Patent Application
20130027686
The invention relates to an analysis device for quantitative and/or qualitative analysis of particles in a substantially liquid sample, and to a method for performing the analysis using the aforementioned device.
It is known to analyze particles, such as cells, in liquids by fluorescence spectroscopy. Hereinafter, the term “particles” includes biological cells of varying origin or optionally solids or molecules. For the analysis, liquid samples are mixed with a dye, such as individual proteomic markers that accumulate on the particles in the sample. It is also known to use these methods for performing the detection and quantification of tumor cells in various body fluids, such as urine. The known methods have the disadvantages that they take longer than 50 minutes until a prepared sample preparation is ready, and that they require many individual work steps, which only skilled persons can perform. Moreover, it is necessary to use the most various kinds of equipment, whose operation again requires specially trained personnel.
The object of the invention is to create both an analysis device and a method which make it possible to shorten the analysis time, compared to known methods, for quantitative and qualitative detection of predetermined particles in a liquid and thus to make them more economical. A further object is to make the analysis capable of being done simply and reliably and to make the outcome visually perceptible.
These objects are attained by an analysis device of the invention, having a sample container unit comprising a sample container for receiving a liquid sample and marking the particles contained in the sample, having a cap for fluid-tight closure of the sample container; a measuring cell unit, which is in fluidic communication with the sample container via an outlet, which measuring cell unit has a liquid-conducting channel, at least one wall of which channel is embodied as at least partially transparent; a carrier unit, which has means for contactlessly transporting and/or concentrating marked particles contained in the sample fluid; and having an optical unit for spectroscopic and/or microscopic detection of the marked particles, having at least one light source for excitation of the marked particles in the sample.
The method of the invention for analysis of a substantially liquid sample having particles that are freely movable in it includes the steps of a) marking the particles with a dye and/or magnetic agents; b) spatially bundling the marked particles, optionally by generating a magnetic field for spatially bundling magnetically sensitive particles and/or sedimentation; and c) performing a spectroscopic and/or microscopic analysis of the particles contained in the sample.
The present invention, with a brief incubation time of 5 to 10 minutes, makes high accuracy possible; that is, a sensitivity and selectivity of >95%, in particular even in a disease in its early stage.
The analysis device of the invention has a compact construction with short fluid channels, so that only tiny volumes of agents and sample fluids are needed, as a result of which, among other advantages, the costs of analysis can be lowered.
In particular, the analysis device of the invention and the method performed with this analysis device enable fast, objectified computer-supported detection of particles that have been altered by disease, especially in body fluids, such as urine or sputum, but also particles in blood as well as tissue cell suspensions. Both the analysis device of the invention and the method of the invention can advantageously be employed for cytological detection of cancer diseases, for checking for doping, or for counting particles and bacteria.
A preferred embodiment is distinguished in that the cap of the sample container is formed from an outer screw-on cap part and a middle cap part connected to the outer cap part via a rated breaking point, and the outer diameter of the middle cap part is approximately equivalent to the inner diameter of the sample container, so that the middle cap part can be lowered into the sample container in form-locking fashion.
A further preferred embodiment is distinguished in that the middle cap part includes an inner cap part that can be moved into the middle cap part, and between the underside of the inner cap part and a foil extending between the lower edge of the middle cap part, a hollow space for receiving the agents for marking the particles is embodied in the sample.
A further preferred embodiment is distinguished in that prestressed elements, which preferably dip into the sample in the tripped state, are additionally provided in the hollow space.
A further preferred embodiment is distinguished in that valves are disposed at the entrance and the exit of the liquid-conducting channel.
A further preferred embodiment is distinguished in that a mixing chamber is disposed between the entrance of the liquid-conducting channel and the spectroscopic and/or microscopic observation chamber.
A further preferred embodiment is distinguished in that a filter is disposed in the liquid-conducting channel on the outlet end of the spectroscopic and/or microscopic observation chamber.
A further preferred embodiment is distinguished in that the sample container unit and the carrier unit are detachably connected to one another.
A further preferred embodiment is distinguished in that the sample container unit can be connected selectively to the carrier unit in terms of orientation by means of shaped elements, and the carrier unit has complementary component means.
A further preferred embodiment is distinguished in that the shaped elements are embodied as a set of at least two holes having different inner diameters.
A further preferred embodiment is distinguished in that the light source is formed by at least one monochromatic LED and that the light is conducted to the spectroscopic and/or microscopic observation chamber by means of an optical waveguide integrated with the carrier unit.
A further preferred embodiment is distinguished in that the carrier unit has at least one coil system for generating magnetic fields, by means of which fields magnetically sensitive particles in the sample can be spatially bundled or distributed.
A further preferred embodiment is distinguished in that the carrier unit further has at least one temperature sensor and at least one heating element for heating the sample upstream and/or downstream of the analysis site.
A further preferred embodiment is distinguished in that the carrier unit has a liquid-conducting channel.
Finally, a further preferred embodiment is distinguished in that the carrier unit has sensors for ascertaining further parameters of the sample.
A further preferred embodiment of the method is distinguished in that after the analysis of the sample, it includes the following step: backflushing both the particulate component and the sample fluid, followed by a cleaning solution, into the sample container and/or disinfecting the carrier unit.
The invention will be explained in further detail below in terms of exemplary embodiments shown in the drawings. In the drawings:
a-1f show a longitudinal section through a sample container unit, comprising a sample container with a cap and a measuring cell unit, in various stages of the analysis method;
a-4e show a schematic view of a plug connection; and
A first function part of the analysis device is the sample container unit 1 shown in
The function of the sample container 2 is to receive the substantially liquid sample to be examined, in particular during the marking of the particles contained in it. In its bottom the sample container has an outlet 43, through which the sample, from the sample container 2, reaches the inside of the measuring cell unit 4 for analysis.
Depending on the analysis task desired, the agents 5 required for the analysis, such as a dye, and/or magnetic beads, can be placed, protected against environmental factors and aging, in the cap 3 of the sample container 2, optionally in chambers separated in sectors from one another and if desired in sealed fashion. Insert elements (not shown) can be placed in the sample container in form-locking fashion and serve the purpose of prefiltration, for example, to prevent clogging of the outlet 43 to the measuring cell unit 4 by coarse contaminants (kidney stone fragments, tissue scrapings from surgical operations), and/or serve as a repository for additional agents. Alternatively to the insert elements, plug-in elements (not shown) having the same function can be connected externally to the container bottom in form-locking, non-detachable, and fluid-tight fashion via connecting pins 6. These plug-in elements, as adaptor pieces (adaptors) can enable a connection between modified forms of the measuring cell unit 4 and the sample container.
Via the connecting pins 6, the measuring cell unit 4 shown in
The sample container unit 1 is preferably embodied as a disposable plastic part. In that case, each sample requires its own sample container unit. Its component parts perform microfluidic functions for separating out the particles present in the fluid, but preferable do not include any sensors. The particulate portion of the sample always remains inside the measuring cell unit 4 of the sample container unit 1 before, during, and also after the analysis and once the analysis has been done can be disposed of properly along with the sample container unit.
Before the sample container unit 1 is inserted into a carrier unit 10 (
A further function part of the analysis device is the carrier unit 10, shown in
Particularly for analysis of more-complex body fluids that contain many different particles, selective separation of target cells in the observation chamber is required, since in such cases, simple sedimentation by gravity is inadequate. The cell precipitation can be accomplished or reinforced in field-induced fashion, for instance by means of magnetic fields. To that end, the carrier unit preferably has controllable coil systems 14. These coil systems 14, disposed in an array, can be switched on and off arbitrarily, and as a result, not only magnetic alternating fields for controlled mixing but also fields for immobilizing particles with magnetic beads adhering to them can be generated.
Advantageously, the controllable coil systems 14 are disposed both above and below the measuring cell unit 4 of the sample container unit 1. To that end, between the sample container unit 1 and the measuring cell unit 4 attached to it, a recess 41 is provided, which receives a crosspiece 18 of the carrier unit 10, in which crosspiece coil systems 14 are provided. This crosspiece 18 of the carrier unit 10 can optionally be integrated as a module with the analysis device, to reinforce the sedimentation of the cells or particles.
The carrier unit 10 is preferably designed for continuous operation. Preferably, ceramic multi-layer circuitry, which is known to the person skilled in the art, is employed. As a result, the coil systems 14 shown in
By a suitable disposition of the components, the ceramic also allows the heat produced to be carried away. A tempering system in the form of heating elements 15 with temperatures sensors can also be integrated with the carrier unit 10, since as a result, the activity of the particles or cells is preserved, and the sensitivity of the entire analysis system can be enhanced. In regions of liquid-conducting channels 54, provided in the carrier unit 10, that are for carrying the sample fluids onward or diverting them, heating elements 15 can also be provided, to enable thermal sterilization of these channels.
Besides the aforementioned components of the carrier unit 10, in a selective analysis portion 16, further sensors 17 for determining additional parameters, such as the liquid portions of the sample, and for determining its pH value, ammonia content and/or protein content can be variably integrated with the carrier unit 10.
A further function part of the analysis device is an optical unit 20, of the kind shown in
Alternatively, however, the excitation can also be done by means of an optically narrow-band-emitting, preferably monochromatic LED 19 via an optical waveguide 30 via the carrier unit 10 lighting controlled by a special index of refraction, as also shown in
Below, the measuring method using the analysis device of the invention will be explained in further detail, again in junction with the drawings. At the beginning, as shown in
For performing the measuring method, the sample container unit 1, in a mistake-proof or selective-orientation position as shown in
Once the incubation has been initiated, the complementary component means 31, on which the sample container 1 is locked, are lowered along with the upper part of the carrier unit 10, as shown in
During the measurement procedure, the sample container 2 takes on the function of a perfusion cartridge. The cap 3 as shown in
The agents 5 are contained, for instance in solid form, in the cap 3, or optionally are applied two-dimensionally to the foil 35, or a in the form of a coating of mixed beads. Alternatively, prestressed elements 37, for instance of plastic, that are concealed in the interior of the cap unfold spontaneously when the foil breaks and reinforce the mixing of the agents 5 and the sample fluid. A special geometry of the inside of the cap, in the form of bucket flaps or interference flaps (not shown), can further promote mixing as the cap 3, as a ram, is moved farther inward in rotating fashion. Any residual air still present in the container 2 can escape through an exhaust valve 38 in the cap 3, which however does not allow any fluid to escape. After the analysis, backflushing the sample into the sample container 2 is optionally done, by means of tensile stress on the cap 3, as shown in
After the inner cap part 36 has been screwed/pushed in, it preferably snaps into a detent in the middle cap part 48 such that the two can no longer be separated from one another even in response to tensile stress, for instance while the sample is being backflushed.
During the measurement procedure, the incubated sample fluid reaches the mixing chamber 7 of the measuring cell unit 4. Here, further agents are delivered as needed via an optional second inlet 51 that can connected into the measuring cell unit 4, as shown in
The thus-marked and mixed sample flows to the observation chamber 8, where the particles thus marked by color and optionally also magnetically settle out or are collected by means of a strong nonhomogeneous magnetic field, brought about for example by neodymium magnets (not shown) or by the coil system 14. After the magnetic field is shut off, the particles can likewise settle out freely. Alternatively, with the field kept in force, the particles can be concentrated by slow mechanically/pneumatically induced lowering of an observation chamber cap 39, made of soft plastic that is kept dark in color, which suppresses interfering background reflections.
The measuring cell unit 4 contains a filter 9 for separating out further particles. Premature closure of the filter membrane of the filter 9 from clogging or occlusion can be detected from a pressure increase in the measuring cell unit and suppressed by means of backflushing pulses, on the one hand orthogonally through the filter membrane and on the other on the prefilter side tangentially along the filter membrane by means of an addition channel unit, not shown, with a valve. It is equally possible, after they have flowed through the entire volume of the sample, for those particles which settle out in the vicinity of the filter chamber to be backflushed in the direction of the observation chamber by means of such a tangential countercurrent. The sample fluid can if desired be subjected to further analyses in an analysis portion 16 and is finally collected in a waste unit 40 for disposal. Alternatively, the sample fluid can be backflushed into the sample container 2 in the course of the disinfection of the analysis device. To achieve this, after the analysis, the particulate portion of the sample, along with the sample fluid, followed by a cleaning solution, is backflushed into the sample container, and the carrier unit 10 is disinfected; after being removed, the closed sample container 2 can be harmlessly disposed of properly. Mechanically, this can be done for instance as shown in
The method and the components of the measuring cell unit 4, the carrier unit 10, and the optical unit 20 are preferably controlled via an electronic device 55, such as a computer. The qualitative and/or quantitative analysis of the marked particles or cells is preferably likewise done with computer support.
It is understood that the exemplary embodiments described can be modified in various ways within the scope of the concept of the invention, for instance with regard to the materials used and the geometrical embodiment of channels and plug connections, without departing from the scope of the invention.
| Number | Date | Country | Kind |
|---|---|---|---|
| A 1582/2009 | Oct 2009 | AT | national |
| Filing Document | Filing Date | Country | Kind | 371c Date |
|---|---|---|---|---|
| PCT/AT2010/000374 | 10/7/2010 | WO | 00 | 10/4/2012 |
