DK2281631T3 - Modular microfluidic sample preparation system and method of mixing and delivering a sample fluid. - Google Patents

Modular microfluidic sample preparation system and method of mixing and delivering a sample fluid. Download PDF

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Publication number
DK2281631T3
DK2281631T3 DK09167507.4T DK09167507T DK2281631T3 DK 2281631 T3 DK2281631 T3 DK 2281631T3 DK 09167507 T DK09167507 T DK 09167507T DK 2281631 T3 DK2281631 T3 DK 2281631T3
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preparation module
preparation
sample
module
fluid
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DK09167507.4T
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Danish (da)
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Reza Nikbakht
Peter Warthoe
Jens Mikkelsen
Iben Schildt Sørensen
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Atonomics As
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    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01LCHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
    • B01L3/00Containers or dishes for laboratory use, e.g. laboratory glassware; Droppers
    • B01L3/56Labware specially adapted for transferring fluids
    • B01L3/563Joints or fittings ; Separable fluid transfer means to transfer fluids between at least two containers, e.g. connectors
    • B01L3/5635Joints or fittings ; Separable fluid transfer means to transfer fluids between at least two containers, e.g. connectors connecting two containers face to face, e.g. comprising a filter
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01LCHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
    • B01L3/00Containers or dishes for laboratory use, e.g. laboratory glassware; Droppers
    • B01L3/50Containers for the purpose of retaining a material to be analysed, e.g. test tubes
    • B01L3/502Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures
    • B01L3/5027Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures by integrated microfluidic structures, i.e. dimensions of channels and chambers are such that surface tension forces are important, e.g. lab-on-a-chip
    • B01L3/502715Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures by integrated microfluidic structures, i.e. dimensions of channels and chambers are such that surface tension forces are important, e.g. lab-on-a-chip characterised by interfacing components, e.g. fluidic, electrical, optical or mechanical interfaces
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01LCHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
    • B01L2200/00Solutions for specific problems relating to chemical or physical laboratory apparatus
    • B01L2200/02Adapting objects or devices to another
    • B01L2200/025Align devices or objects to ensure defined positions relative to each other
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01LCHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
    • B01L2200/00Solutions for specific problems relating to chemical or physical laboratory apparatus
    • B01L2200/02Adapting objects or devices to another
    • B01L2200/028Modular arrangements
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01LCHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
    • B01L2200/00Solutions for specific problems relating to chemical or physical laboratory apparatus
    • B01L2200/06Fluid handling related problems
    • B01L2200/0689Sealing
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01LCHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
    • B01L2200/00Solutions for specific problems relating to chemical or physical laboratory apparatus
    • B01L2200/16Reagents, handling or storing thereof
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01LCHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
    • B01L2300/00Additional constructional details
    • B01L2300/02Identification, exchange or storage of information
    • B01L2300/021Identification, e.g. bar codes
    • B01L2300/022Transponder chips
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01LCHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
    • B01L2300/00Additional constructional details
    • B01L2300/04Closures and closing means
    • B01L2300/041Connecting closures to device or container
    • B01L2300/043Hinged closures
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01LCHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
    • B01L2300/00Additional constructional details
    • B01L2300/06Auxiliary integrated devices, integrated components
    • B01L2300/0681Filter
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01LCHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
    • B01L2300/00Additional constructional details
    • B01L2300/08Geometry, shape and general structure
    • B01L2300/0861Configuration of multiple channels and/or chambers in a single devices
    • B01L2300/0867Multiple inlets and one sample wells, e.g. mixing, dilution
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01LCHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
    • B01L2300/00Additional constructional details
    • B01L2300/08Geometry, shape and general structure
    • B01L2300/0861Configuration of multiple channels and/or chambers in a single devices
    • B01L2300/0874Three dimensional network
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01LCHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
    • B01L2400/00Moving or stopping fluids
    • B01L2400/04Moving fluids with specific forces or mechanical means
    • B01L2400/0403Moving fluids with specific forces or mechanical means specific forces
    • B01L2400/0406Moving fluids with specific forces or mechanical means specific forces capillary forces
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01LCHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
    • B01L2400/00Moving or stopping fluids
    • B01L2400/04Moving fluids with specific forces or mechanical means
    • B01L2400/0475Moving fluids with specific forces or mechanical means specific mechanical means and fluid pressure
    • B01L2400/0481Moving fluids with specific forces or mechanical means specific mechanical means and fluid pressure squeezing of channels or chambers
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01LCHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
    • B01L2400/00Moving or stopping fluids
    • B01L2400/04Moving fluids with specific forces or mechanical means
    • B01L2400/0475Moving fluids with specific forces or mechanical means specific mechanical means and fluid pressure
    • B01L2400/0487Moving fluids with specific forces or mechanical means specific mechanical means and fluid pressure fluid pressure, pneumatics
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01LCHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
    • B01L2400/00Moving or stopping fluids
    • B01L2400/06Valves, specific forms thereof
    • B01L2400/0688Valves, specific forms thereof surface tension valves, capillary stop, capillary break
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01LCHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
    • B01L3/00Containers or dishes for laboratory use, e.g. laboratory glassware; Droppers
    • B01L3/50Containers for the purpose of retaining a material to be analysed, e.g. test tubes
    • B01L3/502Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures
    • B01L3/5027Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures by integrated microfluidic structures, i.e. dimensions of channels and chambers are such that surface tension forces are important, e.g. lab-on-a-chip
    • B01L3/502707Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures by integrated microfluidic structures, i.e. dimensions of channels and chambers are such that surface tension forces are important, e.g. lab-on-a-chip characterised by the manufacture of the container or its components

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  • Chemical & Material Sciences (AREA)
  • Health & Medical Sciences (AREA)
  • Clinical Laboratory Science (AREA)
  • Chemical Kinetics & Catalysis (AREA)
  • Dispersion Chemistry (AREA)
  • Analytical Chemistry (AREA)
  • General Health & Medical Sciences (AREA)
  • Hematology (AREA)
  • Automatic Analysis And Handling Materials Therefor (AREA)
  • Sampling And Sample Adjustment (AREA)

Description

DESCRIPTION
Technical Field [0001] The present invention relates to a modular microfluidic sample preparation system where the system comprises: • a first preparation module arranged in a first plane, o the first preparation module comprising a first surface and an opposing second surface and being delimited by first lateral faces, o the first preparation module further comprising an outlet arranged at the second surface of the first preparation module and an inlet, the inlet and the outlet being connected via a first microfluidic channel system, and • a second preparation module arranged in a second plane substantially parallel to the first plane, o the second preparation module comprising a first surface and an opposing second surface and being delimited by second lateral faces, o the second preparation module further comprising an intake arranged at the first surface of the second preparation module, wherein the intake comprises a blood separation filter, the intake being connected to a second microfluidic channel system.
[0002] Furthermore, the present invention relates to a method of mixing a sample fluid and an additive in a first preparation module and delivering said mixed sample fluid and additive to a second preparation module using a modular microfluidic sample preparation system.
Background Art [0003] Microfluidic systems are used in a number of laboratory automation applications, such as the preparation of fluid samples for further analysis. Such a microfluidic sample preparation system may be formed as a cartridge for insertion into a cooperating slot of an apparatus for performing the actual measurement and analysis of the sample prepared by the microfluidic system.
[0004] Furthermore, sample preparation of complex fluids, such as the preparation of blood samples for a specific measurement/analysis, often requires numerous steps. Some of these sample preparation steps may be of a general nature, and are usually performed in substantially the same manner for different types of measurements/analysis, whereas other sample preparation steps are specific to the specific measurement/analysis to be performed.
[0005] EP0470438 A1 and US5053197 A both relate to a modular microfluidic sample preparation system for separating and analyzing blood, comprising a first preparation module and a second preparation module. According to these disclosures the outlet of the first preparation module is positioned directly at the intake of the second preparation module.
[0006] W02007/004103 also relates to a modular microfluidic sample preparation system for separating and analyzing blood, comprising a first preparation module and a second preparation module.
The modular microfluidic sample preparation system disclosed does not contain a blood filter.
[0007] The numerous processing steps give rise to a complex microfluidic system that requires a large footprint for its implementation on a microfluidic chip. Such a complex microfluidic system is difficult to manufacture, and may lead to substantial problems in production, with low production yields as a consequence. Therefore, the manufacturing of such systems sets high standards for the capabilities of the manufacturing facilities.
[0008] In addition to that, different parts of the systems may require different capabilities of the manufacturing system, for example if active fluids need to be filled into reservoirs of a system, these typically need to be handled differently compared to less fragile parts of the system, e.g. common plastic parts. During the manufacturing of the parts for a microfluidic sample preparation system, the most demanding part sets the general standard of the parameters for all the parts of the system. Such parameters could e.g. be the level of cleanness in the production, sensitivity to heat, sensitivity to pressure or similar parameters. However, manufacturing the system by a standard, which is in fact too high for most of the parts, is expensive. Furthermore, the different parts of the system may require different storing facilities, e.g. if the system contains fluids that need storage in a controlled environment, e.g. with respect to moisture or temperature. Storing both sensitive parts and non-sensitive parts in a controlled environment takes up space in storage facilities and is inefficient as storing in a controlled environment is far more expensive than storing in a standard environment.
[0009] It is an object of the invention to provide a new and improved modular microfluidic sample preparation system which, at least partially, overcomes the disadvantages of the systems mentioned above.
Disclosure of the invention [0010] This aspect is obtained by a modular microfluidic sample preparation system of the above mentioned type, wherein the first preparation module is connected to the second preparation module so that the second surface of the first preparation module is facing towards the first surface of the second preparation module and so that the outlet of the first preparation module faces the intake of the second preparation module and so that the outlet of the first preparation module is positioned at a distance from the intake of the second preparation module.
[0011] Preparation steps performed by the modular microfluidic sample preparation system according to the invention may comprise dosing, mixing, adding additives or reagents, incubation, filtering, temperature stabilisation, presentation of the prepared sample at a measurement port, such as in a sample chamber with an optical window, and the like.
[0012] Hereby, the first preparation module and the second preparation module can be manufactured separately and be mutually connected afterwards. The preparation modules may demand a different level of e.g. cleanness in the manufacturing facilities. By separating the cartridge into at least two preparation modules, it is possible to manufacture the preparation modules at different locations, each complying with different production standard requirements. The outlet of the first preparation module is arranged such that a fluid e.g. a blood sample that has been preconditioned in the first module, is delivered from the outlet of the first preparation module and received by the intake of the second preparation module from where it is transported into the microfluidic channel system of the second preparation module.
[0013] Furthermore, by splitting the sample preparation system into preparation modules for different steps of the preparation process, the complexity of each of the separately produceable preparation modules is reduced, thereby reducing the complexity of the process for producing the preparation modules. This simplifies the production and thereby improves the production yield for the total sample preparation system.
[0014] The modular structure of the sample preparation system also allows for combining different types of first and second preparation modules. For example, the first preparation module may be designed for performing general steps such that the output from the first preparation module is a pre-configured fluid sample that is suited for use as input for different specific sample preparation steps. The specific sample preparation steps for different types of measurements/analyses may be implemented in the second preparation module. Alternatively, first preparation modules for different types of sample pre-configurations may be provided, which are compatible with the same type of second preparation module.
[0015] In another embodiment according to the invention, the first preparation module and the second preparation module may comprise connecting means for detachably connecting the first preparation module with the second preparation module. In this way, it is possible to use each of the modules together with other modular sample preparation systems. The first and the second preparation module being detachable, renders it possible to use the preparation modules together with other sample preparation modules or sample systems.
[0016] The preparation modules may be provided with releasable connection means, e.g. forming a snap lock connection. This allows for an easy assembly/configuration of the desired sample preparation system at the end user site by choosing and connecting the required types of first and second preparation modules. The above-mentioned easy combination/configuration of different types of preparation modules is thus also available to the end user.
[0017] Furthermore, in case of the malfunction of a preparation module, it is possible to exchange a preparation module with another. The connecting means furthermore provide that the preparation modules are correctly positioned in relation to each other. Furthermore, it is possible to store the preparation modules separately and connecting them just before use. In this way, it is possible to store the preparation modules in facilities just suitable for the specific preparation modules, thereby optimizing the storing costs. For example, different preparation modules may have different shelf lives depending on the content of reagents supplied in the module. If active or otherwise time sensitive content is comprised in a module, it is advantageous that such module be kept at a stock number just sufficient to supply the demand within the durability of such content. However, if a first preparation module compared to a second preparation module can be stored for a longer period, the manufacturing costs can be lowered by producing a higher number of less sensitive modules in one batch. Thus, the assembling i.e. connecting of the sensitive and the less sensitive preparation modules just before shipping, or even at the location of the end user may have an influence on the total costs of the modular microfluidic sample preparation system.
[0018] In one embodiment according to the invention, the first lateral faces of the first preparation module may comprise connecting means (e.g. a bead or a ridge) for connecting a recessed area of the second lateral faces of the second preparation module (or vice versa). In this way a simple and reliable system of connecting the two preparation modules is provided. The manufacturing of such connecting means can be carried out during a moulding process and is thus cheap to manufacture.
[0019] In a further embodiment of the invention, the preparation modules of the system, when connected, forms a cartridge. During use, the end user is faced with just one object to handle. Although the microfluidic sample preparation system is modular, the end user is still faced with just one object to handle.
[0020] Preferably, the cartridge comprises all reagents and/or additives to be mixed with the sample during the sample preparation process, thereby ensuring that only the fluid sample to be analysed needs to be handled and presented at the input port of the cartridge. The cartridge provides everything required during the sample preparation process and a measuring port for performing measurements on the prepared sample.
[0021] Preferably, such measurements are optical measurements, and the cartridge presents the prepared sample in a sample chamber/channel that is provided with an optical access port / window. The cartridge may be inserted into a cooperating analysis apparatus activating/driving the sample preparation process, e g. by mechanical, electrical, and/or optical means, by radiation and/or temperature control. The analysing apparatus may further perform measurements on the prepared sample at the above-mentioned measurement port, such as optical or electrical measurements. By configuring the cartridge such as to integrate additive/reagent compartments, it is further achieved that any fluid handling may be confined to filling the cartridge with the sample to be analysed. Any fluid exchange between the cartridge and the analysis apparatus, or any fluid handling by the analysis apparatus may thus be avoided, thereby decreasing the complexity of the analysis apparatus, shrinking the lab-space footprint of the analysis apparatus, and reducing the need for cleaning and maintaining the analysis apparatus to a minimum.
[0022] In a further embodiment of the invention, the modular microfluidic sample preparation system may be a modular microfluidic blood sample preparation system.
[0023] In yet another embodiment according to the invention, the outlet of the first preparation module may be positioned at a distance from the intake of the second preparation module.
[0024] When connected, the first and second preparation modules are aligned such that the outlet of the first preparation module opens towards an intake opening of the second preparation module. The intake of the second preparation module comprises receiving means adapted to receive the fluid from the outlet of the first preparation module and delivery means to deliver the fluid to the microfluidic channel system of the second preparation module.
[0025] Typically, the area of the intake opening/receiving means of the intake of the second preparation (the second preparation module intake) is larger than the cross-sectional area of the outlet of the first preparation module (the first preparation module outlet). Providing a distance between the outlet and the surface of the receiving means of the second preparation module intake facilitates the lateral distribution of the fluid sample expelled from the first preparation module outlet over the reception means surface/intake opening of the second preparation module.
[0026] Fluid may be transferred from the first module to the second preparation module in the following manner; Fluid is expelled from the first preparation module outlet by a driving force, such as hydrostatic pressure applied in/to the first preparation module. The fluid expelled from the first preparation module outlet is accumulated around the outlet of the first preparation module before the fluid is getting into contact with the surface of the intake of the second preparation module. Upon contact with the surface of the second preparation module intake, the fluid may be distributed over the surface of the intake receiving means. Delivery means are provided in the intake for transferring the received fluid sample to the microfluidic channel system of the second preparation module. One advantage of the fluid transfer from the first preparation module to the second preparation module according to the present modular sample preparation system is that it does not require a sealed fluid interconnect between the microfluidic channel systems of the first and second preparation modules, or any critical pressure/fluid tight seal when attaching the first module to the second preparation module. Thereby it is achieved that the sample preparation system may easily be assembled from prefabricated first and second preparation modules at the end user site without requiring special production skills or dedicated equipment.
[0027] The receiving means of the second preparation module intake may be a sheet of woven/non-woven fibrous material adapted to at least partially absorb/imbibe/soak up the fluid sample. The sheet is arranged in the intake opening of the second preparation module and facing towards the outlet opening when the two preparation modules are connected. The sheet is dimensioned such that the fluid sample, when soaked up by the fibrous material, may reach an intake capillary connecting the receiving means to the microfluidic channel system of the second preparation module. The intake capillary may be arranged at one of the edges of the sheet of fibrous material. By capillary action, the intake capillary may retrieve the imbibed fluid sample - or in the case of a multiple component fluid at least one of the components of the multiple component fluid - and deliver it to the microfluidic channels system of the second preparation module for further processing.
[0028] The distance furthermore provides sufficient space if e g. the intake of the second preparation module comprises swelling material that expands when getting into contact with a fluid. In this way, it is possible to use different materials at the intake of the second preparation module.
[0029] In an advantageous embodiment according to the invention, the distance between the outlet of the first preparation module to the intake of the second preparation module may be 0.05 mm -1 mm or 0.1 mm - 0,9 mm or 0.15 mm - 0.8 mm. In this way, a free space is created wherein fluid from the outlet of the first preparation module may bulge out, still being in contact with the outlet, before said fluid is delivered to the intake of the second preparation module. Furthermore, sufficient space for expansion is provided. If the intake of the second preparation module is e.g. a filter having a thickness of approximately 0.32 mm which expands due to swelling upon wetting, such filter may expand approximately 0.15 mm.
[0030] In another embodiment according to the invention, the intake of the second preparation module may comprise a blood separation filter. In this way, it is achieved that the intake of the second preparation module prepares the sample, e.g. blood, for the preparation of the sample following in the second preparation module. Thus, the intake of the second preparation module functions as a first step in the preparation carried out in the second preparation module.
[0031] Blood is a complex multiple component fluid. The separation of a multiple component fluid into different components may be performed in the intake of the second preparation module by providing receiving means and/or delivery means that are configured to preferably transport one or more desired components as compared to the remaining components present in the fluid sample received from the first preparation module. In particular, the blood filter may be configured to retain white and/or red blood cells while blood plasma is selectively transferred to the microfluidic channel system of the second preparation module.
[0032] The selective transport of the blood plasma in the filter may be provided by the capillary effect of the filter, preferably imbibing blood plasma while blood cells are retained by the crosslinked fibres of the filter material. An excess amount of mixed sample fluid, i.e. a blood sample pre-configured with the additive(s) of the first preparation module is provided to the intake of the second preparation module and on the filter, thereby saturating the filter material such that blood plasma reaches the intake capillary connected to the edge of the filter.
[0033] As mentioned above, a distance may be provided between the outlet of the first preparation module and the surface of the blood filter in the intake of the second preparation module. The distance allow/s for delivering the mixed fluid sample onto the blood filter without applying substantial pressure on the filter, thereby avoiding that blood cells are pressed through the filter into the second microfluidic channel system. The filter is dimensioned such that saturation of the filter material with blood plasma may be maintained with the amount of mixed sample fluid delivered to the intake of the second preparation module. Saturation should be maintained as long as needed to retrieve the desired amount of blood plasma into the second preparation module.
[0034] The capillary drag of the intake capillary in contact with the saturated filter material drags the fluid into the microfluidic channel system of the second preparation module. A capillary stop that may be provided in the second microfluidic channel system allows for limiting/controlling the volume of sample fluid, here blood plasma, transferred from the intake into the second module.
[0035] The blood filter may form the receiving means of the intake, wherein the blood filter is a sheet of filter web with a receiving portion arranged in the intake opening such that the receiving portion under operation faces the outlet opening. Typically, a transverse dimension of the receiving portion exceeds the corresponding transverse dimension of the outlet of the first preparation module. Advantageously, the filter web is therefore arranged at a distance from the outer edge of the outlet opening so as to improve the distribution of fluid over the receiving portion. Furthermore, the sheet of filter web may shaped so as to form a delivery tab, said delivery tab extending outwardly from the receiving portion and being connected to the intake capillary so as to establish a fluid communication between the filter web and the intake capillary.
[0036] According to one embodiment, the geometry of the blood filter may have a tapering outline, the wide portion of the tapering outline providing the receiving portion and the pointed portion forming the delivery tab. In this way, it is achieved that the blood filter is directing a fluid contained in the filter in a desired direction, e.g. towards the tapering part. In another embodiment, the filter may exhibit an efficiency of 5 - 50 % or 10 - 25 % output of plasma. The filter may e.g. have a thickness of 0.2 mm to 0.5 mm. Due to capillary drag in the filter, the filter may be wetted by the dispersion of fluid.
[0037] In yet another embodiment according to the invention, the outlet of the first preparation module may have a substantially circular cross section. In this way, the sample fluid delivered from the outlet of the first preparation module is equally distributed from the outlet when delivered from the outlet to the intake of the second preparation module. Due to the surface tension of the fluid, the bulge of fluid around the outlet of the first preparation module will be equally distributed around the outlet. The diameter of the outlet may be 0.5 mm - 2 mm or 0.75 mm -1.75 mm or 1 mm - 1.5 mm.
[0038] According to another embodiment of the invention, the outlet of the first preparation module may have a substantially oval cross section. In this way, it is achieved that the sample fluid delivered from the outlet of the first preparation module is delivered to the intake of the second preparation module so as to focus the flow in a certain direction.
[0039] In an additional embodiment according to the invention, the first preparation module may comprise a passive microfluidic mixing section in fluid communication with the first microfluidic channel system. In this way, it is achieved that fluids and/or additives supplied to the first preparation module can be mixed with the fluid provided through the inlet of the first preparation module.
[0040] In one embodiment according to the invention, the first preparation module may comprise an additive reservoir in fluid communication with the mixing section. In this way, it is possible for the first preparation module to comprise an additive to be added to the sample fluid. The additive reservoir being in fluid communication with the mixing section allows for the additive to be brought into the mixing section, e.g. by letting the sample fluid flow into the additive reservoir, thereby flushing the content of the additive reservoir out, or by forcing the content of the additive reservoir into the mixing section. Once the additive is brought into contact and mixed with the sample fluid, the mixture may require incubation in order to produce an appropriately mixed sample fluid that may be delivered to the second preparation module. For example, the additive may be a reagent comprising a marker, and an appropriate binding of the marker molecules to the target molecules may require such incubation during a given incubation time. Incubation may require temperature stabilisation. Required incubation times depend on the additive in question. For example, when analysing full blood as a sample fluid, the marker additive may be FIRP requiring an incubation time in the order of a few minutes. Alternatively, the additive reservoir may comprise components suitable for providing molecular analysis of the sample by e.g. nucleic acid amplification. Such reagents may comprise e.g. nucleic acid polymerases, helicases, primers and/or probes. In one embodiment reagents suitable for analysing sample material through Polymerase Chain Reaction (PCR) are provided through the additive reservoir. In a more preferred embodiment, reagents suitable for analysing sample material through isothermal amplification are used. Such amplification techniques comprise e.g. Helicase Dependant Amplification (biohelix), Recombinase Polymerase Amplification (TwistDx), Nucleic acid sequence-based amplification (NASBA) (Merieux), Stand displacement amplification (SDA; Becton Dickinson), Transcription mediated amplification (TMA; Gen-Probe), and Loop-mediated isothermal amplification (LAMP; Eiken).
[0041] In another embodiment according to the invention, the first preparation module may comprise an inlet reservoir in fluid communication with the inlet and the first microfluidic channel system of the first preparation module. In this way, it is possible to accumulate a sample fluid in the first preparation module.
[0042] In yet another embodiment according to the invention, the first preparation module may comprise a capillary stop delimiting the inlet reservoir from the mixing section. In this way it is achieved that the inlet reservoir of the first preparation module does not deliver its contents to the following mixing section unless a driving force, such as hydrostatic pressure, is applied forcing the content past the capillary stop. Thus, it is possible for the end user to fill sample fluid into the inlet reservoir without the sample fluid flowing into the mixing section. The inlet reservoir may thus be used for filling the sample preparation system with a pre-defined dosing volume of fluid. The pre-defined dosing volume may be determined by the total volume of the inlet reservoir. The total volume of the inlet reservoir may be less than 200μΙ, alternatively less than 100μΙ, and preferably about 50μΙ.
[0043] Additionally according to the invention, the additive reservoir may comprise a plunger. In this way, it is achieved that the plunger seals the additive reservoir.
[0044] In another embodiment according to the invention, the plunger may be arranged such that the plunger can force the content of the additive reservoir into the mixing section. When forcing the plunger into the additive reservoir, the plunger will cause the content to be forced out of the additive reservoir. The plunger may cause a pressure to be built up in the additive reservoir. A wall, e g. provided by a film or a foil, of the additive reservoir may, upon the build-up of a certain pressure, e.g. provided by pressing the plunger into the additive reservoir, allow the content of the additive reservoir to be delivered to the mixing section of the first preparation module.
[0045] In yet another embodiment according to the invention, the first preparation module may comprise closing means for shutting off the inlet of the first preparation module. In this way it is achieved that the sample fluid is kept in the first reservoir of the first module until a pumping pressure is applied. Thereby, the risk of contaminating other samples or operators is minimised. Furthermore, it is achieved that it is possible to let air, pass the closed inlet, e.g. for forcing the fluid around in the first preparation module, without the risk of air escaping through the inlet. In a further embodiment, the closing means may be a hinged lid. In this way, the closing means is kept near to the place of use and the risk of mislplacing the means is minimised. In another embodiment, the closing means may be an adhering foil or film. In yet another embodiment, the closing means may comprise a projection to be inserted in the inlet, thereby providing an air tight closing.
[0046] In a particular embodiment according to the invention, the first preparation module may comprise a transparent channel (visible to the end user). In this way, it is possible for the end user to easily determine, whether fluid enters the system, i.e. enters a part of the first microfluidic channel system.
[0047] In a further embodiment the transparent channel may be the inlet reservoir of the first preparation module. In this way, it is achieved that the user easily can determine whether the sample is sufficient in order to carry out an analysis of the sample fluid.
[0048] In an embodiment according to the invention at least one of the preparation modules may comprise identification means. In this way it is possible to adjust the machine analyzing the sample to the specific test to be performed. In a further embodiment according to the invention, the identification means may be a bar code, a chip or a RFID tag. In this way, the identification can carry a larger amount of information to be set in relation to the analysis to be performed, e.g. age of the preparation modules, type of content in reservoir(s) or batch number of content in reservoir(s).
[0049] Furthermore, in an embodiment according to the invention, the first preparation module may further comprise a pumping means, thereby ensuring that the fluid situated in the inlet reservoir of the first preparation module i.e. stopped by a capillary stop can be forced pass said capillary stop into the mixing section of the first preparation module. The pumping means may e.g. be an air filled bladder, a pump or be provided by a flexible membrane or foil covering an air filled reservoir or cavity of the first preparation module.
[0050] In one embodiment of the invention a capillary stop may delimit the inlet reservoir and the pumping means, thereby ensuring that the sample fluid does not enter the pumping means.
[0051] Furthermore, the invention relates to the use of a modular microfluidic sample preparation system according to any of above-mentioned embodiments for preparation of a blood sample. The sample prepared by using the microfluidic sample preparation system may subsequently be analysed in a blood analysing apparatus. To that purpose, the modular microfluidic sample preparation system may be inserted as a cartridge into a cooperating slot of such blood analysing apparatus. The blood analysing apparatus may further interact with the modular microfluidic sample preparation system so as to activate/drive the preparation process and analyse the sample. The interaction between the sample preparation system and the analysing apparatus may be e.g. mechanically, electrically, by radiation, heat and/or optically.
[0052] Furthermore, the invention relates to the use of a modular microfluidic sample preparation system in a blood analysing apparatus. The use of such microfluidic sample preparation system in a blood analysing apparatus provides that the end user only needs to fill-in a sample and the analysing apparatus will then perform the rest in order to carry out the analysis. The volume of the fluid provided to the modular microfluidic preparation system through the inlet port may be less than 10Opl.
[0053] Furthermore, the invention relates to a blood analysing apparatus using a modular microfluidic sample preparation system.
[0054] In another embodiment of a blood analysing apparatus according to the invention, the pumping means of a first preparation module may be activated by the blood analysing apparatus. In this way the specific time for performing the analysis is controlled by the analysing machine because the sample fluid is kept in the inlet reservoir, i.e. in a controlled non-damaging environment for the sample fluid, until the pumping means is activated.
[0055] Furthermore, the invention relates to a method of mixing a sample fluid and an additive in a first preparation module and delivering said mixed sample fluid and additive to a second preparation module using a modular microfluidic sample preparation system, the method comprising the steps of: • connecting a first preparation module comprising a first microfluidic channel system to a second preparation module, • supplying a sample fluid to an inlet reservoir through an inlet of the first preparation module, • closing the inlet of the first preparation module, e.g. by a lid, • forcing the sample fluid from the inlet reservoir into a mixing section of the first preparation module by use of air pressure, • supplying an additive from an additive reservoir into the mixing section of the first preparation module, • mixing the additive and the sample fluid by altering the pressure applied from the air to the fluid in the mixing section, thereby creating a mixed sample fluid, • optionally, incubating the sample fluid mixed with the additive during an incubation time, • providing a hydrostatic pressure to the mixed sample fluid, said hydrostatic pressure provided in the first preparation module by the pumping means thereby forcing the mixed sample fluid, through the outlet of the first preparation module positioned at a distance from the intake of the second preparation module to the intake of the second preparation module, wherein the intake comprises a blood separation filter and • at least partially transferring the mixed sample fluid from the intake to the second microfluidic channel system comprised in the second preparation module by means of capillary forces. In this way, it is achieved that the control of the mixing process and the delivery from the first preparation module to the second preparation module is carried out only by means of the applied pressure from the pumping means of the first preparation module in combination with the automatic/passive intake means of the second preparation module. The build-up of the modular microfluidic sample preparation system provides that a minimum of action from external means is necessary in order to carry out the preparation. Furthermore, the module buildup is possible due to the automated functionality of the delivery from the one preparation module to the other.
[0056] According to another method of preparing a blood sample using a modular microfluidic sample preparation system for analysing in a blood analysing apparatus, the method may comprise the steps of: • providing a first preparation module and a second preparation module assembled in such way that the outlet of the first preparation module is positioned at a distance from the intake of the second preparation module, and • supplying a sample fluid to be analysed in the inlet of the first preparation module such that the sample fluid is contained in an inlet reservoir, • closing the inlet of the first preparation module by a closing means, • inserting a microfluidic sample preparation system comprising the first preparation module and the second preparation module in an analysing apparatus, • applying a pressure in the first microfluidic channel system of the first preparation module by activating a pumping means in order to force the sample fluid in the mixing section, • releasing an additive of the additive reservoir into the mixing section of the first preparation module by means of the analysing apparatus, • altering the pressure in the mixing section such that the sample fluid is mixed with the additive in order to produce a mixed sample fluid, • optionally, incubating the sample fluid mixed with the additive during an incubation time, • delivering the mixed sample fluid from the outlet of the first preparation module to the intake of the second preparation module by dragging the mixed sample fluid into the second microfluidic preparation module using a capillary effect of the channels of the second microfluidic preparation system, • performing the sample preparation specified by the second module, and • analysing the blood sample prepared by modular microfluidic sample preparation system using the blood analysing apparatus.
Brief Description of the Drawings [0057]
Fig. 1 shows an embodiment of a modular microfluidic sample preparation system according to the invention,
Fig. 2A shows an exploded view of an embodiment of a first preparation module of a modular microfluidic sample preparation system,
Fig. 2B shows an embodiment of a modular microfluidic sample preparation system according to the invention,
Fig. 3A shows a an embodiment of a the modular microfluidic sample preparation system according to the invention Fig. 3B shows a cross sectional view of the first and second preparation module when connected to each other, and Fig. 4 shows schematically a blood filter for use in the intake of one embodiment of the second preparation module.
Detailed description of the invention [0058] Fig. 1 illustrates a modular microfluidic sample preparation system 1 comprising a first preparation module 2 and a second preparation module 3. The first preparation module 2 comprises an inlet 4 (not visible) closed by a closing means 5. An inlet reservoir 6 is visible for the end user. In this embodiment, the inlet reservoir 6 is a transparent channel of the first preparation module 2 (in the following both the inlet reservoir and the channel are indicated with the number 6). First lateral faces 7 (only partly visible) are arranged to connect the first preparation module 2 to the second preparation module 3. The first lateral faces 7 are arranged so as to connect with the second lateral faces 8 of the second preparation module 3. In the shown embodiment the second lateral faces 8 of the second preparation module comprises a recessed area 9 for receiving connecting means (not visible) of the first preparation module 2. The second preparation module 3 comprises an intake 10 for receiving a fluid delivered from the first preparation module 2. The second preparation module further comprises blisters 11 for containing fluids to be used in the preparation process of the second preparation module 3. When the first preparation module 2 is assembled with and connected to the second preparation module 3, a combined assembly is formed, typically named a cartridge.
[0059] Fig. 2A illustrates an embodiment of the first preparation module 2 in an exploded view. In this embodiment, the first preparation module 2 comprises closing means 5, a first film 20, a second film 21 and a third film 22 attached to an inlet plate 23. The inlet plate having a first surface 24 and a second surface 25 (not visible). The films 20, 21, 22 provide delimiting walls to a first microfluidic channel system 26 of the first preparation module 2. The extend of the first microfluidic channel system 26 is indicated by dotted lines. For illustrative purposes, and due to the fact that the parts of the channel walls in fact are created by both the films 20, 21, 22 and the inlet plate 23, the channels are merely shown as open recesses or indents in the inlet plate 23. Using films 20, 21, 22 for providing delimiting walls to the microfluidic system, the process of manufacturing is made easier. The first preparation module 2 could e g. be produced by an injection moulding process. The first microfluidic channel system 26 comprises an inlet 4 arranged in fluid communication with the inlet reservoir 6. The through-going apertures 27 provide access to the blisters 11 of the second preparation module 3 (not shown). A capillary stop 28 provides delimitation between the inlet reservoir 6 and a mixing section 29 of the microfluidic channel system 26. A recessed area of the inlet plate 23 provides a pumping means cavity 30 for pumping means 31 (not visible). In this embodiment, the pumping means cavity 30 and the second film 21 together form a pumping means 31. In this way, the pumping means cavity 30 is an air reservoir. Pressure from the pumping means 31 is led through a pressure channel 32. When a sample fluid 33 (not shown in this figure) is lead into the inlet 4, the sample fluid 33 is stored in the inlet reservoir 6. In practice, the size for the inlet reservoir may be less than 200μΙ, alternatively less than 10ΟμΙ and preferably about 50μΙ. The sample fluid 33 is dragged by capillary forces and the inlet reservoir 6 is filled. The sample fluid 33 is stopped by a capillary stop 28 in order to be able to control when the sample fluid 33 should be forced into the mixing section 29. In this way, it is achieved that the timeline of performing the desired steps in the preparation modules is controlled by different activation means and does not necessarily take place instantly when the sample fluid is filled into the inlet. The sample fluid 33 is forced into the mixing section 29 by a pressure applied from the pumping means 31 through the pressure channel 32, passing the inlet 4 that has been closed by the closing means 5. The pumping means is e.g. activated by an analysing apparatus simply by pressing the second film 21 e.g. a flexible membrane, whereby an air pressure is generated to be led through the pressure channel 32. A second capillary stop 19 ensures that sample fluid does not enter the pressure channel 32. The pressure from the pumping means 31 then pushes the sample fluid 33 past the capillary stop 28 into the mixing section. The mixing section comprises an additive reservoir 34. The additive reservoir 34 is provided by a through hole 35 in the inlet plate 23 extending from the first surface 24 to the second surface 25, where the through hole 35 on the second surface 25 (not visible) is closed by the third film 22. A plunger 36 arranged in the through hole 35 closes the through hole on the first surface 24. In this way, a reservoir for containing an additive, e.g. a HRP tracer or similar, is created. Upon applying a force on the plunger 36, the plunger is forced towards the second surface 25 and the content of the additive reservoir 34 is forced against the third film 22 covering the through hole 35 on the second surface 25. The third film 22 is arranged such that when a certain pressure is applied to the third film 22 covering the through hole 35, the third film 22 will loosen from the second surface 25 (not visible) of the inlet plate 23, whereby the content of the additive reservoir 34 is forced into the mixing system 29. Thereby and by manipulating the pressure from the pumping means 31, the sample fluid 33 and the content of the additive reservoir 34 is pushed back and forth in the mixing section, whereby they are mixed creating a mixed sample fluid 37 (not shown). The manipulation of the pressure from the pumping means may be carried out by a blood analysing machine. When mixing is complete, the pressure from the pumping means 31 pushes the mixed sample fluid 37 towards the outlet 38 of the first preparation module 2. The final section of the microfluidic channels system 29 towards the outlet 38 is indicated by dotted lines due to the fact that the outlet 38 is situated on the second surface 25 of the first preparation module 2.
[0060] Fig. 2B illustrates the first preparation module 2 of figure 2A seen facing the second surface 25. The third film 22 is partly covering the second surface 25. The position of the inlet 4 is indicated by a dotted circle. Likewise, the position of the additive reservoir 34 is indicated by a dotted circle. The sample fluid 33 (not shown) enters the first preparation module through the inlet 4 placed on the first surface and the mixed sample fluid (not shown) leaves the first preparation module 2 through the outlet 38 placed on the second surface 25. The outlet 38, in this embodiment having a circular cross section, may have an internal diameter of approximately 1,3 mm. The first lateral faces 7 comprises connecting means 39 arranged to engage the second lateral faces 8 (not shown) of the second preparation module 3 (not shown. The first lateral faces 7 is to be understood as the faces delimiting the first surface 24 and the second surface 25 and thus defining the outer perimeter of the first preparation module 2. Furthermore, the first lateral faces 7 may comprise walls 41 projecting from the second surface 25. The projecting walls 41 serve to position the first preparation module 2 correctly in relation to the second preparation module 3.
[0061] Fig. 3A primarily illustrates according to which cut the cross sectional view of Fig. 3B is obtained. The first preparation module 2 is connected to the second preparation module 3 (the second preparation module only indicated by a dotted line). The details of the Fig. 3A is explained in further details in Fig. 2A.
[0062] Fig. 3B illustrates the delivery of a mixed sample fluid 37 i.e. blood being delivered from the outlet 38 to the intake 10 of the second preparation module 3. In this embodiment, the intake 10 comprises a blood filter 40. The blood filter 40 may have a thickness of approximately 0.32 mm. The pressure from the pumping means 31 at the pumping cavity 30 and thus the mixed sample fluid 37 is delivered to the intake 10 as a hydrostatic pressure. By a combination of the hydrostatic pressure applied on the mixed sample fluid 37 and a capillary effect of the intake 10, i.e. the blood filter 40, the mixed sample fluid 37 is dragged towards the second microfluidic channel system 50 of the second preparation module 3. During the process of dragging the mixed sample fluid 37 from the outlet 38 to the second microfluidic channels system 50, the red and white blood cells are filtered from the blood plasma and only blood plasma is delivered to the second microfluidic channels system 50 of the second preparation module 3. A backing material 51 ensures that the surface to which the filter is fastened to the second preparation module 3 exhibits known conditions. Due to the distance d between the outlet 38 and the blood filter 40, the microfluidic channel system 26 of the first preparation module 2 and the microfluidic channel system 50 of the second preparation module 3 are not in direct fluid communication. The mixed sample fluid 37 is placed on top of the blood filter 40. The mixed sample fluid 37 infuses the blood filter 40. When the blood filter 40 is filled with the mixed sample fluid 37, the filtered fluid is forced into contact with the second microfluidic channel system 50 by the capillary drag of the blood filter. When the filtered blood, i.e. blood plasma, is brought in contact with the second microfluidic channel system 50, capillary forces drag the blood plasma into the second microfluidic channel system 50. Due to the controlling of the hydrostatic pressure on the mixed sample fluid 37, i.e. providing a constant supply of mixed sample fluid 37 to the blood filter 40 and the characteristics of the blood filter 40, it is possible to deliver a filtered mixed sample fluid 37 from the outlet 38 of the first microfluidic channel system 26 as a filtered mixed sample fluid to the second microfluidic channel system 50, without the channels of the two systems 26, 50 being in direct fluid communication. The distance d between the outlet 38 and the blood filter 40 provides that the mixed sample fluid 37 is delivered on top of the blood filter 40 as opposed to being forced into the blood filter 40. A blood filter 40 having a thickness of e.g. 0.32 mm may increase approximately 0.15 mm in height when a fluid is infused. The delivery from the first microfluidic system 26 to the intake 10 creates of a fluid column consisting of the mixed sample fluid 37 which keeps supplying the blood filter 40 with fluid. When the supply of mixed sample fluid 37 is continued at such rate that the fluid column does not break apart, the capillary drag of the microfluidic channel system 50 and the capillary properties of the blood filter 40 will continue to supply filtered fluid to the second microfluidic channel system 50. The blood filter 40 is adapted such that approximately 4pl of blood plasma is delivered to the second microfluidic channel system 50 before the filtering effect of the blood filter is decreased, i.e. that e.g. undesired red blood cells will start to be dragged into the second microfluidic channel system 50. A quantity of 4 pi is sufficient to carry out the sample preparation specified in the second preparation module 3. When stopping the hydrostatic pressure applied from the first preparation module 2 the supply of filtered mixed sample fluid to the second microfluidic channel system 50 will stop. The blood filter may have an efficiency of 15 - 20 %.
[0063] Fig. 4 shows schematically the outline shape of a blood filter 40 for use as the receiving means of the intake of one embodiment of the second preparation module. The blood filter 40 has a tapered outline with a receiving portion 42 in the wide end and a delivery tab 43 extending outwardly from the receiving portion 42 to the narrow end of the tapered outline. When installed in the intake 10 of the second module 3, the receiving portion 42 of the blood filter 40 is arranged in the intake opening, and the delivery tab 43, is connected to the intake capillary connecting the blood filter 40 to the second microfluidic channel system 50.
REFERENCES CITED IN THE DESCRIPTION
This list of references cited by the applicant is for the reader's convenience only. It does not form part of the European patent document. Even though great care has been taken in compiling the references, errors or omissions cannot be excluded and the EPO disclaims all liability in this regard.
Patent documents cited in the description • EP0470436A1 [0005] . US5053187Ar0005l • W02007004103A ΡΟΟΟβί

Claims (12)

1. Modulært mikrofluidprøvepræpareringssystem (1), hvor systemet omfatter: - et første præpareringsmodul (2), som er anbragt i et første plan, - idet det første præpareringsmodul (2) omfatter en første overflade (24) og en modsat anden overflade (25) og er afgrænset af første laterale flader (7), - idet det første præpareringsmodul (2) yderligere omfatter en udgang (38), som er anbragt ved den anden overflade (25) af det første præpareringsmodul (2), og en indgang (4), hvor indgangen (4) og udgangen (38) er forbundet via et første mikrofluidkanalsystem (26), - et andet præpareringsmodul (3), som er anbragt i et andet plan, der i det væsentlige er parallelt med det første plan, - idet det andet præpareringsmodul (3) omfatter en første overflade og en modsat anden overflade og er afgrænset af anden laterale flader (8), - idet det andet præpareringsmodul (3) yderligere omfatter et indtag (10), som er anbragt ved den første overflade af det andet præpareringsmodul (3), hvor indtaget (10) omfatter et blodsepareringsfilter (40), idet indtaget (10) er forbundet med et andet mikrofluidkanalsystem (50), og hvor - det første præpareringsmodul (2) er forbundet med det andet præpareringsmodul (3), således at den anden overflade (25) af det første præpareringsmodul (2) vender imod den første overflade af det andet præpareringsmodul (3), og således at udgangen (38) i det første præpareringsmodul (2) vender imod indtaget (10) i det andet præpareringsmodul (2), og således at udgangen (38) i det første præpareringsmodul (2) er anbragt med en afstand (d) fra indtaget (10) i det andet præpareringsmodul (3).A modular microfluidic sample preparation system (1), the system comprising: - a first preparation module (2) disposed in a first plane, - the first preparation module (2) comprising a first surface (24) and an opposite second surface (25). ) and is delimited by first lateral surfaces (7), - the first preparation module (2) further comprises an outlet (38) arranged at the second surface (25) of the first preparation module (2), and an input ( 4), wherein the inlet (4) and the outlet (38) are connected via a first microfluidic channel system (26), - a second preparation module (3), which is arranged in a second plane, which is substantially parallel to the first plane, - the second preparation module (3) comprises a first surface and an opposite second surface and is delimited by second lateral surfaces (8), - the second preparation module (3) further comprises an inlet (10) arranged at the first surface of the second preparation module (3), where the intake (10) o comprising a blood separation filter (40), the inlet (10) being connected to a second microfluidic channel system (50), and wherein - the first preparation module (2) is connected to the second preparation module (3), so that the second surface (25) of the first preparation module (2) faces the first surface of the second preparation module (3), and so that the outlet (38) of the first preparation module (2) faces the inlet (10) of the second preparation module (2), and so that the outlet (38) of the first preparation module (2) is arranged at a distance (d) from the inlet (10) of the second preparation module (3). 2. Modulært mikrofluidprøvepræpareringssystem (1) ifølge krav 1, hvor det første præpareringsmodul (2) og det andet præpareringsmodul (3) omfatter forbindelsesmidler (9, 39) til udløseligt at forbinde det første præpareringsmodul (2) med det andet præpareringsmodul (3).A modular microfluidic sample preparation system (1) according to claim 1, wherein the first preparation module (2) and the second preparation module (3) comprise connecting means (9, 39) for releasably connecting the first preparation module (2) to the second preparation module (3). 3. Modulært mikrofluidprøvepræpareringssystem (1) ifølge krav 1 eller 2, hvor afstanden (d) mellem udgangen (38) i det første præpareringsmodul (2) og indtaget (10) i det andet præpareringsmodul (3) er 0,05-1 mm eller 0,1-0,9 mm eller 0,15-0,8 mm.A modular microfluidic sample preparation system (1) according to claim 1 or 2, wherein the distance (d) between the outlet (38) of the first preparation module (2) and the inlet (10) of the second preparation module (3) is 0.05-1 mm or 0.1-0.9 mm or 0.15-0.8 mm. 4. Modulært mikrofluidprøvepræpareringssystem (1) ifølge et hvilket som helst af de foregående krav, hvor det første præpareringsmodul (2) omfatter et mikrofluidblandingsafsnit (29), der er i fluidforbindelse med det første mi krofluid kanalsystem (26).A modular microfluidic sample preparation system (1) according to any one of the preceding claims, wherein the first preparation module (2) comprises a microfluidic mixing section (29) in fluid communication with the first microfluidic channel system (26). 5. Modulært mikrofluidprøvepræpareringssystem (1) ifølge krav 4, hvor det første præpareringsmodul (2) omfatter et tilsætningsstofreservoir (34), der er i fluidforbindelse med blandingsafsnittet (29).A modular microfluidic sample preparation system (1) according to claim 4, wherein the first preparation module (2) comprises an additive reservoir (34) in fluid communication with the mixing section (29). 6. Modulært mikrofluidprøvepræpareringssystem (1) ifølge et hvilket som helst af de foregående krav, hvor det første præpareringsmodul (2) omfatter et indgangsreservoir (6), der er i fluidforbindelse med indgangen (4) og det første mi krofluid kanalsystem (26) i det første præpareringsmodul (2).A modular microfluidic sample preparation system (1) according to any one of the preceding claims, wherein the first preparation module (2) comprises an inlet reservoir (6) in fluid communication with the inlet (4) and the first microfluidic channel system (26) in the first preparation module (2). 7. Modulært mikrofluidprøvepræpareringssystem (1) ifølge et hvilket som helst af de foregående krav, hvor det første præpareringsmodul (2) omfatter en transparent kanal (6) (synlig for slutbrugeren).A modular microfluidic sample preparation system (1) according to any one of the preceding claims, wherein the first preparation module (2) comprises a transparent channel (6) (visible to the end user). 8. Modulært mikrofluidprøvepræpareringssystem (1) ifølge et hvilket som helst af de foregående krav, hvor det første præpareringsmodul (2) endvidere omfatter et pumpemiddel (31).A modular microfluidic sample preparation system (1) according to any one of the preceding claims, wherein the first preparation module (2) further comprises a pump means (31). 9. Anvendelse af et modulært mikrofluidprøvepræpareringssystem (1) ifølge et hvilket som helst af kravene 1-8 til præparering af en blodprøve.Use of a modular microfluidic sample preparation system (1) according to any one of claims 1-8 for preparing a blood sample. 10. Blodanalyseapparat, hvor der anvendes et modulært mikrofluid-prøvepræpareringssystem (1) ifølge et hvilket som helst af kravene 1-8.A blood analysis apparatus using a modular microfluidic sample preparation system (1) according to any one of claims 1-8. 11. Blodanalyseapparat ifølge krav 10, der omfatter et modulært mikrofluidprøvepræpareringssystem (1) ifølge krav 8, hvor pumpemidlet (31) i det første præpareringsmodul (2) aktiveres af blodanalyseapparatet.A blood analysis apparatus according to claim 10, comprising a modular microfluidic sample preparation system (1) according to claim 8, wherein the pump means (31) in the first preparation module (2) is activated by the blood analysis apparatus. 12. Fremgangsmåde til blanding et prøvefluid (33) og et tilsætningsstof i et første præpareringsmodul (2) og afgivelse af det blandede prøvefluid (37) til et andet præpareringsmodul (3) under anvendelse af et modulært mikrofluidprøvepræpareringssystem (1), hvilken fremgangsmåde omfatter følgende trin: - forbindelse af et første præpareringsmodul (2), der omfatter et første mikrofluidkanalsystem (26), med et andet præpareringsmodul (3), idet det andet præpareringsmodul (3) omfatter et andet mikrofluidkanalsystem (50), - tilførsel af et prøvefluid (33) til et indgangsreservoir (6) gennem en indgang (4) i det første præpareringsmodul (2), - lukning af indgangen (4) i det første præpareringsmodul (2) ved hjælp af lukkemidler (5), - fremdrivning af prøvefluidet (33) fra indgangsreservoiret ind i et blandingsafsnit (26) i det første præpareringsmodul (2) ved hjælp af lufttryk, - tilførsel af et tilsætningsstof fra et tilsætningsstofreservoir (34) til blandingsafsnittet (26) i det første præpareringsmodul (2), - blanding af tilsætningsstoffet og prøvefluidet (33) ved ændring af det tryk, som luften påfører fluidet i blandingsafsnittet (26), hvorved der dannes et blandet prøvefluid (37), - tilvejebringelse af et hydrostatisk tryk på det blandede prøvefluid (37), idet det hydrostatiske tryk, der tilvejebringes i det første præpareringsmodul (2) ved hjælp af pumpemidlerne (31), dermed fremdriver det blandede prøvefluid (37) gennem udgangen (38) i det første præpareringsmodul (2), som er anbragt med en afstand (d) fra indtaget (10) i det andet præpareringsmodul (3), til indtaget (10) i det andet præpareringsmodul (3), hvor indtaget (10) omfatter et blodsepareringsfilter (40), og - mindst delvis overførsel af det blandede prøvefluid (37) fra indtaget til det andet mikrofluidkanalsystem (50), som er omfattet i det andet præpareringsmodul (3), ved hjælp af kapillærkræfter.A method of mixing a sample fluid (33) and an additive in a first preparation module (2) and delivering the mixed sample fluid (37) to a second preparation module (3) using a modular microfluidic sample preparation system (1), the method comprising the following: step: - connecting a first preparation module (2) comprising a first microfluidic channel system (26) to a second preparation module (3), the second preparation module (3) comprising a second microfluidic channel system (50), - supplying a sample fluid ( 33) to an inlet reservoir (6) through an inlet (4) in the first preparation module (2), - closing the inlet (4) in the first preparation module (2) by means of closing means (5), - propelling the sample fluid (33 ) from the inlet reservoir into a mixing section (26) in the first preparation module (2) by means of air pressure, - supply of an additive from an additive reservoir (34) to the mixing section (26) in the first prep mixing module (2), - mixing the additive and the test fluid (33) by changing the pressure which the air applies to the fluid in the mixing section (26), thereby forming a mixed test fluid (37), - providing a hydrostatic pressure on the mixed test fluid (37), the hydrostatic pressure provided in the first preparation module (2) by means of the pump means (31) thereby driving the mixed sample fluid (37) through the outlet (38) of the first preparation module (2) arranged at a distance (d) from the inlet (10) of the second preparation module (3) to the inlet (10) of the second preparation module (3), the inlet (10) comprising a blood separation filter (40), and - at least partial transfer of the mixed sample fluid (37) from the inlet to the second microfluidic channel system (50) included in the second preparation module (3) by capillary forces.
DK09167507.4T 2009-08-07 2009-08-07 Modular microfluidic sample preparation system and method of mixing and delivering a sample fluid. DK2281631T3 (en)

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