Patent Grant
11331012
The present invention relates to a non-invasive biolipid concentration measuring device, a non-invasive biolipid metabolism measuring device, a method of non-invasively measuring biolipid concentration and a method of non-invasively examining biolipid metabolism that can measure the lipid concentration and the lipid metabolism of blood in a living body in a so-called non-invasive manner without collecting blood not only in medical facilities but also at home.
In recent years, public healthcare expenditures are rising, and hence reduction of healthcare expenditures is the government's and public's great concern. The doctor's fees for diseases due to lifestyle related diseases account for one-third of the public healthcare expenditures. Under such circumstances, reduction of public health care expenditures, improvement of health expectancy, and improvement of QOL (Quality of Life) are demanded, and to meet such demands, specific medical examinations have been implemented, and a concept of “very early stages of disease” has been widely spread.
In particular, it is known that metabolic syndrome, which is a subject of screening in specific medical examinations, develops diabetes, dyslipidemia, high blood pressure caused by insulin resistance due to accumulation of visceral fat obesity, and it is expected that early detection of metabolic syndrome will lead to prevention of disease progression and improvement of QOL, and further, reduction of public health care expenditures.
Insulin resistance is important for early detection of lifestyle related diseases as described above; however, the only way of specific medical examinations has been measurement of abdominal girth for estimation of the risk of insulin resistance.
In recent years, a close relationship between insulin resistance and postprandial hyperlipidemia has been revealed, and a possibility that postprandial hyperlipidemia is the cause of insulin resistance has been pointed out, and therefore, postprandial hyperlipidemia can be recognized to be a metabolic error of an origin of metabolic syndrome. As such, postprandial hyperlipidemia is attracting attention not only as a factor for detecting an initial stage of metabolic syndrome (very early stages of diseases), but also as a risk factor of arteriosclerosis. For example, it can be said that when the triglyceride concentration in a non-fasting state is high, the risk of developing coronary heart disease is high.
However, diagnosis of postprandial hyperlipidemia requires observation of variation in lipid concentration in blood during 6 to 10 hours after eating. That is, to measure the state of hyperlipidemia after eating, it is required to hold examinees for about 6 to 10 hours to collect blood multiple times, but such an operation can be implemented only in clinical research and cannot be practically implemented in clinical sites.
In addition, with increasing public health consciousness, specified functional foods that inhibit fat absorption and the like are coming into practical use, and consciousness of dietary ingestion of fat is rising. Although the people are conscious to blood lipid, there is no health management apparatus for easily measuring blood lipid at home. One reason for this is that blood collection itself is restricted by the Medical Practitioners' Act, and even if there is no such restriction, examination apparatuses are not available in the price range for ordinary families. Furthermore, there are problems such as disposal of waste liquid, and long analysis time.
Under such circumstances, the following techniques relating to a blood component measurement method have been proposed.
For example, Japanese Patent Application Laid-Open No. 2004-251673 (PTL 1) discloses a technique relating to an apparatus that calculates the concentration of a measurement object by outputting and emitting light having a wavelength of a near-infrared region and an infrared region with an acoustic optical variable vibration filter to a living body, and by analyzing and computing an absorption spectrum obtained by receiving light that has transmitted through a measurement object or reflected by the measurement object. That is, the technique disclosed in PTL 1 is directed to calculate the amount of absorbed light and the like from the difference between the amount of emitted light and the amount of received light and the like by utilizing a phenomenon in which light is absorbed by blood component, to thereby calculate the blood component concentration from the results of the calculation.
In addition, Japanese Patent Application Laid-Open No. 2010-66280 (PTL 2) discloses a technique relating to a quantitative apparatus for analyzing glucose concentration including: a near-infrared light source; a detection means that detects near-infrared light; a guiding means that introduces near-infrared light emitted by the near-infrared light source to a biological tissue or bodily fluid and guides near-infrared light passing through or deffusely reflected by the biological tissue or the bodily fluid to the detection means; and a computing means that performs a regression analysis of the glucose concentration based on signals obtained by the detection means. The computing means carries out quantification using continuous spectrum signals obtained by continuously measuring wavelengths in at least three adjacent wavelength regions as defined below as explanatory variables, and the glucose concentration as a criterion variable; a first wavelength region is in a range of 1,550 to 1,650 nm to measure absorption derived from OH groups in a glucose molecule, a second wavelength region is in a range of 1,480 to 1,550 nm to measure absorption derived from NH groups in a biological component, and a third wavelength region is in a range of 1,650 to 1,880 nm to measure absorption derived from CH groups in the biological component, within the wavelength region from 1,480 to 1,880 nm in which harmonics of a first harmonic tone is observed, and in which the effect of water absorption is relatively small. That is, as with the technique disclosed in PTL 1, the technique disclosed in PTL 2 utilizes a phenomenon in which light is absorbed by the NH group, CH group and OH group of glucose to calculate the amount of absorbed light from the difference between the amount of emitted light and the amount of received light and the like, to thereby calculate the concentration of the blood component from the results of the calculation.
Further, Japanese Patent Application Laid-Open No. 2002-168775 (PTL 3) discloses a technique relating to a rapid measuring method of a plasma component of a mammal by spectrum information in a visual and near-infrared region, which is characterized by measuring an absorbance in the visual and near-infrared region having a wavelength of 400-2,500 nm by using a near-infrared spectrophotometer relative to separated plasma in measuring the plasma component of the mammal, calculating a primary differential and a secondary differential of the absorbance, using the absorbance, and the primary differential and the secondary differential of the absorbance in the visual and near-infrared region as independent variables, selecting independent variables to the number of two to ten having high explanation power from among the independent variables, predicting triglyceride, inorganic phosphorus, potassium, lactate dehydrogenase and an albumin-globulin ratio in the plasma from the information on the independent variables having high explanation power, and realizing measurement based on the predicted values. That is, as with the techniques of PTL 1 and PTL 2, the technique of PTL 3 utilizes a phenomenon in which plasma absorbs visible light having wavelengths of 400-2500 nm and light of a near-infrared region to calculate the triglyceride concentration and the like in plasma from the difference between the amount of emitted light and the amount of received light and the like.
PTL 1
Japanese Patent Application Laid-Open No. 2004-251673
PTL 2
Japanese Patent Application Laid-Open No. 2010-66280
PTL 3
Japanese Patent Application Laid-Open No. 2002-168775
However, while the techniques disclosed in PTLS 1 to 3 are based on a phenomenon in which light is absorbed by a certain blood component and require elimination of scattering of light, the researches so far show that the influence of absorption is about 1/10 of the influence of scattering, that is, the influence of scattering is about 10 times the influence of absorption, and therefore it is very difficult to eliminate the influence of scattering. In addition, while it is not necessary to eliminate the influence of scattering when the scattering is constant, it is difficult to determine whether the actually measured light intensity has been influenced by absorption or scattering, and the length of the light path also has an influence, thus making it difficult to achieve measurement. In particular, in the case of non-invasive measurement, the influence of absorption by other substances such as cells has to be taken into consideration, and therefore it is practically impossible to achieve non-invasive measurement using the techniques disclosed in PTLS 1 to 3. In addition, the apparatus based on PTLS 1 to 3 has a large size, and is expensive, and therefore, such an apparatus cannot be practically easily used at home. Further, when the distance between the irradiation position and the detection position is increased, the length of the light path is increased, and consequently the light energy may possibly be completely absorbed without being output to the outside in absorption measurement.
In addition, in the technique disclosed in PTL 1, the wavelength range within which light is easily absorbed by lipid, sugar and the like, and the wavelength range within which light is easily absorbed by water and electrolyte of blood overlap each other, and when light of the overlapped wavelength range is used, the influence of light absorption by lipid, sugar and the like is hidden by the influence of light absorption by water and electrolyte, and consequently the amount of light absorbed by lipid, sugar and the like may not possibly be correctly measured.
Further, in the technique disclosed in PTL 2, the glucose concentration in blood is quantified based on a phenomenon in which emitted light is absorbed by a hydrophilic group such as OH group, NH group and CH group of glucose, and therefore the measurement object is disadvantageously limited. In other words, the blood lipid concentration cannot be measured. To be more specific, blood lipid has high hydrophobicity, and has a spherical structure covered by phospholipid and the like. One reason for this is that cholesterol ester and triglyceride in blood have hydrophobicity and poor affinity to water, and exhibit poor solubility to water, thus presenting as scattering members forming micelle covered with amphiphilic phospholipid. In addition, while the triglyceride measured in common medical examinations and diagnoses of disease is triglyceride and the total cholesterol is the sum of cholesterol, cholesterol ester, free cholesterol and the like, it is said that cholesterol ester is important in terms of the risk of arteriosclerosis. As described, since the lipid component that is an important measurement object presents in the center of micelle because of its high hydrophobicity, and the micelle surface has a light reflecting property, it is difficult to measure the concentration of the substance based on absorption. In addition, in the technique disclosed in PTL 2, the concentration is calculated by regression analysis of obtained light absorbance, and therefore cannot be measured in real time.
Furthermore, in the technique disclosed in PTL 3, the measurement object is obtained by collecting blood and then separating plasma from blood, and therefore, the technique disclosed in PTL 3 is not directed to a non-invasive measurement. That is, a triglyceride concentration and the like can be detected only when disturbances such as a living body and other blood components are removed, that is, when a state where the influence of scattering is removed is established. As such, unlike the present invention, in PTL 3 contains no solution for difficulty in non-invasive detection of the triglyceride concentration in blood.
In addition, while a dynamic light scattering method and a static light scattering method are available as techniques for measuring a blood component based on light scattering, the methods are directed to measure the size of blood component, not to calculate concentration. In addition, the dynamic light scattering method is a method for measuring Brownian motion to calculate particle diameter distribution, and the measurement object is required to be statically placed, and therefore it is difficult to measure a dynamic object such as blood flow. Required measurement time is about 30 minutes to one hour per sample. Meanwhile, the static light scattering method is a method for calculating the molecular weight in the case where the component is a single component and the concentration is determined, and the static light scattering method is intended for measurement of particles having a size greater than that can be measured by the dynamic light scattering method, and movement of molecules during analysis is not assumed. Therefore, also in the static light scattering method, the measurement object is required to be statically placed, and therefore it is difficult to measure a dynamic object such as blood flow.
To solve the above-mentioned problems, an object of the present invention is to provide a non-invasive biolipid concentration measuring device, a non-invasive biolipid metabolism measuring device, a method of non-invasively measuring biolipid concentration and a method of non-invasively examining biolipid metabolism which do not require blood collection and allow measurement of blood lipid not only in medical facilities but also at home, and moreover, which achieves instant data acquisition and time-series measurement of blood lipid and can be applied to examination of metabolic errors such as postprandial hyperlipidemia.
A non-invasive biolipid concentration measuring device according to an embodiment of the present invention is configured to non-invasively measure a blood lipid concentration in a living body, the non-invasive biolipid concentration measuring device including:
an irradiator configured to emit light having a given light intensity toward an inside of the living body from an outside;
a light intensity detector disposed at a position separated by a given distance from an irradiation position to which light is emitted by the irradiator, the light intensity detector being configured to detect a light intensity of light emitted from the living body;
a scattering coefficient calculator configured to calculate a light scattering coefficient in the living body based on the light intensity detected by the light intensity detector; and
a lipid concentration calculator configured to calculate a lipid concentration in the living body based on the light scattering coefficient calculated by the scattering coefficient calculator.
Preferably, in the non-invasive biolipid concentration measuring device and the method of non-invasively measuring a biolipid concentration according to the embodiment of the present invention,
the irradiation position and a detection position at which the light intensity is detected are separated by a given irradiation-detection distance, and
a light intensity of light emitted by rearward scattering light scattered by blood lipid in the living body is detected by the light intensity detector detects, or determined by the detection.
Preferably, in the non-invasive biolipid concentration measuring device and the method of non-invasively measuring a biolipid concentration according to the embodiment of the present invention,
the irradiation position and a detection position at which the light intensity is detected are separated by a given irradiation-detection distance, and
the light intensity detector detects a light intensity of light emitted by rearward scattering light scattered by blood lipid in the living body, or a light intensity of light emitted by rearward scattering light scattered by blood lipid in the living body is determined by the detection.
Preferably, in the non-invasive biolipid concentration measuring device and the method of non-invasively measuring a biolipid concentration according to the embodiment of the present invention, the scattering coefficient calculator calculates a light scattering coefficient in the living body based on a ratio of a detected light intensity to an irradiation-detection distance between the irradiation position and a detection position at which the light intensity is detected, or a light scattering coefficient in the living body is determined by the calculation based on a ratio of a detected light intensity to an irradiation-detection distance between the irradiation position and a detection position at which the light intensity is detected.
Preferably, in the non-invasive biolipid concentration measuring device and the method of non-invasively measuring a biolipid concentration according to the embodiment of the present invention, the scattering coefficient calculator calculates a light scattering coefficient in the living body based on a ratio of a detected light intensity to an irradiation-detection distance between the irradiation position and a detection position at which the light intensity is detected, or a light scattering coefficient in the living body is determined by the calculation based on a ratio of a detected light intensity to an irradiation-detection distance between the irradiation position and a detection position at which the light intensity is detected.
Preferably, in the non-invasive biolipid concentration measuring device and the method of non-invasively measuring a biolipid concentration according to the embodiment of the present invention,
the irradiator emits consecutive light, or consecutive light is emitted toward the inside of the living body from the outside during the emission, or consecutive light is emitted toward the inside of the living body from the outside during the emission; and
the scattering coefficient calculator calculates scattering coefficient μs′ by applying light intensity R (ρ) detected by the light intensity detector and the irradiation-detection distance ρ into Expression (1) and Expression (2), or scattering coefficient μs′ is determined by the calculation by applying light intensity R (ρ) determined by the detection and the irradiation-detection distance ρ into Expression (1) and Expression (2)
where μa represents an absorption coefficient, μeff an effective attenuation coefficient, and S0 a light intensity of light emitted by the irradiator.
Preferably, in the non-invasive biolipid concentration measuring device and the method of non-invasively measuring a biolipid concentration according to the embodiment of the present invention,
the irradiator emits consecutive light, or consecutive light is emitted toward the inside of the living body from the outside during the emission;
light intensities at respective detection positions of a plurality of the light intensity detectors are detected by the light intensity detectors, the light intensity detectors being disposed around an irradiation position at respective positions separated by respective different distances from the irradiation position, the irradiation position being a position to which consecutive light is emitted by the irradiator, or light intensities at respective detection positions are detected, the detection positions being disposed around an irradiation position at respective positions separated by respective different distances from the irradiation position, the irradiation position being a position to which consecutive light is emitted during the emission; and
the scattering coefficient calculator calculates a light scattering coefficient in the living body based on a ratio and/or a difference of light intensities detected by the light intensity detectors, or a light scattering coefficient in the living body is determined by the calculation based on a ratio and/or a difference of the light intensities determined by the detection.
Preferably, in the non-invasive biolipid concentration measuring device and the method of non-invasively measuring a biolipid concentration according to the embodiment of the present invention,
the irradiator emits consecutive light, or consecutive light is emitted toward the inside of the living body from the outside during the emission;
a first light intensity detector and a second light intensity detector are arranged in order around an irradiation position at respective positions separated from the irradiation position by respective different distances, the irradiation position being a position to which consecutive light is emitted by the irradiator, or the light intensity is detected at a first detection position and a second detection position disposed around an irradiation position at respective positions separated from the irradiation position by respective different distances, the irradiation position being a position to which consecutive light is emitted during the emission; and
the scattering coefficient calculator calculates scattering coefficient μs′ by applying into Expression (3) first irradiation-detection distance ρ1 between the irradiation position and a first detection position of the first light intensity detector, second irradiation-detection distance ρ2 between the irradiation position and a second detection position of the second light intensity detector, first light intensity R (ρ1) detected by the first light intensity detector, and second light intensity R (ρ2) detected by the second light intensity detector, or scattering coefficient μs′ is determined by the calculation by applying into Expression (3) first irradiation-detection distance ρ1 between the irradiation position and the first detection position, second irradiation-detection distance ρ2 between the irradiation position and the second detection position, first light intensity R (ρ1) detected at the first detection position, and second light intensity R (ρ2) detected at the second detection position.
Preferably, in the non-invasive biolipid concentration measuring device and the method of non-invasively measuring a biolipid concentration according to the embodiment of the present invention,
the irradiator emits pulsed light, or pulsed light is emitted toward the inside of the living body from the outside during the emission;
the light intensity detector detects the light intensity at specified time intervals, or the light intensities at specified time intervals are determined by the detection; and
the scattering coefficient calculator calculates a light scattering coefficient in the living body based on a length of a period until the light intensity detected by the light intensity detector is attenuated to a given intensity after pulsed light is emitted by the irradiator, or a light scattering coefficient in the living body is determined by the calculation based on a length of a period until the light intensity determined by the detection is attenuated to a given intensity after pulsed light is emitted.
Preferably, in the non-invasive biolipid concentration measuring device and the method of non-invasively measuring a biolipid concentration according to the embodiment of the present invention,
the irradiator emits pulsed light, or pulsed light is emitted toward the inside of the living body from the outside during the emission;
the light intensity detector detects the light intensity at specified time intervals, or the light intensities at specified time intervals are determined by the detection; and
the scattering coefficient calculator calculates a light scattering coefficient in the living body based on a length of a period until the light intensity detected by the light intensity detector reaches a highest value after pulsed light is emitted by the irradiator, or a light scattering coefficient in the living body is determined by the calculation based on a length of a period until the light intensity determined by the detection reaches a highest value after pulsed light is emitted.
Preferably, in the non-invasive biolipid concentration measuring device and the method of non-invasively measuring a biolipid concentration according to the embodiment of the present invention,
light obtained by modulating an intensity or a phase of light emitted by the irradiator is emitted, or light obtained by modulating an intensity or a phase of light emitted during the emission is emitted;
the light intensity detector detects the light intensity at specified time intervals, or the light intensities at specified time intervals are determined by the detection; and
the scattering coefficient calculator calculates a light density waveform based on a time variation of the light intensity detected by the light intensity detector, and calculates a scattering coefficient and an absorption coefficient of the blood based on the light density waveform, or, during the calculation, a light density waveform is determined based on a time variation of the light intensity determined by the detection, and a scattering coefficient and an absorption coefficient of the blood are determined based on the light density waveform.
A non-invasive biolipid metabolism measuring device according to the embodiment of the present invention is configured to measure biolipid metabolism from a time variation of a scattering coefficient and/or a lipid concentration calculated by the non-invasive biolipid concentration measuring device.
A method of non-invasively examining biolipid metabolism according to the embodiment of the present invention includes: acquiring a time variation of a scattering coefficient and/or a lipid concentration calculated by the non-invasive biolipid concentration measuring device to examine biolipid metabolism.
According to the present invention, since blood collection is not required, blood lipid can be measured not only in medical facilities but also at home, and moreover, since instant data acquisition is achieved and blood lipid can be measured in a temporally continuous manner, the present invention can be applied to examination of metabolic errors such as postprandial hyperlipidemia.
In the following, a non-invasive biolipid concentration measuring device, a non-invasive biolipid metabolism measuring device, a method of non-invasively measuring biolipid concentration and a method of non-invasively examining biolipid metabolism according to an embodiment of the present invention are described with reference to the drawings.
As illustrated in
In the following, the components are described in detail.
As illustrated in
In addition, the wavelength range within which light is absorbed by inorganic substances of plasma is, mainly, a range within which light absorption by inorganic substances of plasma is significant, and is a range as shown in
That is, as shown in
In this manner, by setting the wavelength range of light source 22 to the above-mentioned range, the influence of light absorption by inorganic substances of plasma and the influence of light absorption by cell components of blood are limited in light detected by light intensity detector 3 described later. With this configuration, absorption that specifies substances does not occur and the loss of light energy due to absorption is negligibly small, and thus light in blood is propagated to a distant position by scattering by blood lipid and emitted to the outside of the body.
In addition, in irradiator 2 of the present embodiment, in accordance with the method of calculating scattering coefficient μs′ of scattering coefficient calculator 4 described later, the time length of consecutive light emission, pulsed light emission and the like can be arbitrarily adjusted, and the intensity or phase of light to be emitted can be arbitrarily modulated.
Alternatively, in irradiator 2, light source 22 that uses fixed wavelength, or light source 22 that uses multiple wavelengths together may be adopted.
Light intensity detector 3 is configured to receive light to detect the intensity of the light. Light intensity detector 3 can receive light emitted to the outside from a living body, and detect the intensity of the light. In addition, in the case where a plurality of light intensity detectors 3 are employed, light intensity detectors 3 are disposed around irradiation position 21 with different distances therebetween. In the present embodiment, as illustrated in
In addition, the distance from irradiation position 21 to detection position 33 is defined as irradiation-detection distance ρ. In the present embodiment, as illustrated in
As illustrated in
In addition, “blood lipid,” which is a measurement object, has a spherical structure covered with apoprotein or the like as illustrated in
It is to be noted that in the case where a plurality of detection positions 33 are provided, the layout of detection positions 33 is not limited to the linear form as long as detection positions 33 are disposed around irradiation position 21 with different distances therebetween, and the layout may be appropriately selected from various forms such as a circular form, a wave form, and a zigzag form. In addition, first irradiation-detection distance ρ1 and second irradiation-detection distance ρ2 between irradiation position 21 and detection position 33, and the distance between detection positions 331 and 332 are not limited to constant distances, and may be appropriately selected.
Scattering coefficient calculator 4 is configured to calculate light scattering coefficient μs′ in a living body based on the light intensity detected by light intensity detector 3. The light intensity detected by light intensity detector 3 is influenced by light scattering of blood lipid as described above, and this feature is utilized to calculate scattering coefficient μs′. It is to be noted that scattering coefficient μs′ in the present embodiment is not limited to a coefficient obtained by digitizing the efficiency of a typical scattering process, and scattering coefficient μs′ in the present embodiment includes a coefficient obtained by digitizing the influence of scattering under a constant condition in consideration of a scattering phenomenon. Details are described below.
As illustrated in
Light intensity/distance calculation unit 41 is configured to calculate scattering coefficient μs′ based on a ratio of the light intensity detected at detection position 33 to irradiation-detection distance ρ between irradiation position 21 and detection position 33. That is, scattering coefficient μs′ is calculated based on a scattering phenomenon in which emitted light is attenuated by scattering as the distance to the detection position is increased. That is, as illustrated in
Therefore, the light intensity detected here contains, as described above, information of light scattering corresponding to the concentration of lipid in a particle form in blood, and information of attenuation of light intensity that is facilitated as the distance between irradiation position 21 and detection position 33 increases. Therefore, light intensity/distance calculation unit 41 calculates the ratio of the light intensity to the distance between irradiation position 21 and detection position 33 which is determined by the setting, that is, a so-called attenuation rate to the distance, and light intensity/distance calculation unit 41 uses the calculated value as scattering coefficient μs′, thus obtaining scattering coefficient μs′ dependent on the blood lipid concentration.
Light intensity/distance calculation unit 41 in the present embodiment emits consecutive light from irradiator 2, and applies light intensity R (ρ) detected by first light intensity detector 31 and irradiation-detection distance ρ1 into the following Expression (1) and Expression (2) to calculate scattering coefficient μs′
where μa is the absorption coefficient, μeff is the effective attenuation coefficient, and S0 is the intensity of the light emitted by irradiator 2.
It is to be noted that Expression (1) and Expression (2) are derived as follows.
First, as illustrated in
Where z0 represents the depth of the light source, that is, the depth from which scattering starts, and is expressed by the following Expression (5).
Where μs′ represents the scattering coefficient.
In addition, μeff represents the effective attenuation coefficient and is expressed by the following Expression (6).
Where D and μa represent the diffusion coefficient and the absorption coefficient, respectively.
In addition, when scattering in a blood vessel near the skin surface or on the skin surface is assumed, the relationship between irradiation-detection distance ρ and depth z0 of the light source can be approximated as the following Expression (7).
Further, as described above, the measurement object of the present embodiment of the present invention is blood lipid, and scattering by blood lipid is considered to be greater than absorption. Therefore, effective attenuation coefficient μeff can be approximated as the following Expression (8).
μeff≈√{square root over (3μaμs′)} [Expression 8]
where
μs′>>μa
When Expression (7) and Expression (8) are applied into Expression (4), the approximate expression of the following Expression (9) is obtained.
Here, regarding irradiation-detection distance ρ and effective attenuation coefficient μeff, when the relationship of the following Expression (10) is satisfied, Expression (9) is expressed as the following Expression (11). Here it is assumed that μeff=5.77 mm (μs′=1/mm, μa=0.01/mm).
When Expression (11) is expressed in a logarithmic expression, Expression (1) is derived.
In addition, regarding irradiation-detection distance ρ and effective attenuation coefficient μeff, when the relationship of the following Expression (12) is satisfied, Expression (9) is expressed as the following Expression (13).
When Expression (13) is expressed in a logarithmic expression, Expression (2) is derived.
It is to be noted that intensity/distance calculation section 41 is not limited to the configuration using Expression (1) and Expression (2) as the present embodiment, and is appropriately selected. For example, it is possible to adopt a configuration in which detected light intensity R (ρ) and scattering coefficient μs′ are simply in proportion to each other.
In addition, intensity/distance calculation section 41 is not limited to the configuration in which detection position 33 is provided at one point. In actual measurement, a large amount of noise may be generated. In such case, by providing multiple detection positions 33, a scattering coefficient may be derived from consecutive light intensities corresponding to irradiation-detection distances ρ. That is, in intensity/distance calculation section 41, when the noise amount of measurement data obtained at a few measurement points is relatively large, the influence of the noise assumed in actual measurement can be alleviated by increasing the number of detection positions 33.
Next, light intensity ratio calculation unit 42 is configured to calculate scattering coefficient μs′ from ratios of light intensities detected by a plurality of light intensity detectors 3. Basically, as with light intensity/distance calculation unit 41, light intensity ratio calculation unit 42 calculates scattering coefficient μs′ based on a scattering phenomenon in which emitted light is attenuated by scattering as the distance to the detection position 33 is increased.
In the present embodiment, consecutive light having a given light intensity is emitted by irradiator 2, and first irradiation-detection distance ρ1 from irradiation position 21 to first detection position 331 of first light intensity detector 31, second irradiation-detection distance ρ2 from irradiation position 21 to second detection position 332 of second light intensity detector 32, first light intensity R (ρ1) detected by first light intensity detector 31, and second light intensity R (ρ2) detected by second light intensity detector 32 are applied into the following Expression (3) to calculate scattering coefficient μs′.
It is to be noted that Expression (3) is derived as follows.
First, in Expression (13), when light intensity R (ρ1) and light intensity R (ρ2) at points separated by different distances ρ1 and ρ2 from irradiation position 21 are measured, scattering coefficient μs′ of a light propagation region in a living body is expressed as the following Expression (14).
When Expression (14) is expressed in a logarithmic expression, the following Expression (15) is obtained.
When Expression (8) is applied into Expression (15), Expression (3) is derived.
As described, with Expression (3), the number of detection positions 33 can be reduced, and thus the size of the apparatus can be reduced. Consequently the apparatus can be manufactured at low cost to be suitable for home-use.
It is to be noted that the configuration of light intensity ratio calculation unit 42 is not limited to the configuration using Expression (3) as the present embodiment, and may be appropriately selected. Alternatively, a configuration may be adopted in which the attenuation rate of the distance between first detection position 331 and second detection position 332 is calculated and scattering coefficient μs′ is calculated based on the calculated attenuation rate.
In addition, the apparatus using Expression (3) is not limited to home-use, and may be an apparatus for medical use or clinical use.
Light intensity difference calculation unit 43 is configured to calculate scattering coefficient μs′ from the difference between light intensities detected by a plurality of light intensity detectors 3. This scattering coefficient μs′ is obtained by calculating the difference between two points corresponding to the distance of detection positions 33, and by using the calculated value as scattering coefficient μs′. That is, as with light intensity/distance calculation unit 41 and light intensity ratio calculation unit 42, light intensity difference calculation unit 43 calculates scattering coefficient μs′ based on a scattering phenomenon in which emitted light is attenuated by scattering as the distance to the detection position 33 is increased.
Light intensity difference calculation unit 43 in the present embodiment acquires light intensity R (ρ1) and light intensity R (ρ2) at first detection position 331 and second detection position 332, calculates the difference therebetween, and uses the calculated value as scattering coefficient μs′.
Attenuation time calculation unit 44 is configured to calculate scattering coefficient μs′ from the period until the light intensity detected by light intensity detector 3 is attenuated to a given intensity after pulsed light is emitted by irradiator 2. That is, attenuation time calculation unit 44 calculates scattering coefficient μs′ based on a scattering phenomenon in which emitted pulsed light is attenuated by scattering with time.
Therefore, the light intensity detected here contains information of light scattering corresponding to the concentration of lipid in blood, and information of attenuation of light intensity that is facilitated as the time from emission to detection is elongated. Thus, attenuation time calculation unit 44 acquires scattering coefficient corresponding to the blood lipid concentration from attenuation of the light intensity.
Attenuation time calculation unit 44 in the present embodiment acquires the light intensities at irradiation position 21 and detection position 33 adjacent thereto, calculates the period until the light intensity is attenuated to a given light intensity, and uses the calculated value as scattering coefficient μs′.
Highest intensity time calculation unit 45 is configured to calculate scattering coefficient μs′ from the period until the light intensity detected by light intensity detector 3 reaches a highest value after pulsed light is emitted by irradiator 2. That is, as with attenuation time calculation unit 414, highest intensity time calculation unit 45 calculates scattering coefficient μs′ based on a scattering phenomenon in which emitted pulsed light is attenuated by scattering with time.
In the present embodiment, as described above, a given distance is provided between irradiation position 21 and detection position 33, and scattering occurs within the distance. Therefore, there is a time lag before the highest light intensity is detected by light intensity detector 3. Highest intensity time calculation unit 45 utilizes the time lag to acquire scattering coefficient μs′ corresponding to blood lipid concentration.
Highest intensity time calculation unit 45 in the present embodiment acquires the light intensities at irradiation position 21 and detection position 33 adjacent thereto, calculates the period until a highest light intensity is obtained, and uses the calculated value as scattering coefficient μs′.
Light-density waveform calculation unit 46 is configured to calculate scattering coefficient μs′ and the absorption coefficient of blood from the light density waveform. The waveform of a light density waveform is changed by modulating the intensity or phase of light emitted by irradiator 2. Such a change of a light density waveform corresponds to the blood concentration, and therefore scattering coefficient μs′ and the absorption coefficient of blood can be calculated therefrom.
Light-density waveform calculation unit 46 in the present embodiment acquires light intensities at irradiation position 21 and detection position 31a adjacent thereto, calculates the time variation of the light density waveform, and calculates scattering coefficient μs′ and the absorption coefficient of blood from the calculated time variation.
It is to be noted that the method of calculating scattering coefficient μs′ of scattering coefficient calculator 4 is not limited to the above-mentioned calculation, and may be appropriately selected from methods of calculating information of the blood lipid concentration contained in light intensity.
Lipid concentration calculator 5 is configured to calculate the blood lipid concentration based on scattering coefficient μs′ calculated by scattering coefficient calculator 4. Although described later in Example 5, scattering coefficient μs′ and the lipid concentration correlate with each other, and lipid concentration calculator 5 calculates the lipid concentration based on the value of scattering coefficient μs′. In the present embodiment, the statistical data on the relationship between scattering coefficient μs′ and the blood lipid concentration is obtained, and scattering coefficient μs′ is compared with the statistical data to calculate the actual blood lipid concentration.
For example, when the blood lipid concentration of a certain living body, Mr. A, is the measurement object, the concentration can be calculated by comparing the measurement result of the blood lipid concentration of Mr. A, which is measured by other blood lipid concentration measurement methods or the like such as blood collection, with the calculated scattering coefficient μs′ to prepare personal statistical data of Mr. A.
Alternatively, personal statistical data of Mr. A may be prepared by comparing the measured blood lipid concentration of Mr. A, which is acquired by a different method of measuring blood lipid concentration or the like, with the measured concentration acquired from the detected light intensity, by calculating the error between the concentration acquired from the comparison and the concentration of a common living body in the statistical data, and by performing calibration for correcting the error.
It is to be noted that the format of the statistical data is not limited, and may be classified by, for example, gender, height, weight, BMI and the like, or may be calculated using tables, graphs, function expressions and the like.
In addition, in clinical sites, the terms “concentration” may sometimes be synonymous with the term “turbidity,” and the term “concentration” used in the present embodiment of the present invention includes the concept of turbidity. Therefore, the results of calculation of the lipid concentration calculator may be in the form of formazin turbidity or the particle number per unit quantity, as well as the concentration.
Next, a configuration of non-invasive biolipid metabolism measuring device 10 is described. Non-invasive biolipid metabolism measuring device 10 is configured to acquire scattering coefficient μs′ or the lipid concentration, or both calculated by non-invasive biolipid concentration measuring device 1 to measure the biolipid metabolism from the time variation thereof. As illustrated in
Non-invasive biolipid metabolism measuring device 10 includes calculated-value acquirer 101 that acquires scattering coefficient μs′ and the lipid concentration calculated by non-invasive biolipid concentration measuring device 1 at specified time intervals, and biolipid metabolism determinator 102 that determines the biolipid function based on the time variation of scattering coefficient μs′ and the lipid concentration acquired by calculated-value acquirer 101.
Calculated-value acquirer 101 is configured to acquire scattering coefficient μs′ and the lipid concentration calculated by non-invasive biolipid concentration measuring device 1 through a communication line or the like at specified time intervals. Time intervals of the acquisition are not limited, and may be adjusted to intervals of several seconds, several tens of minutes, or more in accordance with the examination object.
It is to be noted that scattering coefficient μs′ and the lipid concentration may not be acquired through a communication line, and may be acquired by manually inputting the value of the lipid concentration and the like calculated by non-invasive biolipid concentration measuring device 1. In addition, while non-invasive biolipid concentration measuring device 1 and non-invasive biolipid metabolism measuring device 10 are separately provided in the present embodiment, this is not limitative. Non-invasive biolipid concentration measuring device 1 and non-invasive biolipid metabolism measuring device 10 may be integrally configured, or one of the measuring devices may have the other's function.
Biolipid metabolism determination determinator 102 is configured to determine the biolipid metabolism of the examinee from the time variation of scattering coefficient μs′ and the lipid concentration acquired by calculated-value acquirer 101. For example, since the period until scattering coefficient μs′ and the lipid concentration maximum value reach a highest value corresponds to digestion and absorption of lipid by stomach and small intestine, the health condition is determined based on the time length. In addition, lipolysis effect of liver is determined from the period until scattering coefficient μs′ and the lipid concentration reach the values of the fasting state. Finally, the above-mentioned factors are comprehensively determined to generally determine the health condition.
Next, the following describes operations of a method of non-invasively measuring biolipid concentration and a method of non-invasively examining biolipid metabolism using non-invasive biolipid concentration measuring device 1 and non-invasive biolipid metabolism measuring device 10 of the present embodiment.
First, effects of non-invasive biolipid concentration measuring device 1 and the method of non-invasively measuring biolipid concentration are described for each unit of scattering coefficient calculator 4.
“Concentration Measurement Using Light Intensity/Distance Calculation Unit 411”
An irradiation process in the present embodiment is performed using irradiator 2 of non-invasive biolipid concentration measuring device 1. In the case of concentration measurement using light intensity/distance calculation unit 41, irradiator 2 emits consecutive light having given light intensity S0 toward the inside of the body from outside to irradiate irradiation position 21 with the consecutive light. By using consecutive light to irradiate the living body, the influence of the attenuation with time is prevented from being contained in the light intensity detected by light intensity detector 3.
In addition, in the present embodiment, the light source emits light having wavelengths which do not fall within the wavelength range within which the light is absorbed by inorganic substances of plasma and the wavelength range within which light is absorbed by cell components of blood. Thus, when light passes through the blood, light absorption of inorganic substances of plasma and cell components of blood is limited, and the influence of scattering of blood lipid is left in the light intensity detected by light intensity detector 3.
A light intensity detection process in the present embodiment is performed using light intensity detector 3 of non-invasive biolipid concentration measuring device 1. In the present embodiment, first light intensity detector 31 detects the light intensity at first detection position 331. The light intensity thus detected is passed on to a scattering coefficient calculation process.
The scattering coefficient calculation process in the present embodiment is performed using light intensity/distance calculation unit 41 of scattering coefficient calculator 4 in non-invasive biolipid concentration measuring device 1. In light intensity/distance calculation unit 41, as described above, the light intensity detected in the light intensity detection process, that is, light intensity R (ρ), and irradiation-detection distance ρ are applied into the following Expression (1) and Expression (2) to calculate scattering coefficient μs′. Scattering coefficient μs′ thus calculated is passed on to a lipid concentration calculation process.
The lipid concentration calculation process is performed using lipid concentration calculator 5 in non-invasive biolipid concentration measuring device 1. In lipid concentration calculator 5, based on a correlation between the blood lipid concentration and scattering coefficient μs′, the scattering coefficient μs′ is multiplied by a given coefficient to calculate the blood lipid concentration and the like.
That is, with scattering coefficient calculator 4 and the scattering coefficient calculation process in the present embodiment, scattering coefficient μs′ can be instantly acquired by acquiring a light intensity and applying the acquired light intensity into a given expression. In addition, with lipid concentration calculator 5 and the lipid concentration calculation process, blood lipid concentration, turbidity or the like can be readily calculated by multiplying the scattering coefficient μs′ by a given coefficient. Consequently, the arithmetic processing speed is increased, and real time measurement can be achieved.
“Concentration Measurement Using Light Intensity Ratio Calculation Unit 42”
In the irradiation process, as with light intensity/distance calculation unit 41, irradiation position 21 is irradiated with consecutive light with use of irradiator 2.
In the light intensity detection process, the light intensity at first detection position 331 is detected using first light intensity detector 31, and the light intensity of second detection position 332 is detected using second light intensity detector 32. The light intensities detected at first detection position 331 and second detection position 332 are passed on to a scattering coefficient calculation process.
In the scattering coefficient calculation process, light intensity ratio calculation unit 42 of scattering coefficient calculator 4 calculates the ratio of the acquired light intensities of first detection position 331 and second detection position 332, and calculates scattering coefficient μs′ from the ratio. In the present embodiment, first irradiation-detection distance ρ1 from irradiation position 21 to first detection position 331 of first light intensity detector 31, second irradiation-detection distance ρ2 from irradiation position 21 to second detection position 332 of second light intensity detector 32, first light intensity R (ρ1) detected by first light intensity detector 31, and second light intensity R (ρ2) detected by second light intensity detector 32 are applied into the following Expression (3) to calculate scattering coefficient μs′. Scattering coefficient μs′ thus calculated is passed on to a lipid concentration calculation process.
The lipid concentration calculation process is performed using lipid concentration calculator 5 in non-invasive biolipid concentration measuring device 1. In lipid concentration calculator 5, scattering coefficient μs′ is multiplied by a given coefficient to calculate the blood lipid concentration and the like.
“Concentration Measurement Using Light Intensity Difference Calculation Unit 43”
As with light intensity/distance calculation unit 41 and light intensity ratio calculation unit 42, in the irradiation process, irradiation position 21 is irradiated with consecutive light using irradiator 2, and in the light intensity detection process, the light intensity at first detection position 331 is detected using first light intensity detector 31 whereas the light intensity of second detection position 332 is detected using second light intensity detector 32. The light intensities detected at first detection position 331 and second detection position 332 are passed on to a scattering coefficient calculation process.
In the scattering coefficient calculation process, the difference between the first light intensity at first detection position 331 and the second light intensity at second detection position 332 is calculated, and the difference is used as scattering coefficient μs′. Scattering coefficient μs′ thus calculated is passed on to a lipid concentration calculation process.
The lipid concentration calculation process is performed using lipid concentration calculator 5 in non-invasive biolipid concentration measuring device 1. In lipid concentration calculator 5, scattering coefficient μs′ is multiplied by a given coefficient to calculate the blood lipid concentration and the like.
“Concentration Measurement Using Attenuation Time Calculation Unit 44”
In the irradiation process, irradiation position 21 is irradiated with pulsed light by irradiator 2. By using pulsed light for irradiation of a living body, the influence of the attenuation with time is contained in the light intensity detected by light intensity detector 3.
In the light intensity detection process, the light intensity of first detection position 331 is detected in a temporally continuous manner using first light intensity detector 3. Then, the light intensity detected at first detection position 331 is passed on to a scattering coefficient calculation process at specified time intervals.
In the scattering coefficient calculation process, attenuation time calculation unit 44 acquires the light intensity at first detection position 331 at specified time intervals, and determines whether the acquired light intensity has been attenuated to a given light intensity or lower. When it is determined that the light has been attenuated, the time length from the time when the pulsed light is emitted by irradiator 2 to the time when the light is determined to be attenuated is calculated, and the time length thus calculated is used as scattering coefficient μs′. Scattering coefficient μs′ thus calculated is passed on to a lipid concentration calculation process.
The lipid concentration calculation process is performed using lipid concentration calculator 5 in non-invasive biolipid concentration measuring device 1. In lipid concentration calculator 5, the scattering coefficient μs′ is compared with preliminarily prepared statistical data to calculate the blood lipid concentration and the like.
“Concentration Measurement Using Highest Intensity Time Calculation Unit 45”
As with attenuation time calculation unit 44, in the irradiation process, irradiation position 21 is irradiated with pulsed light using irradiator 2. In the light intensity detection process, the light intensity of first detection position 331 is detected in a temporally continuous manner using first light intensity detector 31. Then, the light intensity detected at first detection position 331 is passed on to a scattering coefficient calculation process at specified time intervals.
In the scattering coefficient calculation process, highest intensity time calculation unit 45 acquires the light intensity at first detection position 331 at specified time intervals, and determines whether the light intensity has a high value. When it is determined that the light intensity has a highest value, the time length from the time when the pulsed light is emitted by irradiator 2 to the time when the light is determined to have a highest value is calculated, and the time length thus calculated is used as scattering coefficient μs′. Scattering coefficient μs′ thus calculated is passed on to a lipid concentration calculation process.
The lipid concentration calculation process is performed using lipid concentration calculator 5 in non-invasive biolipid concentration measuring device 1. In lipid concentration calculator 5, scattering coefficient μs′ is compared with preliminarily prepared statistical data to calculate the blood lipid concentration and the like.
“Concentration Measurement Using Light-Density Waveform Calculation Unit 46”
In the irradiation process, light obtained by modulating the intensity or phase of the light emitted to irradiation position 21 is emitted. In the light intensity detection process, the light intensity of first detection position 331 is detected using first light intensity detector 31. The light intensity detected at first detection position 331 is passed on to a scattering coefficient calculation process at specified time intervals.
In the scattering coefficient calculation process, light-density waveform calculation unit 46 acquires the light intensity at first detection position 331 at specified time intervals, calculates a light density waveform, and calculates the scattering coefficient μs′ and the absorption coefficient of blood based on the light density waveform. Scattering coefficient μs′ thus calculated is passed on to a lipid concentration calculation process.
The lipid concentration calculation process is performed using lipid concentration calculator 5 in non-invasive biolipid concentration measuring device 1. In lipid concentration calculator 5, scattering coefficient μs′ and the absorption coefficient calculated by light-density waveform calculation unit 46 are compared with preliminarily prepared statistical data to calculate the blood lipid concentration and the like.
The following describes effects of non-invasive biolipid metabolism measuring device 10 and the non-invasive biolipid metabolism measurement method.
First, a calculation value acquiring process of the non-invasive biolipid metabolism measurement method is performed using calculated-value acquirer 101 of non-invasive biolipid metabolism measuring device 10. Calculated-value acquirer 101 accesses non-invasive biolipid concentration measuring device 1 to acquire calculated scattering coefficient μs′ and the lipid concentration through a communication line at specified time intervals. In the present embodiment, both of scattering coefficient μs′ and the lipid concentration are acquired and passed on to a biolipid function metabolism determination process.
The biolipid function metabolism determination process is performed using biolipid metabolism determinator 102 of non-invasive biolipid metabolism measuring device 10. Biolipid metabolism determinator 102 monitors time-series changes of the acquired scattering coefficient μs′ and lipid concentration, and acquires a given value representing the biolipid metabolism. In the present embodiment, the maximum values of scattering coefficient μs′ and the lipid concentration, the period until the maximum values are reached, and the period until the value of the fasting state is reached through the maximum values, are acquired.
Then, the values are compared with preliminarily prepared statistical data, and when the values are determined to be normal values, it is determined that the values are normal values, and when the values are determined to fall outside normal values, it is determined that abnormality of biolipid metabolism is present.
For example, when maximum values of scattering coefficient μs′ and the lipid concentration are normal values, it is determined that the basic metabolism of lipid is normal, and when maximum values of scattering coefficient μs′ and the lipid concentration are not normal values, it is determined that the basic metabolism of lipid is abnormal. Likewise, when the period until scattering coefficient μs′ and the lipid concentration reaches the maximum value are normal values, it is determined that the function of digestion and absorption of lipid by stomach and small intestine is normal, and when the period until scattering coefficient μs′ and the lipid concentration reaches the maximum value are not normal values, it is determined that the function of digestion and absorption of lipid by stomach and small intestine is abnormal for some reason. In addition, when the period until scattering coefficient μs′ and the lipid concentration reach the values of the fasting state are normal values, it is determined that lipolysis effect of liver is normal, and when the period until scattering coefficient μs′ and the lipid concentration reach the values of the fasting state are not normal values, it is determined that lipolysis effect of the liver is abnormal.
In clinical sites, the above-mentioned normality and abnormality are comprehensively determined, and thus health condition is comprehensively determined.
With the above-mentioned non-invasive biolipid concentration measuring device 1, non-invasive biolipid metabolism measuring device 10, the method of non-invasively measuring biolipid concentration, and the method of non-invasively examining biolipid metabolism of the present embodiment, the following effects are achieved.
1. The blood lipid concentration can be non-invasively acquired by determining scattering coefficient μs′ in a living body based on the light intensity.
2. Invasive operations such as blood collection are not required, and thus pain and risk of the examinee can be reduced.
3. The blood lipid can be measured at home since medical acts such as blood collection are not required.
4. Data can be instantly acquired since the processes of calculating light intensity scattering coefficient μs′ and the lipid concentration are simple.
5. Application to examination of metabolic errors such as postprandial hyperlipidemia can be achieved since blood lipid and scattering coefficient μs′ well correlated with the blood lipid can be calculated in a temporally continuous manner.
6. The accuracy of measurement of the blood lipid concentration can be enhanced by setting the wavelength range of light to be emitted to a living body to a range falling outside the wavelength range within which light is absorbed by inorganic substances of plasma so as to limit the influence of absorption that results in noise.
7. Blood lipid concentration measurement can be achieved more correctly by further excluding the wavelength range within which light is absorbed by cell components of blood so as to limit the influence of absorption by cell components such as red blood cell.
8. Scattering coefficient μs′ and the lipid concentration can be calculated by various calculation methods by taking into consideration the relationship between the light scattering of blood lipid and the blood lipid concentration.
9. In lipid concentration calculator 5 or the lipid concentration calculation process, conversion to particle number, formazin turbidity or the like, as well as units such as concentration (mg/dL), are also possible in accordance with the demand in the clinical site.
(1) Variation in Whole Blood
First, whether the concentration of blood lipid and the like of examinees changes with time after ingestion of lipid was confirmed. The examinees are Mr. A and Mr. B, each of them ingested lipid (OFTT Cream; Jyoumou Corporation).
The blood lipid concentration was measured as follows. At a time before ingestion of lipid (0 minute), and at 60, 150, 180, 210, 240, 270, 300, 330 and 360 minutes after ingestion, blood was collected to collect blood samples, and the blood samples were put in automatic analysis apparatus H-7170 (Hitachi High-Technologies Corporation.) to measure concentrations of total cholesterol (TC), triglyceride (TG), HDL and LDL. Results of the measurement are shown in
As shown in
Meanwhile, the concentrations of total cholesterol (TC), HDL and LDL were not significantly varied. These results clearly show that ingestion of lipid results in dominant increase of the concentration of triglyceride (TG) in blood.
(2) Variations in Each Lipoprotein
Next, in order to identify the substance that contributes to increase in triglyceride (TG), the blood samples of Example 1 (1) were put in a high-performance liquid chromatography (HPLC) and fractionated into chylomicron (CM)/VLDL, LDL and HDL, and the total cholesterol (TC) and the concentration of triglyceride (TG) in CM/VLDL, LDL and HDL were measured. Results are shown in
As shown in
These results clearly show that increase in concentration of triglyceride (TG) in blood caused after ingestion of fat was caused by increase in TG in large lipoprotein such as CM/VLDL, when the results that total cholesterol (TC) and triglyceride (TG) of LDL and HDL were not substantially varied are taken into consideration.
Next, in Example 2, measurable wavelength ranges when light is non-invasively emitted toward the inside of the body from outside to determine scattering coefficient μs′ from the intensity of light emitted to the outside of the body were studied. In this study, blood was collected from an examinee, and whole blood was put in a spectrophotometer to measure the light absorbance of the blood with light having wavelengths of 300 to 3300 nm, thereby obtaining the absorption spectrum. Results are shown in
As shown in
Next, in Example 3, effectiveness of measurement using transmitted light, and measurement of the blood lipid concentration by non-invasively emitting light toward the inside of the body from outside so as to determine scattering coefficient μs′ from the intensity of light emitted to the outside of the body was studied.
(1) Variation in Light Absorbance of Blood, Blood Cells and Serum in Association with Change in Lipid Concentration
First, by the method of (1) of Example 1, a blood sample of Mr. A was prepared and the blood lipid concentration was measured. Results are shown in Table 1.
Here, blood samples shown in Table 1 having triglyceride (TG) concentration of 390.1, 408.4, 518.2 and 499.6 mg/dL are referred to as samples a, b, c and d, respectively.
Subsequently, samples a, b, c and d are put in a spectrophotometer, and the light absorbance of blood with respect to light having a wavelength of 300 to 1000 nm was measured to obtain absorption spectrums. Likewise, serum and blood cells of samples a, b, c and d were also obtained, and absorption spectrums were obtained by the above-mentioned method. Results are shown in
As shown in
(2) Studies on Absorption Spectrum
Likewise, blood was collected from Mr. A to obtain blood, blood cell and serum. The blood, blood cell and serum thus obtained were put in a spectrophotometer, and the light absorbance of blood with respect to light having a wavelength of 300 to 1000 nm was measured, thus obtaining absorption spectrums. It is to be noted that the basic principle of spectrophotometers is irradiation of a measurement object with light and analyze of transmitted light.
As shown in
In Example 4, with use of non-invasive biolipid concentration measuring device 1 of the embodiment of the present invention, whether the lipid concentration can be measured based on a scattering phenomenon in which emitted light is attenuated with time by scattering was confirmed.
(1) Studies on the Period Until Light is Completely Output (Spread of Waveform)
Irradiation position 21 was set at a center portion of an examinee's back of the hand on the skin over a blood vessel. In addition, detection position 31 is set on the skin over the blood vessel that is common to the irradiation position, at a position separated by 10 mm from irradiation position 21. Ti: Spphirelaser Chameleon Ultra II (variable wavelength type, pulse width: 140 fs FWHM, average output: 400 m W, repetition frequency: 80 MHz; Coherent Inc.) was used as light source 22 of irradiation position 21, and a streak camera was used as light intensity detector 3 of detection position 31.
Lipid was ingested by examinee, and before and after the ingestion of lipid, irradiation position 21 is irradiated with pulsed light having a wavelength of 853 nm, and the light intensity detected at detection position 31 was measured in a time dependent manner. Results are shown in
As shown in
(2) Studies on Peak Top Time
Next, to obtain scattering coefficient μs′, the period (peak top time) until the intensity of detected light reaches a highest value was studied. Results are shown in
As shown in
Next, in Example 5, whether the lipid concentration can be measured based on a scattering phenomenon in which emitted light is attenuated in accordance with the distance by scattering using non-invasive biolipid concentration measuring device 1 of the embodiment of the present invention was determined.
(1) Measurement of Light Intensity at a Plurality of Detection Positions 33
Irradiation position 21 was set at a center portion of the back of the hand of examinees, Mr. A and Mr. B, on the skin over a blood vessel. In addition, three detection positions 33 are set on the skin over the blood vessel that is common to the irradiation positions separated from irradiation position 21 by 10 mm, 15 mm and 20 mm, respectively. Ti: Sapphire (Ti:S) laser Chameleon Ultra (automatic wavelength-sweep femtosecond laser; Coherent Inc.) was used as light source 22 of irradiation position 21, and Femtowatt Photoreceiver FWPR-20-SI (FEMTO Messtechnik GmbH) was used as light intensity detector 3 of detection position 33.
Lipid (OFTT Cream; Jyoumou Corporation) was ingested by the examinees, Mr. A and Mr. B, and at a time before the ingestion of lipid (at 0 minute), and at 60, 150, 180, 210, 240, 270, 300, 330 and 360 minutes after the ingestion of lipid, laser beams of wavelengths of 800 nm, 809 nm, 850 nm and 1000 nm were applied to irradiation position 21 and light intensities detected at respective detection positions 33 were measured. Results are shown in Table 2.
In Table 2, for example, “1000-10” of the left column represents a condition of a wavelength of 1000 mm and an irradiation-detection distance of 10 mm, and light intensities (voltages mV detected with a photodiode) at respective detection positions of Mr. A and Mr. B under respective conditions are shown.
(2) Calculation of Scattering Coefficient μs′ Based on Ratio of Light Intensity
Subsequently, the ratio of light intensities detected at detection positions 33 was calculated, and the ratio thus calculated was used as scattering coefficient μs′. The value of the scattering coefficient μs′ thus obtained is an index that represents scattering of emitted light by blood lipid.
As shown in
In addition,
As shown in
In addition, when the variation in triglyceride concentration can be continuously measured in a time dependent manner in this manner, non-invasive lipid metabolism measurement, which has been conventionally difficult, is achieved, and consequently evaluation of the lever function as well as arteriosclerosis are expected to be achieved.
(3) Calculation of Scattering Coefficient μs′ Based on Difference in Light Intensity
In addition, the difference of light intensities detected at detection positions 33 were calculated, and the calculated difference was used as scattering coefficient μs′.
Comparing
In Example 6, an experiment using a biological tissue simulated phantom and ideal scattering phenomenon were calculated using Monte Carlo simulation, and with use of the value thus obtained, the following Expression (1) and Expression (2) were studied.
(1) Studies on Expression (1) and Expression (2) by Monte Carlo Simulation
First, by Monte Carlo simulation, irradiation-detection distance ρ and number of detected photons were simulated. The condition of this simulation is the absorption coefficient of 0.01, and the number of emitted photons of 10×109. The calculation was performed with scattering coefficients μs′ of 0.5, 1, 1.5, 2, 2.5, 3, 3.5, 4, 4.5 and 5. FIG. shows results of the calculation. In
As shown in
Next, the results of the Monte Carlo simulation were applied into Expression (1). Results are shown in
Here, since it is speculated that the irradiation-detection distance in actual measurement is required to be equal to or greater than 1 cm, the calculation range of the gradients and the intercepts were set to 1 cm to 3 cm. At this time, from Expression (1), the gradients of these values correspond to effective attenuation coefficient μeff, and the intercepts correspond to ln(3μa/2πμeff) of the following Expression (16).
That is, absorption coefficient μa can be determined from the intercepts of the graph of the incident light attenuation rate shown in
Further, the effective attenuation coefficient μeff was calculated from the gradients of the graph of the incident light attenuation rate shown in
μeff≈√{square root over (3μaμs′)} [Expression 8]
Results are shown in
As shown in
(2) Studies on Expression (1) and Expression (2) by Experiment Based on Biological Tissue Simulated Phantom
Next, an experiment was performed based on a biological tissue simulated phantom having a specific scattering coefficient μs′ which was prepared using Intralipid. To be more specific, biological tissue simulated phantoms having scattering coefficients μs′ of 0.5, 1, 1.5, 2, 2.5, 3, 3.5, 4, 4.5 and 5 were prepared. The biological tissue simulated phantoms were irradiated with consecutive light by irradiator 2, and the light intensity was detected by light intensity detector 4. As with Example (1), the light intensity thus detected was applied into Expression (1) and Expression (2) to calculate scattering coefficient μs′. Results are shown in
As shown in
The above-mentioned results show that scattering coefficient μs′ can be measured with use of Expression (1) and Expression (2) even when absorption coefficient μa is unknown. In addition, it was confirmed that, as can be seen in the correlation coefficient, the scattering coefficient can be calculated with higher accuracy by measurement at multiple points even with a large amount of noise in actual measurement of a living body.
In Example 7, the following Expression (3) was studied by an experiment using a biological tissue simulated phantom and calculation of an ideal scattering phenomenon using Monte Carlo simulation.
(1) Studies on Irradiation-Detection Distance
From Expression (3), the sensitivity of scattering coefficient μs′ is enhanced as the ratio of light intensity R (ρ1) to light intensity R (ρ2) at the first detection position is increased. Therefore, the greater the distance between ρ1 and ρ2, the more preferable. However, light intensity R (ρ) exponentially decreases as irradiation-detection distance ρ increases, and S/N ratio, which is the ratio of the signal quantity (signal) to the noise quantity (noise), in measurement are quickly increased, thus degrading the measurement accuracy. In addition, when the difference in distance between ρ1 and ρ2 is increased, common part of internal scattering member propagation region of light intensity of the points is reduced, thus further degrading the measurement accuracy. Given the above, the measurement condition was studied to determine favorable measurement conditions by changing ρ1 and ρ2 in a range of practical use.
(2) Studies on Irradiation-Detection Distance ρ by Biological Tissue Simulated Phantom
First, a biological tissue simulated phantom having a specific scattering coefficient μs′ was prepared using Intralipid. In this experiment, with use of Intralipid, variation of R (ρ1)/R (ρ2) with respect to scattering coefficient μs′ was measured. Exemplary measurement results are shown in
Here, a calibration curve for estimating μs′ from measurement results of (ρ1)/R (ρ2) is desirably a stable simple variation. From this view point, in
(3) Studies on Expression (3) by Monte Carlo Simulation
To verify the adequacy of Expression (3), verification was performed by Monte Carlo simulation. The condition of simulation was absorption coefficient μa of 0.01, 0.05 and 0.1. Scattering coefficient μs′ was set to 0.5, 1, 1.5, 2, 2.5, 3, 3.5 and 4 and calculation was performed for each combination. In addition, irradiation-detection distance ρ was set to ρ1=10 mm and ρ2=20 mm as described above. Then, the value thus obtained was applied into Expression (3), and calculation was performed. Results of the calculation are shown in
As shown in
Likewise, theoretical scattering coefficient μs′ and scattering coefficient μs′ calculated using Expression (3) in the case where noise (±5%) is added to the detected light intensity were also studied. Results of the calculation are shown in
As shown in
(4) Studies on Expression (3) by Experiment Based on Biological Tissue Simulated Phantom
Given the results of Monte Carlo simulation, Expression (3) was studied by an experiment using a biological tissue simulated phantom. Results of measurement are shown in
As shown in
Thus, it was confirmed that scattering coefficient μs′ can be calculated with use of Expression (3) under a condition of a typical living body.
It is to be noted that the non-invasive biolipid concentration measuring device, the non-invasive biolipid metabolism measuring device, the method of non-invasively measuring biolipid concentration and the method of non-invasively examining biolipid metabolism according to the embodiment of the present invention are not limited to the above-described embodiment, and may be appropriately changed.
For example, it is possible to cover irradiator 2 and light intensity detector 3 with a light-shielding cover, or to perform measurement in a dark place, in order to block other light than emitted light and received light.
In addition, while non-invasive measurement with respect to a living body has been described in the present embodiment, the present embodiment is also applicable to non-invasive measurement with respect to a test tube or the like for blood test and serum test in the test tube or the like. In this case, the present embodiment is applicable to turbidity measurement or the like in serum information (hemolysis, high bilirubin, milky fluid and the like) prior to a blood test.
| Number | Date | Country | Kind |
|---|---|---|---|
| 2012267708 | Dec 2012 | JP | national |
This is a Continuation Application of U.S. patent application Ser. No. 14/649,676, filed Jun. 4, 2015, an application filed as a National Phase of PCT/JP2013/080826 on Nov. 14, 2013, an application claiming the benefit from Japanese Application No. 2012267708, filed Dec. 6, 2012, the contents of each of which are hereby incorporated by reference in their entirety.
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| Number | Date | Country | |
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| Child | 16218966 | US |
