (c); and   (e) calculating the metabolism of soluble CSF tau using the measurements from step (d), wherein the amount of labeled tau fragment in the sample at a given time reflects the metabolism of soluble CSF tau.   
     
     
         2 . An in vitro method for measuring the metabolism of soluble cerebral spinal fluid (CSF) tau in a subject, the method comprising:
 (a) separating a tau fragment from at least one blood sample obtained from a subject, using an antibody that has affinity within tau's N-terminus or mid-domain;   (b) detecting and measuring by mass spectrometry the amount of labeled tau, or the amount of labeled and unlabeled tau, in at least blood sample from step (a); and   (b) calculating the metabolism of soluble CSF tau using the measurements from step (b), wherein the amount of labeled tau in the sample at a given time reflects the metabolism of soluble CSF tau; and   wherein
 (i) the label was administered on one or more days to the subject as one or more labeled amino acids, and (ii) at least one blood sample was collected from the subject between day 5 and about day 20, day 20 and day 40, day 40 and day 100, or a combination thereof. 
   
     
     
         3 . The method of  claim 2 , wherein the labeled amino acid was administered on two or more days between day 0 and about day 3. 
     
     
         4 . The method of  claim 2 , wherein the labeled amino acid was administered on two or more days between day 0 and about day 5. 
     
     
         5 . The method of  claim 2 , wherein the labeled amino acid was administered on two or more days between day 0 and about day 10. 
     
     
         6 . The method of  claim 2 , wherein the labeled amino acid was administered daily. 
     
     
         7 . The method of  claim 2 , wherein the labeled amino acid is labeled with a non-radioactive isotope. 
     
     
         8 . The method of  claim 7 , wherein the non-radioactive isotope is selected from the group consisting of  2 H,  13 C,  15 N,  17 O,  18 O,  33 S,  34 S, and  36 S. 
     
     
         9 . The method of  claim 7 , wherein the labeled amino acid is  13 C 6  leucine. 
     
     
         10 . The method of  claim 2 , wherein the labeled amino acid was administered to the subject intravenously or orally. 
     
     
         11 . The method of  claim 10 , wherein the labeled amino acid was administered to the subject orally, at a total daily dose of about 0.1 g to about 10 g, on two or more days between day 0 and about day 10. 
     
     
         12 . The method of  claim 2 , wherein the label is administered to produce an amount of labeled amino acid in the CSF sample selected from the group consisting of about 0.1%, about 0.2%, about 0.5%, about 1%, about 2%, about 5%, about 0.1 to about 20%, and about 0.1 to about 10%. 
     
     
         13 . The method of  claim 2 , wherein the subject is a rodent. 
     
     
         14 . The method of  claim 2 , wherein the subject is a human. 
     
     
         15 . The method of  claim 2 , wherein the tau fragment is separated by immunoprecipitation. 
     
     
         16 . The method of  claim 2 , the method further comprising calculating a metabolic parameter of soluble tau metabolism using the amounts of labeled and/or unlabeled tau determined in step (b), the metabolic parameter selected from the group consisting of relative labeling, fractional synthesis rate, fractional clearance rate, absolute synthesis rate, absolute clearance rate, fractional turnover rate, lag time, half-life, peak time, and peak height. 
     
     
         17 . The method of  claim 2 , wherein tau is a phosphorylated tau isoform. 
     
     
         18 . The method of  claim 2 , wherein at least one blood sample is collected from the subject between about day 20 and about day 40, about day 40 and about day 100, or a combination thereof. 
     
     
         19 . The method of  claim 1 , the method further comprising calculating a metabolic parameter of tau metabolism using the amounts of labeled and/or unlabeled tau determined in  claim 1  step (c), the metabolic parameter selected from the group consisting of relative labeling, fractional synthesis rate, fractional clearance rate, absolute synthesis rate, absolute clearance rate, fractional turnover rate, lag time, half-life, peak time, and peak height.

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