US2019227031A1PendingUtilityA1

Glycan profiling utilizing capillary electrophoresis

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Assignee: BIOPTIC INCPriority: May 22, 2014Filed: Jan 21, 2019Published: Jul 25, 2019
Est. expiryMay 22, 2034(~7.9 yrs left)· nominal 20-yr term from priority
G01N 27/44721G01N 27/44726G01N 27/44791G01N 27/44743G01N 21/64
60
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Claims

Abstract

A method for glycan profiling by capillary electrophoresis (CE), and a CE system for glycan analysis (N-Glycan). The CE system uses integrated dual optical fibers for both radiation excitation and emission detection. The CE system is configured for performing a two-color detection for data analysis. A single radiation excitation source is used to excite two emission fluorophores or dyes in the sample solution to be analyzed. One emission dye is to tag the sample and the other dye is used to provide a reference marker (e.g., a Dextran Ladder) for the sample run. Two detectors (e.g., photomultipler tubes (PMTs)) are applied to simultaneously detect the fluorescent emissions from the dyes. The data collected by both detectors are correlated (e.g., synchronized, and/or super-positioned for analysis) for accurate data peak identification.

Claims

exact text as granted — not AI-modified
We claim: 
     
         1 . A method of glycan profiling, comprising:
 providing a separation channel having a first longitudinal axis along which a glycan sample undergoes separation into sample components, and defining a detection zone defined along the separation channel through which sample components pass, wherein prior to subjecting the glycan sample to separation, the glycan sample is provided with a sample marker corresponding to a first fluorescence emission having a first characteristic wavelength, wherein the sample components are labeled by the sample marker for identification as the glycan sample undergoes separation, wherein the glycan sample is further provided with a reference marker corresponding to a second fluorescence emission having a second characteristic wavelength different from the first characteristic wavelength, wherein the reference marker provides a reference to facilitate identification of the sample components as the glycan sample undergoes separation;   providing a radiation source that provides an incident radiation having a single wavelength to induce the first fluorescence emission from the sample marker having the first characteristic wavelength and the second fluorescence emission from the reference marker having the second characteristic wavelength, and wherein the sample marker comprises a first material that emits the first fluorescence emission when induced by the incident radiation, and the reference marker comprises a second material that emits the second fluorescence emission when induced by the incident radiation;   providing a detector, which detects the first fluorescence emission having the first characteristic wavelength and the second fluorescence emission having the second characteristic wavelength;   providing an incident light guide having a second longitudinal axis, directing the incident radiation from the radiation source to the detection zone, causing radiation to be emitted by sample components as they pass through the detection zone;   providing an emission light guide having a third longitudinal axis, collecting and directing emitted radiation from the detection zone to the detector, wherein the emission light guide and the incident light guide are positioned on opposite sides of the separation channel; and   subjecting the glycan sample to high voltage to effect electrophoresis to separate the glycan sample into the sample components along the separation channel, wherein the detector detects the first fluorescence emission and the second fluorescence emission at the detection zone.   
     
     
         2 . The method of  claim 1 , wherein the radiation source directs same incident radiation to the detection zone to cause the first fluorescence emission having the first characteristic wavelength and the second fluorescence emission having the second characteristic wavelength. 
     
     
         3 . The method of  claim 2 , wherein the separation channel is a capillary channel defined in a capillary column, defining the detection zone. 
     
     
         4 . The method of  claim 3 , wherein the sample marker comprises a sample fluorophore and the reference marker comprises a reference fluorophore, wherein the sample fluorophore and the reference fluorophore are simultaneously subject to the incident radiation as they pass through the detection zone, and wherein the incident radiation induces emitted radiations in the form of the first and second fluorescence emissions of the sample marker and the reference marker as the sample components pass through the detection zone. 
     
     
         5 . The method of  claim 4 , wherein the reference fluorophore provides a Ladder as the reference marker as the glycan sample undergoes separation. 
     
     
         6 . The method of  claim 5 , wherein the emission light guide and the incident light guide are positioned on opposite sides of the separation channel, and wherein the first, second and third longitudinal axis are substantially coplanar at the detection zone. 
     
     
         7 . The method of  claim 6 , wherein at least one of the second and third longitudinal axis is not perpendicular to the first longitudinal axis. 
     
     
         8 . The method of  claim 7 , wherein the incident light guide comprises a first optical fiber having a terminating integral ball-end structure, and the emission light guide comprises a second optical fiber having a terminating integral ball-end structure, and wherein the ball-end structures do not touch exterior of the separation channel. 
     
     
         9 . The method of  claim 8 , wherein the detector comprises a first detector detecting the first fluorescence emission having the first characteristic wavelength, and a second detector detecting the second fluorescence emission having the second characteristic wavelength. 
     
     
         10 . The method of  claim 9 , wherein the glycan sample is N-Glycan. 
     
     
         11 . A method of glycan profiling, comprising:
 providing a separation channel having a first longitudinal axis along which a N-Glycan sample undergoes separation into sample components, and defining a detection zone defined along the separation channel through which sample components pass, wherein prior to subjecting the glycan sample to separation, the glycan sample is provided with a sample marker corresponding to a first fluorescence emission having a first characteristic wavelength, wherein the sample components are labeled by the sample marker for identification as the glycan sample undergoes separation, wherein the glycan sample is further provided with a reference marker corresponding to a second fluorescence emission having a second characteristic wavelength different from the first characteristic wavelength, wherein the reference marker provides a reference to facilitate identification of the sample components as the glycan sample undergoes separation;   providing a radiation source that provides an incident radiation having a single wavelength to induce the first fluorescence emission from the sample marker having the first characteristic wavelength and the second fluorescence emission from the reference marker having the second characteristic wavelength, and wherein the sample marker comprises a first material that emits the first fluorescence emission when induced by the incident radiation, and the reference marker comprises a second material that emits the second fluorescence emission when induced by the incident radiation;   providing a detector, which detects the first fluorescence emission having the first characteristic wavelength and the second fluorescence emission having the second characteristic wavelength;   providing an incident light guide having a second longitudinal axis, directing the incident radiation from the radiation source to the detection zone, causing radiation to be emitted by sample components as they pass through the detection zone;   providing an emission light guide having a third longitudinal axis, collecting and directing emitted radiation from the detection zone to the detector, wherein the emission light guide and the incident light guide are positioned on opposite sides of the separation channel; and   subjecting the glycan sample to high voltage to effect electrophoresis to separate the glycan sample into the sample components along the separation channel, wherein the detector detects the first fluorescence emission and the second fluorescence emission at the detection zone.   
     
     
         12 . The method of  claim 11 , wherein the radiation source directs same incident radiation to the detection zone to cause the first fluorescence emission having the first characteristic wavelength and the second fluorescence emission having the second characteristic wavelength. 
     
     
         13 . The method of  claim 12 , wherein the separation channel is a capillary channel defined in a capillary column, defining the detection zone. 
     
     
         14 . The method of  claim 13 , wherein the sample marker comprises a sample fluorophore and the reference marker comprises a reference fluorophore, wherein the sample fluorophore and the reference fluorophore are simultaneously subject to the incident radiation as they pass through the detection zone, and wherein the incident radiation induces emitted radiations in the form of the first and second fluorescence emissions of the sample marker and the reference marker as the sample components pass through the detection zone. 
     
     
         15 . The method of  claim 14 , wherein the reference fluorophore provides a Ladder as the reference marker as the glycan sample undergoes separation. 
     
     
         16 . The method of  claim 15 , wherein the emission light guide and the incident light guide are positioned on opposite sides of the separation channel, and wherein the first, second and third longitudinal axis are substantially coplanar at the detection zone. 
     
     
         17 . The method of  claim 16 , wherein at least one of the second and third longitudinal axis is not perpendicular to the first longitudinal axis. 
     
     
         18 . The method of  claim 17 , wherein the incident light guide comprises a first optical fiber having a terminating integral ball-end structure, and the emission light guide comprises a second optical fiber having a terminating integral ball-end structure, and wherein the ball-end structures do not touch exterior of the separation channel. 
     
     
         19 . The method of  claim 18 , wherein the detector comprises a first detector detecting the first fluorescence emission having the first characteristic wavelength, and a second detector detecting the second fluorescence emission having the second characteristic wavelength. 
     
     
         20 . An electrophoresis system for profiling glycan, structured and configured to perform the method of  claim 1 .

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