Patent Application
20230341431
The present disclosure relates to an automatic analyzer and an analysis method.
An automatic analyzer, a chemical experiment device, and the like are devices that perform analysis and experiments using various reagents. For example, in an immunoanalyzer for clinical test, magnetic particles are generally used as one of the reagents for separating a measurement target from other substances.
A separation method using the magnetic particles is a method in which a compound that causes specific binding is adsorbed or bound to a surface of the magnetic particles, and components in a specimen solution are recovered and concentrated via the compound. However, since the magnetic particles have a large specific gravity, the magnetic particles gradually settle due to gravity.
PTL 1 discloses that a liquid containing a magnetic substance in a reaction vessel is stirred using a stirring mechanism in an automatic analyzer (see claim 1 of PTL 1).
PTL 1: JP2019-100976A
However, in the automatic analyzer according to PTL 1, since a space for providing the stirring mechanism is essential, it is difficult to save the space of the device.
Therefore, the present disclosure provides a technology that enables stirring of a liquid containing fine particles without providing a dedicated stirring mechanism.
In order to solve the above problem, an automatic analyzer according to the present disclosure includes a probe configured to aspirate and discharge a specimen and a reagent, and a control unit configured to control an operation of the probe, and the control unit controls the probe so that the specimen, the reagent, and fine particles are dispensed to an empty vessel to obtain a liquid mixture, and a first stirring of aspirating, discharging, and stirring the liquid mixture in the vessel before precipitation of the fine particles after the dispensing, and a second stirring of aspirating, discharging, and stirring the liquid mixture in the vessel after the precipitation of the fine particles after the first stirring are performed.
More features relevant to the present disclosure are clarified based on descriptions of the present description and accompanying drawings. Aspects of the present disclosure may be achieved and implemented using elements and various combinations of the elements and the following detailed description and accompanying claims. Descriptions in this specification are merely exemplary, and are not intended to limit the scope of the claims or application of the present disclosure in any sense.
According to the automatic analyzer of the present disclosure, it is possible perform stirring of a liquid containing fine particles without providing a dedicated stirring mechanism. Problems, configurations, and effects other than those described above will become apparent from the following description of the embodiments.
The specimen vessel disk 102 stores a plurality of specimen vessels 101 that accommodate biological samples (hereinafter, referred to as specimens) such as blood and urine. The reagent vessel disk 104 stores a plurality of reagent vessels 103 that accommodate various reagents used for analysis of the specimens. The incubator disk 105 stores a plurality of reaction vessels 34 for reactions of the specimens and the reagents.
The dispensing mechanism 106 drives a probe (not illustrated in
The control device 108 is, for example, a computer device, and controls the overall operations of the automatic analyzer 100. In addition, the control device 108 receives a detection result from the detection unit 107 and analyzes a measurement target component in the specimen.
The reaction vessel storage unit 109 stores a plurality of unused reaction vessels 34. The dispensing tip storage unit 110 stores a plurality of unused dispensing tips 32. The used reaction vessel 34 and dispensing tip 32 are discarded in the disposal unit 111.
The transport device 112 includes an actuator that grips the reaction vessel 34 and the dispensing tip 32 and is movable in three axial directions. The transport device 112 transports the reaction vessel 34 stored in the reaction vessel storage unit 109 to the incubator disk 105, transports the dispensing tip 32 stored in the dispensing tip storage unit 110 to the dispensing tip mounting unit 113, and discards the used reaction vessel 34 to the disposal unit 111. The dispensing tip 32 is mounted on a tip end of the probe of the dispensing mechanism 106 in the dispensing tip mounting unit 113.
In step S1, when a user inputs an instruction to start the operation to the control device 108, the control device 108 activates each unit of the automatic analyzer 100 to start the analysis. Here, the control device 108 drives the dispensing mechanism 106 and the transport device 112 to mount the dispensing tip 32 on the probe in the dispensing tip mounting unit 113.
In step S2, the control device 108 causes the specimen vessel disk 102 to rotate and causes the dispensing mechanism 106 to move, so that the specimen is dispensed from the specimen vessel 101 into the reaction vessel 34 of the incubator disk 105. In addition, the control device 108 causes the reagent vessel disk 104 to rotate and causes the dispensing mechanism 106 to move, so that the reagent is dispensed from the reagent vessel 103 into the reaction vessel 34.
After the reagent and the specimen are dispensed, for example, while the reagent and the specimen are allowed to stand at, for example, 37° C. for 9 minutes, the measurement target component included in the specimen and the label are bound. Further, the measurement target component and the biotinylated modified antibody bind to each other, and the label and biotin are integrated via the measurement target component. It is expected that while the reagent and the specimen are allowed to stand, the reaction continues due to diffusion and an equilibrium state is obtained. After this reaction reaches equilibrium, the process proceeds to a next step.
In step S3, the control device 108 causes the reagent vessel disk 104 to rotate and causes the dispensing mechanism 106 to move, so that the magnetic particle solution is dispensed from the reagent vessel 103 accommodating the magnetic particle solution into the reaction vessel 34.
In step S4, the control device 108 drives the dispensing mechanism 106 to aspirate, discharge, and stir a liquid mixture of the specimen, the reagent, and the magnetic particles before precipitation of the magnetic particles. The stirring performed before the precipitation of the magnetic particles is referred to as a first stirring. Specific conditions of the first stirring will be described later.
After the first stirring, the control device 108 causes the dispensing mechanism 106 to rotate, discards the dispensing tip 32 in the disposal unit 111, drives the transport device 112 to set the new dispensing tip 32 in the dispensing tip mounting unit 113, causes the dispensing mechanism 106 to rotate, and mounts the new dispensing tip 32 on a dispensing probe in the dispensing tip mounting unit 113.
In step S5, the control device 108 determines whether the reaction of the specimen and the reagent has ended after a predetermined period of time has elapsed from the first stirring. Here, when a reaction time set in advance for each reagent or specimen has elapsed, it can be determined that the reaction has ended. When the reaction has not ended, the process proceeds to step S6.
After the magnetic particle solution is dispensed and the first stirring is performed, the liquid mixture is allowed to stand at, for example, 37° C. for 9 minutes, so that the magnetic particles, the measurement target component, and the label react with and bind to one another. However, depending on a measurement target and the reagent, an additional reaction time of a longer time, for example, 9 minutes, 18 minutes, 27 minutes, or 36 minutes may be required in order to perform measurement with high sensitivity. When a long time is required for the reaction, fine particles having a large specific gravity such as the magnetic particles settle in the reaction vessel 34, and thus, there is a possibility that reactivity with the measurement target component present in the reaction liquid decreases, and variations in measurement result occur. Therefore, when a long time is required for the reaction, it is required to stir the reaction liquid every predetermined period of time, for example, every 9 minutes. Each stirring performed for the predetermined period of time is as in the following step S6.
In step S6, the control device 108 drives the dispensing mechanism 106 to aspirate, discharge, and stir the liquid mixture in a state in which the magnetic particles are precipitated. The stirring performed after the precipitation of the magnetic particles is referred to as a second stirring. Specific conditions of the second stirring will be described later. When the second stirring is performed a plurality of times, the stirring can be performed under the same conditions each time.
When it is determined in step S5 that the reaction has ended, in step S7, the control device 108 drives the transport device 112 to transport the reaction vessel 34 to the detection unit 107. The detection unit 107 measures the measurement target component in the reaction vessel 34. At this time, the magnetic particles integrated with the measurement target component and the label in the reaction vessel 34 are captured by a magnet in the detection unit 107. Thereafter, when a voltage is applied, an amount of light emitted by an electrochemical method is detected.
Depending on an analysis item, the specimen and a first reagent may be dispensed in the first dispensing, and a second reagent and the magnetic particle solution may be dispensed in the second dispensing. The specimen, the reagent, and the magnetic particle solution may be dispensed at one time.
As illustrated in
Next, as illustrated in
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Next, as illustrated in
As described above, by performing stirring immediately after the magnetic particles 33 are dispensed and after the magnetic particles 33 settle, it is possible to improve the reactivity of the measurement target component dispersed in the solution and the magnetic particles 33. As a result, the variations in measurement result can be reduced, and thus analysis accuracy can be improved.
As described above, the first stirring operation and the second stirring operation are the same in terms of aspirating and discharging the reaction liquid 35 in the reaction vessel 34, but in the second stirring, the settled magnetic particles 33 are to be stirred, and thus, under the same conditions as the first stirring, it is difficult to disperse the magnetic particles 33 settled at the bottom of the reaction vessel 34. Therefore, by setting the conditions of the second stirring to appropriate conditions different from the conditions of the first stirring, it is possible to provide sufficient stirring efficiency to the settled magnetic particles 33.
Specifically, by setting the discharge rate VD2 in the second stirring faster than the discharge rate VD1 in the first stirring, the settled magnetic particles 33 can be dispersed with high stirring efficiency.
The settled magnetic particles 33 can also be dispersed by setting the discharge position PD2 in the second stirring lower than the discharge position PD1 in the first stirring, that is, at a position closer to the bottom of the reaction vessel 34.
The settled magnetic particles 33 can also be dispersed by setting the aspiration rate VS2 in the second stirring slower than the aspiration rate Vs1 in the first stirring.
The aspiration amount AS2 of the reaction liquid 35 into the dispensing tip 32 in the second stirring can be set to an amount smaller than a total amount of the reaction liquid 35, and specifically, for example, can be set to 95% or less of the total amount of the reaction liquid 35. This is because when the aspiration amount AS2 exceeds the total amount of the reaction liquid 35, air bubbles are also aspirated, and air bubbles are mixed after the discharge, which may result in unstable stirring.
Hereinafter, more specific conditions of the second stirring will be described. The present inventors have studied the conditions of the second stirring capable of providing sufficient stirring efficiency to the magnetic particles settled in the reaction vessel by using a simulator.
Parameters set in this simulation were defined as the aspiration amount, the aspiration rate, the discharge rate, and the discharge position (distance between the tip end of the dispensing tip and the bottom of the reaction vessel at the start of discharge). A diameter of the magnetic particle was set to 2.8 µm, a specific gravity was set to 1.4, and a viscosity of a solvent was set to 0.89 mPa·s. The total amount of the reaction liquid was set to 200 µL. A tip end diameter of the dispensing tip was set to 0.4 mm, and an inner volume was set to 368 µL.
The amount of the stirring liquid of the first stirring was set to 80 µL, whereas the amount of the stirring liquid of the second stirring was set to 95 µL, 140 µL, or 190 µL.
The aspiration rate of the first stirring was set to 200 uL/s, whereas the aspiration rate VS2 of the second stirring was set to 125, 190, or 250 µL/s.
The discharge rate of the first stirring was set to 125 µL/s, whereas the discharge rate VD2 of the second stirring was set to 100, 200, or 300 µL/s.
The discharge position of the first stirring was set to 2.8 mm, whereas the discharge position of the second stirring was set to 0.8 mm, 3.2 mm, or 5.6 mm. In addition, a condition in which the position of the tip end of the dispensing tip at an end of the aspiration of the second stirring was 5.6 mm and the discharge position at the start of discharge was 0.8 mm was also added.
The above parameters were combined to set the conditions of the second stirring from Case 1 to Case 13, and the simulation was performed. As an index indicating the degree of dispersion of the magnetic particles after the second stirring, a standard deviation of a particle density of each layer in the reaction vessel (a region divided into 0 to 2 mm, 2 to 4 mm, 4 to 6 mm, 6 to 8 mm, 8 to 10 mm, and 10 to 11 mm from the bottom of the reaction vessel) was used. For example, when a particle density of a lower layer is high and a particle density of an upper layer is low in the reaction vessel, a particle distribution is biased to the lower layer and the degree of dispersion is low. On the other hand, when the particle density of the lower layer and the particle density of the upper layer in the reaction vessel are equal to each other, it can be determined that the magnetic particles are uniformly dispersed in the entire reaction vessel. Therefore, it can be said that the lower the standard deviation of the particle density of each layer, the more uniform the particle density in the entire reaction vessel, and the higher the degree of dispersion.
Next, based on the results of
First, a relationship between the discharge rate and the degree of dispersion was examined by comparing Cases 1, 4, and 8.
When the discharge rate is increased in the first stirring, the reaction liquid once aspirated into the dispensing tip is likely to remain in the dispensing tip as a liquid film. That is, the magnetic particles tend to remain together with the liquid film in the dispensing tip. As long as there is no purpose of dispersing the settled magnetic particles, the remaining of the magnetic particles can be prevented by slowing down the discharge rate in the first stirring. Therefore, with regard to the discharge rate, by setting the discharge rate of the second stirring to be faster than the discharge rate (126 µL/s) of the first stirring, for example, 200 µL/s to 300 µL/s, it is possible to more uniformly disperse the magnetic particles in the entire reaction liquid in the reaction vessel 34. It is also possible to set the discharge rate of the second stirring faster than 300 µL/s, but when the discharge rate is too fast, the magnetic particles may easily remain in the dispensing tip, and thus, the discharge rate is adjusted in accordance with the diameter of the dispensing tip, the amount of the reaction liquid, and the like. Of course, it is also possible to set the discharge rate of the second stirring slower than 200 µL/s under the condition that the discharge rate of the second stirring is faster than the discharge rate of the first stirring.
Next, a relationship between the discharge position and the degree of dispersion was examined by comparing Cases 4, 5, and 9.
Therefore, by setting the discharge position of the second stirring to a position lower than the discharge position of the first stirring, it is possible to uniformly disperse the magnetic particles in the entire reaction liquid in the reaction vessel. Specifically, when the dimensions of the dispensing tip or the magnetic particles described above are adopted, the distance between the tip end of the dispensing tip and the bottom of the reaction vessel can be set to less than 2.8 mm, and more specifically, can be set to 0.8 mm. Further, the magnetic particles can be dispersed more uniformly by lowering the discharge position as much as possible within a range in which the tip end of the dispensing tip does not come into contact with the settled magnetic particles in accordance with the amount of the magnetic particles.
Next, a relationship between the stirring liquid (aspiration liquid) and the degree of dispersion was examined by comparing Cases 4, 10, and 11.
As compared with Case 4, it can be seen that in Case 11 in which the aspiration liquid is more, the standard deviation of the particle density is smaller, and the dispersibility is better. However, in Case 11, since most of the reaction liquid is aspirated, the reagent containing a larger amount of magnetic particles is aspirated into the dispensing tip, and the amount of magnetic particles remaining in the dispensing tip may increase. Here, even when the aspiration amount of Case 4 is 95 µL which is close to 80 µL of the aspiration amount of the first stirring, since the magnetic particles are dispersed in the entire reaction vessel as illustrated in
First, a relationship between the aspiration rate and the degree of dispersion was examined by comparing Cases 4, 12, and 13.
It can be seen that even when the aspiration rates in Cases 12 and 13 are made faster than the aspiration rate in Case 4, the dispersibility is not improved as compared with Case 4 in which the aspiration rate is low. In addition, when the aspiration rate is increased, the settled magnetic particles may be aspirated into the dispensing tip, and the amount of the magnetic particles remaining without being discharged from the dispensing tip may increase. Therefore, in order to avoid the aspiration of the magnetic particles, the aspiration rate of the second stirring can be made slower than the aspiration rate of the first stirring.
As described above, the automatic analyzer 100 according to the first embodiment uses the dispensing probe that dispenses the specimen and the reagent to perform the first stirring immediately after mixing the magnetic particles (fine particles) and the second stirring after the magnetic particles precipitate after the predetermined period of time has elapsed from the first stirring. As described above, since the reaction liquid in which the magnetic particles are precipitated can be stirred without using a dedicated stirring mechanism, space saving and cost reduction of the device can be achieved. In addition, since the reaction of the magnetic particles, the specimen, and the reagent can be advanced by performing the second stirring, it is possible to reduce the variations in measurement result, and it is possible to improve the analysis accuracy of the specimen.
Further, by setting the conditions of the first stirring to be different from the conditions of the second stirring, the dispersibility of the magnetic particles can be improved, and thus the variations in measurement result can be further reduced.
In the first embodiment, the method of stirring the reaction liquid using the dispensing mechanism including the dispensing probe and the dispensing tip has been described. On the other hand, in the second embodiment, a stirring method in a case of adopting a dispensing mechanism configured to directly aspirate a solution to a dispensing probe without using a dispensing tip is proposed.
The other operations are the same as those of the first embodiment, and thus the description thereof will be omitted. The conditions of the first stirring and the conditions of the second stirring in the present embodiment are also the same as those in the first embodiment.
As described above, in the second embodiment, the reaction liquid 35 containing the magnetic particles 33 is stirred using the dispensing probe 81. As a result, a space for accommodating and discarding the dispensing tip is not required, and thus can further reduce a size of the device as compared with the first embodiment.
In a third embodiment, an analysis method including B/F separation (a step of separating Bound specifically adsorbed to magnetic particles by an antigen-antibody reaction or the like and nonspecifically physically adsorbed Free) will be described.
An analysis method according to the present embodiment is substantially the same as that of the first embodiment, but the operation after the first stirring is different in the following points.
Next, as illustrated in
Next, as illustrated in
Next, as illustrated in
As described above, in the third embodiment, the magnetic particles 33 captured by the magnetic separation device 114 performing the B/F separation can be resuspended by the second stirring.
The present disclosure is not limited to the above embodiments, and includes various modifications. For example, the above embodiments have been described in detail for easy understanding of the present disclosure, and are not necessarily limited to those including all the configurations described above. Further, a part of the configurations in one embodiment can be replaced with a configuration in another configuration. The configuration of another embodiment may be added to the configuration of one embodiment. Further, a part of the configuration of another embodiment may be added to, deleted from, or replaced with a part of the configuration of each embodiment.
31, 81:
32:
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35:
91:
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100, 200:
101:
102:
103:
104:
105:
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107:
108:
109:
110:
111:
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114:
| Number | Date | Country | Kind |
|---|---|---|---|
| 2020-107593 | Jun 2020 | JP | national |
| Filing Document | Filing Date | Country | Kind |
|---|---|---|---|
| PCT/JP2021/004556 | 2/8/2021 | WO |
