The present invention relates to an automatic analyzer that qualitatively and quantitatively analyzes biological samples such as serum and urine.
In a biochemical analysis or immunoassay, an automatic analyzer is often used to examine samples (e.g., blood, urine, or other biological samples to which reagents are often added).
To analyze samples, a biochemical analysis examines color reactions between substrates and enzymes while an immunoassay examines agglutination reactions between antigens and antibodies. To examine such color reactions and agglutination reactions, an automatic analyzer causes a light source to emit light onto a reaction vessel containing a sample-reagent mix and then measures the intensities of transmissive light through and/or scattered light from the reaction vessel.
An example of an automatic analyzer that measures scattered light intensity is the one disclosed in Patent Document 1. In this analyzer, two integrating spheres are disposed in front of and behind a reaction vessel with respect to the direction of light radiated onto the vessel. The analyzer calculates the average of the intensities of light scattered forward and light scattered backward, thereby correcting turbidity changes attributed to cell displacement. Also, Patent Documents 2 and 3 each disclose an automatic analyzer that uses a diaphragm to separate incident light into transmissive light and scattered light, thereby simultaneously measuring the absorbance and scattered light.
Patent Document 1: JP-1998-332582-A
Patent Document 2: JP-2001-141654-A
Patent Document 3: JP-2008-8794-A
In a conventional method of detecting the concentration of a substance in a sample, light is radiated onto the sample mixed with a reagent, and the intensity of the transmissive light that has passed through the sample-reagent mix is measured and converted into the concentration of the substance (the absorbance method). In another conventional method, the scattered light generated from the sample is instead measured and converted into the concentration of the substance. When either of the two methods is employed, the measured intensity of the light radiated onto the sample and the measured intensity of the transmissive light or scattered light need to fall within a given range. In the absorbance method, the intensity of the light source and the sensitivity of the transmissive-light receiver are corrected based on the assumption that the intensity of the light source is equal to the intensity of transmissive light passing through water (zero absorbance) contained within a reaction vessel. Thus, the absorbance method allows simultaneous examination of the light intensity of the light source and baseline transmissive-light intensity.
The latter method of using scattered light, however, has drawbacks. When a reaction vessel contains a substance with no scatterers, scattered light intensity is ideally measured to be zero. However, a small amount of scattered light is often detected because the reaction vessel scatters a small amount of incident light. In addition, because scattered light intensity is strongly proportional to incident light intensity, baseline scattered-light intensity cannot be determined unless the incident light intensity is not accurately determined. Thus, the method of using scattered light involves difficulty in examining the baseline scattered-light intensity, which in turn causes analysis results to vary from analyzer to analyzer.
The present invention has been contrived to address the above issues, and an object of the invention is to provide an automatic analyzer capable of correcting the intensity of light incident on a reaction vessel even when an analysis involves the use of scattered light and also capable of preventing analysis results obtained by the analyzer from differing from those obtained by another analyzer due to inaccurate measurement of the incident light.
To solve the above problems, an automatic analyzer according to the invention comprises: a light source for radiating light onto a reaction vessel in which a sample is caused to react with a reagent; a transmissive-light receiver, located across from the light source with the reaction vessel placed therebetween, for measuring the intensity of transmissive light passing through the reaction vessel; at least one scattered-light receiver, located on the side of the transmissive-light receiver, for measuring the intensity of light scattered from the reaction vessel; and a light-intensity correcting mechanism for correcting the intensity of the light radiated from the light source based on measurement results obtained by the transmissive-light receiver.
In accordance with the present invention, the intensity of light incident on a reaction vessel can be corrected even when an analysis involves the use of scattered light, and analysis results obtained by the analyzer are prevented from differing from those obtained by another analyzer due to inaccurate measurement of the incident light.
An embodiment of the present invention will now be described with reference to the accompanying drawings.
As illustrated in
Arranged along the circumference of the sample disk 5 are multiple sample vessels 6 each containing a sample (e.g., a biological sample such as serum and urine). A rotating mechanism (not illustrated) allows the sample disk 1 to rotate laterally and stop at a particular position.
The first reagent disk 13A and the second reagent disk 13B are housed within reagent refrigerators 9A and 9B, respectively. Arranged and fixed along the circumferences of the reagents disks 13A and 13B are multiple reagent bottles 10A and 10B, respectively, which are used for particular analyses. With rotating mechanisms not illustrated, the first reagent disk 13A and the second reagent disk 13B are allowed to rotate laterally and stop at particular positions. Reading devices 34A and 34B are also disposed adjacent to the first reagent disk 13A and the second reagent disk 13B so that the reagent IDs of the reagent bottles 10A and 10B can be read. Reagent IDs read and their associated bottle positions on the reagent disks 13A and 13B are transmitted through an interface 19 to the computer 18 and then stored on a memory 11. Reagent IDs can take the form of barcodes; in that case, the reading devices 34A and 34B are barcode readers. It should be noted that a first standard reagent and a second standard reagent are placed on the reagent disks 13A and 13B, respectively. These standard reagents are used to perform correction on the measurement unit 40 (discussed later).
The reaction disk 1 is housed within a thermostat tank 3 that is temperature-controlled by a thermostat 4 (the temperature within the thermostat tank 3 is maintained at 37 degrees Celsius, for example). Arranged and fixed along the circumference of the reaction disk 1 are multiple reaction vessels 2 in which to mix a sample and a reagent. A rotating mechanism (not illustrated) allows the reaction disk 1 to rotate laterally and stop at particular positions. The rotation of the reaction disk 1 causes a reaction vessel 2 to move to sample and reagent dispensing positions. At the sample dispensing position, the sample dispenser 7 dispenses a sample into the reaction vessel 2, and at one of the reagent dispensing positions of the first and second reagent disks 13A and 13B, the reagent dispenser 12A or 12B dispenses the reagent required for a particular analysis into the reaction vessel 2. The sample and reagent dispensation is followed by the stirring of the sample-reagent mix by a stirring mechanism 33A or 33B. The operation of the sample dispenser 7 is controlled by a sample dispensation controller 20 while the operation of the reagent dispensers 12A and 12B is controlled by a reagent dispensation controller 21.
The measurement unit 40 is located adjacent to the reaction disk 1 and designed to perform measurement on the sample-reagent mix contained within any reaction vessel 2. As discussed later in detail, the measurement unit 40 includes a light source 14 for radiating light onto a reaction vessel 2 (e.g., a LED: Light Emitting Diode) and a photometric instrument 15 for detecting the transmissive light through and the scattered light from the reaction vessel 2. Measurement is performed on the reaction vessel 2 while the rotation of the reaction disk 1 causes it to traverse the area located between the light source 14 and the photometric instrument 15. The measurement results obtained by the photometric instrument 15 (i.e., analog signals) are converted by an A/D converter 16 into digital signals, which are then transmitted to the computer 18 through the interface 19.
Reaction vessels 2 that have been subjected to measurement are cleaned at the rinse position with the use of a rinse mechanism 17.
The analyzer further includes a keyboard 24, a CRT display 25, a printer 22, and a storage medium drive 23 for recording data on FDs or other external storage media. These devices and the memory 11 are connected to the computer 18 and other functional units through the interface 19. The memory 11 is a data storage device such as a hard disk and used to store analysis results, operator passwords, display settings, analysis parameters, information on requested analysis, calibration results, and so forth.
Next described is the measurement performed by the analyzer of the present embodiment.
As shown in
The transmissive-light receiver 15A is disposed on the axis of the light emitted from the light source 14 to the reaction vessel 2 and detects the transmissive light 14a that passes through the reaction vessel 2 along the light axis. The scattered-light receiver 15B is disposed at a predetermined angle Al with respect to the light axis, with the vertex lying within the reaction vessel 2, and detects the scattered light 14b generated from the reaction vessel 2.
While the light source 14 is meant to be an LED (i.e., a single-wavelength light source), it can instead be a multi-wavelength light source that is capable of changing the wavelength of light. In that case, a multi-wavelength photometer is used as the transmissive-light receiver 15A.
Further, while
By the thus-configured measurement unit 40 measuring the intensities of the transmissive light and the scattered light, the concentration of scatterers in the substance 102 (a sample-reagent mix) within the reaction vessel 2 can be measured.
(2) Principles of Calculating the Concentration of Scatterers
We now describe how to calculate the concentration of scatterers in the substance 102 based on the intensities of transmissive light and scattered light measured by the measurement unit 40. In the present embodiment, those light intensities are converted into concentration data based on calibration curves. Such calibration curves are created in advance according to particular analysis methods.
The following should also be noted. In
As illustrated in the area 50A of
In the measurement according to the present embodiment, the intensity of transmissive light is calculated from the detection results obtained by the transmissive-light receiver 15A, and the intensity of scattered light is calculated from the detection results obtained by the scattered-light receivers 15B and 15C. These intensities of transmissive light and scattered light are then used to calculate the concentration of scatterers based on the relationships illustrated in
(3) Correction (Correction of the Light Intensity of the Light Source and Correction of the Sensitivity of the Light Receivers)
Discussed next is the correction performed by the analyzer of the present embodiment. The correction refers to the act of correcting the light intensity of the light source 14 of the measurement unit 40 and the sensitivity of the transmissive-light receiver 15A and the scattered-light receivers 15B and 15C before the start of an analysis.
The reagent dispenser 12A or 12B first dispenses the first standard reagent into a reaction vessel 2 as instructed by the computer 18 for controlling whole operations (Step S410). The first standard reagent is one with known transmissive and scattering properties and can be, for example, water or other substance that has less influence on light passing through it (i.e., a substance that allows the passage of light and causes less light scattering). The measurement unit 40 then measures the intensity of transmissive light passing through the first standard reagent (Step S420). The measurement result of the reagent at this time would be in an area 50A of
When the transmissive light intensity measured falls within the acceptable range in Step S430, then, the measurement unit 40 measures the intensity of scattered light generated from the first standard reagent (Step S440). The measurement result of the reagent at this time would be in an area 50A of
When the scattered light intensity measured falls within the acceptable range in Step S450, then, the reagent dispenser 12B dispenses the second standard reagent into another empty reaction vessel 2 (Step S460). The second standard reagent is also one with known transmissive and scattering properties and can be, for example, a latex solution or a solution containing other standard scatterers. The measurement unit 40 then measures the intensity of scattered light generated from the second standard reagent (Step S470). The measurement result of the reagent at this time would be in an area 50B of
It should be noted that the first and second standard reagents can be solid substances as long as their transmissive and scattering properties are known. For example, it is also possible to solidify such a substance within a reaction vessel 2 and place the solidified substance on the reaction disk 1. Alternatively, it is also possible to process such a substance into the shape of a reaction vessel 2 and place that substance on the reaction disk 1.
(4) Operation
Described next is the operation of the automatic analyzer of the present embodiment.
Analysis parameters used for particular analyses are input in advance to the analyzer through the keyboard 24 and stored on the memory 11. The operator is supposed to select the patient IDs associated with the samples to be examined and the information on the requested analyses while viewing an operation function screen.
When the operator instructs the analyzer to start analysis, correction is first performed on an as-needed basis before the analysis.
During the correction, the reagent dispenser 12A or 12B first dispenses the first standard reagent into a reaction vessel 2 as instructed by the computer 18, followed by the measurement of the intensity of transmissive light by the measurement unit 40. The light intensity of the light source 14 is then corrected so that the transmissive light intensity measured falls within an acceptable range (Steps S410 through S431 of
During analyses, the sample dispenser 7 first dispenses samples from sample vessels 6 to reaction vessels 2 as needed for the analyses, and the reagent dispensers 12A and 12B then dispense the required reagents into the reaction vessels 2. Thereafter, the sample-reagent mixes within the reaction vessels 2 are stirred by the stirring mechanisms 33A and 33B. When the rotation of the reaction disk 1 causes each of the reaction vessels 2 to move past the measurement unit 40 (measurement position), the measurement unit 40 measures the intensities of transmissive light and scattered light. The measured light intensities are converted by the A/D converter 16 into digital signals, which are then transmitted to the computer 18 through the interface 19. After receiving the digital signals, the computer 18 converts them into concentration data based on the calibration curves created in advance according to particular analysis methods. The concentration data obtained is output to the printer 22 or to the CRT display 25.
(5) Advantages
Next described are the advantages of the automatic analyzer of the present embodiment.
In a conventional method of detecting the concentration of a substance in a sample, light is radiated onto the sample mixed with a reagent, and the intensity of the transmissive light that has passed through the sample-reagent mix is measured and converted into the concentration of the substance (the absorbance method). In another conventional method, the scattered light generated from the sample is instead measured and converted into the concentration of the substance. When either of the two methods is employed, the measured intensity of the light radiated onto the sample and the measured intensity of the transmissive light or scattered light need to fall within a given range. In the absorbance method, the intensity of the light source and the sensitivity of the transmissive-light receiver are corrected based on the assumption that the intensity of the light source is equal to the intensity of transmissive light passing through water (zero absorbance) contained within a reaction vessel. Thus, the absorbance method allows simultaneous examination of the light intensity of the light source and baseline transmissive-light intensity. The latter method of using scattered light, however, has drawbacks. When a reaction vessel contains a substance with no scatterers, scattered light intensity is ideally measured to be zero. However, a small amount of scattered light is often detected because the reaction vessel scatters a small amount of incident light. In addition, because scattered light intensity is strongly proportional to incident light intensity, baseline scattered-light intensity cannot be determined unless the incident light intensity is not accurately determined. Thus, the method of using scattered light involves difficulty in examining the baseline scattered-light intensity, which in turn causes analysis results to vary from analyzer to analyzer.
In contrast, the analyzer of the present embodiment comprises a light source for radiating light onto a reaction vessel in which a sample is caused to react with a reagent; a transmissive-light receiver, located across from the light source with the reaction vessel placed therebetween, for measuring the intensity of transmissive light passing through the reaction vessel; at least one scattered-light receiver, located on the side of the transmissive-light receiver, for measuring the intensity of light scattered from the reaction vessel; and light-intensity correcting means for correcting the light intensity of the light source based on measurement results obtained by the transmissive-light receiver. Thus, the above analyzer is capable of correcting the intensity of the light incident on the reaction vessel even when an analysis involves the use of scattered light. The use of such analyzers prevents analysis results from varying from analyzer to analyzer due to inaccurate measurement of the incident light.
It should also be noted that when multiple scattered-light receivers are used as in the above embodiment, the angles (θ1, θ2, etc.) of at least two of them with respect to the axis of light radiated onto a reaction vessel can be the same. In that case, when those scattered-light receivers detect different scattered light intensities, they are judged to be displaced, followed by the correction of their positions. This is possible because, in principle, scattered-light receivers disposed at the same angle are supposed to detect the same scattered-light intensity.
Number | Date | Country | Kind |
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2010-273437 | Dec 2010 | JP | national |
Filing Document | Filing Date | Country | Kind | 371c Date |
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PCT/JP2011/077525 | 11/29/2011 | WO | 00 | 7/17/2013 |