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    • 专利摘要:
    A device (410) for carrying out heterogeneous immunoassays with the aid of magnetic particles (411) in cuvettes (201) arranged in a row, each cuvette (201) having a filling opening (207) and at least one lateral measurement window (202) which is transparent to the measuring radiation, has the following components: at least one stationary cuvette array (200) in which the cuvettes (201) are arranged to hold liquid media, at least one that can be moved along the cuvette array (200) and in the direction of the filling opening (207) of a selected cuvette (201 ) lowerable holding arm (420) with at least one suction needle (423) which can be lowered towards the bottom (204) of the cuvette (201), and with at least one dispenser (424a to 424d) which can be positioned above or in the respective filling opening (207) the liquid media into the cuvette (201), at least one dispenser (424a, 424b) for delivering a washing solution for the magnetic particles (411) is formed, at least one magnet arrangement (430), which can be moved along the cuvette array (200) and acts on the content of the selected cuvette (201), for separating the magnetic particles (411) on an inner surface of the cuvette (201), and at least one along of the cuvette array (200), which can be moved and aligned with the measurement window (202) of the selected cuvette (201), optical detection device (435) for recording a measurement signal proportional to an analyte concentration in the selected cuvette (201).
    公开号:AT521352A4
    申请号:T50603/2018
    申请日:2018-07-13
    公开日:2020-01-15
    发明作者:Sprengers Wolfgang;Bartel Arnold;Marik Reinhard
    申请人:Meon Medical Solutions Gmbh & Co Kg;
    IPC主号:
    专利说明:

    A device (410) for carrying out heterogeneous immunoassays with the aid of magnetic particles (411) in rows (201) of cells, each cell (201) having a filling opening (207) and at least one side measurement window (202) which is transparent to the measurement radiation, has the following components:
    at least one stationary cuvette array (200) in which the cuvettes (201) are arranged to hold liquid media, at least one holding arm (420) that can be moved along the cuvette array (200) and lowered in the direction of the filling opening (207) of a selected cuvette (201) ) with at least one suction needle (423) that can be lowered towards the bottom (204) of the cuvette (201), and with at least one dispenser (424a to 424d) that can be positioned above or in the respective filling opening (207) for dispensing the liquid media into the Cuvette (201), at least one dispenser (424a, 424b) being designed to deliver a washing solution for the magnetic particles (411), at least one magnet arrangement which can be moved along the cuvette array (200) and acts on the contents of the selected cuvette (201) (430) for separating the magnetic particles (411) on an inner surface of the cuvette (201), as well as at least one that can be moved along the cuvette array (200) and on d The measuring window (202) of the selected cuvette (201) can be aligned with an optical detection device (435) for receiving a measurement signal proportional to an analyte concentration in the selected cuvette (201).
    Fig. 2/37
    22265AT
    The invention relates to a method and a device for carrying out heterogeneous immunoassays with the aid of magnetic particles in rows of cuvettes of an analyzer, each cuvette having a filling opening and at least one lateral measurement window that is transparent to the measuring radiation.
    Heterogeneous immunoassays are routinely used, for example in clinical diagnostics, analytics and microbiology, where there is a need to determine various properties and ingredients of liquid samples quickly, precisely and reproducibly, especially using optical methods.
    Different measuring principles are used in the known devices for performing heterogeneous immunoassays. On the one hand, devices with a stationary detection unit, for example a stationary photomultiplier, and a conveyor device for moving cuvettes for receiving the reaction mixtures to be measured from samples and reagents, such as a conveyor belt or a carousel, are used. The cuvettes are successively guided past the detection unit and measured. As a result, the conveyor must stop each time a new sample or reagent is placed in a cuvette or the cuvette is to be replaced or washed and made available for a new test. With the conceptually rigid cycle times, there is a significant loss in efficiency.
    For a better understanding of the invention, some essential technical terms used in the present application are defined in more detail:
    Analyte / antigen: An analyte - in the case of immunoassays also called an antigen - is an ingredient that can be determined qualitatively and / or quantitatively in a sample. In immunoassays, the analyte is in a liquid phase, usually dissolved in a buffer, in diluted body fluids or other sample fluids. In addition, the analyte can also be a particulate structure, which is present in a suspension and can be detected by immunoassays, with antigenic surface features, such as bacteria, viruses, cells or material particles.
    / 37
    Luminescence / chemiluminescence: With luminescence (e.g. fluorescence,
    Phosphorescence, chemiluminescence), the light emitted by molecules is measured. In the case of chemiluminescence, the light emission is due to a chemical reaction. Luminometric methods are very sensitive and therefore well suited for the detection of markers in immunoassays.
    Immunoassay: A series of methods in bioanalytics are collectively referred to as immunoassay, the common basic principle of which is the detection and detection of an analyte (antigen) in a liquid phase by binding an antigen to an antibody. Immunoassays are used, for example, in laboratory medicine for the determination of a large number of analytes in various body fluids such as blood, serum, urine or cerebrospinal fluid. They are used for the prediction, diagnosis and monitoring of diseases, as well as the detection of toxins or the monitoring of drugs in the body.
    Competitive immunoassay: A competitive immunoassay is used to determine an antigen if either only a single specific antibody is available for it or if the antigen does not have sufficient binding sites for the unhindered binding of two antibodies. For example, an antibody (capture antibody) is used as the recognition component and a labeled antigen is used as the competitive component.
    Sandwich assay: To detect an antigen using a non-competitive assay, also known as a sandwich assay, two different antibodies are required that recognize the antigen and do not interfere with each other in their binding to the antigen. An advantage when comparing with the competitive immunoassay is the higher sensitivity in most applications.
    heterogeneous immunoassay: In a heterogeneous immunoassay of the present invention, in contrast to the homogeneous immunoassay, the liquid phase changes during the process. When using magnetic particles with capture antibodies bound for selective binding of the antigen, this can e.g. can be achieved in that the particles are deposited on the vessel wall by a magnetic field, the first liquid is replaced by a second liquid, and the particles are resuspended in the second liquid / 37. After the removal of the first liquid, any washing steps with the second liquid or a special washing liquid can be carried out on the particles. The washing steps enable the removal of substances which are nonspecifically bound to the particles and of interfering substances present in the first liquid, the removal of interfering substances making the assay much more sensitive and low detection limits and concentration ranges for the antigen to be determined being achieved.
    Magnetic particles (magnetic beads): These are typically small magnetic particles, suspended in an aqueous buffer solution, that are coated with the capture antibody for immunochemical tests.
    Capture Antibody: These are antibodies that bind to at least one epitope of the analyte and are bound to the solid phase - in the case of the present invention - to the surface of solid magnetic particles.
    Tracer antibody (labeled antibody, conjugate): This is a second antibody to which a marker molecule (label) is chemically bound and in the assay selectively binds interactions to analyte molecules by means of antigen-antibodies, or with it to binding sites on an antigen competes (competitive assay). The marker molecule can be a dye that emits light by adding one or more chemical substances (chemiluminescence). Furthermore, the dye can also be stimulated to emit by applying a voltage (electroluminescence) or by irradiating light (e.g. fluorescence). The marker molecule can also catalyze a detection reaction whose reaction products are detectable, such as in the case of an enzymatic reaction (enzymatic immunoassay).
    Bound / free washing, or (B / F) washing: A process step of a heterogeneous immunoassay in which the unbound residue of the labeled tracer antibodies (labeled antibody) added in excess is removed from the surface of the magnetic particles by washing ,
    Pipettor: a device suitable for liquid transfer between a first and second vessel for aspiration and subsequent ejection of a liquid to be transferred to / 37, which can approach different areas of the sample and reagent storage as well as the cuvettes.
    Dispenser (or injector): A dispenser is used to dispense defined amounts of liquid from a storage vessel via a supply line that ends in a nozzle, dispensing opening or dispenser needle, into a vessel, for example into a cuvette.
    State of the art:
    A measuring arrangement is known from US Pat. No. 6,333,008 B1, which is used for carrying out luminometric series analyzes on liquid samples, in which target substances to be detected and labeling substances that can be connected to them in an immunochemical detection reaction and magnetizable carrier particles are contained. As shown in Fig. 1a of the present application, the liquid samples 89 are transported in the wells of a multiple cuvette 90 along a conveying path (see arrow 91) to an optical measuring station 92, permanent magnets and separating stations designed as rotatable double magnets 93 being used for the separation during the transport excess marking substance are determined, act on the multiple cuvette 90. A (B / F) washing step takes place in the individual separation stations with the aid of an injector 94 and a suction needle 95. The luminescence radiation is detected in the measuring station 92 by a photodetector 88. A disadvantage of the known measuring arrangement is the necessity to have to transport the liquid samples to different machine components which are distributed in a fixed manner along a process path during the analysis process. Furthermore, certain components, such as permanent magnets designed as rotatable double magnets 93 and separating stations with injectors 94 and suction needles 95, have to be designed multiple times.
    Devices of this type are distinguished by the fact that all processes are predetermined by rigid clock cycles of the cuvette conveying mechanism and have to run in predetermined time windows. Actions such as dispensing, mixing, separating and measuring can only take place if the respective cuvettes are at the positions of the respective device components.
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    A sample can only be dispensed into an empty cuvette (not at any time, but only) if the empty cuvette passes the position of the sample pipettor and the cuvette transport mechanism stops at this position. A reagent or washing liquid can only be dispensed into a cuvette containing the sample if the cuvette in question passes the position of the reagent dispenser and the cuvette delivery mechanism stops at this position. The same applies analogously to the stirring of reaction mixtures from the sample and the reagents in the cuvettes with mechanical stirring and to the optical measurement at the position of the optical measuring device.
    For example, a specific cuvette cannot be measured optically at any time or repeatedly in small time intervals, since it is necessary to wait until the cuvette in question is at the position of the optical measuring unit.
    When measurements have been completed, a cuvette cannot disadvantageously be washed or changed immediately, and a new test can be started. A cuvette can only be washed or exchanged and thus made available for a new test if the cuvette in question is in the position of the cuvette washing station or the cuvette changer and at a fixed point in time or period from the start of the test accordingly the conceptually rigid cycle times, at which position a wash stop or a cuvette change is or is planned. As a result, all cuvettes are blocked for the same length, regardless of whether the measurement duration of the respective tests is short or long.
    In devices for carrying out heterogeneous immunoassays, individual process steps of an assay in a single cuvette are, for example, separation of the magnetic beads (> 1 min), B / F washing (a few seconds) or antigen / antibody reactions or incubation (approx. 10 -20 min) is particularly time-intensive, while, for example, a luminescence measurement at the respective machine station runs comparatively quickly (a few seconds). If a process step of an assay to be carried out in a cuvette is repeated, the responsible machine component must be present several times / 37 along the process path in order not to have to wait for a full movement cycle of the conveyor mechanism.
    Conventional devices with cuvettes moving stationary along a cyclical movement path from station to station cannot easily afford flexible timing of process steps for parallelizing analyzes in different cuvettes, since the cuvettes can only move together on a cyclic conveyor mechanism and the processing of process steps therefore rigid clock cycles follows.
    The fixed distribution of machine components on a process path for conveyor belts or carousels with moving samples, reagents and cuvettes results in relatively long throughput times for the individual tests and limits the number of tests that can be carried out per hour on a device with a certain number of cuvettes can.
    A device for carrying out heterogeneous immunoassays is known from US Pat. No. 7,718,072 B2. As shown in Fig. 1b of the present application, the cuvettes 96, which hold the sample, the necessary reagents and magnetic particles, are passed in a process path by means of a conveyor belt through a series of thermostattable structures, each structure having a side opening 97a for access of a photomultiplier, has an opposite exemption 97b for a separation magnet 98 which can be brought up to the cuvette and a mixer 99 which engages in the bottom region of the cuvette 96. Several such thermostattable structures for mixing, magnetic separation or measurement can be arranged in a stationary manner along the process path in order to allow the process steps of a heterogeneous immunoassay to be carried out in succession in one or more cuvettes 96. It is also disadvantageous here that the processes taking place on the stationary machine components are predetermined by rigid clock cycles of the cuvette conveyor mechanism and have to run in predetermined time windows.
    The object of the invention is to propose a method and a device for carrying out heterogeneous immunoassays based on the state of the art set out, with which or with which disadvantages, especially in connection with the processes - predetermined by rigid clock cycles and running in predetermined time windows - restricted / 37
    Sample throughput of known systems are avoided and propose improvements that increase the sample throughput without the individual analysis or
    To make the device significantly more expensive, the quality of the analysis should at least be maintained.
    This object is achieved according to the invention by a device for carrying out heterogeneous immunoassays, which is characterized by the following components:
    at least one stationary cuvette array, in which the cuvettes for holding liquid media (samples, reagents, suspensions, washing solutions) are arranged, at least one holding arm that can be moved along the cuvette array and lowered towards the filling opening of a selected cuvette with at least one towards the bottom of the Cuvette that can be lowered, as well as with at least one dispenser that can be positioned above or in the respective filling opening for dispensing the liquid media into the cuvette, at least one dispenser being designed for dispensing a washing solution for the magnetic particles, at least one that can be moved along the cuvette array the contents of the selected cuvette acting magnet arrangement for separating the magnetic particles on an inner surface of the cuvette, and at least one optical detection device that can be moved along the cuvette array and aligned with the measurement window of the selected cuvette for recording a measurement signal proportional to an analyte concentration in the selected cuvette.
    A method according to the invention for determining an antigen by means of a heterogeneous immunoassay is characterized in that, in a first step A, a sample for determining the antigen, a suspension of magnetic particles with a capture antibody, and / 37 if necessary a tracer antibody or a labeled antigen be pipetted into a selected cuvette of a stationary cuvette array, and that the following steps B of an immunochemical analysis, such as
    a) separating the magnetic particles,
    b) introducing and suctioning off a washing solution one or more times,
    c) dosing at least one trigger fluid, as well
    d) luminometric measurement of the sample is carried out with the aid of a measuring and manipulation module which can be moved along the cuvette array and which is stopped in order to carry out individual or all steps a) to d) in the selected cuvette.
    A particular advantage of the invention is that the measurement and manipulation module can be moved to at least one other cuvette of the cuvette array during the course of time-consuming steps in immunochemical analysis, such as incubation, etc., in the selected cuvette, in order to move in the further one Cuvette to perform individual or all steps B of an immunochemical analysis.
    In particular, the measurement and manipulation module according to the invention can move freely between the cuvettes of the stationary cuvette array in order to carry out a second process step in another cuvette during an assay process step in a first cuvette that is not to be carried out with the components of the measurement and manipulation module.
    Before or during the approach of the measuring and manipulation module to a cuvette, the needle group of the dispensers and the suction needle can be washed in a washing station arranged on the measuring and manipulation module.
    For example, in a first parallelization example, during an incubation step of an assay in a first cuvette, a magnetic / 37
    Separation and B / F washing can be carried out in a second cuvette in order to increase the utilization of the machine components and to save time in the processing of the assays.
    If there is an additional, movable magnet arrangement that can be moved along the cuvette array on its own rail independently of the other components of the measuring and manipulation module, then in a second parallelization example, magnetic pre-separation of beads from a third assay can be carried out in a third cuvette , while in a fourth assay of a fourth cuvette the process steps of luminescence triggering and luminescence measurement are carried out with the aid of components of the measurement and manipulation module.
    According to a preferred embodiment variant of the invention, the holding arm for the suction needle and the at least one dispenser has a lifting and rotating device which is arranged on a platform which can be moved along the cuvette array, a common suspension for the magnet arrangement and the detection device being arranged on the moving platform is.
    It is particularly advantageous if the holding arm arranged on the movable platform together with the dispenser platform, together with the magnet arrangement and the detection device, forms a measuring and manipulation module which can be moved along the cuvette array and which contains all robotic, fluidic and measuring technology components for the process steps of magnetic separation of the beads, the so-called B / F washing, as well as the triggering and measurement of the luminescence.
    The invention is explained in more detail below using an exemplary embodiment. Show it:
    1a and 1b two different devices for performing heterogeneous immunoassays according to the prior art,
    2 a device according to the invention for carrying out heterogeneous immunoassays in a three-dimensional view, / 37
    3 shows a detail of the device according to FIG. 2 in an enlarged sectional view,
    4 shows a schematic flow example of a heterogeneous immunoassay,
    5 shows a fluid circuit diagram of the device according to FIG. 2,
    Fig. 6 is a block diagram for electronic control of the device of FIG. 2, and
    7 shows a diagram of the chronological sequence of the individual activities in the device according to the invention during a heterogeneous immunoassay.
    The devices shown in FIGS. 1a and 1b relate to examples of the prior art and have already been explained in detail in the introduction to the description.
    Functionally identical parts are provided with the same reference symbols in the individual illustrations of the invention.
    The device 410 according to the invention shown in FIGS. 2 and 3 is used to carry out heterogeneous immunoassays.
    The device has a one-dimensional, stationary cuvette array 200, for example arranged in an analyzer, in which the cuvettes 201 for receiving liquid media (samples, reagents, suspensions with magnetic particles 411, washing solutions) are arranged in a thermostatted cuvette block 820.
    A pivotable holding arm 420 is designed to be movable along the cell array 200 and can be lowered in the direction of the filling opening 207 of a cell 201 selected by the control logic of the device. The holding arm 420 is equipped with a suction needle 423, which can be lowered in the direction of the bottom 204 of the cuvette 201, together with a suction line 427, and with at least one dispenser 424a to 424d, which can be positioned above or in the respective filling opening 207, for dispensing / 37 the liquid media into the cuvette 201 At least one dispenser 424a, 424b is designed to deliver a washing solution for the magnetic particles 411.
    The supply lines to the dispensers 424a, 424b are designated 426, in particular a washing line 426a leads to the dispenser 424a, a washing line 426b leads to the dispenser 424b, a supply line 426c to the dispenser for a pretrigger solution and a supply line 426d to the dispenser 424d for a trigger solution.
    Furthermore, a magnet arrangement 430, which can be moved along the cuvette array 200 and acts on the contents of the selected cuvette 201, for separating the magnetic particles 411 is provided on an inner surface of the cuvette 201, and an optical detection device 435 which can be moved along the cuvette array 200, which points to the measurement window 202 of the selected cuvette 201 can be aligned in order to obtain a measurement signal proportional to the analyte concentration in the selected cuvette 201.
    For the sake of simplicity, only those components of the device 410 are shown which are essential for the present invention, wherein analyzer components such as sample and reagent storage, pumps, valves, evaluation, control and drive units are not discussed in detail.
    The cuvette array 200 is arranged in a thermostattable cuvette block 820, in particular in FIG. 3 the Peltier elements 831 provided for the thermostatting can be seen, which are arranged between cooling fins 832 and the cuvette block 820. The cuvette block 820 has access openings 825 aligned on the front side with the measurement windows 202 of the cuvettes 201. To mix and thermostate the cuvette contents, an ultrasonic transducer 840 (e.g. piezoelectric thickness transducer) is attached to the bottom 204 of each cuvette 201, contact being made with a spring contact board 846 via contact blocks 847 with spring contacts.
    Alternatively, the cuvette contents can be mixed, for example, by the suction needle 423, or by a manual or automatic pipettor used for introducing the sample and / or reagents, in that the liquid of a cuvette 201 by repeated suction and ejection of at least one / 37
    Part of the liquid volume, introduction of the samples and / or reagents with high flow rate or a suitable combination of these measures is homogenized.
    Other alternative devices for mixing the cuvette contents can include the introduction of magnetically moving stir bars, the immersion of a stirring shaft in the cuvette, and the stirring by a horizontal orbital movement of the cuvette block 820 or by a pipetting needle immersed in the cuvette.
    A dispenser platform 421, which can be lowered onto the filling opening 207 of the cuvette 201 and which has four dispensers 424a to 424d for dispensing liquid media into the cuvette 201 in the example shown, is fastened to the movable holding arm 420 on a resilient holder (see spring element 422). The dispenser platform 421 is penetrated in a central opening by the suction needle 423 attached to the holding arm 420, so that it can be lowered to the bottom 204 of the cuvette 201 after the dispenser platform 421 has been placed against the filling opening 207 of the cuvette 201.
    The dispenser platform 421 has a sealing surface 425 made of an opaque material on the side facing the cuvette 201, so that when the dispenser platform 412 is lowered, access to ambient light during the optical measurement of the cuvette content is excluded.
    According to the invention, a dispenser 424a for dispensing a washing solution for the magnetic particles 411 has an outflow direction (straight washing needle) oriented essentially parallel to the longitudinal axis of the cuvette 201, and a second dispenser 424b - likewise for dispensing a washing solution - one onto an inner side surface of the cuvette 201 directed outflow direction (oblique washing needle).
    A third dispenser 424c for delivering a pretrigger solution and a fourth dispenser 424d for delivering a trigger solution are optionally formed from two further dispensers 424c, 424d of the dispenser platform 412, the outflow directions of which are oriented essentially parallel to the longitudinal axis of the cuvette 201. The third dispenser 424c can remain unused or be omitted for chemo-luminescence-based immunoassays which only require / 37 of a trigger solution.
    The exemplary embodiment shown in FIGS. 2 and 3 is characterized by a platform 440 which can be moved along the cuvette array 200 and which has a lifting and rotating device 445 with which the holding arm 420 together with the suction needle 423 and the dispensers 424a to 424d of the dispenser platform 421 can be lowered , A common suspension 446 for the magnet arrangement 430 and the detection device 435 is preferably also arranged on the movable platform 440, so that a movable measurement and manipulation module 450 is realized which contains all the robotic, fluidic and measurement components for the process steps of the magnetic separation of the beads, the so-called B / F washing, as well as the triggering and measurement of the luminescence.
    The movable platform 440 of the measuring and manipulation module 450 is connected to the frame of the device 410 via a side rail 441 running parallel to the cuvette array 200, and can be moved to the position of a via a moving mechanism such as a stepper motor-driven toothed belt, a spindle or a linear motor selected cuvette 201 are brought. In order to supply and control the measuring and manipulation module 450, flexible electrical and fluidic connecting lines, for example in the form of so-called energy chains (not shown), can be brought to the platform 440.
    According to one embodiment variant, a washing station 442 for the suction needle 423 and the at least one dispenser 424a to 424d of the dispenser platform 421 can also be arranged on the movable platform 440, on the opening 443 of which the holding arm 420 can be lowered after a rotary movement, so that the entire group of needles is on Head of the pivotable support arm 420 can be inserted into the opening 443.
    The needle washing station 442 has an upper suction line 444a and a lower suction line 444b which limit the fill level. It is possible to approach opening 443 by an up and down movement with a 90 ° rotation while simultaneously lowering holding arm 420 below the upper edge of cuvette array 200, as a result of which other robotics components, for example / 37 possible pipettors, etc., can move freely along the cuvette array 200 can move.
    The pivotable holding arm 420 of the measuring and manipulation module 450 is fastened to a tower 449 which can be pivoted in the horizontal plane by 90 ° and is additionally vertically movable, the pivoting movement being made possible by, for example, a stepper motor-driven rotary actuator. In addition, the tower is equipped with a lifting device, which comprises, for example, a stepper motor-driven spindle or a toothed belt for generating a vertical translational movement of the holding arm 420. The two types of movement can be integrated in the combined lifting and rotating device 445 at the base of the vertical tower 449.
    An embodiment variant can also consist in that the needle washing station is positioned stationary at the end of the cuvette array 200, the holding arm of the needle group not having to be designed to be pivotable in this variant.
    According to a preferred embodiment variant, the common suspension 446 for the magnet arrangement 430 and the detection device 435 is suitable for carrying out a translatory or rotary movement in order to exchange the positions of the magnet arrangement 430 and the detection device 435 in front of the selected cuvette 201.
    For example, the magnet arrangement 430 and the detection device 435 can be attached to a rotor arm 447 mounted in the suspension 446 at the same distance from a common axis of rotation 448.
    The rotor arm 447 mounted in the suspension 446 can preferably be designed to be translatable in the direction of the axis of rotation 448 in order to bring the magnet arrangement 430 or the detection device 435 to the access opening 825 in the cuvette block 820 and thus to the measurement window 202 of the selected cuvette 201. The photomultiplier 435 and the magnet arrangement 430 can be aligned with their respective optical main or polar axis to the corresponding access opening 825 in the cuvette block and can be docked light-tight by a horizontal movement to the respective opening, or optimally on the wall to generate the highest possible magnetic flux density the cuvette 201 can be approximated.
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    The magnet assembly 430 may consist of one or more magnets, which are preferably rare earth magnets of high field strength, such as e.g. NdzFe ^ B (neodymium iron borate), but can also be designed as an electromagnet. The magnet arrangement 430 is preferably made from neodymium bar magnets with two different bar radii, an inner bar 431 essentially being surrounded by an outer, hollow-cylindrical bar 432 with the interposition of a non-magnetic intermediate layer 433, and the two bars having different lengths and diameters having a conical transition. The arrangement ends in a slim end region with a selective high magnetic flux density, which can be brought close to the window 201 of the cuvette 201 through the opening 825 in the cuvette block 820. The magnet arrangement 430 can also be composed of a plurality of individual magnets in order to increase the magnetic field strength required for magnetic separation on a cuvette wall or to reduce stray fields in the adjacent cuvettes. An example of a magnet arrangement is shown in FIG. 3, wherein a bipolar end of a concentric magnet arrangement 430 with a non-magnetic intermediate layer 433 is directed onto the cuvette 201.
    According to an embodiment variant, a second magnet arrangement (not shown) which can be moved along the cell array 200 and acts on the content of the selected cell 201 can be provided, which preferably forms a magnetic N-S bridge with at least one of the magnetic poles of the first magnet arrangement 430. The movable platform 440 of the measurement and manipulation module 450 can, for example, have a C-shaped cantilever, which passes under the stationary cell array 200 and allows a second separation magnet to be aligned along the magnetic effective axis of the first separation magnet, and on the other side of the cell block 820 to let go. Here, a second opening comparable to the first access opening 825 of the respective cuvette 201 is not necessary, since the magnetic field lines of the second magnet arrangement work through the material of the cuvette block (aluminum) which is not made of ferromagnetic material. Ideally, the polarity of the two separation magnets is oriented in opposite directions, so that a magnetic series connection (N-S) is created, which leads to a selective increase in the magnetic flux density and a reduction in the undesired stray field on the neighboring cuvettes. The stray field has an unfavorable effect on the magnetic beads / 37 located in the adjacent cuvettes, since the beads in the adjacent cuvettes can be in other process stages in which magnetic separation or agglomeration is undesirable.
    The second magnet arrangement can consist of one or more electromagnets as well as permanent magnets, with an actuator having to be provided in the case of permanent magnets in order to selectively approach or remove the magnet arrangement from the cuvette. The actuator mechanism can be designed analogously to that for the first magnet arrangement 430 and can have a belt drive, a drive spindle or a solenoid in a known manner.
    According to a further conceivable configuration, it is provided that the second magnet arrangement can be moved independently of the first magnet arrangement 430 on a separate rail past the components of the measuring and manipulation module 450, so that in addition to the above-mentioned advantages of a traveling second separation magnet, at the same time magnetic separation on another cuvette is possible in order to prepare magnetic beads for a washing step of a second assay in the other cuvette and thus save time.
    Furthermore, the second magnet arrangement can be used to hold the magnetic beads before the luminescence measurement on the inner wall of the respective cuvette 201, which is opposite the docking direction of the detection device, and thus to obtain a luminescence signal that is not influenced by the magnetic beads.
    The detection device 435 is preferably implemented by a compact photomultiplier and is used to measure the amount of light during the chemiluminescence triggered by the addition of the two trigger solutions, and can be equipped with Peltier cooling in order to obtain a more constant, low-noise signal. To avoid false light during the measurement at one of the access openings 825 of the cuvette block 820, the access openings 825 and the light inlet opening of the photomultiplier can have concentrically stepped contact surfaces at the edge of the two openings. Furthermore, a mechanically operated shutter element can be provided, for example, in order to protect the photomultiplier against the entry of ambient light in the idle state.
    A digital photomultiplier is preferably used to measure the luminescence at low analyte concentration, which triggers for each incoming photon and triggers a digital pulse of 10 ns. These short pulses are counted with the FPGA of the HetIA controller 460 (see FIG. 6) and added up as a counter reading over an adjustable sampling time. As long as the number of photons is small, the irregularly generated pulses can be output individually, the number of pulses per unit of time then corresponds to the number of photons per unit of time.
    According to the invention, a reference light source 436a for the detection device 435 can be arranged on the movable platform 440. The reference light source 436a serves to calibrate the photomultiplier and has a light exit opening which is aligned in the direction of the entry opening of the detection device 435 (e.g. photomultiplier). The reference light source 436a can be arranged at any point along the movement line of the detection device 435, but ideally such that the photomultiplier is calibrated when the magnet arrangement 430 is just in front of the respective access opening 825 of the cuvette block 820.
    As an alternative to this variant, a reference light source 436b can also be arranged in a fixed position at the end of the cuvette block 820 and have a light exit opening along the access openings of the cuvette block 820, as a result of which its thermostating device can also be used for the reference light source 436b.
    The sequence example of a heterogeneous immunoassay is shown by way of example in stages S1 to S9 in FIG. 4.
    The present example of a heterogeneous immunoassay relates to the required mechanical processes in a so-called sandwich assay. Here, the analyte molecule 413 (an endogenous protein, for example prostate-specific antigen) forms a bridge through antigen-antibody interactions between a first antibody (capture antibody 412) immobilized on the surface of the magnetic particles 411 and a second antibody to which signal molecules are bound ( Tracer antibody 414), which after the addition of a / 37
    Pretrigger liquid and a trigger liquid causes chemiluminescence that lasts for a few seconds and is proportional to the amount of analyte. The two types of antibodies are in excess compared to the analyte. So-called competitive immunoassays are used for analyte molecules which are too small to have binding sites for two different antibodies, the tracer antibodies competing directly with the analyte molecules for binding sites on an immobilized antibody.
    In a simple 1-step assay according to FIG. 4, the sample (contains the analyte 413), a suspension of magnetic particles 411 (magnetic beads) with a coating of a capture antibody 412, and a solution of the tracer antibody 414 are first placed in the cuvette 201 pipetted in by means of a pipette (not shown here) (S1, in FIG. 4).
    During the subsequent incubation (approx. 10 min) at 37 ° C., the solution is periodically stirred, for example by means of ultrasound, in order to prevent the beads from sinking and agglomerating. Each analyte molecule is now sandwiched between a capture antibody 412 immobilized on the beads 411 and a tracer antibody 414. There are also non-specifically bound tracer antibodies 415 (S2, in FIG. 4).
    The beads 411 together with the substances bound to them are now fixed to the inner wall of the cuvette 201 with the aid of the magnet arrangement 430 (S3, in FIG. 4) and the entire liquid is removed with the suction needle 423 lowered from the dispenser platform 421 (S4, in FIG 4).
    Subsequently, a washing solution is introduced through a washing needle 424b directed obliquely onto the inner wall of the cuvette 201 in order to remove unbound tracer antibodies adhering to the beads 430 and remaining in the reaction solution by carefully rinsing the beads, the beads 411 still being magnetic be held on the vessel wall (S5, in Fig. 4).
    The cuvette 201 is then sucked dry again, the beads 411 together with the substances bound to them being still magnetically fixed to the inner wall of the cuvettes 201 (S6, in FIG. 4).
    / 37
    A second, vertically aligned washing needle 424a, however, produces the
    Injection of washing solution or diluent into the turbulence
    Liquid so that the beads 411 are resuspended in the liquid when the magnets are undocked (S7, in FIG. 4).
    After this washing step, which can be carried out several times in succession, the photomultiplier 435 is moved towards the cuvette 201. By means of the two dispensers 424c and 424d, pretrigger (S8, in FIG. 4) and trigger solution (S9, in FIG. 4) are now supplied in rapid, immediate succession. This triggers a chemiluminescence L (flash luminescence) that lasts only a few seconds and can be measured by the 435 photomultiplier. The dispenser platform 421 of the holding arm placed on the filling opening 207 of the cuvette 201 at the same time ensures that the cuvette 201 is darkened for this purpose.
    The used cuvette 201 is then sucked empty with the suction needle 423 and either replaced by a disposable cuvette, or cleaned and reused, so that a new immunoassay can take place in the previously used cuvette position.
    To wash the cuvette, the manipulator must be moved away from the cuvette so that the cuvette washing station can move up and start washing.
    In principle, however, other, somewhat modified immunoassays which have a magnetic separation with B / F washing as a process step can also be carried out with the device according to the invention, with another detection method for measuring the chemiluminescence optionally being provided for the detection.
    As shown schematically in FIG. 5, the movable measuring and manipulation module 450 of the invention has a fluidic system 451 for supplying the dispenser platform 421 with washing liquid WF, pretrigger liquid PTF, trigger liquid TF and compressed air DL. Furthermore, devices for suctioning reaction mixture or washing liquid from the cuvettes 201 of the cuvette array 200 and the container or washing trough of the washing station 442 are provided.
    / 37
    The fluidic system 451 is controlled by the HetlA controller 460 (see FIG. 6) and comprises a series of magnetically actuated 3-way valves 457 and precision piston pumps as dispensing pumps 455, which are connected to the movable one
    Platform 440 (see FIG. 2) are connected via flexible hose connections (indicated by wavy lines).
    The dispenser platform 421, which can be moved in the x, y and z directions via the combined degrees of freedom of the movable platform 440 and the pivotable holding arm 420, comprises a group of dispensers 424a to 424d which is supplemented by the lowerable suction needle 423.
    The dispensing unit 452 each has its own dispensing pump 455 for the provision of washing liquid WF, pretrigger PTF and trigger liquid TF, the liquid flow from the dispensing pump 455 for the washing liquid being connected to the straight 424a or the oblique washing needle 424b via a 3-way valve 457 can. The four selectively loadable supply lines are made of flexible plastic at the movable points and are guided in energy chains (not shown).
    The dispensing pumps 455 of the dispensing unit 452 are each connected to the valve network 453 via their own supply lines, whereby for flushing and cleaning purposes, in particular for cleaning the dispensers 424a to 424d and the suction needle 423, alternatively compressed air DL or system water SW (instead of the primary delivery medium) deionized water) can be connected via a corresponding 3-way valve 457 and fed to the dispensing pumps 455.
    The container of the washing station 442 for cleaning the dispensers 424a to 424d and the suction needle 423 has two suction lines 444a, 444b, one of which is 444b in the bottom of the container, a second in the upper half of the container, to act as an overflow for setting one stable filling levels. The suction unit 454 is connected both to the two suction lines 444a, 444b and to the suction needle 423 via flexible hose lines which are guided in energy chains (not shown). Shut-off valves 458 are provided to prevent unwanted backflow of extracted liquids. The three drain lines open into a common feed line of a suction pump 456 (e.g. a / 37 self-priming positive displacement pump), which feeds the extracted waste liquids W to a collection or treatment area in the device (not shown)
    FIG. 6 shows a block diagram for the electronic control of the device according to the invention according to FIG. 2. The HetIA controller 460 of the controller board 461 operates the electrical and mechanical components of the HetIA module and is controlled and programmed by a main computer 588 (e.g. personal computer). The PC controls the sequence and sequence of the sub-processes; the HetIA Controller 460 is responsible for executing the individual actions.
    The functions of the HetIA controller 460 can be summarized as follows (see Fig. 6):
    • Communication with PC 588 via Ethernet interface • Robotic functions RF using stepper motors o Moving platform 440 in the x direction to the respective cuvette 201 of the stationary cuvette array 200 (or to the stationary reference light source 436b in the cuvette block 820, if no moving reference light source 436a is provided) o Rotary movement of the rotor arm 447 for exchanging the position of the detection device 435 (photomultiplier) and magnet arrangement 430 o y movement for docking the photomultiplier 435 or the magnet arrangement 430 to the measurement window of the cuvette 201 or to a reference light source 436a • traveling on the platform 440 FV of the fluidic valves 457, 458 of the fluidic system 451 • DP control for the 455 metering pumps • UM control for the 840 ultrasonic transducer o Has its own US oscillator that is independent of the 461 controller board o Decoder function for the 840 piezoelectric transducers on the individual cuvettes 201/37• Control DE for the detection device 435 and the reference light source 436a • Temperature control TR for thermostatting (37 ° C) o Peltier controller for the detection device 435 (photomultiplier) o Peltier controller for the cuvette block 820
    Certain functions that must be triggered in real-time synchronization (see clamp S in Fig. 6) are implemented in the FPGA of the HetIA controller 460. For example:
    • Time triggering of the control DP of the dosing pump with the time
    Control DE for the detection device 435 (photomultiplier measurement) • Triggering of the reference light source synchronously with the measurement of the photomultiplier • Ultrasonic mixing process of the respective cuvette.
    The sequence of a heterogeneous immunoassay already shown in FIG
    Example of a 1-step sandwich assay will now be described from the perspective of the necessary mechanical processes in the HetIA module. The temporal
    Distribution of the machine activities during the assay is shown in the lines I to XI over the common time axis t in FIG. 7.
    I pipetting samples, reagents and a beads suspension into the
    Cell 201
    II Thermostatization of the cell block
    III Activation of the ultrasonic mixing unit
    IV docking the magnet arrangement 430 for the separation of the beads
    V Suction needle activities 423
    VI washing the fixed beads with the oblique washing needle 424b (laminar)
    VII Re-suspension of the beads with the straight washing needle 424a (turbulent) / 37
    VIII Dispensing of pretrigger liquid via the 424c dispenser (turbulent)
    IX Dispensing of trigger fluid via the 424d dispenser (turbulent)
    X Exchange of the position of magnet arrangement 430 and photomultiplier 435 and luminescence measurement on the cuvette 201
    XI washing the suction needle 423 and the dispensers 424a to 424d
    The individual measures are designated in FIG. 7 in chronological order with 1 to 13.
    1) First, there is a mechanical or manual pipetting of the sample, a suspension of magnetic particles (magnetic beads) with a coating of a capture antibody, and a solution of the tracer antibody in the cuvette (see S1, Fig. 4). Mechanical pipetting can be carried out, for example, by a laboratory robot known from the prior art with x / y / z mobility, while manual pipetting can be carried out by a laboratory technician, for example using hand-held pipettes with disposable tips.
    2) As a constant background activity in all mechanical processes of the assay, the cuvette block 820 with the cuvettes 201 located therein is thermostatted to 37 ° C. (see line II).
    3) The sample-reagent mixture in the cuvette 201 now slowly warms up to the target temperature of 37 ° C. and is incubated for a total of about 10 minutes, while the ultrasound mixing device initially uses the ultrasound transducer 840 on the cuvette 201 to incubate the sample initially homogenized and stirred at short intervals to prevent the beads from sinking and agglomerating (see line III).
    4) After incubation, the magnetic separation of the incubated beads is initiated by rotating the magnet arrangement 430 on the measuring and manipulation module 450 to the corresponding access opening in the cuvette block 820 (see line IV).
    / 37
    5) After separation of the beads on the wall of the cuvette 201, the suction needle 423 is lowered to close to the bottom of the cuvette and all the liquid in the cuvette is sucked off (see S4, FIG. 2), while the magnet arrangement 430 remains in the access opening 825, to hold on to the beads.
    6) Now, washing solution flowing in a laminar manner on the wall of the cuvette 201 is introduced via the oblique washing needle 424b in order to wash the beads fixed on the wall (see line VI).
    7) The cuvette 201 is now sucked dry, the beads still being magnetically fixed to the wall of the cuvette 201 (see line V).
    8) Subsequently, washing liquid is introduced again via a second, vertically oriented, turbulence-generating washing needle 424a, so that the beads are resuspended in the liquid when the magnet arrangement is undocked (see line VII).
    Steps 5-8 can optionally be repeated in order to achieve an even better separation of unbound tracer antibodies.
    9) The position of detection device 435 and magnet arrangement 430 is then exchanged for a 180 ° rotation and the detection device is inserted into the corresponding access opening in the cuvette block 820 (see line X).
    10) Now the pretrigger liquid is first added via a first, vertically oriented, turbulent injection dispenser 424c (see S8, Fig. 4)
    11) The luminescence is now triggered by adding the trigger liquid via a further, vertically oriented, turbulent injection dispenser 424d (see line IX).
    12) Now the suction needle 423 is inserted again and the reaction mixture is suctioned off. The cuvette 201 is now either replaced by a disposable cuvette or washed.
    / 37
    13) Finally, the swivel arm is swiveled horizontally to the side by 90 ° and introduced into the washing station 442. The dispensers 424a to 424d and the
    Suction needles 423 of the dispenser platform 421 are washed by washing solution flowing in from one of the two washing needles for the B / F washing until the filling level is sufficient to wet all the needles (see line XI).
    权利要求:
    Claims (18)
    [1]
    1. Device (410) for carrying out heterogeneous immunoassays with the aid of magnetic particles (411) in cuvettes (201) arranged in a row, each cuvette (201) having a filling opening (207) and at least one lateral measurement window (202) which is transparent to the measuring radiation , characterized by at least one stationary cuvette array (200), in which the cuvettes (201) are arranged to hold liquid media, at least one that can be moved along the cuvette array (200) and in the direction of the filling opening (207) of a selected cuvette (201) Retractable holding arm (420) with at least one suction needle (423) that can be lowered towards the bottom (204) of the cuvette (201), and with at least one dispenser (424a to 424d) that can be positioned above or in the respective filling opening (207) liquid media into the cuvette (201), at least one dispenser (424a, 424b) being designed to deliver a washing solution for the magnetic particles (411) is, at least one magnet arrangement (430) which can be moved along the cuvette array (200) and acts on the content of the selected cuvette (201) for separating the magnetic particles (411) on an inner surface of the cuvette (201), and at least one along the Cuvette arrays (200) which can be moved and which can be aligned with the measurement window (202) of the selected cuvette (201), optical detection device (435) for recording a measurement signal proportional to an analyte concentration in the selected cuvette (201).
    [2]
    2. The device according to claim 1, characterized in that the at least one dispenser (424a to 424d) for dispensing the liquid media is arranged in a dispenser platform (421) which can be lowered onto or into the filling opening (207) of the cuvette (201) the lowerable suction needle (423) is penetrated.
    27/37
    [3]
    3. Device according to claim 1 or 2, characterized in that the dispenser platform (421) on the side facing the cuvette (201) has a sealing surface (425) made of an opaque material.
    [4]
    4. Device according to one of claims 1 to 3, characterized in that a first dispenser (424a) for dispensing a washing solution for the magnetic particles (411) has an outflow direction which is aligned essentially parallel to the longitudinal axis of the cuvette (201), and that a second dispenser (424b) for dispensing a washing solution for the magnetic particles (411) has an outflow direction which is directed towards an inner side surface of the cuvette (201).
    [5]
    5. Device according to one of claims 1 to 4, characterized in that of further dispensers (424c, 424d), the outflow directions of which are aligned essentially parallel to the longitudinal axis of the cuvette (201), optionally a third dispenser (424c) for dispensing a Pretrigger solution and a fourth dispenser (424d) is designed to deliver a trigger solution.
    [6]
    6. Device according to one of claims 1 to 5, characterized in that the holding arm (420) for the suction needle (423) and the at least one dispenser (424a to 424d) has a lifting and rotating device (445) running along one of the cuvette array (200) movable platform (440) is arranged.
    [7]
    7. The device according to claim 6, characterized in that a washing station (442) for the suction needle (423) and the at least one dispenser (424a to 424d) is arranged on the movable platform (440), on the opening (443) of which the holding arm (420) is designed to be lowered after a rotary movement.
    [8]
    8. The device according to claim 6 or 7, characterized in that a common suspension (446) for the magnet arrangement (430) and the detection device (435) is arranged on the movable platform (440).
    [9]
    9. The device according to claim 8, characterized in that the common suspension (446) for the magnet arrangement (430) and the detection device (435) is suitable, a translational or
    28/37 rotary motion to exchange the positions of the magnet assembly (430) and the detection device (435) in front of the selected cuvette (201).
    [10]
    10. The device according to claim 9, characterized in that the magnet arrangement (430) and the detection device (435) are attached at the same distance to a common axis of rotation (448) on a rotor arm (447) mounted in the suspension (446).
    [11]
    11. The device according to claim 10, characterized in that the rotor arm (447) mounted in the suspension (446) is translationally displaceable in the direction of the axis of rotation (448), around the magnet arrangement (430) or the detection device (435) to the measuring window ( 202) of the selected cuvette (201).
    [12]
    12. Device according to one of claims 6 to 11, characterized in that the holding arm (220) arranged on the movable platform (440) together with the dispenser platform (421) together with the magnet arrangement (430) and the detection device (435) along the cuvette array (200) traversable measuring and manipulation module (450), which combines all robotic, fluidic and metrological components for the process steps of a heterogeneous immunoassay.
    [13]
    13. Device according to one of claims 6 to 12, characterized in that a reference light source (436a) for the calibration of the detection device (435) is arranged on the movable platform (440).
    [14]
    14. Device according to one of claims 1 to 13, characterized in that the detection device (435) is designed as a photo multiplier.
    [15]
    15. Device according to one of claims 1 to 14, characterized in that a second, along the cuvette array (200) movable, acting on the content of the selected cuvette (201) magnet arrangement is provided, which preferably with at least one of the magnetic poles of the first Magnet arrangement (430) forms a magnetic LV bridge.
    29/37
    [16]
    16. The apparatus according to claim 15, characterized in that the second magnet arrangement is arranged on the movable platform (440).
    [17]
    17. A method for determining an antigen by means of a heterogeneous immunoassay, characterized in that, in a first step A, a sample for determining the antigen, a suspension of magnetic particles with a capture antibody, and, if appropriate, a tracer antibody or a labeled antigen in a selected cuvette (201) of a stationary cuvette array (200) are pipetted in, and that the following steps B an immunochemical analysis, such as
    e) separating the magnetic particles,
    f) one or more introduction and suction of a washing solution,
    g) metering in at least one trigger liquid, and
    h) luminometric measurement of the sample is carried out with the aid of a measuring and manipulation module (450) which can be moved along the cuvette array and which is stopped in order to carry out individual or all steps a) to d) in the selected cuvette (201).
    [18]
    18. The method according to claim 19, characterized in that the measuring and manipulation module (450) during the course of time-consuming steps in immunochemical analysis, such as incubation, etc., in the selected cuvette, to at least one other cuvette (201) of the cuvette array (200) is carried out in order to carry out individual or all steps B of an immunochemical analysis.
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    同族专利:
    公开号 | 公开日
    EP3821247A1|2021-05-19|
    WO2020010379A1|2020-01-16|
    US20210270819A1|2021-09-02|
    CN112424603A|2021-02-26|
    AT521352B1|2020-01-15|
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    法律状态:
    优先权:
    申请号 | 申请日 | 专利标题
    ATA50603/2018A|AT521352B1|2018-07-13|2018-07-13|METHOD AND DEVICE FOR CARRYING OUT HETEROGENIC IMMUNOASSAYS|ATA50603/2018A| AT521352B1|2018-07-13|2018-07-13|METHOD AND DEVICE FOR CARRYING OUT HETEROGENIC IMMUNOASSAYS|
    EP19742670.3A| EP3821247A1|2018-07-13|2019-07-11|Method and device for performing heterogeneous immunoassays|
    PCT/AT2019/060230| WO2020010379A1|2018-07-13|2019-07-11|Method and device for performing heterogeneous immunoassays|
    CN201980046702.4A| CN112424603A|2018-07-13|2019-07-11|Method and apparatus for performing heterogeneous immunoassays|
    US17/260,195| US20210270819A1|2018-07-13|2019-07-11|Method and device for performing heterogeneous immunoassays|
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