The present invention concerns an analysis method and a system for performing this analysis. Specifically the invention concerns a method for determination of hemoglobin in unaltered whole blood and a system which can be used in this determination.
A disposable cuvette for sampling a fluid, mixing the sample with a reagent and directly making optical analyses of the sample mixed with the reagent is previously known from U.S. Pat. No. 4,088,448. This known cuvette has several advantages as it i.a. simplifies the sampling procedure, reduces the number of utensils and considerably improves the accuracy of analysis by making the analysing procedure independent of the operating technique of the operator making the analysis. A cuvette construction based on the same principle and with improved flow characteristics is disclosed in the U.S. Pat. No. 5,674,457.
A disposable cuvette developed according to these patents is currently widely used for hemoglobin measurement (Hb determination) of undiluted whole blood. To this end the cuvette cavity has been pre-treated with a reagent, such that when a blood sample is drawn into the cuvette, the walls of the red blood cells are disintegrated and a chemical reaction is initiated. The result of the reaction allows Hb determination by absorption measurement directly through the transparent walls of the cuvette which, in the measuring zone, also called the optical window, has a predetermined and accurately defined distance between the inner surfaces of the opposing planar walls. The measurement method is based on a modified azidmethemoglobin method according to Vanzetti, G., “An azide-methaemoglobin method for haemoglobin determination in blood”, Am. J. Lab. & Clin. Med. 67, 116-126 (1966).
The spectrophotometric measurements are made at 570 and 880 nm. This quantitative measurement method based on dry chemistry has met with considerable success as can be seen in e.g. the article by von Schenck, H., Falkensson, M. and Lundberg, B., “Evaluation of ‘HemoCue’, a new device for determining hemoglobin”, Clinical Chemistry, vol 32, No 3, pages 526-529, 1986, as the method gives equal or even superior results in comparison with the results obtained with standardised wet methods for the determination of Hb. The reagent used is comprised of sodium deoxycholate which hemolyses the red blood cells, sodium azide and sodium nitrite, which converts hemoglobin to azidmethemoglobin.
Due to the hygroscopic properties of the reagents used, the shelf life is limited and the storage of the cuvettes in sealed packages including a drying agent is required. Even more troublesome is the fact that, in climates with high humidity, the cuvette has to be used within a few minutes after the removal from the package, as otherwise the reagents will be destroyed and the measurement will be inaccurate and thus useless.
The problems originating from the hygroscopic properties of the reagents used may however be eliminated as it has been found that these reagents must not be used, as disclosed in U.S. Pat. No. 6,638,769, according to which the first absorption measurement is performed at a wavelength range 490-520 nm directly on the sample in the microcuvette. According to the invention disclosed in this patent application it is however necessary that the blood is hemolysed before the measurement is performed. The cuvette cavity must thus include a hemolysing agent for disintegrating the red blood cells and releasing the hemoglobin contained in these cells. The necessity of using a hemolysing agent when performing photometric absorbance measurements of hemoglobin in a blood sample is also disclosed in e.g. the U.S. Pat. No. 5,064,282 (Artel).
Quantitative methods for optical determination of hemoglobin in whole blood without using hemolysing agent are known but these methods have in common that they are all comparatively complicated. This depends above all on the inhomogeneity of the blood due to the high concentration of red blood cells, a consequence of which is that light is scattered upon interaction with these particles of inhomogeneous blood samples. Accordingly the light is not transmitted directly through the sample but deflected over a range of scattering angles. Another factor that causes problems is the fact that blood may contain as many as five different species of hemoglobin. Patent publications addressing these problems are i.a. the U.S. Pat. No. 6,262,798 (Shepherd) and WO 01/53806 (Radiometer).
According to the invention disclosed in the U.S. Pat. No. 6,262,798 a plurality of wavelengths are needed in order to achieve a correct measurement. The fact that many wavelengths are needed makes the spectrophotometer comparatively complicated. The wavelengths are selected by their ability to distinguish the hemoglobin species at minimum scatter and maximum absorbance. The patent also discloses the use of a large detector which reduces the problem of scattering beyond the detection range.
WO 01/53806 discloses an apparatus which is especially applicable for optical measurements on whole blood. This apparatus comprises an absorption filter or an interference filter, which provides correction for variations in the detector sensitivity and in the effective optical path length as observed upon varying level of scattering. The apparatus uses a large detector for detecting scattered light transmitted through the absorption filter or the interference filter.
In U.S. Pat. No. 6,831,733, it has been shown that an accurate determination of the total amount of hemoglobin in whole blood can be made not only without using a hemolysing agent but also without using a plurality of wavelengths as disclosed in the U.S. Pat. No. 6,262,798. According to U.S. Pat. No. 6,831,733, the total amount of hemoglobin in whole blood could be determined by performing two absorbance measurements, at a first wavelength in the range 490-520 nm, and at a second wavelength at which the absorption is substantially smaller than at the first wavelength. The concentration of hemoglobin in the sample may then be determined by processing results of the first and second absorption measurements. The difference in absorption between the first and second absorption measurements is mainly due to the difference in absorption of the hemoglobin. However, there are other factors that affect the difference in absorption. The most important other factor is the difference in scattering in the sample. According to U.S. Pat. No. 6,831,733, the effect of scattering is regarded as being dependent of the absorbance measured in the second absorption measurement. Thus, it has been unexpectedly found that the concentration of hemoglobin in the sample could be measured as the difference in absorption between merely two absorption measurements, by using a term to compensate for scattering. The compensation term is dependent on the result of the second absorption measurement.
It is an object of the present invention to provide a rapid, quantitative method for the determination of hemoglobin in unaltered whole blood.
A second object is to provide a method for the determination of hemoglobin in unaltered whole blood, which may be performed in a microcuvette that may also be used for acquiring a sample of blood.
A third object is to provide a simple method of processing results of absorption measurements for determination of hemoglobin in unaltered whole blood.
A fourth object is to provide a system for implementing the methods for the determination of hemoglobin in unaltered whole blood.
Other objects will be apparent from the following description and the accompanying claims.
In accordance with an aspect of the present invention a method for providing such a hemoglobin determination comprises: acquiring a sample of unaltered whole blood into a capillary cuvette; presenting said cuvette to a set-up for an absorption measurement; delaying absorption measurement for a determined period of time; performing a first absorption measurement at a first wavelength in the range 490-520 nm directly on the sample in the cuvette; further conducting a second absorption measurement at a second wavelength different from the first wavelength and at which the absorption is substantially smaller than at the first wavelength; and processing results of the first and second absorption measurements to determine the concentration of hemoglobin in the sample.
In accordance with another aspect of the present invention a system for providing such a hemoglobin determination comprises: means for emitting light at a first wavelength in a first range of 490-520 nm and at a second wavelength in a second range at which absorption of light in blood is substantially smaller than at the first wavelength; a cuvette holder arranged to receive a capillary cuvette, which holds a sample of unaltered whole blood; a detector for detecting light transmitted through the sample in a first absorption measurement for light in said first range and in a second absorption measurement for light in said second range; a controller for creating a delay of a determined period of time between placement of the cuvette in the cuvette holder and performing absorption measurements; and a processing unit for processing results of the first and second absorption measurements to determine the concentration of hemoglobin in the sample.
According to the invention it has been unexpectedly found that quantitative determinations of hemoglobin can not only be easily performed directly on an unaltered, i.e. undiluted and unhemolyzed, sample of whole blood, but may also be achieved by simply conducting two absorption measurements at different wavelengths and processing these results.
The determination may be performed on a blood sample without using hygroscopic reagents, such as sodium azide and sodium nitrate, or a hemolysing agent. Thus, the hemoglobin determination is based on measurements of absorption, while the hemoglobin is bound inside red blood cells. The hemoglobin level may thus be determined without lysing the red blood cells to release the hemoglobin.
Further, it has now been unexpectedly realized that it is not even necessary to compensate for the effect of scattering of the red blood cells. A difference between two absorption measurement reflects both an effect due to absorption of light in hemoglobin and an effect due to scattering of light by the red blood cells. However, by using a delay in performing the absorption measurements, it may be controlled at which time the absorption measurements are performed. In development of the invention it has been observed that the results of the absorption measurements vary with time in respect to the acquiring of a blood sample. The result of the first absorption measurement varies more heavily. This implies that the difference between the two absorption measurements will vary depending on at which point of time the measurements were performed. Thus, the delay in performing the absorption measurements may control at which time the absorption measurements are performed and the processing of the results may be calibrated accordingly to output a correct value of the hemoglobin concentration in the blood sample.
In particular, the difference between the absorption measurement results decrease heavily the first period of time after the blood sample is acquired. Thereafter, the difference is relatively stable for a period of time and after a while the difference start to increase again. The delay may thus be adapted to allow the measurements to be performed at a time when the measurement results are relatively stable. This makes the result of the determined hemoglobin concentration quite insensitive to the exact point of time at which it is performed. Thus, the result is not dependent on whether the acquired sample is presented instantly to the measurement apparatus or a minute passes before the acquired sample is presented to the measurement apparatus.
It is believed that the variation in measurement results is at least partly due to movements within the sample as the sample is acquired into the cuvette. After a while, the movements have been allowed to settle and the measurement results are more stable. The effect of scattering of the red blood cells is then also diminished and, therefore, the processing of the results of the absorption measurements need not account for effects of the scattering of the red blood cells being different for the first and second absorption measurements. The measurement results may later start to increase again as the red blood cells are beginning to settle within the bottom portion of the cuvette. The red blood cells will therefore collect at the bottom of the cuvette, which will increase the effect of scattering.
Thus, according to the invention, the hemoglobin determination is performed in a simple manner. Only two absorption measurements are needed using a sample of unaltered whole blood. Further, the hemoglobin content may be determined using a simple algorithm for processing the results of the two absorption measurements. This implies that it is easy to calibrate an instrument to present correct results with the algorithm. However, the ease of calibration is achieved at the cost of a somewhat prolonged time for obtaining an analysis result, since the analysis need to be delayed in order to ensure that effects of scattering need not be accounted for.
In the context of this application, the term “absorption measurement” should be construed as a measurement related to the absorption in a sample. In an absorption measurement, the intensity of light detected after interacting with a sample is compared with the intensity of light irradiated on the sample. The detected light corresponds to the transmittance through the sample. The light that does not reach the detector is considered to be absorbed. Thus, in the results of the measurements the transmittance may be used instead of the absorption. As the transmittance is the inverse of the absorption, detecting transmittance would still be an absorption measurement. However, the measured absorption does not only correspond to light that has been truly absorbed in the sample, since some of the light has been scattered in the sample so that it does not reach the detector.
Further, the term “determination” should be construed as the measurement not necessarily obtaining an absolutely exact value of the concentration of hemoglobin in the sample. Thus, the concentration of hemoglobin is “determined” within reasonable margins of error such that the result not merely gives an order of magnitude of the concentration, while not necessarily giving an absolute value.
The processing may be performed by a predetermined algorithm. This implies that the algorithm may be programmed into an instrument and that the instrument may directly return analysis results after the absorption measurements have been performed.
The processing may determine the concentration of hemoglobin in the sample by computing the following formula:
[Tot Hb]=(Abs1−Abs2)·k1+k2
wherein [Tot Hb] is the total concentration of hemoglobin in the sample, Abs1 is the measured absorbance of the first absorption measurement, Abs2 is the measured absorbance of the second absorption measurement, and k1 and k2 are calibration coefficients, which depend on the measurement arrangement.
This implies that the total concentration of hemoglobin in a sample is simply determined by computing a difference between the two absorption measurements. There is only a need for two calibration coefficients which may handle the slope of the curve and the offset of the curve from the origin of coordinates. Thus, it is only necessary to determine two values of calibration coefficients, whereby calibration of instruments may be achieved in a simple manner.
The presenting may comprise placing the cuvette in a holder of an instrument for performing absorption measurements. This implies that the cuvette may be guided to a correct position for absorption measurements within the instrument.
According to one embodiment, the delaying is made for a predetermined period of time that is pre-set before acquiring the sample. Thus, a measurement apparatus may be pre-set to delay the performing of the absorption measurements by a predetermined period of time. The measurement apparatus may be calibrated accordingly. This predetermined period of time may be controlled by means of a timer that enables performing the absorption measurements after the period of time has passed.
The predetermined period of time may be started when the cuvette is placed in the holder. Thus, the instrument may control that the analysis is delayed for a minimum amount of time in order for the scattering effects of red blood cells to be insubstantial. The instrument may thus be arranged to enable absorption measurements at a specific time after receiving a cuvette in the holder.
The predetermined period of time is at least 30 seconds, and more preferably in the range of 60-90 seconds. This gives the sample a possibility to settle appropriately such that the scattering effects of the red blood cells will not affect the analysis result.
According to another embodiment, the delaying is made by monitoring results of absorption measurements and, when the results are substantially constant, allowing the first and second absorption measurements to be performed for determining the concentration of hemoglobin in the sample. This implies that a first check is made to ensure that the absorption measurements are performed at a point of time where the effect of scattering in the blood sample will not significantly affect the determining of the concentration of hemoglobin. When this has been established, the absorption measurements are performed. Alternatively, the first check may be made in any other way to determine that the movements within the blood sample have settled.
The first absorption measurement may be performed at a wavelength in the range 500-510 nm, more preferably at 506 nm. In the wavelength range of 490-520 nm, and especially 500-510 nm, the absorptions of the five different forms of hemoglobin, namely oxy-, deoxy-, carboxy-, met- and sulfhemoglobin, are significant and similar. Thus, the absorption in this wavelength range will depend only slightly on the distribution between the different forms of hemoglobin in the blood. Especially, at 506 nm, the difference between the absorbances of oxy- and deoxyhemoglobin is close to zero. Since these forms of hemoglobin are predominant in normal blood, the absorption of oxy- and deoxyhemoglobin could advantageously be used for determining an absorption coefficient for relating a measured absorption to the concentration of hemoglobin at 506 nm. Accordingly, some assumptions are made regarding the contents of different forms of hemoglobin in the blood sample. Thus, the hemoglobin determination will not be as accurate or the processing of the measurement results will have to be modified, if a measurement is made on a blood sample having a very differing distribution of the forms of hemoglobin. Further, the measurements will only determine the total concentration of hemoglobin and not the concentrations of the specific forms of hemoglobin.
The second absorption measurement may be performed at a wavelength in the range 650-1200 nm, more preferably in the range 850-910 nm, most preferably in the range 860-900 nm. At these wavelength ranges, the absorption of hemoglobin is significantly lower than at the first wavelength. Further, the wavelength should be chosen such that absorption of other substances in the blood sample is substantially the same at the first and second wavelengths. This implies that the difference in absorption may be related to the concentration of hemoglobin in the sample. The second wavelength may advantageously be selected in the range 860-900 nm, whereby the absorption of other substances will not affect the analysis result.
The cuvette may have an optical path length of less than 1 mm, more preferably less than 0.2 mm. This ensures that a sufficient intensity of light may be transmitted through the sample in order for the absorption measurements to be statistically significant. A smaller optical path would allow higher intensities of light to be detected.
The cuvette may have an optical path length in the range 0.05-0.2 mm. This implies that light is transmitted through a sufficient amount of blood in order to enable determination of hemoglobin concentration, while sufficient intensities of light may be detected without use of a strong light source.
The means for emitting light, the cuvette holder and the detector may be arranged in a photometer. The photometer would thereby provide an adapted set-up for performing the analysis. The photometer may easily be carried such that the analysis may be performed where it is needed, e.g. at a point of care.
The processing unit may be embedded in the photometer. Thus, the photometer could return results of an analysis in a display of the photometer and there is no need to use additional equipment. However, the processing unit may alternatively be connected to the photometer. This implies that the processing unit may be arranged in a computer, to which the photometer may be connected. This would allow a user to analyse the results of the absorption measurements in further detail.
The detector may have a detecting area of a size such that essentially only directly transmitted light is detected. This implies that light that is scattered into a substantially different direction is not detected, whereby the absorption measurement determines the amount of light being transmitted without being scattered or absorbed. Thus, the measurement may assume that all light that is scattered into another direction is not detected.
The detector may be arranged closer than 10 mm to the sample holder. This further implies that only light being scattered in small angles is detected.
The means for emitting light may comprise one light source, which is arranged to emit light at the first wavelength and to emit light at the second wavelength. Then, filters may be used for ensuring that the sample is illuminated with the correct wavelength. Alternatively, the means for emitting light may comprise a first light source, which is arranged to emit light at the first wavelength, and a second light source, which is arranged to emit light at the second wavelength. The different light sources may then be appropriately turned on and off in order to illuminate the sample with the correct wavelength.
The invention will now by way of example be described in more detail with reference to the accompanying drawings.
Referring now to
The disposable microcuvette used according to the present invention may be of the type disclosed in the U.S. Pat. No. 4,088,448 or preferably in the U.S. Pat. No. 5,674,457 which are hereby incorporated by reference. The cuvette may be defined as a unitary body member including at least one cavity with an optical window (measuring zone) wherein two, plane or curved, surfaces facing the cavity are placed at a predetermined distance from one another and thus define a predetermined optical path length. This distance between the surfaces defining the measuring zone is a critical parameter in providing the proper optical path length for the hemoglobin measurement. The optical path length should be less than 1 mm in order to ensure that the intensity of light transmitted through a sample in the cuvette is sufficient to enable determination of hemoglobin in the sample. In a preferred embodiment, this distance is less than 0.2 mm, and more preferably between 0.05 and 0.2 mm. The distance between the inner surfaces of the rest of the cavity is preferably in the order of 0.1-2 mm which is effective to permit the sample to enter the cavity by capillary force through the cavity inlet, which is communicating with the exterior of the body member. Furthermore, the cavity has a predetermined fixed volume of less than about 25 μl. No active additives, such as reagents or hemolysing agents, are necessary for the determination according to the inventive method.
The cuvettes according to the present invention may be formed by any suitable material, which allows the formation of the necessary tight tolerance levels. Preferably the cuvette is manufactured by injection moulding of a transparent polymeric material.
In order to overcome problems related to the capillary filling of the cuvette it may be necessary to pre-treat the inner surfaces of the cuvette in order to impart a hydrophilic character to these surfaces. This may be achieved by coating the surfaces with a suitable detergent, such as Brij 35. Another possibility is to select a hydrophilic material for the manufacturing of the cuvette.
A feature of the inventive method is that the absorption determination should be carried out at a wavelength in a range of 490-520 nm, more preferably in the range 500-510 nm, and most preferably at 506 nm. The secondary absorption measurement is preferably performed at a wavelength in the range 650-1200 nm, more preferably in the range 850-910 nm, and most preferably in the range 860-900 nm.
The absorption measurements are performed directly on the whole blood in the sample, i.e. the blood is unaltered (undiluted and unhemolyzed).
In the wavelength range of 490-520 nm, the absorptions of the five different forms of hemoglobin, namely oxy-, deoxy-, carboxy-, met- and sulfhemoglobin, are similar and significant. Thus, the absorption in this wavelength range will depend only slightly on the distribution between the different forms of hemoglobin in the blood. Especially, at 506 nm, the difference between the absorbances of oxy- and deoxyhemoglobin is close to zero. Since these forms of hemoglobin are predominant in normal blood, the absorption of oxy- and deoxyhemoglobin could advantageously be used for determining an absorption coefficient for relating a measured absorption to the concentration of hemoglobin at 506 nm. Accordingly, some assumptions are made regarding the contents of different forms of hemoglobin in the blood sample. Thus, the hemoglobin determination will not be as accurate or the processing of the measurement results will have to be modified, if a measurement is made on a blood sample having a very differing distribution of the forms of hemoglobin. Further, the measurements will only determine the total concentration of hemoglobin and not the concentrations of the specific forms of hemoglobin.
A second absorption measurement is performed at a wavelength, where the absorption of light in blood is substantially smaller. Such an absorption measurement could suitably be performed at a wavelength in the range 650-1200 nm. The differences between the absorption measurements is then considered to be due to absorption of hemoglobin.
However, the scattering of light varies with the concentration of hemoglobin in the sample, but the scattering of light is not only dependent on the concentration of hemoglobin. The scattering of light is due to light interaction with particles in the blood, such as red blood cells, white blood cells, and lipid particles. According to the invention, it has been found that by delaying the analysis, movements within the sample will settle and the effect of scattering in the sample will decrease. Thus, it has been unexpectedly found that calibration of a measurement instrument may be used to handle the scattering effects and that the concentration of hemoglobin in a sample may be directly related to the difference in absorption between the two absorption measurements.
The principle of an algorithm for determining the concentration of hemoglobin will now be described with reference to the schematic diagram in
According to the above, the results of the absorption measurements should be processed for determining the concentration of hemoglobin in the sample. This processing may be performed by a predetermined algorithm. This algorithm calculates the concentration of hemoglobin according to the above-described scheme.
The processing may determine the concentration of hemoglobin in the sample by computing the following formula:
[Tot Hb]=(Abs1−Abs2)·k1+k2
wherein [Tot Hb] is the total concentration of hemoglobin in the sample, Abs1 is the measured absorbance of the first absorption measurement, Abs2 is the measured absorbance of the second absorption measurement, and k1 and k2 are calibration coefficients, which depend on the measurement arrangement. The calibration coefficients k1 and k2 may be specific for each instrument used for hemoglobin determination.
The calibration coefficients may be determined by performing absorption measurements on a set of blood samples having known concentrations of hemoglobin. These calibration measurements may be performed when an instrument is manufactured. Further, calibration measurements may be performed at regular intervals in order to ensure that the instrument returns correct analysis results. Then, the calibration coefficients may be updated regularly to handle any differences in the performance of the instrument.
In
The delay may be achieved by simply not allowing absorption measurements to be performed until a pre-set period of time has passed from placement of the cuvette in a holder of the instrument. However, the delay may alternatively be achieved by allowing absorption measurements to be performed when it is confirmed that the drifting of the value of the absorption measurements has stopped. This may be done by monitoring the value of at least one of the absorption measurements for a period of time and, when the drifting has stopped, determining results of the absorption measurements to be used in processing.
Referring now to
Preferably, the first wavelength emitted by the means 10 for emitting light is in the range 500-510 nm, more preferably at 506 nm. Further, the second wavelength emitted by the means 10 for emitting light is preferably in the range 850-910 nm, and more preferably in the range 860-900 nm.
The system further comprises a cuvette holder 12 arranged to receive a capillary cuvette, which has an optical path length of less than 1 mm and holds a sample of unaltered whole blood. When a cuvette is placed in the holder 12, the optical window will be correctly positioned so that it will be irradiated with the light from the light source. Preferably, the cuvette holder 12 is arranged to receive a cuvette, which has an optical path length of less than 0.2 mm, and more preferably in the range 0.05-0.2 mm.
The system also comprises a controller 13 for creating a delay of a determined period of time between placement of the cuvette in the cuvette holder and performing absorption measurements. The controller 13 will thus ensure that a sufficient period of time passes from the acquiring of a sample into the cuvette and the performing of absorption measurements of the sample. This may be accomplished by means of a timer that provides a delay of a predetermined period of time. The timer 13 may receive input from a sensor 13a that detects when a cuvette is placed in the cuvette holder 12. The timer 13 may be arranged in a processing unit of the system in order to receive a clock signal for determining the period of time of the delay. When the predetermined period of time has passed, the timer 13 may transmit a signal to a control unit 13b, which controls the function of the light source 12. The control unit 13b is thus enabled such that absorption measurements may be initiated.
Alternatively, the controller comprises an analyser that monitors results of absorption measurements. The analyser may receive input from a detector 14 that detects light transmitted through the sample. When the analyser identifies that the result from the detector 14 becomes substantially constant, the analyser may conclude that the required period of time has passed. Thus, the results of the absorption measurements will now be stable and the controller may enable the control unit 13b such that the absorption measurements giving results to be processed may be initiated.
The light transmitted through the sample will be detected by a detector 14 so that a first absorption measurement may be obtained for light in the first range and a second absorption measurement may be obtained for light in the second range.
The system further comprises a processing unit 16 for processing results of the first and second absorption measurements to determine the concentration of hemoglobin in the sample according to the algorithm described above.
The system may suitably be implemented in a photometer comprising the means 10 for emitting light, the cuvette holder 12, and the detector 14. Photometers suitable for performing these measurements may be obtained by using photometers modified with suitable wave length filters and light emitting diodes. According to a preferred embodiment of the invention a photometer measures the absorbance at the two wavelengths and a built-in micro processor calculates, according to a programmed algorithm, the total concentration of hemoglobin in blood. Thus, no special absorption or interference filter which provide correction for variations in the detector sensitivity and in the effective optical path length as disclosed in WO 01/53806 are necessary.
In the above case, the processing unit 16 is embedded in the photometer. However, the processing unit 16 may also be connected to the photometer, and thus be implemented outside the photometer. For example, a computer connected to the photometer may be used.
The detector 14 may be arranged to detect essentially only directly transmitted light, since the scattered light need not be detected. This implies that the detector 14 detects light which is essentially within the diameter of the light beam irradiated on the sample and directly transmitted through the sample. Of course, some light may be scattered, while still being within this diameter. According to a preferred embodiment, the diameter of a detecting area of the detector 14 may typically be approximately 2 mm. The detector 14 is preferably arranged closer than 10 mm to the sample holder. This implies that light which has been scattered to small angles is detected.
The foregoing has been a description of a certain preferred embodiment of the present invention, but it is not intended to limit the invention in any way. Rather, many modifications, variations, and changes in details may be made within the scope of the present invention.
Number | Date | Country | Kind |
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0601025-0 | May 2006 | SE | national |
Filing Document | Filing Date | Country | Kind | 371c Date |
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PCT/SE2007/000406 | 4/27/2007 | WO | 00 | 10/17/2008 |