WO1999064851A1 - Control of flow and materials for micro devices - Google Patents
Control of flow and materials for micro devices Download PDFInfo
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- WO1999064851A1 WO1999064851A1 PCT/US1999/013340 US9913340W WO9964851A1 WO 1999064851 A1 WO1999064851 A1 WO 1999064851A1 US 9913340 W US9913340 W US 9913340W WO 9964851 A1 WO9964851 A1 WO 9964851A1
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- fluid pathway
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Classifications
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N27/00—Investigating or analysing materials by the use of electric, electrochemical, or magnetic means
- G01N27/26—Investigating or analysing materials by the use of electric, electrochemical, or magnetic means by investigating electrochemical variables; by using electrolysis or electrophoresis
- G01N27/416—Systems
- G01N27/447—Systems using electrophoresis
- G01N27/44704—Details; Accessories
Definitions
- the present invention generally relates to methods and devices for the control of the movement of fluids and electrically charged sample components within those fluids. More particularly, the present invention permits exclusion or concentration of specifically chosen sample components within a fluid.
- the present invention provides an analytical device, either microchip- or capillary-based, having the means to exclude specific sample components of interest from a capillary or channel for the purpose of preconcentration or control of movement of sample components.
- a control system includes a means for controlling the flow of the fluid in the channel and the placement of an electrode at the immediate entrance of each channel on such devices so that material may be directly manipulated by either or both of the effects of both bulk flow and electrically driven migration.
- Capillary zone electrophoresis is an efficient analytical separation technique which utilizes differences in mobility of sample components in an electric field based on the electrical charge and molecular site and shape of the sample component.
- Conventional CZE systems typically comprise a buffer- filled capillary with outlet and inlet ends disposed in two reservoirs into which one sample is injected, a means for applying voltage to the capillary resulting in migration of the sample through the capillary, and a means for detecting the sample zone.
- pressu ⁇ zed flow and countermigration can be used to increase the overall concentration as described by Ho ⁇ et al (1993, Anal Chem 65 2882-2886)
- the sample is introduced into a first vessel containing buffer which is connected to another vessel by a glass tube
- An electrode extending into the first vessel applies a voltage to the sample while suction pressure is applied
- the sample concentration increases throughout the first vessel rather than concentrating the sample in a discrete portion of that vessel because the applied potential field is unconstrained throughout the buffei volume Because the concentration increase and electric fields are dispersed throughout the entire first vessel volume this technique is not applicable as a small volume ln ection/preconcentration technique Moreover, this arrangement does not allow for micromampulations such as electrophoretic separation withm the vessel containing the concentrated sample
- sample components fluids and electrically charged species
- analytical electrophoretic arrangement including microchips or capillaries which excludes specific sample components of interest from a capillary or channel for the purposes of preconcentration or control of movement of materials.
- preconcentration and manipulation is achieved within a single constrained flow pathway system. More particularly, the sample is preconcentrated in a portion of the constrained flow pathway and is manipulated as it travels through the pathway.
- the invention further provides an electrophoretic apparatus for controlling the movement of an sample component in a fluid sample comprising:
- the present invention can be utilized m methods and devices for manipulating, testing, probing, or analyzing sample fluids of any kind where fluid manipulations are utilized for preconcentration, chemical reaction, injection, detection, or movement, or cessation of movement, of components of interest m a sample fluid
- the present invention is directed to an analytical device having a plurality of channels with electrodes placed at the immediate entrance of all or selected channels and a method for regulating the bulk flow withm the channels
- the bulk flow is set approximately equal to and opposite the electrophoretic migration of specific sample components of interest, the movement of those specific sample components ceases
- the introduction of an electric field between the electrodes within the channel, coupled with control of bulk flow, allows selected sample components of interest to be excluded or preconcentrated immediately upon introduction of the fluid sample into the channel.
- Figure 1 is a schematic drawing of a fused silica capillary arrangement with electrodes placed immediately at the mlet to provide the voltage control withm the capillary in accordance with the invention
- Figures 2(a), 2(b) and 2(c) are schematic drawings of a micro-device apparatus having an injection channel and a separation channel in accordance with the invention
- Figure 3 is a schematic drawing of a micro-device apparatus indicating the preconcentration of materials at the immediate entrance to a channel where the voltage with in the buffer reservoir is held constant in accordance with the invention
- Figure 4 is a schematic drawing of the theoretical profile of the preconcentration of material at the immediate entrance to a capillary showing the concentration of desired materials
- Figure 5 is a graph showing the normalized fluorescence intensity versus distance outside the capillary entrance for two control experiments
- Figure 6 is a graph showing the normalized fluorescence intensity versus number of pixels (1 pixel - 0.24 ⁇ m) outside a capillary entrance ;and Figures 7(a) and (b) are fluorescence micrographs of a capillary entrance before and after, respectively, preconcentration of 200 nm fluorescently labeled latex micro spheres for 270 seconds.
- the present invention provides novel methods and devices for exclusion or concentration of specifically chosen sample components within fluids through the control of fluid movement and electrophoretic migration of charged sample components within those fluids.
- the fluid sample is delivered or injected into a restricted flow path such as a channel or capillary.
- the flow path is preferably less than 200 microns in diameter. Precise control of fluid manipulation, sample component movement and solution injection systems are accomplished by carefully controlling the voltage field gradients and the bulk flow within each channel on a micro-device.
- microchip includes a semiconductor device comprising silica or any other substrate which may be used m micro fluidic devices, which may be used in or in conjunction with a computer
- the present invention also provides for the placement of an electrode at the immediate entrance of each channel on a micro-device so that material movement may be dnectly manipulated by elect ⁇ cally-d ⁇ ven migration, 1 e , electrophoretic migration
- the present invention also provides control of bulk flow of the fluid withm the channel Bulk flow may be positive or negative depending upon the magnitude and direction of electrically-driven flow, l e , electroosmosis, or various other sources of flow such as pressure, convection, capillarity, etc Voltage gradients may likewise be manipulated to provide electrophoretic migration m either direction
- the independent control of these parameters provides for absolute control of movement of sample components withm the fluid about a micro-device
- the method of the invention comp ⁇ ses as a first step, the introduction of a sample containing the sample component of interest into a channel or capillary that has been filled with buffer Sample introduction may be accomplished using a syringe by which the sample solution is injected into the channel Alternatively, the introduction of the sample can be performed according to standard procedures, including but not limited to the use of electroosmotic flow, electro-kmetic pumping, or pneumatic pumping
- FIG. 1 An electrophoretic arrangement in which a capillary is utilized to create the rest ⁇ cted flow path is shown m Figure 1
- electrodes 20 are located external to and mounted onto a fused silica capillary
- a counter electrode 24 is placed at a location remote from electrodes 20 and fornis a circuit therewith
- a high voltage is applied to the electrodes 20 and 24 by power supply 26
- a reservoir 28 including buffer bulk flow mate ⁇ als is in fluid contact with the capillary
- a sample 5 including charged components is introduced into the reservoir and moves towards the entrance 9 of the capillary m the presence of the applied voltage which induces electrophoretic migration
- the charged components m analyte 5 aie concentrated at the entrance 9 of the capillary 22
- the present invention also provides a micro-analytical separation device comprised of etched or molded channels whereby various channels are used for separation and analysis purposes and others are distinctly used for the purpose of injection or material movement illustrated in Figs 2(a-c)
- the system includes an injection channel 2 and sepaiation channel 4
- Sample material is injected to fill the injection channel 2 m between the separation channels 4 as depicted m Figure 2b
- a small voltage is applied to the two injection channel electrodes 5
- the electrodes are used to create an appropriate voltage gradient to prevent unwanted introduction of materials into the separation channel thereby concentrating desired components m separation channel 4
- positive, negative and neutral molecules may be manipulated as a group or individually
- a high voltage is applied by power supply means between the mlet and outlet end of the channel or capillary through electrode means
- the voltage used is not critical to the invention and may vary widely depending on the sample component(s) to be excluded or concentrated Conditions for selecting appropriate voltage conditions will depend on the physical properties of the sample component(s) and can be determined by those of skill m the art
- the method of the invention further comprises setting the bulk flow in the channel or capillary approximately equal to and opposite to the electrophoretic migration rate of the material
- the bulk flow m the capillary may be generated and controlled by either electroosmosis, pressure or various other mechanisms Bulk flow may be created and controlled by electroosmotic pumping devices, pneumatic devices, or directly by electroosmosis with dynamic control and monitoring.
- electroosmotic pumping devices pneumatic devices
- electroosmosis with dynamic control and monitoring.
- any constrained fluid pathway for example a fused silica or teflon capillary, where separation or injection of materials of interest are performed may be included in the device.
- Each channel or continuous fluid pathway where control of material movement is desired is constructed with an electrode adjoining the entrance and exit of the channel or pathway. Electrodes are placed at the entrance of the side channels to control the voltage field allowing electrophoretic migration to occur, and electroosmosis if the source of flow in the particular channel. In this manner the invention provides for integration of preconcentration and analysis within the constrained fluid pathway.
- the injection channel 2 is perpendicular to the separation channel 4, although the geometry of this intersection is not of direct importance to the concepts presented here.
- Electrodes 5, 6 are located at the immediate entrances of channels 5, 6 and are electrically connected to the junction where the two channels 2, 4 intersect.
- materials of interest may be totally excluded from entering the adjoining channel or selectively permitted to enter the channel by using electrophoretic focusing techniques.
- a reservoir containing a buffer solution 5 is placed in fluid contact with a channel 12 and an electrode 9 is placed at the immediate entrance to that channel 11.
- the buffer reservoir is maintained at the same voltage as the entrance electrode, thus the material will not undergo electrophoretic migration within the reservoir. However, the charged materials will move toward the channel entrance at the same rate as the bulk flow.
- the effects of the applied voltage field influences the charged materials, thus inducing electrophoretic migration. Since the bulk flow within the channel is approximately equal to and opposite the electrophoretic migration, the charged material of interest stops.
- the flow rate of fluids may be controlled by, for example, the following techniques: pressure induced flow, capillary, and electroosmosis as taught by Giddings (1991, Unified Separations Science, Wiley-Interscience, New York, Chapt. 3). More specifically, pressure can be controlled by any physical or chemical means which will generate controllable flow or pressure. Capillarity can be controlled via chemical, electrochemical or photo-induced surface or solution changes as taught by Gallardo et al. (1999, Science 283:57-60). Electroosmosis can be controlled by external radial electrostatic fields as taught by Tsuda ( 1998, Handbook of Capillary Electrophoresis, Ed. J.P. Landers, 2 nd ed., CRC Press, Boca Raton , Chap. 22).
- the methods and devices of the present invention may be used for purposes of manipulating, testing, probing, or analyzing fluids of any kind where fluid manipulations may be used for preconcentration, chemical reaction, injection, detection, or movement or restriction of movement, of the materials of interest.
- the manipulations provided for by the methods and devices described herein will allow for precise liquid injection and handling within a micro-chemical analysis device in addition to the ability to increase local concentration of materials by several orders of magnitude.
- the capillary electrophoresis system was built and used a CZE1000R high voltage power supply from Spellman High Voltage Electronics Corporation (Hauppauge, New York).
- the vacuum pump system was purchased from Cenco Hyvac (Fort Wayne, IN).
- the laser source was a 442/325 nm 100 MPA: (Omnichrome Laser, Chino, Cat Scan).
- Image viewing was accomplished with a case closed-5E CCD camera (HutchNet, East Hartford, Construction) integrated to an Olympus Vanex stereo microscope (Tokyo, apan).
- Data collection and analysis were accomplished using Labview software and an Imaq Pci- 1408 image acquisition board by in-house program development (National Instruments, Austin, TX). Data analysis was also performed on Microsoft Excel spreadsheet program using an Optiplex GXI Pentium 233 (Dell Computer Corporation, Round Rock, TX).
- the fluorescent signal was monitored from the carboxylate modified latex micro spheres as vacuum and voltage fields were adjusted.
- Example 1 Experiments were performed to effectively demonstrate the increased local concentration of specific materials using a capillary 30 and reservoir 32 arrangement shown in Fig. 4.
- the tip of the capillary was coated with metal 34 thereby providing a metal electrode.
- These experiments were performed with fluorescence microscopy, fluorescently labeled latex microspheres, vacuum flow and a metal-coated capillary tip.
- the preconcentration build-up over time can be modeled as the formation as an exponential zone superimposed on a background of constant solute concentration for materials accumulating up behind a partially rejecting bar ⁇ er such a filter
- the filter in this case is the exclusion of the micro spheres from the capillary by the applied voltage field and the resulting electrophoretic migration rate
- the background concentration of the micro spheres is equal to J ⁇ /v
- the concentration of the micro spheres is given by c
- the flux of the micro spheres is given by J ⁇
- the velocity of the flow towards the barrier is v
- the original concentration of micro spheres is given by c 0
- the distance from the bar ⁇ er is given by y
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Abstract
The present invention generally relates to methods and devices for the control of the movement of fluids and electrically charged sample components within those fluids. More particularly, the present invention permits exclusion or concentration of specifically chosen sample components within a fluid. The present invention provides an analytical device, either microchip- or capillary-based, having the means to exclude specific sample components of interest from a capillary or channel for the purpose of preconcentration or control of movement of sample components. Such a control system includes a means for controlling the flow of the fluid in the channel and the placement of an electrode at the immediate entrance of each channel on such devices so that material may be directly manipulated by effects of both bulk flow and electrically driven migration.
Description
CONTROL OF FLOW AND MATERIALS FOR MICRO DEVTCES
INTRODUCTION
The present invention generally relates to methods and devices for the control of the movement of fluids and electrically charged sample components within those fluids. More particularly, the present invention permits exclusion or concentration of specifically chosen sample components within a fluid.
The present invention provides an analytical device, either microchip- or capillary-based, having the means to exclude specific sample components of interest from a capillary or channel for the purpose of preconcentration or control of movement of sample components. Such a control system includes a means for controlling the flow of the fluid in the channel and the placement of an electrode at the immediate entrance of each channel on such devices so that material may be directly manipulated by either or both of the effects of both bulk flow and electrically driven migration.
BACKGROUND OF THE INVENTION Capillary zone electrophoresis (CZE) is an efficient analytical separation technique which utilizes differences in mobility of sample components in an electric field based on the electrical charge and molecular site and shape of the sample component. Conventional CZE systems typically comprise a buffer- filled capillary with outlet and inlet ends disposed in two reservoirs into which one sample is injected, a means for applying voltage to the capillary resulting in migration of the sample through the capillary, and a means for detecting the sample zone.
Sample injection systems and capillary zone electrophoresis channel systems have been integrated together on planar glass substrates for separation of sample components as described by Harrison et al. (1992, Anal. Chem. 64:19261932) and Seiler et al. (1993, Anal. Cem. 65:1481-1488). Additionally, capillary electrophoresis on microchips has been described by Manz et al., (1992, J. of
Chromatography 593 253-258) Total chemical analysis systems (TAS) in which sample transport, chromatography or electrophoretic separations and detection are all performed have also been developed
One of the limitations of conventional CZE is the extremely small amount of sample which must be used in order to obtain separation or resolution of sample components The use of small volume samples results m low amount of sample components of interest representing a major limitation in the detectabihty of sample components On the other hand, the larger the sample volume introduced into the capillary, the broader the sample component peaks will be Attempts to increase injection sample volume typically leads to a breakdown in resolution due to broadening of the peaks attributable to individual sample components which one is actually trying to resolve or separate and possibly leads to generation of laminar flow mside the capillary
A number of techniques have been developed for increasing the concentration of specific sample components of interest and narrowing the width of the injected sample One such technique involves the use of a solid-phase adsorption medium followed by a sequential combination of pressure- and electrically-driven flows as described in United States Patent No 5,453,382 Using such a technique, the solution containing the sample component of interest is applied to the solid phase adsorption medium under conditions which permit sorption of the sample component of interest to the adsorption medium The environment of the medium is then altered to promote desorption of the concentrated sample component and a voltage gradient is induced across the medium to induce electroosmosis United States Patent No 5,340,452 also describes a similar method for increasing the concentration of sample components prior to electrophoresis by using an active material which selectively retains the sample components of interest at the inlet end of the capillary tube
For some specialized samples, another obstacle to successful separation of components of a solution results from the low strength of the electric field in the buffer bordering the sample solution and the column buffer To circumvent this problem, water or diluted buffer may be removed from the capillary or column using electro-osmotic flow while the sample components are stacked m a
support buffer thereby concentrating the sample components in a sample with a minimum amount of laminar flow Such a method is described in United States Patent No 5,116,471
For large volume samples m constrained containers, pressuπzed flow and countermigration can be used to increase the overall concentration as described by Hoπ et al (1993, Anal Chem 65 2882-2886) The sample is introduced into a first vessel containing buffer which is connected to another vessel by a glass tube An electrode extending into the first vessel applies a voltage to the sample while suction pressure is applied The sample concentration increases throughout the first vessel rather than concentrating the sample in a discrete portion of that vessel because the applied potential field is unconstrained throughout the buffei volume Because the concentration increase and electric fields are dispersed throughout the entire first vessel volume this technique is not applicable as a small volume ln ection/preconcentration technique Moreover, this arrangement does not allow for micromampulations such as electrophoretic separation withm the vessel containing the concentrated sample
Hence, none of the aforedescπbed methods provide for concentration of sample components upon immediate introduction into a constrained small volume flow path which receives a fluid sample without the use of complicated systems such as discontinuous buffer systems and, in some instances, microengmeered absorption devices Accordingly, there exists a need in the art for more precise and efficient methods and devices for increasing the concentiation of sample components of interest withm a fluid sample while maintaining a consistent buffer and without microengmeeπng absorption systems
SUMMARY OF THE INVENTION Accordingly, it is an object of the present invention to provide a novel, more efficient method for controlling the movement of fluids and electrically charged species, referred to as sample components, withm those fluids which permits exclusion or concentration of specifically chosen species withm a constrained fluid flow path
It is another object of the invention to provide an analytical electrophoretic arrangement including microchips or capillaries which excludes specific sample components of interest from a capillary or channel for the purposes of preconcentration or control of movement of materials. It is a further object of the present invention to provide an arrangement in which preconcentration and manipulation is achieved within a single constrained flow pathway system. More particularly, the sample is preconcentrated in a portion of the constrained flow pathway and is manipulated as it travels through the pathway.
These and other objects of the invention are obtained by a method for controlling the movement of a specific sample component in a fluid sample comprising:
(a) providing a constrained fluid pathway having an inlet;
(b) introducing the fluid sample into the inlet of the constrained fluid pathway; (c) providing an electrode mounted at the inlet of the fluid pathway, the electrode being entirely external to the constrained fluid pathway;
(d) applying voltage to the electrode to create a voltage gradient within the constrained fluid pathway to promote electrophoretic migration of the sample component; and
(e) adjusting the flow rate of the fluid approximately equal to and opposite to the electrophoretic migration of the sample.
(f) adjusting the electrophoretic migration rate to be approximately equal and opposite to the flow rate of the fluid. wherein movement of the specific sample component ceases.
The invention further provides an electrophoretic apparatus for controlling the movement of an sample component in a fluid sample comprising:
(a) at least one constrained fluid pathway having an inlet and an electrode mounted at the inlet of the constrained fluid pathway and entirely external to the constrained fluid pathway; and -
(b) a power supply for supplying a voltage to the electrode.
It is another object of the invention to provide an electrophoretic apparatus for controlling the movement of an sample component in a fluid sample comprising
(a) at least one injection fluid pathway having an electrode mounted at the inlet of said the pathway,
(b) at least one separation fluid pathway having an electrode mounted at the mlet of said pathway,
(c) at least one power supply for providing voltage between the electrodes, and (d) means for regulating the bulk flow withm the channels
The present invention can be utilized m methods and devices for manipulating, testing, probing, or analyzing sample fluids of any kind where fluid manipulations are utilized for preconcentration, chemical reaction, injection, detection, or movement, or cessation of movement, of components of interest m a sample fluid
In one embodiment, the present invention is directed to an analytical device having a plurality of channels with electrodes placed at the immediate entrance of all or selected channels and a method for regulating the bulk flow withm the channels When the bulk flow is set approximately equal to and opposite the electrophoretic migration of specific sample components of interest, the movement of those specific sample components ceases The introduction of an electric field between the electrodes within the channel, coupled with control of bulk flow, allows selected sample components of interest to be excluded or preconcentrated immediately upon introduction of the fluid sample into the channel.
BRIEF DESCRIPTION OF THE DRAWINGS Further objects and advantages of the invention will be apparant from a reading of the following description m conjunction with the accompanying drawings, in which: Figure 1 is a schematic drawing of a fused silica capillary arrangement with electrodes placed immediately at the mlet to provide the voltage control withm
the capillary in accordance with the invention;
Figures 2(a), 2(b) and 2(c) are schematic drawings of a micro-device apparatus having an injection channel and a separation channel in accordance with the invention; Figure 3 is a schematic drawing of a micro-device apparatus indicating the preconcentration of materials at the immediate entrance to a channel where the voltage with in the buffer reservoir is held constant in accordance with the invention;
Figure 4 is a schematic drawing of the theoretical profile of the preconcentration of material at the immediate entrance to a capillary showing the concentration of desired materials;
Figure 5 is a graph showing the normalized fluorescence intensity versus distance outside the capillary entrance for two control experiments;
Figure 6 is a graph showing the normalized fluorescence intensity versus number of pixels (1 pixel - 0.24 μm) outside a capillary entrance ;and Figures 7(a) and (b) are fluorescence micrographs of a capillary entrance before and after, respectively, preconcentration of 200 nm fluorescently labeled latex micro spheres for 270 seconds.
DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENTS The present invention provides novel methods and devices for exclusion or concentration of specifically chosen sample components within fluids through the control of fluid movement and electrophoretic migration of charged sample components within those fluids. Typically the fluid sample is delivered or injected into a restricted flow path such as a channel or capillary. For purposes of the present invention, the flow path is preferably less than 200 microns in diameter. Precise control of fluid manipulation, sample component movement and solution injection systems are accomplished by carefully controlling the voltage field gradients and the bulk flow within each channel on a micro-device.
The principle of electrophoretic focusing as a means of sample component exclusion from a capillary or channel can be applied to the microscale analytical device described herein. The apparatus and processes disclosed herein may
be used on microchip instrumentation in conjunction with control fluid dynamics in channels formed into oi onto semiconductor devices As used herein, the term "microchip" includes a semiconductor device comprising silica or any other substrate which may be used m micro fluidic devices, which may be used in or in conjunction with a computer
The present invention also provides for the placement of an electrode at the immediate entrance of each channel on a micro-device so that material movement may be dnectly manipulated by electπcally-dπven migration, 1 e , electrophoretic migration The present invention also provides control of bulk flow of the fluid withm the channel Bulk flow may be positive or negative depending upon the magnitude and direction of electrically-driven flow, l e , electroosmosis, or various other sources of flow such as pressure, convection, capillarity, etc Voltage gradients may likewise be manipulated to provide electrophoretic migration m either direction The introduction of an electric field lesultmg in electrophoretic migration of a specific sample component, coupled with manipulation of bulk flow equal and opposite to electrophoretic migration, results in cessation of movement of those specific sample components Thus, the independent control of these parameters provides for absolute control of movement of sample components withm the fluid about a micro-device
The method of the invention compπses as a first step, the introduction of a sample containing the sample component of interest into a channel or capillary that has been filled with buffer Sample introduction may be accomplished using a syringe by which the sample solution is injected into the channel Alternatively, the introduction of the sample can be performed according to standard procedures, including but not limited to the use of electroosmotic flow, electro-kmetic pumping, or pneumatic pumping
An electrophoretic arrangement in which a capillary is utilized to create the restπcted flow path is shown m Figure 1 In this arrangement electrodes 20 are located external to and mounted onto a fused silica capillary A counter electrode 24 is placed at a location remote from electrodes 20 and fornis a circuit therewith A
high voltage is applied to the electrodes 20 and 24 by power supply 26 A reservoir 28 including buffer bulk flow mateπals is in fluid contact with the capillary A sample 5 including charged components is introduced into the reservoir and moves towards the entrance 9 of the capillary m the presence of the applied voltage which induces electrophoretic migration Thus, the charged components m analyte 5 aie concentrated at the entrance 9 of the capillary 22
The present invention also provides a micro-analytical separation device comprised of etched or molded channels whereby various channels are used for separation and analysis purposes and others are distinctly used for the purpose of injection or material movement illustrated in Figs 2(a-c) As shown m Figure 2a the system includes an injection channel 2 and sepaiation channel 4 Sample material is injected to fill the injection channel 2 m between the separation channels 4 as depicted m Figure 2b To prevent unintentional introduction of material movement, commonly referred to as trailing or leaking, into the mam separation channel after injection ceases, a small voltage is applied to the two injection channel electrodes 5 As illustrated m Figure 2c, after the initial injection the electrodes are used to create an appropriate voltage gradient to prevent unwanted introduction of materials into the separation channel thereby concentrating desired components m separation channel 4 By manipulating flow and the voltage fields independently, positive, negative and neutral molecules may be manipulated as a group or individually
A high voltage is applied by power supply means between the mlet and outlet end of the channel or capillary through electrode means The voltage used is not critical to the invention and may vary widely depending on the sample component(s) to be excluded or concentrated Conditions for selecting appropriate voltage conditions will depend on the physical properties of the sample component(s) and can be determined by those of skill m the art
To preconcentrate sample components of either positive or negative charge, the method of the invention further comprises setting the bulk flow in the channel or capillary approximately equal to and opposite to the electrophoretic migration rate of the material The bulk flow m the capillary may be generated and controlled by either electroosmosis, pressure or various other mechanisms Bulk flow
may be created and controlled by electroosmotic pumping devices, pneumatic devices, or directly by electroosmosis with dynamic control and monitoring. Thus the sample component of interest is drawn toward the channel by bulk flow, but is excluded from the channel by the voltage field effects on a narrow range of materials with similar electrophoretic migration rates thereby excluding or concentrating the sample component of interest at the immediate entrance of the capillary or channel.
Alternatively, any constrained fluid pathway, for example a fused silica or teflon capillary, where separation or injection of materials of interest are performed may be included in the device. Each channel or continuous fluid pathway where control of material movement is desired is constructed with an electrode adjoining the entrance and exit of the channel or pathway. Electrodes are placed at the entrance of the side channels to control the voltage field allowing electrophoretic migration to occur, and electroosmosis if the source of flow in the particular channel. In this manner the invention provides for integration of preconcentration and analysis within the constrained fluid pathway.
In the preferred embodiment of the invention as shown in Figure 2a-c, the injection channel 2 is perpendicular to the separation channel 4, although the geometry of this intersection is not of direct importance to the concepts presented here. Electrodes 5, 6 are located at the immediate entrances of channels 5, 6 and are electrically connected to the junction where the two channels 2, 4 intersect.
Placement of an electrode at the immediate entrance of a capillary or channel and at the junction with another channel or buffer reservoir, creates a chemical voltage gate, in that movement of materials may be independently controlled by simply varying the voltage field gradient and the flow rate within the particular channel. At this chemical voltage gate, materials of interest may be totally excluded from entering the adjoining channel or selectively permitted to enter the channel by using electrophoretic focusing techniques.
In another embodiment of the invention shown in Figure 3 a reservoir containing a buffer solution 5 is placed in fluid contact with a channel 12 and an electrode 9 is placed at the immediate entrance to that channel 11. The buffer reservoir is maintained at the same voltage as the entrance electrode, thus the material
will not undergo electrophoretic migration within the reservoir. However, the charged materials will move toward the channel entrance at the same rate as the bulk flow. At the immediate entrance of the channel the effects of the applied voltage field influences the charged materials, thus inducing electrophoretic migration. Since the bulk flow within the channel is approximately equal to and opposite the electrophoretic migration, the charged material of interest stops.
The flow rate of fluids may be controlled by, for example, the following techniques: pressure induced flow, capillary, and electroosmosis as taught by Giddings (1991, Unified Separations Science, Wiley-Interscience, New York, Chapt. 3). More specifically, pressure can be controlled by any physical or chemical means which will generate controllable flow or pressure. Capillarity can be controlled via chemical, electrochemical or photo-induced surface or solution changes as taught by Gallardo et al. (1999, Science 283:57-60). Electroosmosis can be controlled by external radial electrostatic fields as taught by Tsuda ( 1998, Handbook of Capillary Electrophoresis, Ed. J.P. Landers, 2nd ed., CRC Press, Boca Raton , Chap. 22).
The methods and devices of the present invention may be used for purposes of manipulating, testing, probing, or analyzing fluids of any kind where fluid manipulations may be used for preconcentration, chemical reaction, injection, detection, or movement or restriction of movement, of the materials of interest. The manipulations provided for by the methods and devices described herein will allow for precise liquid injection and handling within a micro-chemical analysis device in addition to the ability to increase local concentration of materials by several orders of magnitude.
Preparation of specific embodiments in accordance with the present invention will now be described in further detail. These examples are intended to be illustrative and the invention is not limited to the specific materials and methods set forth in these embodiments.
The examples discussed hereinafter were conducted using the following standard chemicals and instrumentation, unless otherwise stated: Chemicals and Materials. Sodium dihydrogen phosphate and anhydrous ethyl alcohol (Aldrich Chemical Company, Milwaukee, WI); and
phosphoric acid (EMG NCV Science, Gibbstown, NEW IERSEY) were used as received. Capillaries were 45 cm in length (150 μm o.d. - 20 μm i.d.) fused silica and were purchased from Polymicro Technologies (Phoenix, AZ). 0.2 μm carboxylate modified yellow-green fluorescent (505/515) latex micro spheres were purchased from Molecular Probes (Eugene, OR). The capillary electrophoresis buffer used for the latex micro sphere experiments was 100 mM phosphate buffer, adjusted with phosphoric acid to pH 5.1.
Instrumentation. The capillary electrophoresis system was built and used a CZE1000R high voltage power supply from Spellman High Voltage Electronics Corporation (Hauppauge, New York). The vacuum pump system was purchased from Cenco Hyvac (Fort Wayne, IN). The laser source was a 442/325 nm 100 MPA: (Omnichrome Laser, Chino, Cat Scan). Image viewing was accomplished with a case closed-5E CCD camera (HutchNet, East Hartford, Construction) integrated to an Olympus Vanex stereo microscope (Tokyo, apan). Data collection and analysis were accomplished using Labview software and an Imaq Pci- 1408 image acquisition board by in-house program development (National Instruments, Austin, TX). Data analysis was also performed on Microsoft Excel spreadsheet program using an Optiplex GXI Pentium 233 (Dell Computer Corporation, Round Rock, TX). The fluorescent signal was monitored from the carboxylate modified latex micro spheres as vacuum and voltage fields were adjusted.
Example 1 Experiments were performed to effectively demonstrate the increased local concentration of specific materials using a capillary 30 and reservoir 32 arrangement shown in Fig. 4. The tip of the capillary was coated with metal 34 thereby providing a metal electrode. These experiments were performed with fluorescence microscopy, fluorescently labeled latex microspheres, vacuum flow and a metal-coated capillary tip.
The presence or location of carboxylate-modified latex spheres were directly observed with the microscope under the effects of vacuum induced flow. The voltage was then empirically adjusted until the micro spheres were excluded from entering the capillary due to the electrophoretic migration rate of the micro spheres.
The intensity of the fluorescent signal which is directly related to concentration was monitored Only a selected probe area, of approximately 2 5 μm x 120 μm parallel, and centered with the bore of the capillary immediately outside the entrance was quantitated for the fluorescence intensity changes First, control experiments were performed to determine if adsorption or other unknown processes were responsible for the increased fluorescence These control experiments consisted of using either the voltage field only (- 14 kV) or the vacuum-induced flow only 1 2 m Hg across a 45 cm long, 20 μm l d capillary As illustrated in Figure 5 the fluorescent signal was monitored and quantitated for 4 minutes The fluorescent signal was normalized with the fluorescent signal obtained at t = 0 minutes to eliminate any existing background fluorescence from the temporal data The normalized fluorescent signal of the control experiments remained at a value of 1 75±9 32 (n = 11 ) thioughout the 4 minutes of the experiment (Figure 6) No increase m fluorescent intensity was observed over the experimental period indicating that no unknown mechanisms nor adsorption to the capillary tip and walls contributed to the mci eased fluorescent intensity m the following experiments
Experiments were performed to demonstrate preconcentration once the electrophoretic migration rate withm the channel in the capillary was adjusted to be equal to and opposite the bulk buffer low rate As with the control experiments, the fluorescence intensity was nonnahzed and then monitored for 4 minutes (n = 4), The voltage empirically determined to generate an electrophoretic migration rate which counterbalanced the bulk flow rate was 14kV Figures 7(a) and (b) are fluorescence micrographs of a capillary entrance before and after, respectively, preconcentration of 200 nm fluorescently labeled latex micro spheres for 270 seconds As illustrated Figure 7b and Figure 4 the largest fluorescence intensity changes occurred withm 33 μm of the capillary entrance Due to dynamic range limitations, the fluorescent intensity at the entrance to the capillary saturated the CCD and therefore quantitation of this effect must be performed some 19 2 μm outside the entrance to the capillary The normalized fluorescent signal at 19 2 μm resulted in an increase in fluorescence intensity approximated by a linear equation (y = mx + b) where m is 0 042 arb units/mm and b is 0 99 arb units (R2= 0 938, P _: 0 01) The initial concentration of
the micro-spheres was 1 473 x 1010 micro spheres/mL
The preconcentration build-up over time can be modeled as the formation as an exponential zone superimposed on a background of constant solute concentration for materials accumulating up behind a partially rejecting barπer such a filter The filter in this case is the exclusion of the micro spheres from the capillary by the applied voltage field and the resulting electrophoretic migration rate Assuming the system will reach steady state conditions after a given time, the background concentration of the micro spheres is equal to Jα/v , initial flux over velocity The concentration build-up of the micro spheres is given by the following equation c = JBv + (c0-Jαl v)exp(-lvly/D7) where the concentration of the micro spheres is given by c, the flux of the micro spheres is given by Jα, the velocity of the flow towards the barrier is v, the original concentration of micro spheres is given by c0, the distance from the barπer is given by y, and the total diffusion of the micro spheres is given by D, A plot of concentration of desired components versus location m the arrangement is shown m Figure 4
Although the present invention has been described with reference to latex micro spheres and fused silica capillaries piovidmg the constrained fluid pathway, it should be understood that various modifications and variations can be easily made by those skilled m the art without departing from the spirit of the invention Such modifications are intended to fall withm the scope of the claims Accordingly, the foregoing disclosure should be interpreted as illustrative only and not m a limiting sense Vaπous publications are cited herein, the contents of which are incorporated, by reference, in their entireties
Claims
1. A method for controlling the movement of a specific sample component in a fluid sample comprising:
(a) providing a constrained fluid pathway having an inlet; (b) introducing the fluid sample into the inlet of the constrained fluid pathway; (c) providing an electrode mounted at the inlet of the fluid pathway, the electrode being entirely external to the constrained fluid pathway; (d) applying voltage to the electrode to create a voltage gradient within the constrained fluid pathway to promote electrophoretic migration of the sample component; and (e) adjusting the flow rate of the fluid approximately equal to and opposite to the electrophoretic migration; wherein movement of the specific sample component ceases.
2. The method of claim 1 wherein the constrained fluid pathway is a channel.
3. The method of claim 1 wherein the constrained fluid pathway is a capillary tube.
4. The method of claim 1 wherein the constrained fluid pathway is less than 200 microns in diameter.
5. The method of claim 1 wherein the flow rate of the fluid sample is controlled by electroosmosis.
6. The method of claim 1 wherein the flow rate of the fluid sample is controlled by pressure. 7 The method of claim 1 wherein the constrained fluid pathway is a channel on a microchip
8 An electrophoretic apparatus for controlling the movement of an sample component m a fluid sample comprising (a) at least one constrained fluid pathway having an mlet and an electrode mounted at the mlet of the constrained fluid pathway and entirely external to the constrained fluid pathway, and (b) a power supply for supplying a voltage to the electrode
9 The apparatus of claim 8 wherein the constrained fluid pathway is a channel located on a microchip
10 The apparatus of claim 8 wherein the constrained fluid pathway is a capillary
11 The apparatus of claim 8 further comprising a buffer reservoir for containing a buffer solution in fluid contact with the constrained fluid pathway
12 The apparatus of claim 8 wherein the constrained fluid pathway is a channel m a microchip
13 The apparatus of claim 8 wherein the constrained fluid pathway is a capillary
14 The apparatus of claim 8 wherein the diameter of the constrained fluid pathway is less than 200 microns m diameter
15 An electrophoretic apparatus for controlling the movement of an sample component m a fluid sample comprising
(a) at least one injection fluid pathway having an electrode mounted at the mlet of said the pathway, (b) at least one separation or further fluid transfer fluid pathway having an electrode mounted at the inlet of said pathway,
(c) at least one power supply for providing voltage to the electrodes, and
(d) means for regulating the bulk flow withm the channels
The method of claim 15 wherein the constrained fluid pathway is a channel m a microchip
The method of claim 15 wherein the constrained fluid pathway is a capillary
Priority Applications (4)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| JP2000553795A JP2002517751A (en) | 1998-06-11 | 1999-06-11 | Flow and material control for microdevices |
| CA002328400A CA2328400A1 (en) | 1998-06-11 | 1999-06-11 | Control of flow and materials for micro devices |
| EP99927515A EP1092147A1 (en) | 1998-06-11 | 1999-06-11 | Control of flow and materials for micro devices |
| US09/701,662 US6890411B1 (en) | 1998-06-11 | 1999-06-29 | Control of flow and materials for micro devices |
Applications Claiming Priority (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US8895698P | 1998-06-11 | 1998-06-11 | |
| US60/088,956 | 1998-06-11 |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| WO1999064851A1 true WO1999064851A1 (en) | 1999-12-16 |
Family
ID=22214492
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| PCT/US1999/013340 WO1999064851A1 (en) | 1998-06-11 | 1999-06-11 | Control of flow and materials for micro devices |
Country Status (4)
| Country | Link |
|---|---|
| EP (1) | EP1092147A1 (en) |
| JP (1) | JP2002517751A (en) |
| CA (1) | CA2328400A1 (en) |
| WO (1) | WO1999064851A1 (en) |
Cited By (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US9052262B2 (en) | 2010-01-27 | 2015-06-09 | Izon Science Limited | Control of particle flow in an aperture |
| US11090660B2 (en) | 2016-08-10 | 2021-08-17 | Arizona Board Of Regents On Behalf Of Arizona State University | Hyper efficient separations device |
Families Citing this family (1)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US7695689B2 (en) | 2002-07-18 | 2010-04-13 | National Institute Of Advanced Industrial Science And Technology | Micro reactor device and method of manufacturing micro reactor device |
Citations (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US5200050A (en) * | 1991-10-25 | 1993-04-06 | Washington State University Research Foundation | Electrophoretic processor and methods |
| US5453382A (en) * | 1991-08-05 | 1995-09-26 | Indiana University Foundation | Electrochromatographic preconcentration method |
| WO1996004547A1 (en) * | 1994-08-01 | 1996-02-15 | Lockheed Martin Energy Systems, Inc. | Apparatus and method for performing microfluidic manipulations for chemical analysis and synthesis |
| WO1996027793A1 (en) * | 1995-03-03 | 1996-09-12 | Alltech Associates, Inc. | Apparatus/method for electrochemically modifying chromatographic material |
-
1999
- 1999-06-11 CA CA002328400A patent/CA2328400A1/en not_active Abandoned
- 1999-06-11 JP JP2000553795A patent/JP2002517751A/en active Pending
- 1999-06-11 EP EP99927515A patent/EP1092147A1/en not_active Withdrawn
- 1999-06-11 WO PCT/US1999/013340 patent/WO1999064851A1/en not_active Application Discontinuation
Patent Citations (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US5453382A (en) * | 1991-08-05 | 1995-09-26 | Indiana University Foundation | Electrochromatographic preconcentration method |
| US5200050A (en) * | 1991-10-25 | 1993-04-06 | Washington State University Research Foundation | Electrophoretic processor and methods |
| WO1996004547A1 (en) * | 1994-08-01 | 1996-02-15 | Lockheed Martin Energy Systems, Inc. | Apparatus and method for performing microfluidic manipulations for chemical analysis and synthesis |
| WO1996027793A1 (en) * | 1995-03-03 | 1996-09-12 | Alltech Associates, Inc. | Apparatus/method for electrochemically modifying chromatographic material |
Non-Patent Citations (1)
| Title |
|---|
| MANZ A ET AL: "ELECTROOSMOTIC PUMPING AND ELECTROPHORETIC SEPARATIONS FOR MINIATURIZED CHEMICAL ANALYSIS SYSTEMS", JOURNAL OF MICROMECHANICS & MICROENGINEERING, vol. 4, no. 4, 1 December 1994 (1994-12-01), pages 257 - 265, XP000601273, ISSN: 0960-1317 * |
Cited By (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US9052262B2 (en) | 2010-01-27 | 2015-06-09 | Izon Science Limited | Control of particle flow in an aperture |
| US11090660B2 (en) | 2016-08-10 | 2021-08-17 | Arizona Board Of Regents On Behalf Of Arizona State University | Hyper efficient separations device |
| US11806729B2 (en) | 2016-08-10 | 2023-11-07 | Arizona Board Of Regents On Behalf Of Arizona State University | Hyper efficient separations device |
Also Published As
| Publication number | Publication date |
|---|---|
| JP2002517751A (en) | 2002-06-18 |
| EP1092147A1 (en) | 2001-04-18 |
| CA2328400A1 (en) | 1999-12-16 |
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