WO2001087485A2 - Dispositifs microfluidiques et procedes de criblage a haut debit - Google Patents

Dispositifs microfluidiques et procedes de criblage a haut debit Download PDF

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Publication number
WO2001087485A2
WO2001087485A2 PCT/US2001/015743 US0115743W WO0187485A2 WO 2001087485 A2 WO2001087485 A2 WO 2001087485A2 US 0115743 W US0115743 W US 0115743W WO 0187485 A2 WO0187485 A2 WO 0187485A2
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Prior art keywords
platform
reagent
fluid
ofthe
reservoirs
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PCT/US2001/015743
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English (en)
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WO2001087485A3 (fr
Inventor
Gregory J. Kellogg
David Duffy
Aaron Pelta
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Tecan Trading Ag
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Priority claimed from US09/595,239 external-priority patent/US6582662B1/en
Application filed by Tecan Trading Ag filed Critical Tecan Trading Ag
Priority to EP01937420A priority Critical patent/EP1284819A2/fr
Priority to AU2001263162A priority patent/AU2001263162A1/en
Priority to JP2001583935A priority patent/JP2004501360A/ja
Publication of WO2001087485A2 publication Critical patent/WO2001087485A2/fr
Publication of WO2001087485A3 publication Critical patent/WO2001087485A3/fr

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    • B01J19/0046Sequential or parallel reactions, e.g. for the synthesis of polypeptides or polynucleotides; Apparatus and devices for combinatorial chemistry or for making molecular arrays
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    • BPERFORMING OPERATIONS; TRANSPORTING
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    • CCHEMISTRY; METALLURGY
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Definitions

  • This invention relates to methods and apparatus for performing microanalytic and microsynthetic analyses and procedures.
  • the invention relates to microminiaturization of genetic, biochemical and bioanalytic processes.
  • the present invention provides devices and methods for the performance of miniaturized biochemical assays. These assays may be performed for a variety of purposes, including but not limited to screening of drug candidate compounds, life sciences research, and clinical and molecular diagnostics. Methods for performing any of a wide variety of such microanalytical or microsynthetic processes using the microsystems apparatus of he invention are also provided.
  • More traditional approaches to compound library development are also yielding growing numbers of candidates, including the use of naturally-derived compounds extracted from plants, fungi, and bacteria. In part, this is due to an increased understanding of the function of these compounds, including how they affect the metabolic pathways of the organisms which synthesize and use them; the increasing refinement in identifying and understanding compounds based on small structural and compositional differences; and improved methods for extracting and purifying these compounds.
  • the function of drug candidates, targets, and the effect of the candidates on targets is assessed in the early stages of pharmaceutical development through a process of screening that typically includes: binding of a drug candidate to a portion or domain of the target molecule; immunoassays that bind to drug candidate target domains correlated with drug efficacy; enzymatic assays, in which the inhibition of an enzymatic activity of the target by the drug candidate can be used as a sign of efficacy; protein/protein binding; and protein/DNA(RNA) binding.
  • Additional assays involve the use of living cells and include gene expression, in which levels of transcription in response to a drug candidate are monitored, and functional assays designed to investigate both macroscopic effects, such as cell viability, as well as biochemical effects and products produced in and by the cells as a result of treatment with the drug lead compound.
  • Miniaturization has been accompanied by the development of more sensitive detection schemes, including both better detectors for conventional signals (e.g., colorimetric absorption, fluorescence, and chemiluminescence) as well as new chemistries or assay formats (e.g., imaging, optical scanning, and confocal microscopy).
  • Miniaturization can also confer performance advantages. At short length scales, diffusionally-limited mixing is rapid and can be exploited to create sensitive assays (Brody et al, 1996, Biophysical J. IV. 3430-3431). Because fluid flow in miniaturized pressure-driven systems is laminar, rather than turbulent, processes such as washing and fluid replacement are well-controlled.
  • Microfabricated systems also enable assays that rely on a large surface area to volume ratio such as those that require binding to a surface and a variety of chromatographic approaches.
  • microdevices Integration of microdevices with existent laboratory infrastructure is also desirable and has been poorly addressed in the art. This integration is one of both scale and format.
  • scale fluids must be transferred to devices from the external world, where the volumes in which they are handled are typically one or more orders of magnitude greater than the volumes required by the microdevice. It is desirable that this transition be done in a way that does not introduce excessively complex processes or machinery and which does not create excessive errors, such as in the volume of fluid transferred.
  • format it is desirable that microdevices have a similar physical aspect to macroscale devices already used in laboratories, especially in regard to the manner in which fluids are added to or removed from the devices. Microdevices that can be loaded with fluids using standard methods, such as pipettors, will be more easily and widely used in a variety of settings.
  • Fluid processing in microtiter plates is also difficult.
  • washing an important step in many assays can be problematic.
  • Methods that reduce both the number of manipulations of fluids on the plate as well as manipulations ofthe plate itself can reduce cost while improving assay quality through suppression of contamination, carry-over, and fluid loss.
  • This invention provides microsystems platforms as disclosed in co-owned U.S. Patent No. 6,063,589, issued May 16, 2000, and co-owned and co-pending patent applications U.S. Serial Nos. 08/761,063, filed December 5, 1996; 08/768,990, filed December 18, 1996; 08/910,726, filed August 12, 1997; 08/995,056, filed December 19, 1997; and 09/315,114, filed May 19, 1999, the disclosures of each of which are explicitly incorporated by reference herein.
  • the invention provides apparatus and methods for performing microscale processes on a microplatform, whereby fluid is moved on the platform in defined channels motivated by centripetal force arising from rotation of the platform.
  • the first element of the apparatus ofthe invention is a microplatform that is a rotatable structure, most preferably a disk, the disk comprising fluid (sample) inlet ports, fluidic microchannels, reagent reservoirs, collection chambers, detection chambers and sample outlet ports, genetically termed "microfluidic structures.”
  • the disk is rotated at speeds from about 1 to about 30,000 rpm for generating centripetal acceleration that enables fluid movement through the microfluidic structures of the platform.
  • the disks of the invention also preferably comprise air outlet ports and air displacement channels.
  • the air outlet ports and in particular the air displacement ports provide a means for fluids to displace air, thus ensuring uninhibited movement of fluids on the disk.
  • Specific sites on the disk also preferably comprise elements that allow fluids to be analyzed, as well as detectors for each of these effectors.
  • the discs of this invention have several advantages over those that exist in the centrifugal analyzer art. Foremost is the fact that flow is laminar due to the small dimensions of the fluid channels; this allows for better control of processes such as mixing and washing. Secondly, the small dimensions conferred by microfabrication enable the use of "passive" valving, dependent upon capillary forces, over much wider ranges of rotational velocities and with greater reliability than in more macroscopic systems. To this are added the already described advantages of miniaturization.
  • the second element ofthe invention is a micromanipulation device that is a disk player/ reader device that controls the function of the disk. This device comprises mechanisms and motors that enable the disk to be loaded and rotated.
  • the device provides means for a user to operate the microsystems in the disk and access and analyze data, preferably using a keypad and computer display.
  • the micromanipulation device also advantageous provides means for actuation of on-disc elements, such as active valves; the application and control of heat to the disc for purposes of chemical or biological incubation; and means for adding fluids to and removing fluids from the discs.
  • the micromanipulation devices of this invention are more particularly described in co-owned U.S. Patent No. 6,063,589, issued May 16, 2000, and co-owned and co- pending patent applications U.S. Serial Nos.
  • the invention specifically provides microsystems platforms comprising microfluidics components contained in one or a multiplicity of platfomi layers that are fluidly connected to permit transfer, mixing and assay performance on the sealed surface of the platform.
  • the platforms preferably comprise reagent reservoirs containing a sufficient volume, preferably from about InL to about lmL, of a reagent solution for a multiplicity of individual assays.
  • the reagent reservoirs are fluidly connected by microchannels to one or more preferably a multiplicity of collection, and more preferably detection, chambers, and the microfluidics components arranged so that a specific volume ofthe reagent solution is delivered to each collection chamber.
  • said reagent reservoirs are fluidly connected to mixing structures, most preferably a mixing microchannel that is also fluidly connected to a sample reservoir, so that one or a plurality of reagents are mixed with sample and the resulting mixture delivered into the detection chamber.
  • the platform comprises a multiplicity of sample reservoirs and mixing structures fluidly connected with a multiplicity of detection chambers.
  • the platforms of the invention permit the use of a detector, most preferably an optical detector, for detecting the products of the assay, whereby the collection chambers comprise optical cuvettes, preferably at the outer edge of the platform, most preferably wherein the platform is scanned past a fixed detector through the action of the rotary motor.
  • the platforms of the invention are most preferably constructed using microfabrication techniques as described more fully below, the volumes of fluids used may be made arbitrarily small as long as the detectors used have sufficient sensitivity.
  • the present invention solves problems in the current art through the use of a microfluidic disc in which centripetal acceleration is used to move fluids. It is an advantage of the microfluidics platforms of the present invention that the fluid- containing components are constructed to contain a small volume, thus reducing reagent costs, reaction times and the amount of biological material required to perform an assay. It is also an advantage that the fluid-containing components are sealed, thus eliminating experimental error due to differential evaporation of different fluids and the resulting changes in reagent concentration. Because the microfluidic devices ofthe invention are completely enclosed, both evaporation and optical distortion are reduced to negligible levels.
  • the platforms ofthe invention also advantageously permit "passive" mixing and valving, i.e., mixing and valving are performed as a consequence of the structural arrangements ofthe components on the platforms (such as shape, length, position on the platform surface relative to the axis of rotation, and surface properties of the interior surfaces of the components, such as wettability as discussed below), and the dynamics of platform rotation (speed, acceleration, direction and change-of-direction), and permit control of assay timing and reagent delivery.
  • “passive" mixing and valving i.e., mixing and valving are performed as a consequence of the structural arrangements ofthe components on the platforms (such as shape, length, position on the platform surface relative to the axis of rotation, and surface properties of the interior surfaces of the components, such as wettability as discussed below), and the dynamics of platform rotation (speed, acceleration, direction and change-of-direction), and permit control of assay timing and reagent delivery.
  • the disclosed invention is a microfluidic disc comprising metering structures and a microfluidic network that is used to distribute aliquots of reagent to each of a multiplicity of mixing structures, each mixing structure being fluidly connected to one of a multiplicity of sample reservoirs, thereby permitting parallel processing and mixing of the samples with one or more common reagents.
  • the fluidic network defined as the overall pattern of channels, reservoirs, microvalves, and air vents, may be planar or three-dimensional, depending upon the application under consideration.
  • the use of such metering and distribution reduces the need for automated reagent distribution mechanisms, reduces the amount of time required for reagent dispensing (that can be performed in parallel with distribution of reagent to a multiplicity of reaction chambers), and permits delivery of small (nL-to- ⁇ L) volumes without using externally- applied electromotive means.
  • the assembly of a multiplicity of collection chambers on the platforms of the invention also permits simplified detectors to be used, whereby each individual collection/detection chamber can be scanned using mechanisms well-developed in the art for use with, for example, CD-ROM technology.
  • the platforms of the invention are advantageously provided with sample and reagent entry ports for filling with samples and reagents, respectively, that can be adapted to liquid delivery means known in the art (such as micropipettors).
  • the platforms of the invention reduce the demands on automation in at least three ways.
  • the total number of fluid "delivery” events on the microfluidic platform is reduced relative to microtiter plates.
  • microfluidic structures that sub-divide and aliquot common reagents (such as reagent solutions, buffers, and enzyme substrates) used in all assays performed on the platform, the number of manual or automated pipetting steps are reduced by at least half (depending on the complexity of the assay). Examples of these structures have been disclosed in co-owned U.S. Patent 6,063,589, issued May 16, 2000, and incorporated by reference herein; and are disclosed below.
  • Figure 1 depicts an exploded, oblique view of a microsystems platform of the invention.
  • Figure 2a depicts a plan view of the upper face of one component of the microsystems platform shown in exploded, oblique view in Figure 1, the reservoir layer.
  • Figure 2b is a detail of one component of the upper face of the reservoir layer illustrated in Figure 2a.
  • Figure 3 is a plan view of another component of the microsystems platform of
  • Figure 1 the upper sealing film.
  • Figure 4a depicts a plan view ofthe lower face ofthe reservoir layer.
  • Figure 4b is a detail of the lower face of the reservoir layer showing the second reagent addition reservoir and first reagent overflow reservoir.
  • Figure 4c is a detail of the lower face of the reservoir layer showing the first reagent addition reservoir and second reagent overflow reservoir.
  • Figure 4d is a detail of the lower face ofthe reservoir layer showing one series of sample and reagent reservoirs, channels, and a detection cuvette for a single microdevice that performs a single measurement.
  • Figure 5 a depicts a plan view of another component of the microsystems platform of Figure 1, the microfluidic layer.
  • Figure 5b is a detail of one segment of the microfluidic layer of Figure 5 comprising the microfluidic channels of a single microfluidic assay structure.
  • Figure 5c is a detail of the microfluidic layer of Figure 5 illustrating the overflow valve and channels for the first reagent.
  • Figure 5d is a detail of the microfluidic layer of Figure 5 illustrating the overflow valve and channels for the second reagent.
  • Figure 6 is a segment of the assembled reservoir and microfluidic layers comprising the microsystems platform of Figure 1.
  • Figures 7a through 7g illustrate the sequence of fluid motions as sample, reagent 1, and reagent 2 are distributed to the reservoirs ofthe device of Figure 1.
  • Figures 8a through 81 illustrate the sequence of fluid motions into a single microfluidic assay structure ofthe device of Figure 1.
  • Figure 9 illustrates a first alternative construction of the microsystems platform in which the sample volume is metered by the construction ofthe device.
  • Figure 10 illustrates a second alternative construction of the microsystems platform in which two common reagents are isolated through the introduction of a bubble.
  • Figure 11 illustrates a third alternative construction of the microsystems platform in which a series of mixtures of two reagents are delivered to the assay structures ofthe device.
  • Figure 12 shows a device developed for the performance of 24 parallel assays.
  • Figure 13 shows a dose-response curve illustrating enzymatic activity as a function of inhibitor concentration for enzymatic inhibition assays performed with the devices ofthe invention, as disclosed in Example 1 and illustrated in Figure 12.
  • This invention provides a microplatform and a micromanipulation device as disclosed in co-owned U.S. Patent No. 6,063,589, issued May 16, 2000, and co-owned and co-pending patent applications U.S. Serial Nos. 08/761,063, filed December 5, 1996; 08/768,990, filed December 18, 1996; 08/910,726, filed August 12, 1997; 08/995,056, filed December 19, 1997; 09/315,114, filed May 19, 1999, the disclosures of each of which are explicitly incorporated by reference herein, adapted for performing microanalytical and microsynthetic assays of biological samples.
  • sample will be understood to encompass any fluid, solution or mixture, either isolated or detected as a constituent of a more complex mixture, or synthesized from precursor species, h particular, the term “sample” will be understood to encompass any biological species of interest.
  • biological sample or “biological fluid sample” will be understood to mean any biologically-derived sample, including but not limited to blood, plasma, serum, lymph, saliva, tears, cerebrospinal fluid, urine, sweat, plant and vegetable extracts, semen, and ascites fluid.
  • a centripetally motivated fluid micromanipulation apparatus is intended to include analytical centrifuges and rotors, microscale centrifugal separation apparatuses, and most particularly the microsystems platforms and disk handling apparatuses as described in co-owned U.S. Patent No. 6,063,589, issued May 16, 2000, and co-owned and co-pending patent applications U.S. Serial Nos. 08/761,063, filed December 5, 1996; 08/768,990, filed December 18, 1996; 08/910,726, filed August 12, 1997; 08/995,056, filed December 19, 1997; 09/315,114, filed May 19, 1999, the disclosures of each of which are explicitly incorporated by reference herein.
  • microsystems platform is intended to include centripetally-motivated microfluidics arrays as described in co-owned U.S. Patent No. 6,063,589, issued May 16, 2000, and co-owned and co-pending patent applications U.S. Serial Nos. 08/761,063, filed December 5, 1996; 08/768,990, filed December 18, 1996; 08/910,726, filed August 12, 1997; 08/995,056, filed December 19, 1997; 09/315,114, filed May 19, 1999, the disclosures of each of which are explicitly incorporated by reference herein.
  • the terms “capillary”, “microcapillary” and “microchannel” will be understood to be interchangeable and to be constructed of either wetting or non-wetting materials where appropriate.
  • the term “reservoir,” “assay chamber,” “fluid holding chamber,” “collection chamber” and “detection chamber” will be understood to mean ' a defined volume on a microsystems platform ofthe invention comprising a fluid.
  • the terms "entry port” and “fluid input port” will be understood to mean an opening on a microsystems platform of the invention comprising a means for applying a fluid to the platform.
  • exit port and "fluid outlet port” will be understood to mean a defined volume on a microsystems platform of the invention comprising a means for removing a fluid from the platform.
  • capillary junction will be understood to mean a region in a capillary or other flow path where surface or capillary forces are exploited to retard or promote fluid flow.
  • a capillary junction is provided as a pocket, depression or chamber in a hydrophilic substrate that has a greater depth (vertically within the platform layer) and/ or a greater width (horizontally within the platform layer) that the fluidics component (such as a microchannel) to which it is fluidly connected.
  • the fluidics component such as a microchannel
  • the force hindering flow is produced by capillary pressure, that is inversely proportional to the cross sectional dimensions of the channel and directly proportional to the surface tension of the liquid, multiplied by the cosine of the contact angle of the fluid in contact with the material comprising the channel.
  • capillary pressure that is inversely proportional to the cross sectional dimensions of the channel and directly proportional to the surface tension of the liquid, multiplied by the cosine of the contact angle of the fluid in contact with the material comprising the channel.
  • Capillary junctions can be constructed in at least three ways, one embodiment, a capillary junction is formed at the junction of two components wherein one or both of the lateral dimensions of one component is larger than the lateral dimension(s) of the other component.
  • a capillary junction occurs at an enlargement of a capillary as described in co-owned and co-pending U.S. Serial Nos. U.S. Serial Nos. 08/761,063, filed December 5, 1996; 08/768,990, filed December 18, 1996; and 08/910,726, filed August 12, 1997. Fluid flow through capillaries is inhibited at such junctions.
  • capillary junctions are formed when the dimensions of the components change from a small diameter (such as a capillary) to a larger diameter (such as a chamber) in wetting systems, in contrast to non-wettable systems, where capillary junctions form when the dimensions of the components change from a larger diameter (such as a chamber) to a small diameter (such as a capillary).
  • a second embodiment of a capillary junction is formed using a component having differential surface treatment of a capillary or flow-path.
  • a channel that is hydrophilic that is, wettable
  • hydrophobicity that is, non-wettable
  • a fluid flowing through such a channel will do so through the hydrophilic areas, while flow will be impeded as the fluid-vapor meniscus impinges upon the hydrophobic zone.
  • the third embodiment of a capillary junction according to the invention is provided for components having changes in both lateral dimension and surface properties.
  • An example of such a junction is a microchannel opening into a hydrophobic component (microchannel or reservoir) having a larger lateral dimension.
  • capillary action will be understood to mean fluid flow in the absence of rotational motion or centripetal force applied to a fluid on a rotor or platform of the invention and is due to a partially or completely wettable surface.
  • capillary microvalve will be understood to mean a capillary microchannel comprising a capillary junction whereby fluid flow is impeded and can be motivated by the application of pressure on a fluid, typically by centripetal force created by rotation of the rotor or platform of the invention.
  • Capillary microvalves will be understood to comprise capillary junctions that can be overcome by increasing the hydrodynamic pressure on the fluid at the junction, most preferably by increasing the rotational speed ofthe platform.
  • in fluid communication or "fluidly connected” is intended to define components that are operably interconnected to allow fluid flow between components.
  • air displacement channels will be understood to include ports in the surface of the platform that are contiguous with the components (such as microchannels, chambers and reservoirs) on the platform, and that comprise vents and microchannels that permit displacement of air from components of the platforms and rotors by fluid movement.
  • microplatforms of the invention are provided to comprise one or a multiplicity of microsynthetic or microanalytic systems (termed “microfluidics structures” herein).
  • microfluidics structures comprise combinations of related components as described in further detail herein that are operably interconnected to allow fluid flow between components upon rotation of the disk.
  • These components can be microfabricated as described below either integral to the disk or as modules attached to, placed upon, in contact with or embedded in the disk.
  • microfabricated refers to processes that allow production of these structures on the sub-millimeter scale. These processes include but are not restricted to molding, photolithography, etching, stamping and other means that are familiar to those skilled in the art.
  • the invention also comprises a micromanipulation device for manipulating the disks of the invention, wherein the disk is rotated within the device to provide centripetal force to effect fluid flow on the disk. Accordingly, the device provides means for rotating the disk at a controlled rotational velocity, for stopping and starting disk rotation, and advantageously for changing the direction of rotation of the disk.
  • electromechanical means and control means are provided as components of the devices of the invention.
  • User interface means (such as a keypad and a display) are also provided, as further described in co-owned U.S. Patent No. 6,063,589, issued May 16, 2000, and co-owned and co-pending patent applications U.S. Serial Nos.
  • the invention provides a combination of specifically-adapted microplatforms that are rotatable, analytic/synthetic microvolume assay platforms, and a micromanipulation device for manipulating the platform to achieve fluid movement on the platform arising from centripetal force on the platform as result of rotation.
  • the platform ofthe invention is preferably and advantageously a circular disk; however, any platform capable of being rotated to impart centripetal for a fluid on the platform is intended to fall within the scope ofthe invention.
  • the micromanipulation devices ofthe invention are more fully described in co-owned and co-pending U.S. Serial Nos. U.S. Serial Nos.
  • Fluid (including reagents, samples and other liquid components) movement is controlled by centripetal acceleration due to rotation of the platform.
  • the magnitude of centripetal acceleration required for fluid to flow at a rate and under a pressure appropriate for a particular microfluidics structure on the microsystems platform is determined by factors including but not limited to the effective radius of the platform, the interior diameter of microchannels, the position angle of the microchannels on the platform with respect to the direction of rotation, and the speed of rotation of the platform.
  • an unmetered amount of a fluid is applied to the platform and a metered amount is transferred from a fluid reservoir to a microchannel, as described in co-owned U.S. Patent No.
  • the metered amount of the fluid sample provided on an inventive platform is from about InL to
  • metering manifolds comprising one or a multiplicity of metering capillaries are provided to distribute the fluid to a plurality of components ofthe microfluidics structure.
  • microchannels comprising the surface of the platforms of the invention.
  • MicroChannel sizes are optimally determined by specific applications and by the amount of and delivery rates of fluids required for each particular embodiment of the platforms and methods of the invention.
  • MicroChannel sizes can range from 0.1 ⁇ m to a value close to the thickness of the disk (e.g., about 1mm); in preferred embodiments, the interior dimension of the microchannel is from 0.5 ⁇ m to about 500 ⁇ m.
  • MicroChannel and reservoir shapes can be trapezoid, circular or other geometric shapes as required.
  • Microchannels preferably are embedded in a microsystem platform having a thicl ⁇ iess of about 0.1 to 25mm, wherein the cross-sectional dimension of the microchannels across the thickness dimension of the platform is less than 1mm, and can be from 1 to 90 percent of said cross-sectional dimension of the platform.
  • Sample reservoirs, reagent reservoirs, reaction chambers, collection chambers, detections chambers and sample inlet and outlet ports preferably are embedded in a microsystem platform having a thickness of about 0.1 to 25mm, wherein the cross-sectional dimension of the microchannels across the thickness dimension of the platform is from 1 to 75 percent of said cross-sectional dimension of the platform.
  • delivery of fluids through such channels is achieved by the coincident rotation of the platform for a time and at a rotational velocity sufficient to motivate fluid movement between the desired components.
  • the flow rate through a microchannel of the invention is inversely proportional to the length of the longitudinal extent or path of the microchannel and the viscosity of the fluid and directly proportional to the product ofthe square ofthe hydraulic diameter of the microchannel, the square of the rotational speed of the platform, the average distance of the fluid in the channels from the center of the disk and the radial extent of the fluid subject to the centripetal force. Since the hydraulic diameter of a channel is proportional to the ratio of the cross-sectional area to cross-sectional perimeter of a channel, one can judiciously vary the depth and width of a channel to affect fluid flow (see Duffy et al, 1998, Anal. Chem. 71: 4669-4678 and co-owned and co-pending patent applications U.S. Serial Nos. 08/761,063, filed December 5, 1996 and 08/768,990, filed December 18, 1996, incorporated by reference).
  • fluids of higher densities flow more rapidly than those of lower densities given the same geometric and rotational parameters.
  • fluids of lower viscosity flow more rapidly than fluids of higher viscosity given the same geometric and rotational parameters. If a microfluidics structure is displaced along the radial direction, thereby changing the average distance of the fluid from the center of the disc but maintaining all other parameters, the flow rate is affected: greater distances from the center result in greater flow rates. An increase or a decrease in the radial extent of the fluid also leads to an increase or decrease in the flow rate. These depencies are all linear.
  • Variation in the hydraulic diameter results in a quartic dependence of flow rate on hydraulic diameter (or quadratic dependence of fluid flow velocity on hydraulic diameter), with larger flow rates corresponding to larger diameters. Finally, an increase in the rotational rate results in a quadratic increase in the flow rate or fluid flow velocity.
  • Input and output (entry and exit) ports are components of the microplatforms of the invention that are used for the introduction or removal of fluid components. Entry ports are provided to allow samples and reagents to be placed on or injected onto the disk; these types of ports are generally located towards the center ofthe disk. Exit ports are also provided to allow products to be removed from the disk. Port shape and design vary according specific applications. For example, sample input ports are designed, inter alia, to allow capillary action to efficiently draw the sample into the disk, addition, ports can be configured to enable automated sample/reagent loading or product removal. Entry and exit ports are most advantageously provided in arrays, whereby multiple samples are applied to the disk or to effect product removal from the microplatform.
  • the inlet and outlet ports are adapted to the use of manual pipettors and other means of delivering fluids to the reservoirs of the platform
  • the platform is adapted to the use of automated fluid loading devices.
  • an automated device is a single pipette head located on a robotic arm that moves in a direction radially along the surface of the platform.
  • the platform could be indexed upon the spindle of the rotary motor in the azimuthal direction beneath the pipette head, which would travel in the radial direction to address the appropriate reservoir.
  • Another embodiment is a pipettor head adapted to address multiple reservoirs, either a subset of or all of the reservoirs on the platform surface.
  • a single head may for example be composed of a linear array of pipette heads.
  • the entry ports of Figure 1 might be addressed by indexing such a linear head in the direction transverse to the pipette tips, other embodiments, pipette heads may be used which can simultaneously address all entry ports (for example, a 96-tip head).
  • sample entry ports needed for the delivery of many samples — and reagent entry ports, through which larger volumes or reagent are delivered for use in reactions with all samples.
  • a pipetting device that can simultaneously address all sample entry ports as well as reagent ports might consist of a standard multipipettor with a few added, large-volume delivery tips. Also included in air handling systems on the disk are air displacement channels, whereby the movement of fluids displaces air through channels that connect to the fluid- containing microchannels retrograde to the direction of movement of the fluid, thereby providing a positive pressure to further motivate movement ofthe fluid.
  • Platforms of the invention such as disks and the microfluidics components comprising such platforms are advantageously provided having a variety of composition and surface coatings appropriate for particular applications.
  • Platform composition will be a function of structural requirements, manufacturing processes, and reagent compatibility/chemical resistance properties.
  • platforms are provided that are made from inorganic crystalline or amorphous materials, e.g. silicon, silica, quartz, inert metals, or from organic materials such as plastics, for example, poly(methyl methacrylate) (PMMA), acetonitrile-butadiene-styrene (ABS), polycarbonate, polyethylene, polystyrene, polyolefins, polypropylene and metallocene.
  • PMMA poly(methyl methacrylate)
  • ABS acetonitrile-butadiene-styrene
  • PCC polycarbonate
  • polyethylene polystyrene
  • polyolefins polypropylene and metallocene
  • the platforms may also be made from thermoset materials such as polyurethane and poly(dimethyl siloxane) (PDMS).
  • thermoset materials such as polyurethane and poly(dimethyl siloxane) (PDMS).
  • platforms made of composites or combinations of these materials for example, platforms manufactures of a plastic material having embedded therein an optically transparent glass surface comprising the detection chamber of the platform.
  • platforms composed of layers made from different materials may be made. The surface properties of these materials may be modified for specific applications, as disclosed in co-owned U.S. Patent No. 6,063,589, issued May 16, 2000, and co-owned and co-pending patent applications U.S. Serial Nos.
  • the disk incorporates microfabricated mechanical, optical, and fluidic control components on platforms made from, for example, plastic, silica, quartz, metal or ceramic. These structures are constructed on a sub-millimeter scale by molding, photolithography, etching, stamping or other appropriate means, as described in more detail below. It will also be recognized that platforms comprising a multiplicity ofthe microfluidic structures are also encompassed by the invention, wherein individual combinations of microfluidics and reservoirs, or such reservoirs shared in common, are provided fluidly connected thereto. An example of such a platform is shown in Figure 1.
  • Figure 1 shows an exploded view of an example of a disc appropriate for large numbers of similar or identical microfluidics structures for performing, inter alia, liquid-phase assays.
  • the disc shown here enables the performance of 96 parallel assays of the same form.
  • the assays have the general form: mix first fluid A with second fluid B, and then mix the combined fluids (A+B) with third fluid C.
  • the fluid A may actually be a number of fluids, Ai, A 2 ,..Aj,...A shadow s where n is the total number of assays to be performed on independent fluids.
  • the disc is designed for loading fluids thereupon through ports constructed in the platform.
  • one fluid, A herein termed “sample” is loaded through 96 independent entry ports.
  • the second fluid, B is loaded in a volume somewhat greater than 96 times the volume required for each assay into a single entry port.
  • the third fluid, C is similarly loaded into a single entry port.
  • the volumes of each of the reservoirs containing fluids A, B and C, or the amount of fluid A, B or C loaded onto the disk, can be different, depending on the requirements of the assay.
  • the disc is configured so that rotation of the disc after loading, under a prescribed rotational profile, effects the following fluid motions: Delivery of individual samples A, to assay structures within the disc; delivery of metered aliquots of fluid B to individual assay structures within the disc; delivery of metered aliquots of fluid C to individual assay structures within the disc; "isolation" of individual assay structure volumes of fluids B and C through the use of overflow reservoirs which take excess fluid and introduce air bubbles between individual assay structures; and the performance of the assay as described above, wherein the discs effect two fluid mixing steps.
  • the number of fluids and sequence of mixing steps can be arbitrary, e.g., ( ⁇ +B) + (B+C).
  • the total number of fluids can also be arbitrary, and the three-dimensional nature of the microfluidic network allows the "crossing over" of numerous channels.
  • This device include: a) "samples” that must be loaded in large numbers can be loaded into a standard format accessible to laboratory robotics or standard automated pipetting systems; b) common reagents need to be loaded only once each, and without high precision.
  • This disc illustrates that identical assays may be made by repeating assay structures around the disc at a given radius as well as modifying the structures for placement at different radial positions. In this way, it is possible to fully cover the surface of the disc with microfluidics structures for performing assays.
  • the maximum number of assays that may be performed will depend upon the volume of fluid that cay be manipulated reproducibly, i.e., the minimum reproducible dimensions with which the disc may be fabricated, and the amount of hydrodynamic pressure required to drive small volumes of fluid through microchannels at convenient rotational rates. Taking these considerations into account, it is estimated that greater than 10,000 assays having volumes of l-5nL can be created in a circular platform having a 6cm radius.
  • platform 100 is composed of at least 3 component layers.
  • a reservoir layer 201 having features on the lower face, or both the upper and lower faces, is used.
  • a sealing film 301 is used to enclose those channels.
  • the "lower" surface of the reservoir layer 201 is bonded to a microfluidics layer 500.
  • the upper surface of the reservoir layer contains the fluid entry ports; it may also contain one or more distribution manifolds as described herein for distributing one or more common fluids.
  • Fluid flow permits mixing of various component fluids in the assay and movement of the fluids from sample and reagent chambers through mixing structures and into assay reaction chambers.
  • fluid flow can be effectuated to include incubation and wash steps, using structures disclosed in co-owned U.S. Patent No. 6,063,589, issued May 16, 2000 and incorporated by reference herein. Fluid flow rates range from about InL/s to about lOOO ⁇ L/s at rotational speeds of from about 4- 30,000rpm.
  • Passive or capillary valves are preferably used to control fluid flow in the platform as described in co-owned U.S. Patent No. 6,063,589, issued May 16, 2000, and co-owned and co-pending patent applications U.S. Serial Nos. 08/761,063, filed December 5, 1996; 08/768,990, filed December 18, 1996; 08/910,726, filed August 12, 1997; 08/995,056, filed December 19, 1997; 09/315,114, filed May 19, 1999, the disclosures of each of which are explicitly incorporated by reference herein.
  • Platform 100 is preferably provided in the shape of a disc, a circular planar platform having a diameter of from about 10 mm to about 50mm and a thickness of from about 0.1mm to about 25mm.
  • Each layer comprising the platform preferably has a diameter that is substantially the same as the other layers, although in some embodiments the diameters of the different layers are not required to completely match.
  • Each layer has a thickness ranging from about 0.1mm to about 25mm, said thickness depending in part on the volumetric capacity of the microfluidics components contained therein.
  • top surface ofthe reservoir layer 201 is shown in Figure 2a.
  • Reservoir layer 201 is preferably provided in the shape of a disc, a circular planar platform having a diameter of from about 10mm to about 50mm and a thickness of from about 0.1mm to about 25mm.
  • the layer preferably comprises a center hole 202 for mounting on a spindle, having a diameter of from about 1mm to about 20mm. Center hole 202 can be replaced by an extruded fitting for connection to a spindle, or may be absent entirely, in which case registry and connection to the spindle is accomplished using the attached microfluidic layer or another portion of the surface of the platform.
  • Figure 2a illustrates a variety of structures necessary for device function. These include “sample” or fluid entry ports that are comprised of a through hole 204 communicating between the two faces of the disc and in some embodiments a conical or cup-like depression 203. The depression aids in the placement of pipette tips when the device is used manually. These entry holes are typically arrayed in a rectangular pattern with a spacing to permit an automated pipetting device such as an 8-tip linear or 96-tip rectangular pipetting head to be used. For such devices the spacing of entry ports is typically 9mm or 4.5mm, and the arrays are typically 8x12 or 16x24 elements in size.
  • These ports may also be placed in the pattern of a 1536-well plate, which has a spacing of 2.25mm and consists of 32x48 elements. They may also be placed in an arbitrary pattern for manual use or use with custom devices.
  • the upper surface also contains entry ports for the addition of the two common reagents, comprised respectively of 214+215 and 216+217.
  • These ports have dimensions adapted to automated loading devices such as micropipettors, for example, a standard 200 ⁇ L plastic pipette tip of tip diameter 1.5mm; micropipette tips of diameter 1mm; piezoelectric or ceramic drop delivery systems; and inkjet-based fluid delivery systems.
  • the dimensions of the ports must be a few times greater than the size of the droplets, e.g., 0.2mm for a InL drop.
  • entry ports are air ports 205 and 206 that allow air to escape from the common reagent reservoirs 401 and 402 (discussed below).
  • the disc is able to distribute three fluids to an arbitrary port only by having a three-dimensional construction: fluid paths must "cross over" one another. As a result, some of the fluid motion occurs on the upper face of 201.
  • Reagent aliquotting manifold 210 is such a distribution channel; its connection to bulk reagent reservoir 402 is via through hole 207 and exit channel 208.
  • vias 211 which penetrate from one side of the disc to the other, allowing fluids to be distributed from the top to the bottom of the disc.
  • the manifold 210 terminates in a via 218 which communicates with an overflow reservoir 403 discussed below. Also visible on the upper surface are air-ports 212 and 213 whose function will be discussed further below.
  • Figure 2b is a detail of the fluid entry to the manifold.
  • the through-hole 207 connects the upper surface ofthe disc within the channel 208 to the reservoir 402 on the lower surface ofthe disc.
  • Figure 3 shows the sealing film 301.
  • the sealing film is typically of a thin, flexible material that can be sealed to the upper surface ofthe disc using an adhesive or heat-bonded into place, such that it seals all fluid channels. It is also shaped such that fluid entry ports and air vents are not blocked.
  • Figure 4a illustrates the bottom surface of the reservoir layer 201. Shown here are a number of through features from Figure 2b, including the entry vias 204. Also shown are the common reagent reservoirs 401 and 402. Reservoir 401 distributes fluids along the lower face ofthe reservoir layer, while 402 distributes fluids through manifold 210 on the upper surface. Also shown are the overflow reservoirs 403 and 404 corresponding to reagent reservoirs 402 and 401, respectively.
  • Figure 4b is a detail ofthe region around reagent reservoir 401. The reservoir is accessed through hole 215 and entry passageway 406; this may be shaped as shown to prevent flow of fluid toward the air vent 206.
  • the depth ofthe reservoir 407 can be contoured to prevent fluid from reaching the hole 206 before the remainder of the reservoir has been filled.
  • the reservoir 401 is connected via a channel 408 to a distribution manifold 409 through which the reagent is distributed.
  • the fluid samples enter via ports 204 and channels 411.
  • Figure 4c is a detail ofthe region around reagent reservoir 402.
  • the reservoir is accessed through hole 217 and entry passageway 412; this may be shaped as shown to prevent flow of fluid toward the air vent 205.
  • a restriction in depth of the reservoir 407 can successfully prevent fluid from reaching the hole 206 before the remainder of the reservoir has been filled.
  • the reservoir 402 also contains a via 207 which communicates with the manifold 210 on the upper surface ofthe disc.
  • Figure 4d illustrates an expanded view of a section of the reservoir layer showing the reservoirs involved in a single assay.
  • this embodiment of the platforms of the invention contains three reservoirs plus one detection chamber for each assay.
  • Each reservoir has dimensions of from about 0.05mm to about 5mm wide, from about 0.05mm to about 20mm long, and from about 0.05mm to about 5mm thick, and has a volumetric capacity of from about O.lnL to about 500 ⁇ L.
  • Reservoirs 417, 418, and 416 are designed to contain fluids Ai(in some embodiments, this will the a sample), B, and C.
  • reservoir such as reservoir 418 that is fluidly connected to the reagent manifold is terms an "aliquotted reagent reservoir".
  • the detection cuvette for this assay is detection chamber 420 with air-port 213 leading to air displacement hole 214.
  • Air displacement holes 214 that allow air displaced by the motion of fluids to escape, have a cross- sectional dimension of from about 100 to about 500 ⁇ m. These holes may optionally be replaced by a manifold or series of channels connecting the receiving reservoirs to one or more air holes.
  • the detecting reservoirs are designed to be accessible to optical interrogation, for example, by being composed of optically-transparent plastics or other materials. Also shown is the distribution manifold 409 that communicates with the filling channel 415. Filling channel 415 terminates at aliquotted reagent reservoir 418.
  • a narrow passageway 414 is connected to filling channel 415.
  • Passageway 414 passes through one or more capillary junctions 413 to air port 212.
  • Reservoir 416 is connected via passageway 419 and via 211 to the distribution manifold 210 on the upper surface of the disc.
  • reservoir 417 is connected via sample input port 204 to the interface
  • This collection of reservoirs and structures — 416, 417, 418, 420, 415, 414, 413, 212, 416, 419, 211, 417, and 411 — is repeated on the illustrated platform of the invention a total of 96 times azimuthally around the disc with an angular spacing of about 3.5°.
  • the 96 arrays are sub-divided into two groups of 48; which are placed with azimuthal symmetry around the disc.
  • Platforms having a smaller or greater number of arrays of such reservoirs are within the scope of the invention being most preferably evenly spaced around the surface area of the platform in configurations that match the pattern of microfluidics components on the microfluidics layer.
  • Microfluidics Layer The microfluidics layer of the embodiment of the platform of the invention is shown in Figures 5a through 5d.
  • Microfluidics layer 500 is optimally of the same lateral dimensions as the reservoir layer. There is also an optional center hole for mounting on a spindle, although this is not required in all configurations.
  • the microfluidics layer contains an array 501 of microfluidic structures 502, the number of structures in the array being equal to the number of parallel assays to be run on the platform. In the embodiment illustrated in the Figures, there are 96 such structures evenly repeated with angular spacing of about 3.5°.
  • Microfluidics structures 502 preferably comprise microchannels having cross-sectional dimensions of from about 5 ⁇ m to about 500 ⁇ m and a depth in the microfluidics layer of from about lO ⁇ m to about 3mm.
  • FIG. 5b is an expanded view of a single unit of microfluidic structures.
  • Each microfluidics structure comprises one microfluidics assay.
  • the microfluidic structure consists of depressions in the surface of the microfluidic disc of a single or multiple depths ranging between 2 microns and lOOOmicrons, while the widths of the depressions varies from about 2 ⁇ m to about 500 ⁇ m, as further described below.
  • microchannels 505 and 506 are aligned by assembly between the reservoir layer and microfluidics layer so that the microchannels protrude into reservoirs 416 and 417, respectively.
  • Microchannels 505 and 506 in some embodiments narrow to form capillary junctions 508 before joining mixing microchannel 509.
  • Mixing microchannels are configured to provide mixing of different solutions as the mixture traverses the longitudinal extent of the microchannel. The degree of mixing is dependent on the flow rate of the fluids and the longitudinal extent of the mixing microchannel, which is proportional to the amount of time the two fluids are in contact and are mixed together.
  • the degree of mixing is also dependent on the lateral extent of the mixing microchannel, and is further dependent on the diffusion constants of the fluids to be mixed, i order to accommodate mixing microchannels having sufficient lengths for mixing fluids having a useful range of viscosities, the mixing microchannels are provided as shown in Figure 5b, wherein mixing is promoted as illustrated in Figure 5b by configuring the microchannel to bend several times as it traverses a path on the platform surface that is perpendicular to the direction of rotation, but extends radially on the surface of the platform from a position more proximal to a position more distal to the axis of rotation.
  • Mixing microchannel 509 has a length of from about 1mm to about 100mm, its length in some cases achieved through the use of bends.
  • Mixing microchannel 509 is provided with a capillary junction of a restriction in the lateral dimension at 510 wherein the interior diameter of the microchannel is reduced by about 0 to 95%, and then joins capillary junction 511.
  • Capillary junction 511 is larger in the lateral or vertical direction or both than the restriction 510.
  • the mixing time is 500 seconds, an unacceptably long time for most reactions.
  • This mixing time may be reduced by mechanical stirring, for example, but stirring is difficult to obtain in fluids confined in small structures because the flow ofthe fluid is laminar and does not contain turbulent eddies that are known to promote mixing. If, instead of placing fluids A and then B in a 1mm 3 container, fluids A and B were placed side-by-side in a long, thin capillary of lateral dimension d, the relevant time for mixing is much shorter. If, for example, d is 100 microns, mixing time t is 20 seconds.
  • the mixing channels of the device simulate the placement of fluid in a long capillary by co-injecting fluid streams A and B into a capillary microchannel. These fluids flow side-by-side down the channel initially. As the fluid is pushed through the microchannel due to centrifugal force produced by rotation of the platform, diffusion occurs between the fluids.
  • a capillary of sufficiently narrow diameter, sufficient length, and a pumping rate that is sufficiently low the portion of A and B of the total volumes of A and B present in the channel during pumping can be caused to mix.
  • These choices may be determined by setting the required time for mixing equal to the amount of time necessary for the fluid to traverse the channel.
  • the required time for diffusion is
  • the fluid properties are the density p and viscosity ⁇ , ⁇ R and ⁇ R> are the extent along the radius and average radial position of the fluid subject to centripetal acceleration, and / and d H are the length and hydraulic diameter of the channel.
  • MicroChannel 514 passes through a restriction in the lateral dimension at 515 wherein the interior diameter of the microchannel is reduced by about 1-99%, and then joins capillary junction 511.
  • the capillary junction leads to a further mixing microchannel 516 that terminates at end 517 and that protrudes into detection chamber 420.
  • Mixing microchannel 516 has a length of from about 1 mm to about 100mm.
  • overflow reservoirs 503 and 504 as shown in Figure 5c and 5d.
  • Each overflow structure abuts at 518 with the terminus of a distribution manifold. Entry 518 passes through passageway 519 to enlargement 520, forming a capillary junction. This is then connected via channel 521 that ends at 522, internal to an overflow chamber.
  • FIG. 6 illustrates three assay sectors of the assembled platform, in which the reservoirs of the reservoir layer are mated to microchannels from the microfluidics layer.
  • the platform layers are mated as described in more detail below.
  • capillary valving is understood to depend on geometry, fluid properties and rotational rate, as disclosed more fully in U.S. Serial Nos. 08/761,063, filed December 5, 1996; 08/768,990, filed December 18, 1996; and 08/910,726, filed August 12, 1997, incorporated by reference herein.
  • Alternative arrangements of the microfluidic layers of the platforms of the invention can be provided to contain any number of concentric rings of assays consistent with the amount of surface area available on the platform surface and the extent of the surface taken up by any one embodiment of microfluidics required to perform an assay.
  • the fluid channels described here are preferably of a size that the residence time within the channel of a fluid element under centrifugal flow is sufficient to allow diffusional mixing across the diameter of the channel.
  • the design of such mixing elements is defined in co-owned and co-pending application U.S. Serial NO. 09/595,239, filed June 16, 2000, incorporated by reference.
  • the total number of assays that can be fit onto the disc is 706.
  • the collection/detection chamber should be closer to the edge of the platform than the reagent reservoirs, so that there will be sufficient hydrodynamic pressure produced by convenient rotational speeds to motivate the fluid through the microchannels and mixing elements and into the collection/detection chambers. Placement of the collection/detection chambers at the outer edge of the platform also facilitates detection using a fixed optical detector. However, for extremely high-density platforms this may not be the most efficient way to arrange the assay components.
  • a detector that can access cuvettes at a variety of radial and azimuthal positions.
  • An example of a scanning optical system would be one in which the optical signal is scanned radially, while the disc could be indexed beneath the optics azimuthally. In this way the optics can address any point on the disc surface.
  • Scanning methods include a detector on a linear drive that moves radially; alternately, the optical signal may be scanned radially through the use of a galvanometrically-controlled mirror system.
  • the platform of the invention is used for the performance of assays in the following fashion, referring to Figures 7 and 8, which illustrate fluid motion in the vicinity of the reservoirs 401, 402, 403, 404 and an assay structure, respectively.
  • the assays were run as follows. Aliquots of fluid A are added ports 203+204; the volume of the individual aliquots are identical, but may range depending upon the design of the device from InL to 50 microliters. The chosen volume for the aliquot is such that, when fluid fills reservoir 417, it protrudes into 411 for a short distance, typically less than 1/3 of the length of 417.
  • Figures 7 and 8 illustrate the sequence of fluid flows in the vicinity of the reservoirs of microfluidic assay elements.
  • Figure 7a illustrates the flow of fluids entering reservoirs 401 and 402, as well as of samples of fluid A enter ports 217 and channels 414.
  • the platform is then placed on a device that is capable of performing rotations. At a first rotational speed ranging from 100-1000 rpm, fluids A are driven through channels 411 into the reservoirs 417, where they are retained by capillary junctions508.
  • fluid B is driven through hole 207 into manifold 210. As fluid B travels 210, it flows through the vias 211 into passageways 419 and finally reservoirs 416, where it was retained by capillary junctions 508. Fluid B also pases through via 218 and is retained at capillary junction 520 of overflow structure 503. Also at this rotation rate, fluid C is driven through channel 408 and manifold 409 to the fill channels 414, and then to aliquotted reagent reservoirs 418. Fluid in aliquotted reagent reservoir 418 is stopped at capillary junction 513. Fluid C also enters capillary 414 and is stopped at capillary junction 413.
  • Fluid C completely fills 409 and is also stopped at capillary junction 520 over overflow structure 503.
  • the rotational rate is then increased to a second speed.
  • the overflow capillary valves formed 520 on the overflow structures 503 and 504 release.
  • Fluid A in manifold 210 flows into the overflow reservoir 403, leaving behind solution in the reservoirs 416.
  • fluid C flows into reservoir 402; as it flows, the fluid in each assay structure at capillary junctions 413 is "pulled".
  • the fact that aliquotted reagent reservoir 418 is radially-outward from 413 means that there is rotationally-induced resistance to drawing the fluid from aliquotted reagent reservoir 418.
  • the tension in the fluid at 413 is relieved through the introduction of air via the channel and port 212; by introduction of this air bubble, solution C within the manifold 409+415 is effectively separated from fluid remaining in aliquotted reagent reservoir 418.
  • the speed is then increased to a third value, at which point the capillary junctions at 508 and 513 allows fluid to flow.
  • the fluids from reservoirs 505 and 506 flow through channel 509 and are halted at the junction 510; similarly, the fluid flowing through 514 was halted at the junction 515.
  • the capillary junctions at 511 allow the fluids to flow.
  • the mixing fluids are then pumped via centrifugation into the detection reservoir 420. hi the case of the junctions 507 and 511, whichever fluid flows first is forced to wet the exit capillary of the other fluid in the capillary junction, thereby inducing it to flow as well.
  • the various rotational rates need not be monotonically increasing.
  • the velocity may be "spiked" momentarily from a low value to high value when a capillary valving event is desired; if it is then reduced quickly to a lower value, the next capillary valving event may be designed to operate at the same rotational rate as the first, or even a lower rate.
  • a large number of events may be designed to function serially.
  • microfluidic layer 500 are sized and spaced so that they mate with those of layer 201 in the preceding example.
  • the additional elements in this embodiment are capillary 901, a combined capillary junction and overflow chamber 902, and air-vent 903.
  • This embodiment is designed to meter an imprecise volume of "sample" fluid for each assay structure.
  • the function of this alternative is the same as in the previous embodiment, with these additional features: At the first rotational speed, sample fluid is delivered via channel 411 to reservoir 417. As it flows to the reservoir, some fluid enters capillary 901 but is retained at the expansion of 901 into capillary junction 902.
  • capillary 901 The fluid fills the reservoir and is halted by capillary junction 508 in the microfluidics layer (not shown in this figure).
  • the dimensions of capillary 901 are chosen so that fluid is able to pass opening 902 at a rotational speed intermediate between the first and second rotational speeds discussed above. Displaced air is vented through 903, and fluid which extends radially-inward of the inersection of cahnnel 411 and capillary junction 902 flows into capillary junction 902.
  • Air vent 903 may be chosen to be small enough that fluids cannot escape it at any rotational speed normally used for the device. The selection ofthe diameter of capillary 901 depends on the expected amount of excess volume.
  • the device may be designed so that the user is required to add 0.75 ⁇ L, as long as the volume of channel 901 is 0.05 ⁇ L or less.
  • the radial position of 902 is the same as that of capillary junction 508 on microfluidic layer 500, the diameter of capillary 901 at capillary junction 902 need only be somewhat larger than that ofthe channels that meet at capillary junction 507 in order to function.
  • a lOO ⁇ m wide and lOO ⁇ m deep channel 901 meets requirements.
  • FIG. 10 A second alternative construct is shown in Figure 10.
  • the manifold 210 is positioned radially-outward of reservoirs 416, 417, and 418.
  • Via 211 connects with channel 1003 that leads radially-inward to a microchannel configuration identical to that associated with aliquotted reagent reservoir 418 described above, consisting of capillary 1004, capillary junctions 1005, and air vent 1006. It will be understood that this structure behaves like that associated with aliquotted reagent reservoir 418 in the previous description, by isolating fluids in the multiple reservoirs 416 from one another.
  • channel 1003 resides on the "upper" face of the layer 201 are within the scope of the invention, as long as a via connecting the fluid path to the lower face is made, for example, at the radially-proximal end of 416; this may be advantageous in order to "pack" structures most effectively in the azimuthal direction.
  • This alternate construction may provide advantages for liquids that have unpredictable properties such as viscosity and surface tension. With such fluids, it is possible that bubbles may accidentally be introduced in manifold 210 in the previously described embodiment. These bubbles make draining of the manifold, and isolation of the reservoirs 416, difficult. By introducing bubbles at each reservoir, the need for maintaining a single plug of fluid in manifold 210 is relaxed
  • FIG. 11 A third alternative construction with additional functionality is shown Figure 11.
  • a microfluidic network for the creation of a dilution series is illustrated and is part of a larger network of structures used for various purposes.
  • the fluid distribution scheme illustrated here is advantageous not only for the three-fluid homogeneous assays disclosed herein but can be applied to any centrifugally-based process which requires the creation of such dilution series.
  • the platform has only three ports and reservoirs for fluid addition: Reservoirs 401 and 402 for common reagents, as previously discussed, and reservoirs 601 and 602 placed on a surface of the platform 201 and accessed by entry ports 618 and 619 respectively. Reservoirs 401 and 402 lead to distribution manifolds, overflows, and assay reservoirs as previously discussed. Fluid channel 603 exits reservoir 601 and is split into two components at what will be called a T-junction 604, a portion of which continues to further T-junctions and a portion of which, 607, terminates at a capillary junction 609.
  • reservoir 602 leads to channel 605, which is split at T-junction 606; one arm of the split channel continues to further T- junctions, while the other arm, 608, terminates at the capillary junction 609.
  • the structure 650 composed of reservoirs and channels as previously disclosed, embodies the same functionality as that given in Figure 6.
  • Channel 419 for example, is the passage for the entry of first reagent into reservoir 416.
  • the other portion of channel 603 terminates at capillary junction 615.
  • channel 605 leads to T-junction 612, where it is split into channel 613 which terminates at capillary junction 618 and a portion which continues to assay structure 651.
  • the capillary junctions 609, 615, and 616 all are fluidly connected to channels 614, 640, and 641, respectively.
  • Channels 640 and 641 lead respectively to assay structures 653 and 654.
  • Channel 614 is further split at a 4-armed junction 617 into 3 channels: A continuation of 614, which leads assay structure 652, and side channels 618 and 619 which terminate at capillary junctions 615 and 616, respectively.
  • the disc may be used to distribute liquids for an assay in the following fashion.
  • Common reagents are loaded into reservoirs 401 and 402.
  • Sample (fluid A) is loaded into reservoirs 601 and a diluent buffer (fluid B) into reservoir 602.
  • the common reagents are distributed to reservoirs 416 and 418 as previously described.
  • Sample and diluent enter channels 603 and 605. Fluid A reaches the T- junction 604, at which point a portion of the fluid continues down channel 603 and a portion flows into channel 607.
  • fluid B splits at 606 into channels 605 and 608.
  • the portion of A present in 607 reaches capillary junction 609, as does the fluid B present in 608.
  • the fluid in channel 614 After sufficient time for diffusional mixing in the channel, arrives at junction 617 with a volume fraction of A equal to 0.5 and B equal to 0.5, i.e., the fluids A and B are "mixed".
  • the mixed fluid arriving at 617 is denoted fluid Cl.
  • Fluid Cl is split into 3 streams at junction 617.
  • a portion of that mixed liquid Cl now mixes with the original A solution which has been directed by channel 603 to junction 610 and channel 611, by passing through capillary junction 615.
  • This fluid, denoted C2 is in channel 640 and has volume fraction of A of 0.75 and B of 0.25.
  • the fluid in 641 has volume fraction of A of 0.25 and B of 0.75.
  • the fluidic network delivers 5 concentrations of A — 1.0, 0.75, 0.5, 0.25, 0.0— to the structures 650, 651, 652, 653, and 654, respectively.
  • the flow rates of the two fluids entering any mixing channel 614, 640, and 641 must be equal. This is assured by the diameter of the channels, as fluid flow is controlled by the fluidic impedances of the various mixing channels. It will be understood that the process of dividing and recombining channels illustrated may be continued indefinitely. One further splitting and recombination in the manner shown would lead to a total of 9 concentrations of A: 1.0, 0.875, 0.75, 0.625, 0.5, 0.375, 0.125, 0.0625, 0.0.
  • this mixing scheme need not be restricted to use with the three-fluid homogeneous assays previously discussed, but may be used to deliver a fluid of arbitrary composition to a point on the platform.
  • fluidic design A number of variations in fluidic design are possible, either dictated by assay requirements, fluidic requirements, ease-of-use or reduction in automation or all of these factors.
  • capillary valves have been shown to retain fluids in an intermediate chamber at elevated temperatures, used for incubation (as disclosed more extensively in co-owned U.S. Patent No. 6,063,589, issued May 16, 2000, incorporated by reference).
  • Assays that require intermediate incubations, for example, because of slow chemical kinetics, may be performed in such structures.
  • assays for which diffusional mixing is insufficient may require agitation of the fluid to effect mixing, hi such a case, active valves can be used, which retain the fluids against the sudden pressure changes induced by agitation, as described in more fully in co-owned and co-pending U.S. Serial No. 09/315,114, filed May 19,
  • Figure 11 is functionally identical to that of Figures 1-8, the only significant difference being that that of Figure 11 is designed for the performance of 24 assays, while that of Figures 1-8 is designed for the performance of 96 assays.
  • the platform was prepared as follows.
  • the macrofluidic reservoir layer 201 was manufactured through machining of acrylic using computer/numerical code machining using a Light Machines VMC5000 milling machine running Light Machines "Benchman” software (Light Machines Corporation, Manchester, NH).
  • the sealing film of as shown in Figure 3 was made by applying a double-sided tape to a thin sheet of heat-stabilized polyester (mylar). A section of mylar bonded to tape was cut from the combined sheet to the correct shape, leaving one adhesive face of the tape for application to the macrofluidic layer.
  • mylar heat-stabilized polyester
  • microfluidics layer was manufactured as follows.
  • a microfluidics structure such as the structure shown in Figures 5a through 5d was designed using in a computer aided design package such as AutoCAD (Autodesk, San Rafael CA) and Freehand (Macromedia Inc., San Francisco, CA). This design was converted into a photomask by printing at high resolution (3386 dpi) on a transparent plastic sheet.
  • a 125-mm diameter silicon wafer was coated with a layer of negative photoresist (SU-8(50)) and spun on a spin-coater (Chemat Technology, Northridge, CA) at a speed sufficient (200 to 8000 rpm) to give a desired thickness between 5 ⁇ m and 500 ⁇ m.
  • SU-8(50) negative photoresist
  • spin-coater Chemat Technology, Northridge, CA
  • the silicon wafer was baked to have a smooth surface and then the photoresist partially cured.
  • the silicon wafer was exposed to ultraviolet (UV) light using a conventional UV source and mask aligner.
  • UV ultraviolet
  • the photoresist was then developed in propylene glycol methyl ether acetate and non-crosslinked photoresist removed through washing in dichloromethane.
  • the resulting relief was then passivated by exposure to a vapor of tridecafluoro- 1,1,2,2- tetrhydrooctyl-1-trichlorosilane and used as a mold for microfabrication (Duffy et al, 1998, Anal Chem. 70: 4974-4984).
  • PDMS polydimethylsiloxane
  • crosslinking agent Sylgard 184, Dow Corning
  • Sealing film with adhesive exposed was first applied to the upper surface ofthe macrofluidic layer so that it completely covered the holes and channels 207, 208, 211, 218.
  • Final assembly was completed by forming a reversible, conforming seal between the PDMS microfluidics layer and the bottom surface of the macrofluidic reservoir layer 201 made through simple physical contact ofthe two components. This seal is based on physical adhesion forces alone — an der Waals attraction forces and potentially static electrical charge present on the surfaces — and was sufficient to seal the disc against leakage due to the centripetally-induced pressures used.
  • the platform shown in Figure 11 and prepared as described herein was used to perform simultaneously and in parallel 24 enzyme inhibition assays. Fluids were deposited in the reservoirs formed in reservoir layer 201 when reservoir layer is mated or bonded with microfluidics layer 500. Platform 100 is then rotated using a rotational profile designed to drive fluids through the channels within the macrofluidic disc 201 and the microfluidic disc 500.
  • the platform shown in Figure 11 possesses the same features as that shown in
  • fluid A if an inhibitor was present in fluid A, mixing fluid A with fluid B will, after a sufficient time resulted in a chemical reaction or other change induced by the inhibitor in most or all of the enzyme molecules, rendering them incapable of catalyzing the desired reaction. If this solution was mixed with the substrate solution, little or no change in the measured parameter was seen.
  • the system chosen to model homogeneous assays consisted of theophylline as inhibitor, alkaline phosphatase as the enzyme, and 7-nitrophenol phosphate (PNPP) as the substrate.
  • PNPP 7-nitrophenol phosphate
  • Theophylline was used in concentrations of O.OlmM to lOOmM to provide a standard dose-response curve in the inhibitor.
  • Alkaline phosphatase was used in a lmg/mL solution.
  • PNPP was used as a 0.5mM solution. All solutions were made in a buffer of 0.1 M glycine and 0.5mM MgCl 2 in deionized water.
  • the dimensions of the platform used for these assays were as follows.
  • the overall platform diameter was 12cm.
  • the macrofluidic disc was about 1.6mm thick.
  • the diameter of the sample entry ports through-holes 204 was 0.5mm; the depression 203 was conical, with an outer diameter of 2mm and a depth of 1mm, allowing the cones to "guide" the placement of pipette tips when loaded manually.
  • the common reagent entry ports consisted here of only through holes 215 and 217, also of diameter 0.5mm.
  • the air ports 205 and 206 were also 0.5mm in diameter.
  • the reagent manifold through-hole 207 was also 0.5mm in diameter, and the exit channel 208 was of larger diameter and depth of 0.43mm.
  • the exit channel narrowed to join the channel 209 of width 0.45mm.
  • the manifold 210 was also 0.43mm deep and0.45mm wide.
  • the vias 211 were 0.45mm in diameter and penetrated through the macrofluidic disc from the top surface to the bottom surface.
  • the terminal via 218 had a diameter of 0.53mm and penetrated to the bottom surface ofthe layer.
  • the dimensions of the features on the lower face of the macrofluidic disc were as follows.
  • the common reagent reservoirs 401 and 402 had a depth of 1.14mm.
  • the radial positions of the ends of these reservoirs most proximal to the center of the disc were 1.59cm and that of the ends most distal from the center of the disc were 3.4cm.
  • the volume allowable in reagent reservoir 402 was bO ⁇ L, while that of reservoir 401 was llO ⁇ .
  • Entry passageway 406 was 0.25mm deep and 0.25mm wide.
  • Channel 408 was 0.25mm wide x 0.25mm deep, as was manifold 409.
  • Entry channels 411 were 0.25mm wide x 0.25mm deep; their lengths varied according to the relative positions of the reservoir 417 and entry port 204 that each channel connected, from about 12mm to about 27mm.
  • Channel 411 preferably opens at its connection to reservoir 417 such that acute angles are not presented within the plane ofthe disc that might impede fluid flow.
  • the inner radii of reservoirs 416, 417, and 418 were about 4.1cm and outer of reservoirs 416, 417, and 418 were about 4.5cm. Both inner and outer ends of the reservoirs were rounded with radii of 0.5m to prevent fluid from both "stopping" at the inner end during loading due to capillary forces and being retained as the reservoirs emptied.
  • Reservoirs 416, 417, and 418 were about 0.57mm, 0.57mm, and 1.14mm deep, respectively. Each reservoir was 0.6mm in width. The lengths, depths, and widths of the reservoirs were chosen such that the volumes contained within 416 and 417 were 0.91microliters while that contained with aliquotted reagent reservoir 418 was twice that volume, 1.82 microliters.
  • Detection reservoirs 420 were constructed of optically-transparent material and had an outer radius of about 5.7cm and an inner radius of about 5.2cm, were 0.7mm deep, and had a subtended angle of 3.2° and were thus designed to accommodate the combined volumes of reservoirs 416, 417, and 418 (approximately 3.6 microliters).
  • Distribution manifold 409 is connected to aliquotted reagent reservoir 418 via a filling channel 415 which as 0.25mm wide x 0.25mm deep; the end of 415 was also enlarged at its connection to aliquotted reagent reservoir 418.
  • Capillary channel 414 was 0.13mm wide x 0.13mm deep.
  • the capillary junctions 413 were 0.25mm deep x 0.5mm wide; they were formed so that the opening of 414 into 414 formed a backward angle of 45°, thus increasing the capillary stopping power of the junction.
  • the connection to reservoir 416 is via passsageway 419, which was about 0.25mm deep and widened by 0.25mm wide to 0.6mm wide at its joining with 416.
  • the microfluidics layer 500 was also 12cm in diameter and had a thickness between 1 and 2mm (although the thickness is not important) and was composed of white PDMS.
  • the depth of all microfluidic structures (that was determined by the height of the SU-8 relief) was lOO ⁇ m.
  • the width of the entrance to the mixing channels, 505, 506, and 512, was 200 ⁇ m.
  • the channels narrowed to lOO ⁇ m before reaching the capillary junction at 508.
  • the width of the junction 508 was 120 ⁇ m.
  • the entrance 512 narrowed to lOO ⁇ m prior to the junction 513 that was 200 ⁇ m.
  • the widths of channels 509 and 514 was lOO ⁇ m.
  • the lengths of the mixing channels was chosen to provide sufficient time for mixing via diffusion with liquids of moderate diffusion constant (5xl0 "6 cm 2 /s) as fluids are pumped through them under the influence of centripetal acceleration.
  • the lengths of channels 509 and 514 was about 17mm. These channels narrowed to 50 ⁇ m at 510 and 515 before joining the junction 511, which was about 0.4mm square.
  • Channel 516 was lOO ⁇ m wide and about 38mm long. These dimensions resulted in the fluids talcing > 2sec to transit the mixing microchannels.
  • the entry 518 was 0.4mm x 1.8mm, while the capillary passageway 519 was 120 ⁇ m wide.
  • Enlargement 520 was about 200 ⁇ m wide by 200 ⁇ m long, and 521 was also lOO ⁇ m long.
  • the assays were run as follows. 1 ⁇ L aliquots of theophylline solutions having the concentrations set forth above were loaded into entry ports 203+204 using a pipette. A total of ⁇ "f ⁇ L of alkaline phosphatase was loaded into reservoir 402 through entry port 217, and a total of PNPP solution was loaded into reservoir 401 through entry port 215. The platform was placed on the spindle of an instrument containing a diffuse reflectance optical head capable of three-color measurements. Figures 7 and 8 illustrate the sequence of fluid flows in the vicinity of the reservoirs of microfluidic assay elements. The platform was first rotated at 300rpm for 30seconds.
  • the theophylline solutions were driven completely through channels 411 into the reservoirs 417, where it was retained by capillary junctions 508.
  • the alkaline phosphatase solutions were driven through hole 207 into manifold 210.
  • the alkaline phosphatase solution traveled 210, it flowed through the vias 211 into passageways 419 and finally reservoirs 416, where it was retained by capillary junctions 508.
  • the PNPP solution was driven through channel 408 and manifold 409 to the fill channels 415.
  • the PNPP solution was driven through 414 to the aliquotted reagent reservoirs 418; PNPP solution also entered capillary 414 and was stopped at capillary junction 413 and at capillary junction 513.
  • the rotational rate was then increased to 500rpm.
  • the overflow capillary valves formed by 519 and 520 on the overflow structures released.
  • the alkaline phosphatase solution in manifold 210 then flowed into the overflow reservoir 403, leaving behind solution in the reservoirs 416.
  • the draining of excess PNPP solution into the overflow reservoir 402 exerted an inward "pull" on the solution at the capillary junctions 413.
  • the tension in the fluid in channel 415 so created was relieved through the introduction of air via channel 413; this effectively separated the draining PNPP solution in 415+409 from the solution in the aliquotted reagent reservoirs 418.
  • the speed was increased to 600rpm, at which point the capillary junctions at 508 and 513 allowed fluid to flow.
  • the fluids from reservoirs 505 and 506 flow through channel 509 and were halted at the junction 510; similarly, the fluid flowing through 514 was halted at the junction 515.
  • the capillary junctions at 511 allowed the fluids to flow.
  • the mixed fluids were then pumped into the detection reservoir 420. hi the case ofthe junctions 507 and 511, whichever fluid flows first is forced to wet the exit capillary ofthe other fluid in the capillary junction, thereby inducing it to flow as well.
  • the ratio of the alkaline phosphatase and theophylline flow-rates as a function of time in mixing microchannel 509 is given exactly by where A A and B B are the cross-sectional area ofthe reservoirs 416 and 417 as a function of time, or alternately, radial position of the meniscus as fluid is removed from the reservoirs. If it was desired that the ratio of flows is constant (as was the case here), it was sufficient to maintain a constant ratio of cross-sectional areas as a function of radial position. Note that this does not imply that the cross sections are constant, just that their ratio is.
  • the ratio expressed in the equation can be manipulated by altering the ratio of cross-sectional areas of the reservoirs, as disclosed more fully in co-owned U.S. Patent No. 6,063,589, issued May 16, 2000 and incorporated by reference.
  • microchannel 509 and 516 are long and the flow rates can be controlled by rotational rate, the co-flowing streams are present in those channels for a time sufficient enough for diffusion across the interface between these streams to effect complete mixing ofthe solutions.
  • the optical system also advantageously contained a beam-splitter that sent a fraction of the incident light to a reference photodiode.
  • Two detectors used in this optics system were the assay detector, which measured diffusely-reflected light; and the reference detector, which measured a fraction ofthe incident light. Measurements at each detector were made when both the 430nm and 630nm light sources were active as well as when they were "dark" or off. The measured voltages were thus: V D ° dark measurement in assay detector V R D dark measurement in reference detector
  • V D measurement at absorbing wavelength ⁇ i (430nm) in assay detector
  • V D 2 measurement at non-absorbing wavelength in ⁇ 2 (660nm) assay detector
  • the absorbance at 430nm is calculated from
  • C PN p is the concentration of yellow product, j ⁇ -nifrophenol; this concentration is inversely related to the concentration of theophylline in the initial solution.
  • Figure 12 shows data for 24 assays run simultaneously on the platform, representing four-fold replicates for each of six theophylline concentrations ranging from 0 to lOmM. The data are consistent with those generated on the laboratory bench using absorbance and that contained in co-owned and co-pending U.S. application Serial No. 09/595,239, filed June 16, 2000, incorporated by reference herein.
  • microplatform systems according to the invention can be used as a substitute for conventional 96-well microtiter plates for performing enzyme assays to determine enzymatic activity thereof.

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  • Chemical Kinetics & Catalysis (AREA)
  • Health & Medical Sciences (AREA)
  • Dispersion Chemistry (AREA)
  • General Health & Medical Sciences (AREA)
  • Analytical Chemistry (AREA)
  • Organic Chemistry (AREA)
  • Hematology (AREA)
  • Clinical Laboratory Science (AREA)
  • Apparatus Associated With Microorganisms And Enzymes (AREA)
  • Investigating Or Analysing Biological Materials (AREA)
  • Investigating Or Analysing Materials By The Use Of Chemical Reactions (AREA)
  • Optical Measuring Cells (AREA)
  • Automatic Analysis And Handling Materials Therefor (AREA)
  • Physical Or Chemical Processes And Apparatus (AREA)

Abstract

L'invention concerne des procédés et un dispositif servant à mettre en oeuvre des analyses et des procédures de microanalyse et de microsynthèse. L'invention concerne une plate-forme pour microsystèmes et un dispositif de micromanipulation de la plate-forme qui utilise la force centripète résultant de la rotation de la plate-forme pour produire un déplacement de fluides dans des microcanaux. Ces techniques peuvent être mises en oeuvre à diverses fins, notamment mais pas exclusivement dans le criblage de composés candidats thérapeutiques, la recherche biologique et le diagnostic clinique et moléculaire. L'invention concerne des procédés propres au dispositif de l'invention, qui permettent de mettre en oeuvre une gamme très variée de processus de microanalyse et de microsynthèse.
PCT/US2001/015743 2000-05-15 2001-05-15 Dispositifs microfluidiques et procedes de criblage a haut debit WO2001087485A2 (fr)

Priority Applications (3)

Application Number Priority Date Filing Date Title
EP01937420A EP1284819A2 (fr) 2000-05-15 2001-05-15 Dispositifs microfluidiques et procedes de criblage a haut debit
AU2001263162A AU2001263162A1 (en) 2000-05-15 2001-05-15 Microfluidics devices and methods for high throughput screening
JP2001583935A JP2004501360A (ja) 2000-05-15 2001-05-15 ミクロ流体装置および高スループット・スクリーニングのための方法

Applications Claiming Priority (8)

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US20427300P 2000-05-15 2000-05-15
US20427200P 2000-05-15 2000-05-15
US60/204,272 2000-05-15
US60/204,273 2000-05-15
US09/595,239 2000-06-16
US09/595,239 US6582662B1 (en) 1999-06-18 2000-06-16 Devices and methods for the performance of miniaturized homogeneous assays
USPCT/US00/16653 2000-06-16
PCT/US2000/016653 WO2000079285A2 (fr) 1999-06-18 2000-06-16 Dispositifs et methodes permettant d"effectuer des analyses homogenes miniature

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WO2001087485A2 true WO2001087485A2 (fr) 2001-11-22
WO2001087485A3 WO2001087485A3 (fr) 2002-04-04

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JP (1) JP2004501360A (fr)
AU (1) AU2001263162A1 (fr)
WO (1) WO2001087485A2 (fr)

Cited By (23)

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WO2003018198A1 (fr) * 2001-08-28 2003-03-06 Gyros Ab Microcavite microfluidique de retention microfluidique et autres structures microfluidiques
WO2004007079A1 (fr) * 2002-07-12 2004-01-22 Applera Corporation Disque rotatif de support d'echantillons et son procede de chargement
EP1534429A2 (fr) * 2002-07-26 2005-06-01 Applera Corporation Caracteristiques de conception de micro-canal facilitant un transfert de fluide centripete
US6919058B2 (en) 2001-08-28 2005-07-19 Gyros Ab Retaining microfluidic microcavity and other microfluidic structures
EP1566215A2 (fr) * 2004-02-17 2005-08-24 Boehringer Ingelheim microParts GmbH Plateforme microstructurée et procédé de manipulation d'un liquide
WO2006030218A1 (fr) 2004-09-15 2006-03-23 Bp Oil International Limited Procede d'evaluation d'une charge d'alimentation de raffinerie
US7033747B2 (en) 2001-04-11 2006-04-25 Nagaoka & Co., Ltd Multi-parameter assays including analysis discs and methods relating thereto
US7041258B2 (en) 2002-07-26 2006-05-09 Applera Corporation Micro-channel design features that facilitate centripetal fluid transfer
US7054258B2 (en) 2000-12-08 2006-05-30 Nagaoka & Co., Ltd. Optical disc assemblies for performing assays
US7079468B2 (en) 2000-12-08 2006-07-18 Burstein Technologies, Inc. Optical discs for measuring analytes
US7091034B2 (en) 2000-12-15 2006-08-15 Burstein Technologies, Inc. Detection system for disk-based laboratory and improved optical bio-disc including same
JP2007527517A (ja) * 2003-07-01 2007-09-27 スリーエム イノベイティブ プロパティズ カンパニー 開口部のないチャンネルを備えたサンプル処理装置
US7390464B2 (en) 2003-06-19 2008-06-24 Burstein Technologies, Inc. Fluidic circuits for sample preparation including bio-discs and methods relating thereto
US7429354B2 (en) 2001-03-19 2008-09-30 Gyros Patent Ab Structural units that define fluidic functions
EP2096341A1 (fr) 2002-12-04 2009-09-02 Spinx, Inc, Dispositifs et procédé pour la manipulation de microfiltration programmable de fluides
EP1955770A3 (fr) * 2007-02-12 2013-07-24 Samsung Electronics Co., Ltd. Dispositif microfluidique à base de force centrifuge pour la dilution et système microfluidique l'incluant
US8592219B2 (en) 2005-01-17 2013-11-26 Gyros Patent Ab Protecting agent
CN109211860A (zh) * 2018-09-29 2019-01-15 厦门大学 一种多项式检测光盘和检测方法
US10309976B2 (en) 2014-06-30 2019-06-04 Phc Holdings Corporation Substrate for sample analysis, sample analysis device, sample analysis system, and program for sample analysis system
US10520521B2 (en) 2014-06-30 2019-12-31 Phc Holdings Corporation Substrate for sample analysis, sample analysis device, sample analysis system, and program for sample analysis system
US10539582B2 (en) 2014-06-30 2020-01-21 Phc Holdings Corporation Substrate for sample analysis, sample analysis device, sample analysis system, and method for removing liquid from liquid that contains magnetic particles
US10539560B2 (en) 2014-06-30 2020-01-21 Phc Holdings Corporation Substrate for sample analysis, and sample analysis apparatus
US10539583B2 (en) 2014-12-12 2020-01-21 Phc Holdings Corporation Substrate for sample analysis, sample analysis device, sample analysis system, and program for sample analysis system

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US7459127B2 (en) 2002-02-26 2008-12-02 Siemens Healthcare Diagnostics Inc. Method and apparatus for precise transfer and manipulation of fluids by centrifugal and/or capillary forces
US7754151B2 (en) * 2005-04-04 2010-07-13 Panasonic Corporation Liquid homogenizer and analyzer employing the same
WO2006108559A2 (fr) * 2005-04-09 2006-10-19 Boehringer Ingelheim Microparts Gmbh Dispositif et procede pour analyser un echantillon liquide
EP2490005A1 (fr) * 2011-02-18 2012-08-22 Koninklijke Philips Electronics N.V. Réseau de résistance microfluidique et dispositif microfluidique

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US5912134A (en) * 1994-09-02 1999-06-15 Biometric Imaging, Inc. Disposable cartridge and method for an assay of a biological sample
GB2341924A (en) * 1998-05-08 2000-03-29 Amersham Pharm Biotech Ab Microfluidic device
WO2000078455A1 (fr) * 1999-06-22 2000-12-28 Tecan Trading Ag Dispositifs et methodes servant au fonctionnement d'essais d'amplification miniaturises in vitro

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EP0608006A2 (fr) * 1990-06-04 1994-07-27 Abaxis, Inc. Rotors analytiques et procédés d'analyse de fluides biologiques
US5912134A (en) * 1994-09-02 1999-06-15 Biometric Imaging, Inc. Disposable cartridge and method for an assay of a biological sample
GB2341924A (en) * 1998-05-08 2000-03-29 Amersham Pharm Biotech Ab Microfluidic device
WO2000078455A1 (fr) * 1999-06-22 2000-12-28 Tecan Trading Ag Dispositifs et methodes servant au fonctionnement d'essais d'amplification miniaturises in vitro

Cited By (36)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US7079468B2 (en) 2000-12-08 2006-07-18 Burstein Technologies, Inc. Optical discs for measuring analytes
US7542383B2 (en) 2000-12-08 2009-06-02 Vindur Technologies, Inc. Optical disc assemblies for performing assays
US7366063B2 (en) 2000-12-08 2008-04-29 Burstein Technologies, Inc. Optical discs for measuring analytes
US7599275B2 (en) 2000-12-08 2009-10-06 Vindur Technologies, Inc. Optical discs for measuring analytes
US7200100B2 (en) 2000-12-08 2007-04-03 Nagaoka & Co., Ltd. Optical disc assemblies for performing assays
US7889615B2 (en) 2000-12-08 2011-02-15 Vindur Technologies, Inc. Optical discs for measuring analytes
US7054258B2 (en) 2000-12-08 2006-05-30 Nagaoka & Co., Ltd. Optical disc assemblies for performing assays
US7091034B2 (en) 2000-12-15 2006-08-15 Burstein Technologies, Inc. Detection system for disk-based laboratory and improved optical bio-disc including same
US7429354B2 (en) 2001-03-19 2008-09-30 Gyros Patent Ab Structural units that define fluidic functions
US7033747B2 (en) 2001-04-11 2006-04-25 Nagaoka & Co., Ltd Multi-parameter assays including analysis discs and methods relating thereto
US7275858B2 (en) 2001-08-28 2007-10-02 Gyros Patent Ab Retaining microfluidic microcavity and other microfluidic structures
US7300199B2 (en) 2001-08-28 2007-11-27 Gyros Ab Retaining microfluidic microcavity and other microfluidic structures
US6919058B2 (en) 2001-08-28 2005-07-19 Gyros Ab Retaining microfluidic microcavity and other microfluidic structures
WO2003018198A1 (fr) * 2001-08-28 2003-03-06 Gyros Ab Microcavite microfluidique de retention microfluidique et autres structures microfluidiques
US7083974B2 (en) 2002-07-12 2006-08-01 Applera Corporation Rotatable sample disk and method of loading a sample disk
US9555409B2 (en) 2002-07-12 2017-01-31 Applied Biosystems, Llc Rotatable sample disk and method of loading a sample disk
US7592172B2 (en) 2002-07-12 2009-09-22 Applied Biosystems, Llc Rotatable sample disk and method of loading a sample disk
WO2004007079A1 (fr) * 2002-07-12 2004-01-22 Applera Corporation Disque rotatif de support d'echantillons et son procede de chargement
US7041258B2 (en) 2002-07-26 2006-05-09 Applera Corporation Micro-channel design features that facilitate centripetal fluid transfer
EP1534429A4 (fr) * 2002-07-26 2005-09-07 Applera Corp Caracteristiques de conception de micro-canal facilitant un transfert de fluide centripete
EP1534429A2 (fr) * 2002-07-26 2005-06-01 Applera Corporation Caracteristiques de conception de micro-canal facilitant un transfert de fluide centripete
EP2096341A1 (fr) 2002-12-04 2009-09-02 Spinx, Inc, Dispositifs et procédé pour la manipulation de microfiltration programmable de fluides
US7390464B2 (en) 2003-06-19 2008-06-24 Burstein Technologies, Inc. Fluidic circuits for sample preparation including bio-discs and methods relating thereto
JP2007527517A (ja) * 2003-07-01 2007-09-27 スリーエム イノベイティブ プロパティズ カンパニー 開口部のないチャンネルを備えたサンプル処理装置
EP1566215A3 (fr) * 2004-02-17 2011-05-25 Boehringer Ingelheim microParts GmbH Plateforme microstructurée et procédé de manipulation d'un liquide
EP1566215A2 (fr) * 2004-02-17 2005-08-24 Boehringer Ingelheim microParts GmbH Plateforme microstructurée et procédé de manipulation d'un liquide
WO2006030218A1 (fr) 2004-09-15 2006-03-23 Bp Oil International Limited Procede d'evaluation d'une charge d'alimentation de raffinerie
US8592219B2 (en) 2005-01-17 2013-11-26 Gyros Patent Ab Protecting agent
EP1955770A3 (fr) * 2007-02-12 2013-07-24 Samsung Electronics Co., Ltd. Dispositif microfluidique à base de force centrifuge pour la dilution et système microfluidique l'incluant
US10539582B2 (en) 2014-06-30 2020-01-21 Phc Holdings Corporation Substrate for sample analysis, sample analysis device, sample analysis system, and method for removing liquid from liquid that contains magnetic particles
US10309976B2 (en) 2014-06-30 2019-06-04 Phc Holdings Corporation Substrate for sample analysis, sample analysis device, sample analysis system, and program for sample analysis system
US10520521B2 (en) 2014-06-30 2019-12-31 Phc Holdings Corporation Substrate for sample analysis, sample analysis device, sample analysis system, and program for sample analysis system
US10539560B2 (en) 2014-06-30 2020-01-21 Phc Holdings Corporation Substrate for sample analysis, and sample analysis apparatus
US10539583B2 (en) 2014-12-12 2020-01-21 Phc Holdings Corporation Substrate for sample analysis, sample analysis device, sample analysis system, and program for sample analysis system
CN109211860A (zh) * 2018-09-29 2019-01-15 厦门大学 一种多项式检测光盘和检测方法
CN109211860B (zh) * 2018-09-29 2023-11-17 厦门大学 一种多项式检测光盘和检测方法

Also Published As

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JP2004501360A (ja) 2004-01-15
AU2001263162A1 (en) 2001-11-26
WO2001087485A3 (fr) 2002-04-04
EP1284819A2 (fr) 2003-02-26

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