Apparatuses and methods consistent with exemplary embodiments relate to a microfluidic structure in which a sample is efficiently distributed to a plurality of chambers and distribution speed and supply speed of a fluid are adjustable, and a microfluidic device having the same.
Microfluidic devices are used to perform biological or chemical reactions by manipulating small amounts of fluid.
A microfluidic structure provided in a microfluidic device to perform an independent function generally includes a chamber to accommodate a fluid, a channel allowing the fluid to flow therethrough, and a member (e.g., valve) to regulate the flow of the fluid. The microfluidic structure may include various combinations of such structures. A device fabricated by disposing such a microfluidic structure on a chip-shaped substrate to perform multi-step processing and manipulation to conduct a test involving an immune serum reaction or biochemical reaction on a small chip is referred to as a lab-on-a chip.
To transfer a fluid in a microfluidic structure, driving pressure is needed. Capillary pressure or pressure generated by a separate pump may be used as the driving pressure. Recently, a disc type microfluidic device which has a microfluidic structure arranged on a disc-shaped platform to move a fluid using centrifugal force to perform a series of operations has been proposed. This device is referred to as a “Lab CD” or “Lab-on a CD.”
In a microfluidic structure, adjusting a fluid such as a sample or reaction solution to a fixed amount and regulating the flow of the fluid through the chambers may be important. To perform such adjustment and regulation, a separate valve may be mounted to a channel. However, a separate driving source may be required to open and/or close the valve in this case.
A siphon channel that does not require such a separate driving source has been proposed to overcome this problem. However, the conventional siphon channel is installed between a sample supply chamber and a distribution channel and is used only for distribution of a sample, and conventional cases have not proposed how to transfer the distributed sample.
Exemplary embodiments provide a microfluidic structure in which a plurality of chambers are arranged at different positions and connected in parallel, and a fixed amount of fluid may thus be efficiently distributed to the chambers without using a separate driving source by connecting one chamber to another chamber for subsequent operation through a siphon channel, and a microfluidic device having the same.
In accordance with an aspect of an exemplary embodiment, there is provided a microfluidic device including a platform having a center of rotation and including a microfluidic structure, wherein the microfluidic structure includes a plurality of first chambers arranged in a circumferential direction of the platform at different distances from the center of rotation; and a plurality of first siphon channels, each of the plurality of first siphon channels being connected to a corresponding first chamber of the plurality of the first chambers.
The microfluidic structure further includes a sample supply chamber configured to accommodate a sample and including a discharge outlet, and a distribution channel connected to the discharge outlet of the sample supply chamber and to the plurality of first chambers, the distribution channel being configured to distribute the sample in the sample supply chamber to the plurality of first chambers.
The first chambers may be arranged such that each of the plurality of first chambers is arranged further from the center of rotation than an adjacent first chamber of the plurality of first chambers to which the sample flows earlier.
The plurality of first chambers may be arranged such that a first chamber of the plurality of first chambers having a larger sequence number along the distribution channel is more distant from the center of rotation than another first chamber having a smaller sequence number.
The first chambers may be arranged in a direction along the distribution channel such that a first chamber of the plurality of first chambers positioned at a greater distance from the discharge outlet of the sample supply chamber than another first chamber of the plurality of first chambers is more distant from the center of rotation of the platform than the other first chamber.
The plurality of first chambers may be spirally arranged around the center of rotation of the platform.
Each of the plurality of first siphon channels may have a crest point at a position higher than a full fluid level of a corresponding first chamber connected thereto.
Widths of the plurality of first siphon channels may be between about 0.01 mm and about 3 mm, and depths of the plurality of first siphon channels may be between about 0.01 mm and about 3 mm.
The microfluidic structure may further include at least one reaction chamber connected to at least one second chamber of the plurality of second chambers.
The plurality of first chambers, the plurality of second chambers and the reaction chamber may be arranged further from the center of rotation than the sample supply chamber.
At least one of the plurality of second chambers may accommodate a first marker conjugate to specifically bind with an analyte in the sample, wherein the first marker conjugate may be a conjugate of a marker and a capture material to specifically bind with the analyte.
The reaction chamber may include a detection region having the capture material and the capture material specifically binds with the analyte immobilized thereon.
The detection region may be formed by one selected from the group consisting of a porous membrane, a micropore and a micro-pillar to move the sample according to capillary force.
The microfluidic structure may further include a magnetic body disposed in a chamber disposed at a position adjacent to the reaction chamber.
In accordance with an aspect of another exemplary embodiment, there is provided a microfluidic structure formed on a platform, the microfluidic structure including a sample supply chamber configured to accommodate a sample and including a discharge outlet, a distribution channel connected to the discharge outlet of the sample supply chamber, a plurality of first chambers connected to the distribution channel, configured to receive the sample supplied through the distribution channel, and respectively arranged at different radii from a center of rotation of the platform, and a plurality of siphon channels, each of the plurality of siphon channels being connected to a corresponding first chamber of the plurality of first chambers.
The plurality of first chambers may be arranged at an increasing order of the radii from the center of rotation which may correspond to a sequence of supply of the sample to the plurality of first chambers.
The plurality of first chambers may be arranged at an increasing order of the radii from the center of rotation which may correspond to a sequence of flow of the sample through the distribution channel.
The plurality of first chambers may be arranged at an increasing order of the radii from the center of rotation which may correspond to a sequence of supply of the sample.
The plurality of first chambers may be arranged at an increasing order of the radii from the center of rotation which may correspond to an increasing order of distances of the first chambers from the discharge outlet of the sample supply chamber along the distribution channel.
Each of the plurality of siphon channels may have a crest point at a position higher than a full fluid level of the corresponding first chamber connected thereto.
Widths of the plurality of siphon channels may be between about 0.01 mm and about 3 mm, and depths of the plurality of siphon channels may be between about 0.01 mm and about 3 mm.
The microfluidic structure may further include at least one reaction chamber connected to at least one of the plurality of second chambers.
The plurality of first chambers, the plurality of second chambers and the reaction chamber may be arranged further from a center of rotation than the sample supply chamber.
Disposed in at least one of the second chambers may be a first marker conjugate, wherein the first marker conjugate specifically binds to an analyte in the sample.
The reaction chamber may include a detection region having a capture material to specifically bind with the analyte immobilized thereon.
The detection region may be formed by one selected from the group consisting of a porous membrane, a micropore and a micro-pillar to move the sample according to capillary force.
The microfluidic structure may further include a magnetic body disposed in a chamber disposed at a position adjacent to the reaction chamber.
The microfluidic structure may further include a metering chamber disposed between the at least one second chamber and the at least one reaction chamber and configured to meter an amount of a fluid transferred from the at least one second chamber, and a fluid transfer assist unit connected between the metering chamber and the at least one reaction chamber.
The fluid transfer assist unit may include a fluid passage configured to transfer the fluid accommodated in the metering chamber to into the reaction chamber.
The fluid transfer assist unit may further include a fluid guide configured to guide movement of the fluid accommodated in the metering chamber to the fluid passage.
The microfluidic structure may further include a second siphon channel having one end connected to the metering chamber, and a waste chamber connected to the other end of the second siphon channel.
After the fluid accommodated in the metering chamber is transferred to the reaction chamber, the second siphon channel may transfer the fluid sample flowing thereinto to the waste chamber.
The microfluidic structure may further include a magnetic body accommodated in a chamber.
In accordance with another aspect, a test device is provided. The test device includes the microfluidic device, a rotary drive unit configured to rotate a platform of the microfluidic device, a magnetic module configured to be movable in a radial direction of the platform; and a controller configured to control the rotary drive unit and the magnetic module.
When a fluid is to be transferred from the metering chamber to the reaction chamber, the controller is configured to rotate the platform and at a predefined time during rotation of the platform, move the magnetic module to a position over or under the platform such that the magnetic module faces the magnetic body.
In accordance with an aspect of another exemplary embodiment, there is provided a method of controlling a microfluidic device including a platform provided with a second chamber configured to accommodate a fluid, a third chamber configured to meter the amount of the fluid, a fourth chamber configured to have a chromatographic reaction to occur therein using the fluid metered in the third chamber and introduced thereinto, and a channel to connect the second chamber, the third chamber and the fourth chamber to each other, the method including rotating the platform and transferring the fluid accommodated in the second chamber to the third chamber, and repeating intervals comprising increasing a rotational speed of the platform and stopping thereof, such that the fluid flows into the fourth chamber.
The method may further include, upon transferring the fluid to the third chamber, stopping the platform such that a first order reaction occurs between the fluid and a marker conjugate accommodated in the third chamber.
The method may further include, upon introduction of the fluid into the fourth chamber, stopping the platform.
The method may further include, when the platform is stopped, absorbing the fluid a detection region provided in the fourth chamber, and transferring the fluid remaining in the third chamber to the fourth chamber.
The method may further include, allowing a chromatographic reaction to occur in the fourth chamber, and thereafter, rotating the platform to remove the fluid remaining in the fourth chamber.
The above and/or other aspects will become apparent and more readily appreciated from the following description of exemplary embodiments, taken in conjunction with the accompanying drawings of which:
Reference will now be made in detail to exemplary embodiments, examples of which are illustrated in the accompanying drawings, wherein like reference numerals refer to tike elements throughout.
Referring to
The microfluidic structure includes a plurality of chambers to accommodate a fluid and a channel to connect the chambers.
Here, the microfluidic structure is not limited to a structure with a specific shape, but comprehensively refers to structures including channels connecting the chambers to each other and formed on or within the microfluidic device, especially on the platform of the microfluidic device to allow the flow of a fluid. The microfluidic structure may perform different functions depending on the arrangements of the chambers and the channels, and the kind of the fluid accommodated in the chambers or flowing along the channels.
The platform 100 may be made of various materials including plastics such as polymethylmethacrylate (PMMA), polydimethylsiloxane (PDMS), polycarbonate (PC), polypropylene, polyvinyl alcohol and polyethylene, glass, mica, silica and silicon (in the form of a wafer), which are easy to work with and whose surfaces are biologically inactive. The above materials are simply examples of materials usable for the platform 100, and the exemplary embodiments disclosed herein are not limited thereto. Thus, any material having proper chemical and biological stability, optical transparency and mechanical workability may be used as a material of the platform 100.
The platform 100 may be formed in multiple layers of plates. A space to accommodate a fluid within the platform 100 and a channel allowing the fluid to flow therethrough may be provided by forming intaglio structures corresponding to the microfluidic structures, such as the chambers and the channels, on the contact surfaces of two plates, and thereafter, joining the plates. The joining of two plates may be accomplished using any of various techniques such as bonding with an adhesive agent or a double-sided adhesive tape, ultrasonic welding, and laser welding.
The illustrated exemplary embodiment of
The microfluidic device 10 may be mounted to a test device 300 including a drive unit 310 and a controller 320, and may be rotated by the drive unit 310 as shown in
More specifically, the drive unit 310 includes a motor to provide rotational force to the platform 100, thereby enabling fluids accommodated in chambers disposed in the platform 100 to move to other chambers according to centrifugal force. Rotation of the platform 100 through the drive unit 310, as well as overall operations of the test device 300 including positioning a magnet and detecting by a detection unit, which will be described later, may be controlled by the controller 320.
A platform 100 may be provided with one test unit. However, for faster throughput at lower cost, the platform 100 may be divided into a plurality of sections, and each section may be provided with independently operable microfluidic structures. The microfluidic structures may perform different tests and/or may perform several tests at the same time. Alternatively, a plurality of test units that perform the same test may be provided. For convenience of description of the illustrated exemplary embodiment, a description will be given of a case in which a chamber to receive a sample from a sample supply chamber and a channel connected to the chamber form a single unit, and different units may receive the sample from different sample supply chambers.
Since the microfluidic device to according to the illustrated embodiment causes a fluid to move using centrifugal force, the chamber 130 to receive the fluid is disposed at a position more distant from the center C of the platform 100 than the position of the chamber 120 to supply the fluid, as shown in
The two chambers are connected by a channel 125, and in the microfluidic device 10 of the illustrated embodiment, a siphon channel may be used as the channel 125 to control the fluid flowing therethrough.
As used herein, the term “siphon” refers to a channel that causes a fluid to move using a pressure difference. In the microfluidic device 10, the flow of the fluid through the siphon channel is controlled using capillary pressure that forces the fluid to move up through a tube having a very small cross-sectional area and centrifugal force generated by rotation of the platform 100.
The graph of
Referring to
In the illustrated embodiment as described below, the chambers to receive a fluid sample from the sample supply chamber 110 are referred to as first chambers 120, and the chambers to which the fluid sample is transferred from the first chambers are referred to as second chambers 130. In addition, according to the sample supply sequence, the first chambers 120 are respectively referred to as a “1-1”-th chamber 120-1 to a “1-n”-th chamber 120-n. The second chambers 130 are respectively referred to as a “2-1”-th chamber 130-1 to a “2-n”-th chamber 130-n according to the first chambers connected thereto. The other chambers subsequently connected are defined in the same manner. Also, for convenience of description, when the term “first chambers 120” is used throughout, it means at least one of the first chambers 120-1 to 120-n. This is also applied to the other structures ranging from the second chambers 130 to the fifth chambers 170 (see
The “1-1”-th chamber 120-1 to the “1-n”-th chamber 120-n, which are the first chambers 120, are connected to the sample supply chamber 110 through the distribution channel 115, and are respectively connected to the “2-1”-th chamber 130-1 to the “2-n”-th chamber 130-n, which are the second chambers 120, through the siphon channel 125.
As shown in
Specifically, the “1-1”-th chamber 120-1 that first receives the sample from the sample supply chamber 110 is disposed on a circumference closest to the center of the platform 100, i.e., the circumference having the shortest radial distance from the center of rotation C of the platform 100, and the “1-2”-th chamber 120-2 is disposed on a circumference more distant from the center of rotation C of the platform 100 than the “1-1”-th chamber 120-1, i.e., on a circumference having a larger radial distance from the center of rotation.
As described above, the platform 100 may be formed in various shapes including circles, circular sectors and polygons, and in the illustrated embodiment, the platform 100 has a circular shape. In addition, as shown in
When the platform 100 rotates, the fluid sample accommodated in the sample supply chamber 110 flows through the distribution channel 115. When the “1-1”-th chamber 120-1 is filled with the sample, the sample flowing through the distribution channel 115 is introduced, by centrifugal force, into the “1-2”-th chamber 120-2 arranged more distant from the center of the platform 100. In the same manner, the “1-2”-th to “1-n”-th chambers are filled with the sample. After the first chambers 120-1 to 120-n are all filled with the sample, the remaining sample flows into an excess chamber 180 to accommodate excess fluid.
After filling the first chambers 120, the sample flows into the second chambers 130 through the siphon channels 125, and thus, to transfer the sample through the siphon channel 125, the crest point of the siphon channel 125 should be higher than the highest level of the fluid accommodated in the sample supply chamber 110, as shown in
The capillary force of the siphon channel 125 may be established by narrowing the cross-sectional area of the siphon channel 125 or by hydrophilic treatment of the inner surfaces of the siphon channel 125. In the illustrated embodiment, the cross-sectional area of the siphon channel 125 is not limited, but the width and depth thereof may be adjusted to have a value between 0.01 mm and 3 mm, between 0.05 mm and 1 mm, or between 0.01 mm and 0.5 mm to establish a high capillary pressure. The capillary force may also be established by plasma treatment or hydrophilic polymer treatment of the inner surfaces of the siphon channel 125.
In the microfluidic device 10 according to the illustrated embodiment, the fluid sample may be a biosample of a bodily fluid such as blood, lymph and tissue fluid or urine, or an environmental sample for water quality control or soil management. However, the embodiment is not limited so long as the fluid is movable by centrifugal force.
A microfluidic structure may be formed as one unit as in the illustrated embodiment of
Referring to
Referring to
Thus, when the platform 100 rotates, the sample accommodated in the sample supply chamber 110 of each unit is independently distributed to the respective first chambers 120 and thereafter, introduced into the respective second chambers 130 through the respective siphon channels 125.
As shown in
For example, a bodily fluid sample may be used to conduct an immunoserologic test in the first test unit and a biochemical test in the second test unit. Alternatively, immuno-serological tests of different kinds or biochemical tests of different kinds may be independently conducted using different samples in each of the first test unit and the second test unit.
As shown in
Thus, when a platform 100 is provided with a plurality of test units to simultaneously perform several tests as shown in
It should be understood that
First, as shown in
Then, the platform 100 is rotated such that the sample accommodated in the sample supply chamber 110 is distributed to all of the first chambers 120 through the distribution channel 115, as shown in
Referring to
When the “1-1”-th chamber 120-1 is filled with sample, the fluid flowing through the distribution channel 115 does not flow into the “1-1” chamber 120-1 anymore and instead moves up to the inlet of the “1-2” chamber 120-2 and flows into the “1-2” chamber 120-2. Similarly, when the “1-2” chamber 120-2 is filled with sample, the fluid flowing through the distribution channel 115 does not flow into the “1-2” chamber 120-2 anymore and instead moves up to the inlet of the next chamber, i.e., the “1-2” chamber 120-2 and flows into the “1-2” chamber 120-2. In a similar manner, all the chambers from the “1-1”-th chamber 120-1 to the “1-n”-th chamber 120-n are filled with the sample. The portion of the sample remaining after filling the “1-n”-th chamber 120-n is accommodated in the excess chamber 180.
Referring to
The portion of the sample remaining after filling the first chambers 120-1 to 120-n is accommodated in the excess chamber 180.
Once distribution of the sample to the first chambers 120-1 to 120-n is completed, rotation of the platform is stopped. When the platform 100 is stopped, the sample contained in the first chambers 120-1 to 120-n flows into the siphon channels 125-1 to 125-n by capillary pressure, thereby filling all of the siphon channels 125-1 to 125-n, as shown in
When the siphon channels 125-1 to 125-n are filled with the sample, the platform 100 is rotated again causing the sample to flow into the second chambers 130-1 to 130-n by centrifugal force, as shown in
Thus, the sample accommodated in the sample supply chamber 110 is distributed to the second chambers 130 in a fixed amount via the first chambers 120 and the siphon channels 125 according to the operations of
When the outlets of the first chambers 120 connected to the inlets of the siphon channels 125 are located at the lowest portions of the first chambers 120 (i.e., the portions distal to the center of rotation), as shown in
In the illustrated exemplary embodiment of
Hereinafter, the structure and operation of the microfluidic device according to the illustrated exemplary embodiment will be described in detail with reference to
As described above, the platform 100 may be formed in various shapes including circles, circular sectors and polygons. Also, for convenience of description, in the illustrated exemplary embodiment, it will be assumed that three first chambers 120, namely, chambers 120-1, 120-2 and 120-3 are connected in parallel to the distribution channel 115 and three second chambers 130-1, 130-2 and 130-3 are connected to the respective first chambers 120.
Each of the first chambers 120, each of the corresponding second chambers 130 connected thereto, and any microfluidic structures connected to the corresponding second chambers 130 form a single test part, and in the illustrated embodiment, three test parts are provided. Each test part may be provided with a different configuration and a different material to be accommodated therein such that a different test may be independently conducted.
The sample supply chamber 110 is arranged closest to the center of rotation C to accommodate a sample supplied from the outside. The sample supply chamber 110 accommodates a fluid sample, and for illustration purposes only, blood is supplied as the fluid sample.
A sample introduction inlet 111 is provided at one side of the sample supply chamber 110, through which an instrument such as a pipette may be used to introduce blood into the sample supply chamber 110. Blood may be spilled near the sample introduction inlet 111 during the introduction of blood, or the blood may flow backward through the sample introduction inlet 111 during rotation of the platform 100. To prevent the microfluidic device 10 from being contaminated in this manner, a backflow receiving chamber 112 may be formed at a position adjacent to the sample introduction inlet 111 to accommodate any spilled sample during introduction thereof or any sample that flows backward.
In another exemplary embodiment, to prevent backflow of the blood introduced into the sample supply chamber 110, a structure that functions as a capillary valve may be formed in the sample supply chamber 110. Such a capillary valve allows passage of the sample only when a pressure greater than or equal to a predetermined level is applied.
In another exemplary embodiment, to prevent backflow of the blood introduced into the sample supply chamber 110, a rib-shaped backflow prevention device may be formed in the sample supply chamber 110. Such a rib-shaped back flow prevention device may include one or more protrusions formed on a surface of the sample supply chamber 110. Arranging the backflow prevention device in a direction crossing the direction of flow of the sample from the sample introduction inlet 111 to the sample discharge outlet may produce resistance to flow of the sample, thereby preventing the sample from flowing toward the sample introduction inlet 111.
The sample supply chamber 110 may be formed to have a width that gradually increases from the sample introduction inlet 111 to the sample discharge outlet 113 in order to facilitate discharge of the sample accommodated therein through the sample discharge outlet 113. In other words, the radius of curvature of at least one side wall of the sample supply chamber 110 may gradually increase from the sample introduction inlet 111 to the sample discharge outlet 113.
The sample discharge outlet 113 of the sample supply chamber 110 is connected to a distribution channel 115 formed on the platform 100 in the circumferential direction of the platform 100. Thus, the distribution channel 115 is sequentially connected to the “1-1”-th chamber 120-1, the “1-2”-th chamber 120-2 and the “1-3”-th chamber 120-3 proceeding counterclockwise. A Quality Control (QC) chamber 128 to indicate completion of supply of the sample and an excess chamber 180 to accommodate any excess sample remaining after supply of the sample may be connected to the end of the distribution channel 115.
The fast chambers 120 (i.e., 120-1, 120-2, and 120-3) may accommodate the sample supplied from the sample supply chamber 110 and cause the sample to separate into a supernatant and sediment through centrifugal force. Since the exemplary sample used in the illustrated embodiment is blood, the blood may separate into a supernatant including serum and plasma and sediment including corpuscles in the first chambers 120.
Each of the first chambers 120-1, 120-2 and 120-3 is connected to a corresponding siphon channel 125-1, 125-2 and 125-3. As described above, the crest points (i.e., bend) of the siphon channels 125-1, 125-2 and 125-3 should be higher than the highest level of the fluid accommodated in the first chambers 120-1, 120-2 and 120-3. To secure a difference in height, the “1-2”-th chamber 120-2 is positioned on a circumference that is further from the center of rotation C, or a circumference of a larger radius, than the circumference on which the “1-1”-th chamber 120-1 is positioned, and the “1-3”-th chamber 120-3 is positioned on a circumference that, is further from the center of rotation C, or a circumference of a larger radius, than the circumference on which the “1-2”-th chamber 120-2 is positioned.
In this arrangement, a chamber 120 positioned farther away from the sample discharge outlet 113 along the direction of How of the distribution channel 115, will have a shorter length in a radial direction. Accordingly, if the first chambers 120 are set to have the same volume, the first chamber 120 positioned farther away from the sample discharge outlet 113 has a larger width in a circumferential direction, as shown in
As described above, the positions at which the inlets of the siphon channels 125-1, 125-2 and 125-3 meet the outlets of the first chambers 120-1, 120-2 and 120-3 may vary depending on the amount of fluid to be transferred. Thus, if the sample is blood, as in the illustrated exemplary embodiment, a test is often performed only on the supernatant, and therefore the outlets of the first chambers 120 may be arranged at upper portions (i.e., above the middle portion) thereof, at which the supernatant is positioned. This is simply an embodiment provided for illustration, and if the sample is not blood or the test is performed on the sediment in addition to the supernatant, outlets may be provided at lower portions of the first chambers 120.
The outlets of the siphon channels 125-1, 125-2 and 125-3 are connected to the respective second chambers 130-1, 130-2 and 130-3. The second chambers 130 may accommodate only a sample (e.g., blood), or may have a reagent or reactant pre-stored therein. The reagent or reactant may be used, for example, to perform pretreatment or first order reaction for blood, or to perform a simple test prior to the main test. In the illustrated exemplary embodiment, binding between an analyte and a first marker conjugate occurs in the second chambers 130.
Specifically, the first marker conjugate may remain in the second chamber 130 in a liquid phase or solid phase. When the marker conjugate is solid phase, the inner wall of the second chamber 130 may be coated with the marker conjugate or the marker conjugate may be temporarily immobilized on a porous pad disposed therein.
The first marker conjugate is a complex formed by combining a marker and a capture material which specifically reacts with an analyte in the sample. For example, if the analyte is antigen Q, the first marker conjugate may be a conjugate of the marker and antibody Q which specifically reacts with antigen Q.
Exemplary markers include, but are not limited to, latex beads, metal colloids including gold colloids and silver colloids, enzymes including peroxidase, fluorescent materials, luminescent materials, superparamagnetic materials, materials containing lanthanum (III) chelates, and radioactive isotopes.
Also, if test paper on which a chromatographic reaction occurs is inserted into the reaction chamber 150, as described below, a second marker conjugate which binds with a second capture material may be immobilized on the control line of the test paper to confirm reliability of the reaction. In various exemplary embodiments, the second marker conjugate may also be in a liquid phase or solid phase and, when in solid phase, the inner wall of the second chamber 130 may be coated with the second marker conjugate or the second marker conjugate may be temporarily immobilized on a porous pad disposed therein.
The second marker conjugate is a conjugate of the marker and a material specifically reacting with the second capture material immobilized on the control line. The marker may be one of the aforementioned exemplary materials. If the second capture material immobilized on the control line is biotin, a conjugate of streptavidin and the marker may be temporarily immobilized in the second chamber 130.
Accordingly, when blood flows into the second chamber 130, antigen Q present in the blood binds with the first marker conjugated with antibody Q and is discharged to the third chamber 140. At this time, the second marker conjugated with streptavidin is also discharged.
The second chambers 130-1, 130-2 and 130-3 are connected to the third chambers 140-1, 140-2 and 140-3, and in the illustrated embodiment, the third chambers 140-1, 140-2 and 140-3 are used as metering chambers. The metering chambers 140 function to meter a fixed amount of sample (e.g., blood) accommodated in the second chamber 130 and supply the fixed amount of blood to the respective fourth chambers 150 (150-1, 150-2, and 150-3). The metering operation of the metering chambers will be described below with reference to
The residue in the metering chambers 140 which has not been supplied to the fourth chambers 150 may be transferred to the respective waste chambers 170 (170-1, 170-2, and 170-3). In the illustrated exemplary embodiment, the connection between the metering chambers 140 and the waste chambers 170 is not limited to
The third chambers 140-1, 140-2 and 140-3 are connected to the reaction chambers 150-1, 150-2 and 150-3 which are the fourth chambers. Although not shown in detail, the third chambers may be connected to the fourth chambers via channels, or by a specific structure to transfer the fluid. The latter case will be described in detail with reference to
A reaction may occur in the reaction chambers 150 in various ways. For example, in the illustrated embodiment, chromatography based on capillary pressure is used in the reaction chambers 150. To this end, the reaction chamber 150 includes a detection region 20 to detect the presence of an analyte through chromatography.
The detection region 20 is formed from a material selected from a micropore, micro pillar, and thin porous membrane such as cellulose, upon which capillary pressure acts. Referring to
Referring to
When the analyte is antigen Q, the capture material 24a permanently immobilized on the test line 24 may be antibody Q. In this case, when the biosample flowing according to the capillary pressure reaches the test line 24, the conjugate 22a of antigen Q and the first marker conjugate binds with antibody Q 24a to form a sandwich conjugate 24b. Therefore, if the analyte is contained in the biosample, it may be detected by the marker on the test line 24.
A normal test may fail for various reasons such as small sample amount and/or sample contamination. Accordingly, to determine whether the test has been properly performed, the detection region 20 may be provided with a control line 25 on which is permanently immobilized a second capture material 25a that specifically reacts with a material contained in the sample regardless of presence of the analyte.
As the second capture material 25a immobilized on the control line 25, biotin may be used, and thus the second marker conjugate 23a contained in the sample in the second chamber 130 may be a streptavidin-marker conjugate, which has a high affinity to biotin.
Referring to
In other words, if a mark by the marker appears on both the control line 25 and the test line 24, the sample will be deemed positive, which indicates that the analyte is present in the sample. If the mark appears only on the control line 25, the sample will be deemed negative, which indicates that the analyte is not present in the sample. However, if the mark does not appear on the control line 25, test malfunction may be determined.
As shown in
Referring to
Referring to
As the flowing biosample reaches the test line 24 and the control line 25, the capture material 24a binds with the conjugate 22a to form a sandwich conjugate 24b on the test line 24, as shown in
If the reaction chamber 150 of the microfluidic device is provided with the detection region 20 of
In another exemplary embodiment, rather than using chromatography, a capture antigen or capture antibody may be provided in the reaction chamber 150 to react with a certain antigen or antibody in the sample such that a binding reaction with the capture antigen or capture antibody occurs in the reaction chamber 150.
Referring to
Meanwhile, the platform 100 may be provided with one or more magnetic bodies for position identification. For example, in addition to chambers in which a sample or residue is accommodated or a reaction occurs, the platform 100 may be provided with magnetic body accommodating chambers 160-1, 160-2, 160-3 and 160-4. The magnetic body accommodating chambers 160-1, 160-2, 160-3 and 160-4 accommodate a magnetic body, which may be formed of a ferromagnetic material such as iron, cobalt and nickel which have a high intensity of magnetization and form a strong magnet like a permanent magnet, a paramagnetic material such as chromium, platinum, manganese and aluminum which have a low intensity of magnetization and thus do not form a magnet alone, but may become magnetized when a magnet approaches to increase the intensity of magnetization, or a diamagnetic material such as bismuth, antimony, gold and mercury which are repelled by magnetic fields.
Referring to
The magnetic module 330 may be positioned so as not to influence the rotation of the platform 100, and may be transported to a position under the platform 100 when the operation of position identification is required. When the magnetic module 330 is positioned under the platform 100, it may attract the magnetic body accommodated in the magnetic body accommodating chamber 160, thereby causing the platform 100 to rotate according to magnetic attractive force such that the magnetic body accommodating chamber 160 is aligned with the magnetic module 330. To allow the magnetic body accommodating chamber 160 to be easily attracted by the magnet module 330, the magnetic body accommodating chamber 160 may be formed to protrude downward from the platform 100.
Since the detection unit 350 is located adjacent to a position facing the magnetic module 330, information contained in a detection area may be detected by the detection unit 350 by forming the magnetic body accommodating chamber 160 at a position adjacent to the detection object region within the platform 100. The detection area may be a QC chamber 128 or a reaction chamber 140. Any area which has detectable information may be used as the detection area.
The detection unit 350 may be provided with a light emitting unit and a light receiving unit. The light emitting unit and the light receiving unit may be integrally formed and arranged facing in the same direction, as shown in
In the illustrated exemplary embodiment, the magnetic module 330 is adapted to move on the lower side of the platform. Alternatively, it may be adapted to move on the upper side of the platform.
Allowing the magnetic body accommodating chambers 160-1, 160-2 and 160-3 to perform the operation of position identification as in the illustrated embodiment is simply one example. In another example, instead of providing the magnetic body accommodating chamber 160 in the microfluidic device, a motor may be used to control an angular position of the platform 100 such that a certain position on the platform 100 faces the detection unit 350.
Referring to
As illustrated in
In addition, as describe above with reference to
As shown in
The second chambers 130 may simply serve to temporarily accommodate the blood flowing thereinto, or allow, as described above, binding between a specific antigen in the blood and a marker conjugate pre-provided in the second chambers 130-1, 130-2 and 130-3.
The reaction occurring in the reaction chambers 150 may be immunochromatography or a binding reaction with a capture antigen or capture antibody, as described above.
As shown in
Accordingly, when the reaction is completed, the magnet is moved to a position under the platform 100, thereby causing the detection unit 350 and the reaction chamber 150 to be positioned facing each other due to attractive force between the magnet 330 and the magnetic body. The detection unit 350 may therefore detect the result of the reaction in the reaction chamber 150 by capturing an image of the reaction chamber.
Hereinafter, another example of metering a fluid in the microfluidic device will be described in detail.
Referring to
The fluid transfer assist unit 155 includes a fluid guide 155b to guide movement of the fluid from the metering chamber 140 to the reaction chamber 150, and a fluid passage 155a allowing the fluid to flow from the metering chamber 140 to the reaction chamber 150 therethrough. The fluid guide 155b is shaped to protrude from the reaction chamber 150 toward the metering chamber 140, and the fluid passage is formed to have a greater width than other channels so as to facilitate passage of the fluid. However, the fluid transfer assist unit 155 does not necessarily require inclusion of the fluid guide 155b. Alternatively, only the fluid passage 155a may be provided.
In addition, in the illustrated embodiment, the reaction occurs in the reaction chamber using chromatography, and to this end, the reaction chamber 150 is provided with the detection region 20 described above with reference to
The fluid transfer assist unit 155 not only serves to control the rotational speed of the platform 100, but also causes the fluid accommodated in the metering chamber to be transferred to the reaction chamber 150 by the amount desired by a user. Hereinafter, the function of the fluid transfer assist unit 155 will be described with reference to
When the platform 100 is rotated, the sample and the marker conjugate in the second chamber 130 move to the metering chamber 140. As shown in the interval (a) in
In the metering chamber 140, a first order reaction occurs between the sample and the first marker conjugate, i.e., between the analyte and the first marker conjugate. In addition, rotation of the platform 100 is stopped as shown in the interval (b) in
Referring to the interval (c) of
In this case, the combination of the magnetic force of the magnetic body and inertial force resulting from rotation of the sample act simultaneously to rotate the platform 100, thereby driving the fluid sample toward the reaction chamber 150 as shown in
Therefore, the fluid sample positioned outside the point at which the metering chamber 140 and the reaction chamber 150 are connected to each other may be transferred to the reaction chamber 150 by control of the rotational speed as previously described. Thus, the occurrence of the second order reaction within the reaction chamber 150 at a desired time may be accomplished by adjustment of the control timing by the user, thereby supplying a desired amount of the fluid sample to the reaction chamber 150 with a small amount of torque applied to the platform 100. Here, the second order reaction is the chromatography reaction by the detection region 20.
If there is any fluid sample remaining in the first chamber 120, the siphon channels may be filled with the fluid sample by capillary force, and when the platform 100 is rotated at a high speed, the fluid sample filling the siphon channels 125 may pass through the second chambers 130, thereby flowing into the metering chambers 140. However if the fluid sample in the metering chambers 140 flows into the reaction chamber 150, the detection region 20 indicating the result of the second order reaction may be contaminated. Accordingly, the microfluidic device 10 may further include a second siphon channel to transfer additional inflow of the fluid sample to the waste chamber 170.
Referring to
Therefore, additional inflow of the fluid sample into the reaction chamber in which the reaction has been completed may be prevented even when there is remaining fluid sample in the first chamber.
As is apparent from the above description, a microfluidic structure and a microfluidic device having the same according to an exemplary embodiment allows for the efficient distribution of a fixed amount of a fluid to a plurality of chambers. Adjustment of the distribution speed and supply speed of the fluid, without a separate driving source, may thus be accomplished by arranging the chambers at different positions on the platform 100 and connecting them in parallel using a siphon channel.
Also, a multi-step reaction is allowed by connection of a first chamber (an accommodation chamber), a second chamber (a first order reaction chamber), a third chamber (a metering chamber) and a fourth chamber (a second order reaction chamber), and therefore reaction sensitivity is enhanced.
Further contamination of a reaction result may be prevented by arranging a second siphon channel between the metering chamber and the waste chamber, and directing a fluid sample flowing to the reaction chamber to the waste chamber after completion of reaction.
Although a few exemplary embodiments have been shown and described, it would be appreciated by those skilled in the art that changes may be made in these embodiments without departing from the principles and spirit of the inventive concept, the scope of which is defined in the claims and their equivalents.
Number | Date | Country | Kind |
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10-2012-0075711 | Jul 2012 | KR | national |
10-2012-0085361 | Aug 2012 | KR | national |
This application is a continuation of U.S. patent application Ser. No. 14/803,161, now U.S. Pat. No. 10,058,864, filed Jul. 20, 2015, which is a divisional of U.S. application Ser. No. 13/934,857, filed Jul. 3, 2013, which claims priority from Korean Patent Applications No. 10-2012-0075711, filed on Jul. 11, 2012, and No. 10-2012-0085361, filed on Aug. 3, 2012, in the Korean Intellectual Property Office, the disclosure of each of which is incorporated herein by reference in its entirety.
Number | Name | Date | Kind |
---|---|---|---|
3706413 | Blum | Dec 1972 | A |
5160702 | Kopf-Sill | Nov 1992 | A |
5976472 | Chatterjee | Nov 1999 | A |
7125711 | Pugia | Oct 2006 | B2 |
10058864 | Lee | Aug 2018 | B2 |
20060223103 | Klapproth | Oct 2006 | A1 |
20070128652 | Woudenberg | Jun 2007 | A1 |
20100081213 | Lee | Apr 2010 | A1 |
20100093105 | Lee | Apr 2010 | A1 |
20100288949 | Yoo | Nov 2010 | A1 |
20110094600 | Bergeron | Apr 2011 | A1 |
20110111987 | Siegreist | May 2011 | A1 |
20120295781 | Amasia | Nov 2012 | A1 |
Number | Date | Country |
---|---|---|
101918528 | Dec 2010 | CN |
102177439 | Sep 2011 | CN |
1288648 | Mar 2003 | EP |
2479139 | Oct 2011 | GB |
WO 2007006049 | Jan 2007 | WO |
Entry |
---|
Communication dated Sep. 14, 2016, issued by the State Intellectual Property Office of the People's Republic of China in counterpart Chinese Application No. 201310291257.2. |
Communication dated Mar. 27, 2017, issued by the State Intellectual Property Office of the People's Republic of China in counterpart Chinese Application No. 201310291257.2. |
Communication dated Apr. 6, 2017, from the European Patent Office in counterpart European Application No. 13176051.4. |
Communication dated Mar. 24, 2017, issued by the Canadian Intellectual Property Office in counterpart Canadian Application No. 2,820,181. |
Communication dated Oct. 17, 2017, issued by the State Intellectual Property Office of the PR's China in counterpart Chinese Application No. 201310291257.2. |
Communication dated Mar. 8, 2018, issued by the State Intellectual Property Office of the People's Republic of China in counterpart Chinese Application No. 201310291257.2. |
Communication dated Mar. 28, 2018, issued by the Canadian Intellectual Property Office in counterpart Canadian Application No. 2,820,181. |
Communication dated Dec. 28, 2015, issued by the State Intellectual Property Office of the People's Republic of China in counterpart Chinese Application No. 201310291257.2. |
Gorkin et al., “Centrifugal microfluidics for biomedical applications,” Lab on a Chip, first published May 28, 2010, 10, 1758-1773. |
Communication dated Feb. 11, 2015, from the European Patent Office in counterpart European Application No. 13176051.4. |
Focke et al. “Centrifugal Microfluidic System for Primary Amplification and Secondary Real-Time PCR”, Lab Chip, 2010, Vo. 10, pp. 3210-3212, accepted Sep. 14, 2010. |
Siegrist, J. et al., “Serial Siphon Valving for Centrifugal Microfluidic Platforms”, Microfluid Nanofluid, 2010, vol. 9, pp. 55-63, published online Nov. 4, 2009. |
International Search Report dated Sep. 16, 2013, issued by the International Searching Authority in counterpart International Application No. PCT/KR2013/006118. |
Office Action dated Apr. 12, 2017 in U.S. Appl. No. 14/803,161. |
Final Office Action dated Nov. 7, 2017 in U.S. Appl. No. 14/803,161. |
Notice of Allowance dated Jun. 7, 2018 in U.S. Appl. No. 14/803,161. |
Supplemental Notice of Allowance dated Jun. 27, 2018 in U.S. Appl. No. 14/803,161. |
Number | Date | Country | |
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20190091680 A1 | Mar 2019 | US |
Number | Date | Country | |
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Parent | 13934857 | Jul 2013 | US |
Child | 14803161 | US |
Number | Date | Country | |
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Parent | 14803161 | Jul 2015 | US |
Child | 16115379 | US |