REAGENT AND METHOD FOR MEASURING HEMOGLOBINS

TECHNICAL FIELD

The present invention relates to a reagent for measuring hemoglobins including a surfactant. The present invention also relates to a method for measuring hemoglobins using the reagent for measuring hemoglobins.

BACKGROUND ART

Conventionally, the concentration of hemoglobins is measured for the diagnosis of diabetes, hemoglobinopathy and the like. For example, the concentration of hemoglobins including normal hemoglobins such as hemoglobin A1a, hemoglobin A1b, hemoglobin F, hemoglobin A1c, hemoglobin AG, and hemoglobin A2, modified hemoglobins such as acetylated hemoglobin and carbamylated hemoglobin, and abnormal hemoglobins such as hemoglobin S and hemoglobin C is measured. Among these hemoglobins, in particular, the value of hemoglobin A1c is measured. Examples of the method for measuring the concentration of hemoglobins mainly includes a liquid chromatography method.

In the liquid chromatography method, a hemolytic reagent is added to a sample such as blood, the sample after hemolysis is measured by cation exchange liquid chromatography, and the peak of the obtained chromatogram is arithmetically processed to determine the concentration of hemoglobins such as the value of hemoglobin A1c. Conventionally, as a hemolytic reagent, a composition containing polyoxyethylene octyl phenyl ether having an average number of moles of an oxyethylene group added of 10 (for example, trade name “Triton X-100”) is used.

Patent Document 1 below discloses a method for separating hemoglobin A1c for separating hemoglobin A1c in a sample of human blood from other glycosylated and non-glycosylated hemoglobins and a Schiff base of a precursor of hemoglobin A1c. In Example of Patent Document 1, a hemolytic reagent containing 0.33% by weight of Triton X-100 is used.

Patent Document 2 below discloses a hemolytic reagent used for hemolyzing a blood sample in a method for measuring hemoglobins by cation exchange liquid chromatography. The hemolytic reagent contains chaotropic ions. In Example of Patent Document 2, a hemolytic reagent containing 0.1% by weight of Triton X-100 is used.

RELATED ART DOCUMENT
Patent Documents

Patent Document 1: JP S58-191968 A

Patent Document 2: JP 2001-021555 A

SUMMARY OF THE INVENTION
Problems to be Solved by the Invention

Hemolytic reagents (reagents for measuring hemoglobins) including polyoxyethylene octyl phenyl ether having an average number of moles of an oxyethylene group added of 10 as described in Patent Documents 1 and 2 are excellent in hemolytic performance. Thus, when a sample such as whole blood is treated with such a hemolytic reagent and is measured by cation exchange liquid chromatography, a peak of hemoglobins is satisfactorily obtained. In addition, a shoulder peak and a split peak are less likely to occur in all the obtained peaks. Thus, hemoglobins can be measured with high accuracy.

Hemolytic reagents including polyoxyethylene octyl phenyl ether having an average number of moles of an oxyethylene group added of 10 cause less carryover in measurement by cation exchange liquid chromatography. Thus, even when a large number of samples are continuously measured, hemoglobins can be measured with high accuracy.

Meanwhile, in Europe, the REACH regulation (Registration, Evaluation, Authorization and Restriction of Chemicals) has come into effect in 2007, and the use of specific chemicals have been limited. In 2017, products containing 0.1% by weight or more of polyoxyethylene octyl phenyl ether having an average number of moles of an oxyethylene group added of 10 have become subject to the REACH regulation. Also, in countries other than Europe, reduction of the amount of polyoxyethylene octyl phenyl ether having an average number of moles of an oxyethylene group added of 10 used contributes to the reduction of the environmental load and the improvement of the safety of a human body.

An object of the present invention is to provide a reagent for measuring hemoglobins capable of satisfactorily causing hemolysis and measuring hemoglobins with high accuracy. More specifically, an object of the present invention is to provide a reagent for measuring hemoglobins capable of, without including polyoxyethylene octyl phenyl ether having an average number of moles of an oxyethylene group added of 10, causing hemolysis at a level equivalent to that of a reagent for measuring hemoglobins containing the component, and measuring hemoglobins with equivalent accuracy.

Another object of the present invention is to provide a method for measuring hemoglobins using the reagent for measuring hemoglobins.

Means for Solving the Problems

According to a broad aspect of the present invention, there is provided a reagent for measuring hemoglobins used for measuring hemoglobins by cation exchange liquid chromatography, including: a nonionic surfactant or an amphoteric surfactant, the nonionic surfactant being Component A1 below, Component A2 below, Component A3 below, Component A4 below, Component A5 below, Component A6 below, Component A7 below, Component A8 below, or Component A9 below, and the amphoteric surfactant being Component B1 below, Component B2 below, or Component B3 below.

Component A1: Polyoxyethylene alkyl ether having an average number of moles of an oxyethylene group added of 8 or more and 20 or less, and a carbon number of an alkyl group of 12 or more and 17 or less

Component A2: Polyoxyethylene stearyl ether having an average number of moles of an oxyethylene group added of 40 or more and 60 or less

Component A3: Polyoxyethylene oleyl ether having an average number of moles of an oxyethylene group added of 9 or more and 15 or less

Component A4: Polyoxyethylene-sec-alkyl ether having an average number of moles of an oxyethylene group added of 6 or more and 10 or less, and a carbon number of an alkyl group of 11 or more and 15 or less

Component A5: Polyoxyethylene tridecyl ether having an average number of moles of an oxyethylene group added of

Component A6: Polyoxyethylene polyoxypropylene alkyl ether having an HLB value of 11 or more and 15 or less

Component A7: n-nonanoyl-N-methyl-D-glucamine

Component A8: n-octyl-β-D-glucopyranoside

Component A9: Saponin

Component B1: 3-[(3-cholamidopropyl)dimethylammonio]propane sulfonate

Component B2: 3-[(3-cholamidopropyl)dimethylammonio]-2-hydroxypropane sulfonate

Component B3: Lauryl dimethylamine oxide

In a particular aspect of the reagent for measuring hemoglobins according to the present invention, the reagent for measuring hemoglobins includes the nonionic surfactant, the nonionic surfactant includes the Component A1, the Component A2, the Component A3, the Component A4, the Component A5, or the Component A6, the Component A1 is polyoxyethylene lauryl ether having an average number of moles of an oxyethylene group added of 9, 12, or 19, or polyoxyethylene cetyl ether having an average number of moles of an oxyethylene group added of 13 or 20, the Component A2 is polyoxyethylene stearyl ether having an average number of moles of an oxyethylene group added of 50, the Component A3 is polyoxyethylene oleyl ether having an average number of moles of an oxyethylene group added of 9 or 13, the Component A4 is polyoxyethylene-sec-alkyl ether having an average number of moles of an oxyethylene group added of 7 or 9 and a carbon number of an alkyl group of 11 or more and 15 or less, and the Component A6 is polyoxyethylene polyoxypropylene alkyl ether having an HLB value of 12.5, 12.7, or 14.0.

In a particular aspect of the reagent for measuring hemoglobins according to the present invention, the Component A1 is polyoxyethylene lauryl ether having an average number of moles of an oxyethylene group added of 12, or polyoxyethylene cetyl ether having an average number of moles of an oxyethylene group added of 13, and the Component A3 is polyoxyethylene oleyl ether having an average number of moles of an oxyethylene group added of 13.

In a particular aspect of the reagent for measuring hemoglobins according to the present invention, the reagent for measuring hemoglobins includes the nonionic surfactant, and the reagent for measuring hemoglobins has a content of the nonionic surfactant of 0.01% by weight or more and 1.0% by weight or less.

In a particular aspect of the reagent for measuring hemoglobins according to the present invention, the reagent for measuring hemoglobins includes the amphoteric surfactant, and the reagent for measuring hemoglobins has a content of the amphoteric surfactant of 0.01% by weight or more and 1.0% by weight or less.

According to a broad aspect of the present invention, there is provided a method for measuring hemoglobins, including the steps of: mixing an erythrocyte-containing sample and the reagent for measuring hemoglobins to obtain a mixed solution; and measuring the mixed solution by cation exchange liquid chromatography.

Effect of the Invention

The reagent for measuring hemoglobins according to the present invention is used for measuring hemoglobins by cation exchange liquid chromatography. The reagent for measuring hemoglobins according to the present invention includes a nonionic surfactant or an amphoteric surfactant. In the reagent for measuring hemoglobins according to the present invention, the nonionic surfactant is any of Components A1 to A9 below, or the amphoteric surfactant is any of Components B1 to B3 below. Component A1: Polyoxyethylene alkyl ether having an average number of moles of an oxyethylene group added of 8 or more and 20 or less, and a carbon number of an alkyl group of 12 or more and 17 or less. Component A2: Polyoxyethylene stearyl ether having an average number of moles of an oxyethylene group added of 40 or more and 60 or less. Component A3: Polyoxyethylene oleyl ether having an average number of moles of an oxyethylene group added of 9 or more and 15 or less. Component A4: Polyoxyethylene-sec-alkyl ether having an average number of moles of an oxyethylene group added of 6 or more and 10 or less, and a carbon number of an alkyl group of 11 or more and 15 or less. Component A5: Polyoxyethylene tridecyl ether having an average number of moles of an oxyethylene group added of 15. Component A6: Polyoxyethylene polyoxypropylene alkyl ether having an HLB value of 11 or more and 15 or less. Component A7: n-nonanoyl-N-methyl-D-glucamine. Component A8: n-octyl-3-D-glucopyranoside. Component A9: Saponin. Component B1: 3-[(3-cholamidopropyl)dimethylammonio]propane sulfonate. Component B2: 3-[(3-cholamidopropyl)dimethylammonio]-2-hydroxypropane sulfonate. Component B3: Lauryl dimethylamine oxide. The reagent for measuring hemoglobins according to the present invention has the above-mentioned configuration, and thus is capable of satisfactorily causing hemolysis and measuring hemoglobins with high accuracy.

BRIEF DESCRIPTION OF DRAWINGS

FIG. 1 is an example of a chromatogram obtained when measurement is performed by cation exchange liquid chromatography using the reagent for measuring hemoglobins according to one embodiment of the present invention.

FIG. 2 is an example of a chromatogram obtained when measurement is performed by cation exchange liquid chromatography using a conventional reagent for measuring hemoglobins.

FIGS. 3(a) and 3(b) are examples of chromatograms for evaluating the shape of the peak of hemoglobin A0.

FIGS. 4(a) and 4(b) are examples of chromatograms for evaluating the peak shape of the first fraction.

FIGS. 5(a) to 5(c) are examples of chromatograms for evaluating the height of the peak of hemoglobin A0.

FIGS. 6 (a) and 6(b) are figures showing the relationship between the number of storage days and the value of hemoglobin A1c, and the relationship between the number of storage days and the variation in the value of hemoglobin A1c in a mixed solution of a reagent for measuring hemoglobins and whole blood.

FIGS. 7(a) and 7(b) are figures showing the relationship between the number of storage days and the value of hemoglobin A1c, and the relationship between the number of storage days and the variation in the value of hemoglobin A1c in a mixed solution of a reagent for measuring hemoglobins and a hemoglobin A1c substance for measurement control (low concentration) (IRC-L).

FIGS. 8(a) and 8(b) are figures showing the relationship between the number of storage days and the value of hemoglobin A1c, and the relationship between the number of storage days and the variation in the value of hemoglobin A1c in a mixed solution of a reagent for measuring hemoglobins and a hemoglobin A1c substance for measurement control (high concentration) (IRC-H).

FIGS. 9(a) and 9(b) are figures showing column durability in a mixed solution of a reagent for measuring hemoglobins and a hemoglobin A1c substance for measurement control (high concentration) (IRC-H).

MODES FOR CARRYING OUT THE INVENTION

Hereinafter, the present invention will be described in detail.

In the reagent for measuring hemoglobins according to the present invention, the nonionic surfactant is polyoxyethylene alkyl ether having an average number of moles of an oxyethylene group added of 8 or more and 20 or less, and a carbon number of an alkyl group of 12 or more and 17 or less, polyoxyethylene stearyl ether having an average number of moles of an oxyethylene group added of 40 or more and 60 or less, polyoxyethylene oleyl ether having an average number of moles of an oxyethylene group added of 9 or more and 15 or less, polyoxyethylene-sec-alkyl ether having an average number of moles of an oxyethylene group added of 6 or more and 10 or less, and a carbon number of an alkyl group of 11 or more and 15 or less, polyoxyethylene tridecyl ether having an average number of moles of an oxyethylene group added of 15, polyoxyethylene polyoxypropylene alkyl ether having an HLB value of 11 or more and 15 or less, n-nonanoyl-N-methyl-D-glucamine, n-octyl-β-D-glucopyranoside, or saponin.

In the reagent for measuring hemoglobins according to the present invention, the amphoteric surfactant is 3-[(3-cholamidopropyl)dimethylammonio]propane sulfonate, 3-[(3-cholamidopropyl)dimethylammonio]-2-hydroxypropane sulfonate, or lauryl dimethylamine oxide.

In the present specification, “Polyoxyethylene alkyl ether having an average number of moles of an oxyethylene group added of 8 or more and 20 or less, and a carbon number of an alkyl group of 12 or more and 17 or less” may be referred to as “Component A1”.

In the present specification, for Component A1, “polyoxyethylene alkyl ether having an average number of moles of an oxyethylene group added of 10 or more and 15 or less, and a carbon number of an alkyl group of 12 or more and 17 or less” may be referred to as “Component A1′”.

In the present specification, “Polyoxyethylene stearyl ether having an average number of moles of an oxyethylene group added of 40 or more and 60 or less” may be referred to as “Component A2”.

In the present specification, “Polyoxyethylene oleyl ether having an average number of moles of an oxyethylene group added of 9 or more and 15 or less” may be referred to as “Component A3”.

In the present specification, for Component A3, “Polyoxyethylene oleyl ether having an average number of moles of an oxyethylene group added of 10 or more and 15 or less” may be referred to as “Component A3′”.

In the present specification, “Polyoxyethylene-sec-alkyl ether having an average number of moles of an oxyethylene group added of 6 or more and 10 or less, and a carbon number of an alkyl group of 11 or more and 15 or less” may be referred to as “Component A4”.

In the present specification, “Polyoxyethylene tridecyl ether having an average number of moles of an oxyethylene group added of 15” may be referred to as “Component A5”.

In the present specification, “Polyoxyethylene polyoxypropylene alkyl ether having an HLB value of 11 or more and 15 or less” may be referred to as “Component A6”.

In the present specification, “n-nonanoyl-N-methyl-D-glucamine” may be referred to as “Component A7”.

In the present specification, “n-octyl-@-D-glucopyranoside” may be referred to as “Component A8”.

In the present specification, “Saponin” may be referred to as “Component A9”.

In the present specification, “3-[(3-cholamidopropyl)dimethylammonio]propane sulfonate” may be referred to as “Component B1”.

In the present specification, “3-[(3-cholamidopropyl)dimethylammonio]-2-hydroxypropane sulfonate” may be referred to as “Component B2”.

In the present specification, “Lauryl dimethylamine oxide” may be referred to as “Component B3”.

In the present specification, “Polyoxyethylene octyl phenyl ether having an average number of moles of an oxyethylene group added of 10” may be referred to as “Component X”.

The reagent for measuring hemoglobins according to the present invention includes a nonionic surfactant or an amphoteric surfactant, and the nonionic surfactant is Component A1, Component A2, Component A3, Component A4, Component A5, Component A6, Component A7, Component A8, or Component A9, or the amphoteric surfactant is Component B1, Component B2, or Component B3.

The reagent for measuring hemoglobins according to the present invention has the above-mentioned configuration, and thus is capable of satisfactorily causing hemolysis and measuring hemoglobins with high accuracy.

A conventional reagent for measuring hemoglobins including Component X is capable of satisfactorily causing hemolysis and measuring hemoglobins with high accuracy. On the other hand, a reagent for measuring hemoglobins not including Component X is not capable of satisfactorily causing hemolysis and measuring hemoglobins with high accuracy.

In contrast, the reagent for measuring hemoglobins according to the present invention has the above-mentioned configuration, and thus is capable of, without including Component X, causing hemolysis at a level equivalent to that of a reagent for measuring hemoglobins including Component X, and measuring hemoglobins with equivalent accuracy.

The reagent for measuring hemoglobins according to the present invention is capable of satisfactorily causing hemolysis, and thus the peak of hemoglobins can be satisfactorily obtained when measurement is performed by cation exchange liquid chromatography. In addition, a shoulder peak and a split peak are less likely to occur in all the obtained peaks. Thus, hemoglobins can be measured with high accuracy. With the reagent for measuring hemoglobins according to the present invention, carryover can be reduced. Thus, even when a large number of samples are continuously measured, hemoglobins can be measured with high accuracy.

At a test center, after a hemolytic reagent (a reagent for measuring hemoglobins) and a substance to be tested are mixed, the mixed solution may be stored for a certain period (for example, several days) before the mixed solution is measured by cation exchange chromatography. The reagent for measuring hemoglobins according to the present invention can increase the storage stability of a mixed solution obtained by mixing the reagent and the substance to be tested. The substance to be tested includes, in addition to an erythrocyte-containing sample such as blood (for example, blood of a subject), a hemoglobin-containing sample without an erythrocyte (for example, a standard substance for hemoglobins and a hemoglobin substance for measurement control). With the reagent for measuring hemoglobins according to the present invention, even when the mixed solution is stored for a certain period of time, the peak shape of hemoglobins is less likely to change before and after storage, and the measurement value is less likely to vary.

Particularly, when the reagent for measuring hemoglobins according to the present invention includes Component A1′ or Component A3′, the storage stability of the mixed solution obtained by mixing the reagent for measuring hemoglobins and the substance to be tested can be further increased, and the storage stability of the reagent for measuring hemoglobins can also be increased.

Examples of the hemoglobins include normal hemoglobins such as hemoglobin A1a, hemoglobin A1b, hemoglobin F, hemoglobin A1c, hemoglobin A0, and hemoglobin A2, modified hemoglobins such as acetylated hemoglobin and carbamylated hemoglobin, and abnormal hemoglobins such as hemoglobin S and hemoglobin C.

The reagent for measuring hemoglobins according to the present invention is suitably used for measuring the value of the hemoglobin A1c (the concentration of hemoglobin A1c).

FIG. 2 is an example of a chromatogram obtained when measurement is performed by cation exchange liquid chromatography using a conventional reagent for measuring hemoglobins (a conventional reagent for measuring hemoglobins including Component X).

In FIGS. 1 and 2, the peak detected at about 19 seconds is the peak of hemoglobin A1c, and the peak detected at about 40 seconds is the peak of hemoglobin AG. FIGS. 1 and 2 are, for example, examples of chromatograms when measurement is performed under the measurement conditions used in Examples below.

With the reagent for measuring hemoglobins according to the present invention, a peak shape equivalent to that of a conventional reagent for measuring hemoglobins including Component X can be obtained.

With the reagent for measuring hemoglobins according to the present invention, a component that is subject to the REACH regulation can be eliminated, and thus the influence on the environment can be reduced and the safety can be increased compared to the conventional reagent for measuring hemoglobins including Component X.

The reagent for measuring hemoglobins according to the present invention can include the nonionic surfactant, can include the amphoteric surfactant, or can include both of the nonionic surfactant and the amphoteric surfactant.

(Nonionic Surfactant)

The reagent for measuring hemoglobins preferably includes a nonionic surfactant. The nonionic surfactant is any of Components A1 to A9. As the above-mentioned nonionic surfactant, only one of Components A1 to A9 can be used, or two or more can be used in combination.

Component A1 is polyoxyethylene alkyl ether having an average number of moles of an oxyethylene group added of 8 or more and 20 or less, and a carbon number of an alkyl group of 12 or more and 17 or less. Component A1 is a component represented by the formula (1) below. As Component A1, only one type can be used, or two or more types can be used in combination.

R—O(CH₂CH₂O)_nH (1)

In the formula (1) above, R represents an alkyl group having 12 or more and 17 or less carbon atoms, and n represents a number of 8 or more and 20 or less.

In the case of polyoxyethylene alkyl ether having an average number of moles of an oxyethylene group added of less than 8 and a carbon number of an alkyl group of less than 12, the surfactant is less likely to dissolve and a reagent for measuring hemoglobins may not be prepared. In the case of polyoxyethylene alkyl ether having an average number of moles of an oxyethylene group added of less than 8 and a carbon number of an alkyl group of less than 12, a good peak may not be obtained. In the case of polyoxyethylene alkyl ether having an average number of moles of an oxyethylene group added of more than 20 and a carbon number of an alkyl group of more than 17, a good peak may not be obtained or carryover may occur.

From the viewpoint of effectively exhibiting the effect of the present invention, and from the viewpoint of increasing the storage stability of the mixed solution obtained by mixing the reagent for measuring hemoglobins and the substance to be tested, the carbon number of the alkyl group of Component A1 is preferably 17 or less, more preferably 16 or less, and particularly preferably 12 or 16. When the carbon number of the alkyl group is 12, Component A1 is polyoxyethylene lauryl ether, and when the carbon number of the alkyl group is 16, Component A1 is polyoxyethylene cetyl ether.

Thus, Component A1 is particularly preferably polyoxyethylene lauryl ether having an average number of moles of an oxyethylene group added of 8 or more and 20 or less, or polyoxyethylene cetyl ether having an average number of moles of an oxyethylene group added of 8 or more and 20 or less.

When Component A1 is polyoxyethylene lauryl ether, the average number of moles of an oxyethylene group added in the polyoxyethylene lauryl ether is preferably 9 or more, more preferably 10 or more, further preferably 11 or more, and preferably 19 or less, more preferably 16 or less, further preferably 13 or less. The average number of moles of an oxyethylene group added in the polyoxyethylene lauryl ether is also preferably 9, 12, or 19, and most preferably 12. When the average number of moles of an oxyethylene group added is in the above-mentioned preferred range or value, the solubility of the surfactant can be further increased, the hemolysis can be satisfactorily performed, hemoglobins can be measured with even higher accuracy, and the storage stability of the mixed solution obtained by mixing the reagent for measuring hemoglobins and the substance to be tested can be further increased.

When Component A1 is polyoxyethylene cetyl ether, the average number of moles of an oxyethylene group added in the polyoxyethylene cetyl ether is preferably 10 or more, more preferably 12 or more, and preferably 19 or less, more preferably 16 or less, further preferably 14 or less. The average number of moles of an oxyethylene group added in the polyoxyethylene cetyl ether is also preferably 13 or 20, and most preferably 13. When the average number of moles of an oxyethylene group added is in the above-mentioned preferred range or value, the solubility of the surfactant can be further increased, the hemolysis can be satisfactorily performed, hemoglobins can be measured with even higher accuracy, and the storage stability of the mixed solution obtained by mixing the reagent for measuring hemoglobins and the substance to be tested can be further increased.

Thus, Component A1 is preferably polyoxyethylene lauryl ether having an average number of moles of an oxyethylene group added of 9, 12, or 19, or polyoxyethylene cetyl ether having an average number of moles of an oxyethylene group added of 13 or 20. Component A1 is most preferably polyoxyethylene lauryl ether having an average number of moles of an oxyethylene group added of 12, or polyoxyethylene cetyl ether having an average number of moles of an oxyethylene group added of 13.

From the viewpoint of effectively exhibiting the effect of the present invention, and from the viewpoint of increasing the storage stability of the reagent for measuring hemoglobins and the storage stability of the mixed solution obtained by mixing the reagent and the substance to be tested, Component A1 is preferably polyoxyethylene alkyl ether having an average number of moles of an oxyethylene group added of 10 or more and 15 or less, and a carbon number of an alkyl group of 12 or more and 17 or less. That is, Component A1 is preferably Component A1′.

The HLB (Hydrophilic Lipophilic Balance) value of Component A1 is preferably 10 or more, more preferably 12 or more, and preferably 18 or less, more preferably 16 or less. When the HLB value is greater than or equal to the lower limit, generation of micelles can be suppressed, and column clogging can be effectively suppressed. When the HLB value is less than or equal to the upper limit, the cell membrane of blood cell components can be sufficiently dissolved, and column clogging can be effectively suppressed.

The HLB value of Component A1 and the HLB value of each component described later are the HLB value determined by Griffin method. The HLB value is 0 or more and 20 or less. The smaller the HLB value, the stronger the hydrophobicity (lipophilicity), and the larger the HLB value, the stronger the hydrophilicity. The HLB value determined by Griffin method is calculated by the following formula.

HLB value=20×(molecular weight of hydrophilic group/molecular weight)

The clouding point of Component A1 is preferably 80° C. or more, more preferably 90° C. or more, and preferably 150° C. or less, more preferably 120° C. or less. When the clouding point is greater than or equal to the lower limit and less than or equal to the upper limit, the solubility of the surfactant can be increased, and the reagent for measuring hemoglobins can be sufficiently prepared.

The clouding point is the temperature at which a transparent or translucent liquid undergoes phase separation due to a temperature change, and as a result, the liquid becomes opaque. The clouding point is also generally referred to as the lower critical solution temperature.

The content of Component A1 is preferably 0.01% by weight or more, more preferably 0.05% by weight or more, further preferably 0.08% by weight or more, particularly preferably 0.1% by weight or more in 100% by weight of the reagent for measuring hemoglobins. The content of Component A1 is preferably 1.0% by weight or less, more preferably 0.8% by weight or less, further preferably 0.6% by weight or less, particularly preferably 0.5% by weight or less in 100% by weight of the reagent for measuring hemoglobins. When the content of Component A1 is greater than or equal to the lower limit and less than or equal to the upper limit, the effect of the present invention can be even more effectively exhibited, and the storage stability of the mixed solution obtained by mixing the reagent for measuring hemoglobins and the substance to be tested can be further increased.

Examples of the commercially available product of Component A1 include “EMULGEN 109P” manufactured by Kao Corporation (polyoxyethylene lauryl ether having an average number of moles of an oxyethylene group added of 9, polyoxyethylene (9) lauryl ether), “EMULGEN 120” manufactured by Kao Corporation (polyoxyethylene lauryl ether having an average number of moles of an oxyethylene group added of 12, polyoxyethylene (12) lauryl ether), “EMULGEN 147” manufactured by Kao Corporation (polyoxyethylene lauryl ether having an average number of moles of an oxyethylene group added of 19, polyoxyethylene (19) lauryl ether), “EMULGEN 220” manufactured by Kao Corporation (polyoxyethylene cetyl ether having an average number of moles of an oxyethylene group added of 13, polyoxyethylene (13) cetyl ether), and “Brij (registered trademark) 58” manufactured by Sigma-Aldrich (polyoxyethylene cetyl ether having an average number of moles of an oxyethylene group added of 20, polyoxyethylene (20) cetyl ether).

Component A2 is polyoxyethylene stearyl ether having an average number of moles of an oxyethylene group added of 40 or more and 60 or less. Component A2 is a component represented by the formula (2) below. As Component A2, only one type can be used, or two or more types can be used in combination.

C₁₈H₃₇O(CH₂CH₂O)_nH (2)

In the formula (2) above, n represents a number of 40 or more and 60 or less.

In the case of polyoxyethylene stearyl ether having an average number of moles of an oxyethylene group added of less than 40, the surfactant is less likely to dissolve and a reagent for measuring hemoglobins may not be prepared. In the case of polyoxyethylene stearyl ether having an average number of moles of an oxyethylene group added of less than 40, a good peak may not be obtained. In the case of polyoxyethylene stearyl ether having an average number of moles of an oxyethylene group added of more than 60, a good peak may not be obtained or carryover may occur.

From the viewpoint of increasing the solubility of the surfactant, and from the viewpoint of satisfactorily causing hemolysis and measuring hemoglobins with high accuracy, the average number of moles of an oxyethylene group added in Component A2 is preferably 45 or more, and preferably 55 or less. From the viewpoint of further increasing the solubility of the surfactant, and from the viewpoint of even more satisfactorily causing hemolysis and measuring hemoglobins with even higher accuracy, the average number of moles of an oxyethylene group added in Component A2 is most preferably 50.

The HLB value of Component A2 is preferably 13 or more, more preferably 15 or more, and preferably 19 or less, more preferably 18 or less. When the HLB value is greater than or equal to the lower limit, generation of micelles can be suppressed, and column clogging can be effectively suppressed. When the HLB value is less than or equal to the upper limit, the cell membrane of blood cell components can be sufficiently dissolved, and column clogging can be effectively suppressed.

The HLB value of Component A2 can be determined by the above-mentioned method.

The clouding point of Component A2 is preferably 80° C. or more, more preferably 90° C. or more. When the clouding point is greater than or equal to the lower limit, the solubility of the surfactant can be increased, and the reagent for measuring hemoglobins can be sufficiently prepared.

The content of Component A2 is preferably 0.01% by weight or more, more preferably 0.05% by weight or more, further preferably 0.08% by weight or more, particularly preferably 0.1% by weight or more in 100% by weight of the reagent for measuring hemoglobins. The content of Component A2 is preferably 1.0% by weight or less, more preferably 0.8% by weight or less, further preferably 0.6% by weight or less, particularly preferably 0.5% by weight or less in 100% by weight of the reagent for measuring hemoglobins. When the content of Component A2 is greater than or equal to the lower limit and less than or equal to the upper limit, the effect of the present invention can be even more effectively exhibited.

Examples of the commercially available product of Component A2 include “EMULGEN 350” manufactured by Kao Corporation (polyoxyethylene stearyl ether having an average number of moles of an oxyethylene group added of 50, polyoxyethylene (50) stearyl ether).

Component A3 is polyoxyethylene oleyl ether having an average number of moles of an oxyethylene group added of 9 or more and 15 or less. Component A3 is a component represented by the formula (3) below. As Component A3, only one type can be used, or two or more types can be used in combination.

C₁₈H₃₅O(CH₂CH₂O)_nH (3)

In the formula (3) above, n represents a number of 9 or more and 15 or less.

In the case of polyoxyethylene oleyl ether having an average number of moles of an oxyethylene group added of less than 9, the surfactant is less likely to dissolve and a reagent for measuring hemoglobins may not be prepared. In the case of polyoxyethylene oleyl ether having an average number of moles of an oxyethylene group added of less than 9, a good peak may not be obtained. In the case of polyoxyethylene oleyl ether having an average number of moles of an oxyethylene group added of more than 15, a good peak may not be obtained or carryover may occur.

From the viewpoint of increasing the solubility of the surfactant, and from the viewpoint of satisfactorily causing hemolysis and measuring hemoglobins with high accuracy, the average number of moles of an oxyethylene group added in Component A3 is preferably 14 or less. From the viewpoint of further increasing the solubility of the surfactant, and from the viewpoint of even more satisfactorily causing hemolysis and measuring hemoglobins with even higher accuracy, the average number of moles of an oxyethylene group added in Component A3 is particularly preferably 9 or 13, most preferably 13.

From the viewpoint of effectively exhibiting the effect of the present invention, and from the viewpoint of increasing the storage stability of the reagent for measuring hemoglobins and the storage stability of the mixed solution obtained by mixing the reagent and the substance to be tested, Component A3 is preferably polyoxyethylene oleyl ether having an average number of moles of an oxyethylene group added of 10 or more and 15 or less. That is, Component A3 is preferably Component A3′.

The HLB value of Component A3 is preferably 10 or more, more preferably 12 or more, and preferably 17 or less, more preferably 15 or less. When the HLB value is greater than or equal to the lower limit, generation of micelles can be suppressed, and column clogging can be effectively suppressed. When the HLB value is less than or equal to the upper limit, the cell membrane of blood cell components can be sufficiently dissolved, and column clogging can be effectively suppressed.

The HLB value of Component A3 can be determined by the above-mentioned method.

The clouding point of Component A3 is preferably 50° C. or more, more preferably 85° C. or more, and preferably 100° C. or less, more preferably 95° C. or less. When the clouding point is greater than or equal to the lower limit and less than or equal to the upper limit, the solubility of the surfactant can be increased, and the reagent for measuring hemoglobins can be sufficiently prepared.

The content of Component A3 is preferably 0.01% by weight or more, more preferably 0.05% by weight or more, further preferably 0.08% by weight or more, particularly preferably 0.1% by weight or more in 100% by weight of the reagent for measuring hemoglobins. The content of Component A3 is preferably 1.0% by weight or less, more preferably 0.8% by weight or less, further preferably 0.6% by weight or less, particularly preferably 0.5% by weight or less in 100% by weight of the reagent for measuring hemoglobins. When the content of Component A3 is greater than or equal to the lower limit and less than or equal to the upper limit, the effect of the present invention can be even more effectively exhibited.

Examples of the commercially available product of Component A3 include “EMULGEN 409PV” manufactured by Kao Corporation (polyoxyethylene oleyl ether having an average number of moles of an oxyethylene group added of 9, polyoxyethylene (9) oleyl ether) and “EMULGEN 420” manufactured by Kao Corporation (polyoxyethylene oleyl ether having an average number of moles of an oxyethylene group added of 13, polyoxyethylene (13) oleyl ether).

Component A4 is polyoxyethylene-sec-alkyl ether having an average number of moles of an oxyethylene group added of 6 or more and 10 or less, and a carbon number of an alkyl group of 11 or more and 15 or less. Component A4 is a component represented by the formula (4) below. Component A4 is an adduct of ethylene oxide and a secondary alcohol having 11 to 15 carbon atoms. Component A4 is different from Component A1. As Component A4, only one type can be used, or two or more types can be used in combination.

C_mH_2m+1O(CH₂CH₂O)_nH (4)

In the formula (4) above, m represents a number of 11 or more and 15 or less, and n represents a number of 6 or more and 10 or less.

In the case of polyoxyethylene-sec-alkyl ether having an average number of moles of an oxyethylene group added of less than 6 and a carbon number of an alkyl group of 11 or more and 15 or less, the surfactant is less likely to dissolve and a reagent for measuring hemoglobins may not be prepared. In addition, in the case of polyoxyethylene-sec-alkyl ether having an average number of moles of an oxyethylene group added of less than 6 and a carbon number of an alkyl group of 11 or more and 15 or less, a good peak may not be obtained.

The HLB value of Component A4 is preferably 10 or more, more preferably 12 or more, and preferably 17 or less, more preferably 15 or less. When the HLB value is greater than or equal to the lower limit, generation of micelles can be suppressed, and column clogging can be effectively suppressed. When the HLB value is less than or equal to the upper limit, the cell membrane of blood cell components can be sufficiently dissolved, and column clogging can be effectively suppressed.

The HLB value of Component A4 can be determined by the above-mentioned method.

The clouding point of Component A4 is preferably 30° C. or more, and preferably 60° C. or less. When the clouding point is greater than or equal to the lower limit and less than or equal to the upper limit, the solubility of the surfactant can be increased, and the reagent for measuring hemoglobins can be sufficiently prepared.

The content of Component A4 is preferably 0.01% by weight or more, more preferably 0.05% by weight or more, further preferably 0.08% by weight or more, particularly preferably 0.1% by weight or more in 100% by weight of the reagent for measuring hemoglobins. The content of Component A4 is preferably 1.0% by weight or less, more preferably 0.8% by weight or less, further preferably 0.6% by weight or less, particularly preferably 0.5% by weight or less in 100% by weight of the reagent for measuring hemoglobins. When the content of Component A4 is greater than or equal to the lower limit and less than or equal to the upper limit, the effect of the present invention can be even more effectively exhibited.

Examples of the commercially available product of Component A4 include “EMULGEN 707” manufactured by Kao Corporation (polyoxyethylene-sec-alkyl ether having an average number of moles of an oxyethylene group added of 7 and a carbon number of an alkyl group of 11 or more and 15 or less) and “EMULGEN 709” manufactured by Kao Corporation (polyoxyethylene-sec-alkyl ether having an average number of moles of an oxyethylene group added of 9 and a carbon number of an alkyl group of 11 or more and 15 or less).

Component A5 is polyoxyethylene tridecyl ether having an average number of moles of an oxyethylene group added of 15. Component A5 is a component represented by the formula (5) below. As Component A5, only one type can be used, or two or more types can be used in combination.

C₁₃H₂₇O(CH₂CH₂O)₁₅H (5)

The content of Component A5 is preferably 0.01% by weight or more, more preferably 0.05% by weight or more, further preferably 0.08% by weight or more, particularly preferably 0.1% by weight or more in 100% by weight of the reagent for measuring hemoglobins. The content of Component A5 is preferably 1.0% by weight or less, more preferably 0.8% by weight or less, further preferably 0.6% by weight or less, particularly preferably 0.5% by weight or less in 100% by weight of the reagent for measuring hemoglobins. When the content of Component A5 is greater than or equal to the lower limit and less than or equal to the upper limit, the effect of the present invention can be even more effectively exhibited.

Examples of the commercially available product of Component A5 include “LEOCOL TD-150” manufactured by Lion Corporation.

Component A6 is polyoxyethylene polyoxypropylene alkyl ether having an HLB value of 11 or more and 15 or less. The polyoxyethylene polyoxypropylene alkyl ether has an oxypropylene group and an oxyethylene group. Component A6 is a component represented by the formula (6) below. As Component A6, only one type can be used, or two or more types can be used in combination.

R—(CH₂CH(CH₃)O)_m(CH₂CH₂O)_nH (6)

In the formula (6) above, R represents an alkyl group, m represents a number of 1 or more, and n represents a number of 1 or more.

The HLB value of Component A6 is preferably 11.5 or more, more preferably 12 or more, and preferably 14.5 or less. When the HLB value is greater than or equal to the lower limit, generation of micelles can be suppressed, and column clogging can be effectively suppressed. When the HLB value is less than or equal to the upper limit, the cell membrane of blood cell components can be sufficiently dissolved, and column clogging can be effectively suppressed. From the viewpoint of even more effectively exhibiting the effects of the present invention, and from the viewpoint of even more effectively suppressing the column clogging, the HLB value of Component A6 is preferably 12.5, 12.7, or 14.0.

The HLB value of Component A6 can be determined by the above-mentioned method.

The clouding point of Component A6 is preferably 30° C. or more, more preferably 50° C. or more, and preferably 95° C. or less, more preferably 90° C. or less. When the clouding point is greater than or equal to the lower limit and less than or equal to the upper limit, the solubility of the surfactant can be increased, and the reagent for measuring hemoglobins can be sufficiently prepared.

The content of Component A6 is preferably 0.01% by weight or more, more preferably 0.05% by weight or more, further preferably 0.08% by weight or more, particularly preferably 0.1% by weight or more in 100% by weight of the reagent for measuring hemoglobins. The content of Component A6 is preferably 1.0% by weight or less, more preferably 0.8% by weight or less, further preferably 0.6% by weight or less, particularly preferably 0.5% by weight or less in 100% by weight of the reagent for measuring hemoglobins. When the content of Component A6 is greater than or equal to the lower limit and less than or equal to the upper limit, the effect of the present invention can be even more effectively exhibited.

Examples of the commercially available product of Component A6 include “EMULGEN LS-106” manufactured by Kao Corporation (polyoxyethylene polyoxypropylene alkyl ether having an HLB value of 12.5), “EMULGEN LS-114” manufactured by Kao Corporation (polyoxyethylene polyoxypropylene alkyl (C12 to 14) ether having an HLB value of 14.0), and “EMULGEN MS-110” manufactured by Kao Corporation (polyoxyethylene polyoxypropylene alkyl ether having an HLB value of 12.7).

Component A7 is n-nonanoyl-N-methyl-D-glucamine.

The content of Component A7 is preferably 0.01% by weight or more, more preferably 0.05% by weight or more, further preferably 0.08% by weight or more, particularly preferably 0.1% by weight or more in 100% by weight of the reagent for measuring hemoglobins. The content of Component A7 is preferably 1.0% by weight or less, more preferably 0.8% by weight or less, further preferably 0.6% by weight or less, particularly preferably 0.5% by weight or less in 100% by weight of the reagent for measuring hemoglobins. When the content of Component A7 is greater than or equal to the lower limit and less than or equal to the upper limit, the effect of the present invention can be even more effectively exhibited.

Examples of the commercially available product of Component A7 include “MEGA-9” manufactured by Dojindo Molecular Technologies, Inc.

Component A8 is n-octyl-β-D-glucopyranoside.

The content of Component A8 is preferably 0.01% by weight or more, more preferably 0.05% by weight or more, further preferably 0.08% by weight or more, particularly preferably 0.1% by weight or more in 100% by weight of the reagent for measuring hemoglobins. The content of Component A8 is preferably 1.0% by weight or less, more preferably 0.8% by weight or less, further preferably 0.6% by weight or less, particularly preferably 0.5% by weight or less in 100% by weight of the reagent for measuring hemoglobins. When the content of Component A8 is greater than or equal to the lower limit and less than or equal to the upper limit, the effect of the present invention can be even more effectively exhibited.

Examples of the commercially available product of Component A8 include “n-octyl-β-D-glucopyranoside” manufactured by Dojindo Molecular Technologies, Inc.

Component A9 is saponin. As Component A9, only one type can be used, or two or more types can be used in combination.

Component A9 is preferably soybean saponin, more preferably soybean saponin represented by the formula (9) below.

embedded image

The content of Component A9 is preferably 0.01% by weight or more, more preferably 0.05% by weight or more, further preferably 0.08% by weight or more, particularly preferably 0.1% by weight or more in 100% by weight of the reagent for measuring hemoglobins. The content of Component A9 is preferably 1.0% by weight or less, more preferably 0.8% by weight or less, further preferably 0.6% by weight or less, particularly preferably 0.5% by weight or less in 100% by weight of the reagent for measuring hemoglobins. When the content of Component A9 is greater than or equal to the lower limit and less than or equal to the upper limit, the effect of the present invention can be even more effectively exhibited.

Examples of the commercially available product of Component A9 include “Saponin” manufactured by NACALAI TESQUE, INC.

(Amphoteric Surfactant)

The reagent for measuring hemoglobins preferably includes an amphoteric surfactant. The surfactant is any of Components B1 to B3. As the above-mentioned amphoteric surfactant, only one of Components B1 to B3 can be used, or two or more can be used in combination.

Component B1 is 3-[(3-cholamidopropyl)dimethylammonio]propane sulfonate (CHAPS).

The content of Component B1 is preferably 0.01% by weight or more, more preferably 0.05% by weight or more, further preferably 0.08% by weight or more, particularly preferably 0.1% by weight or more in 100% by weight of the reagent for measuring hemoglobins. The content of Component B1 is preferably 1.0% by weight or less, more preferably 0.8% by weight or less, further preferably 0.6% by weight or less, particularly preferably 0.5% by weight or less in 100% by weight of the reagent for measuring hemoglobins. When the content of Component B1 is greater than or equal to the lower limit and less than or equal to the upper limit, the effect of the present invention can be even more effectively exhibited.

Examples of the commercially available product of Component B1 include “CHAPS” manufactured by Dojindo Molecular Technologies, Inc.

Component B2 is 3-[(3-cholamidopropyl)dimethylammonio]-2-hydroxypropane sulfonate (CHAPSO).

The content of Component B2 is preferably 0.01% by weight or more, more preferably 0.05% by weight or more, further preferably 0.08% by weight or more, particularly preferably 0.1% by weight or more in 100% by weight of the reagent for measuring hemoglobins. The content of Component B2 is preferably 1.0% by weight or less, more preferably 0.8% by weight or less, further preferably 0.6% by weight or less, particularly preferably 0.5% by weight or less in 100% by weight of the reagent for measuring hemoglobins. When the content of Component B2 is greater than or equal to the lower limit and less than or equal to the upper limit, the effect of the present invention can be even more effectively exhibited.

Examples of the commercially available product of Component B2 include “CHAPSO” manufactured by Dojindo Molecular Technologies, Inc.

Component B3 is lauryl dimethylamine oxide.

The content of Component B3 is preferably 0.01% by weight or more, more preferably 0.05% by weight or more, further preferably 0.08% by weight or more, particularly preferably 0.1% by weight or more in 100% by weight of the reagent for measuring hemoglobins. The content of Component B3 is preferably 1.0% by weight or less, more preferably 0.8% by weight or less, further preferably 0.6% by weight or less, particularly preferably 0.5% by weight or less in 100% by weight of the reagent for measuring hemoglobins. When the content of Component B3 is greater than or equal to the lower limit and less than or equal to the upper limit, the effect of the present invention can be even more effectively exhibited.

Examples of the commercially available product of Component B3 include “AMPHITOL 20N” manufactured by Kao Corporation.

(Buffering Agent)

The reagent for measuring hemoglobins preferably includes a buffering agent. By inclusion of the buffering agent, variation in pH can be suppressed. As the buffering agent, only one type can be used, or two or more types can be used in combination.

Examples of the buffering agent include phosphates such as sodium phosphate, disodium hydrogen phosphate, sodium dihydrogen phosphate, potassium phosphate, dipotassium hydrogen phosphate, and potassium dihydrogen phosphate, carbonates such as sodium carbonate and sodium hydrogen carbonate, borate such as sodium borate, and carboxylic acid, dicarboxylic acid, carboxylic acid derivative, hydroxycarboxylic acid, aniline, aniline derivative, amino acid, an amine compound, an imidazole compound, an alcohol compound, ethylenediaminetetraacetic acid, pyrophosphoric acid, pyridine, cacodylic acid, glycerol phosphate, 2,4,6-collidine, N-ethylmorpholine, morpholine, 4-aminopyridine, ammonia, ephedrine, hydroxyproline, piperidine, tris(hydroxymethyl)aminomethane, and glycylglycine.

From the viewpoint of maintaining the pH of the reagent for measuring hemoglobins in a preferred range described below, the buffering agent is preferably phosphate.

The content of the buffering agent in the reagent for measuring hemoglobins is not particularly limited as long as buffer action is exhibited. The content of the buffering agent can be 0.01% by weight or more, can be 0.02% by weight or more, and can be 0.2% by weight or less, 0.1% by weight or less in 100% by weight of the reagent for measuring hemoglobins.

(Inorganic Salt)

The reagent for measuring hemoglobins preferably includes an inorganic salt. By inclusion of the inorganic salt, the osmotic pressure can be satisfactorily adjusted. As the inorganic salt, only one type can be used, or two or more types can be used in combination.

Examples of the inorganic salt include sodium chloride, potassium chloride, sodium sulfate, and potassium sulfate.

From the viewpoint of maintaining the osmotic pressure of the reagent for measuring hemoglobins in the preferred range described below, the inorganic salt is preferably sodium chloride, potassium chloride, sodium sulfate, or potassium sulfate, and more preferably sodium chloride.

The content of the inorganic salt in the reagent for measuring hemoglobins is not particularly limited. The content of the inorganic salt can be 0.1% by weight or more, and can be 1.0% by weight or less in 100% by weight of the reagent for measuring hemoglobins.

(Water)

The reagent for measuring hemoglobins preferably includes water.

The content of water is preferably 80% by weight or more, more preferably 90% by weight or more, further preferably 95% by weight in 100% by weight of the reagent for measuring hemoglobins.

(Other Components)

The reagent for measuring hemoglobins can include other components other than the above-mentioned components. Examples of the other components include a preservative, a hemoglobin stabilizer, and a pH adjuster. As the other components, only one type can be used, or two or more types can be used in combination.

Examples of the preservative include sodium azide, thymol, and sodium propionate.

Examples of the hemoglobin stabilizer include chelating agents such as ethylenediaminetetraacetic acid (EDTA), and glutathione.

Examples of the pH adjuster include acids such as hydrochloric acid, phosphoric acid, nitric acid, and sulfuric acid, and bases such as sodium hydroxide, potassium hydroxide, lithium hydroxide, magnesium hydroxide, barium hydroxide, and calcium hydroxide.

(Other Details of Reagent for Measuring Hemoglobins)

The reagent for measuring hemoglobins preferably includes the nonionic surfactant, more preferably includes, as the nonionic surfactant, Component A1, Component A2, Component A3, Component A4, Component A5, or Component A6, further preferably includes Component A1 or Component A3, and particularly preferably includes Component A1′ or Component A3′. In this case, the effect of the present invention can be even more effectively exhibited. The storage stability of the mixed solution obtained by mixing the reagent for measuring hemoglobins and the substance to be tested can be further increased.

When the reagent for measuring hemoglobins includes the nonionic surfactant, the content of the nonionic surfactant (the total content of Components A1 to A9) is preferably 0.01% by weight or more, more preferably 0.05% by weight or more, further preferably 0.08% by weight or more, and particularly preferably 0.1% by weight or more in 100% by weight of the reagent for measuring hemoglobins. The content of the nonionic surfactant (the total content of Components A1 to A9) is preferably 1.0% by weight or less, more preferably 0.8% by weight or less, further preferably 0.6% by weight or less, particularly preferably 0.5% by weight or less in 100% by weight of the reagent for measuring hemoglobins. When the content of the nonionic surfactant (the total content of Components A1 to A9) is greater than or equal to the lower limit and less than or equal to the upper limit, the effect of the present invention can be even more effectively exhibited. The storage stability of the mixed solution obtained by mixing the reagent for measuring hemoglobins and the substance to be tested can be further increased.

When the reagent for measuring hemoglobins includes the amphoteric surfactant, the content of the amphoteric surfactant (the total content of Components B1 to B3) is preferably 0.01% by weight or more, more preferably 0.05% by weight or more, further preferably 0.08% by weight or more, and particularly preferably 0.1% by weight or more in 100% by weight of the reagent for measuring hemoglobins. The content of the amphoteric surfactant (the total content of Components B1 to B3) is preferably 1.0% by weight or less, more preferably 0.8% by weight or less, further preferably 0.6% by weight or less, particularly preferably 0.5% by weight or less in 100% by weight of the reagent for measuring hemoglobins. When the content of the amphoteric surfactant (the total content of Components B1 to B3) is greater than or equal to the lower limit and less than or equal to the upper limit, the effect of the present invention can be even more effectively exhibited.

The reagent for measuring hemoglobins preferably does not include Component X. In the present invention, the effects of the present invention can be exhibited without including Component X. In the present invention, the storage stability of the mixed solution obtained by mixing the reagent for measuring hemoglobins and the substance to be tested can be increased without including Component X. However, the reagent for measuring hemoglobins can include Component X. For example, the reagent for measuring hemoglobins can include Component X at a concentration not subject to the REACH regulation (the content of Component X of less than 0.1% by weight in 100% by weight of the reagent for measuring hemoglobins).

The pH of the reagent for measuring hemoglobins is preferably 6.0 or more, more preferably 7.0 or more, and preferably 8.5 or less, more preferably 8.0 or less. When the pH is greater than or equal to the lower limit and less than or equal to the upper limit, hemolysis can be even more satisfactorily caused.

The osmotic pressure of the reagent for measuring hemoglobins is preferably 50 mOsm or more, more preferably 75 mOsm or more, and preferably 200 mOsm or less, more preferably 150 mOsm or less. When the osmotic pressure is greater than or equal to the lower limit and less than or equal to the upper limit, hemolysis can be even more satisfactorily caused.

The osmotic pressure can be measured using an osmometer (for example, “Osmometer 3250” manufactured by Advanced Instruments, Inc.).

The reagent for measuring hemoglobins is suitably used for hemolyzing erythrocyte. The reagent for measuring hemoglobins is preferably a hemolytic reagent.

The reagent for measuring hemoglobins is suitably mixed with a substance to be tested and used. Examples of the substance to be tested include an erythrocyte-containing sample such as blood, a standard substance for hemoglobins, and a hemoglobin substance for measurement control.

The reagent for measuring hemoglobins is suitably used as a diluting solution for dissolving or diluting a sample not containing erythrocyte and having a known hemoglobin concentration (a standard substance for hemoglobins, a hemoglobin substance for measurement control and the like). Further, the reagent for measuring hemoglobins is also suitably used as a washing liquid for a liquid chromatograph and a washing liquid for a column.

(Method for Measuring Hemoglobins)

The method for measuring hemoglobins according to the present invention includes the steps of: mixing an erythrocyte-containing sample and the reagent for measuring hemoglobins to obtain a mixed solution; and measuring the mixed solution by cation exchange liquid chromatography.

The cation exchange liquid chromatography is preferably cation exchange high performance liquid chromatography.

Examples of the erythrocyte-containing sample include blood.

Generally, in the cation exchange liquid chromatography, in addition to a mixed solution prepared from blood collected from a patient or the like (an erythrocyte-containing sample), a mixed solution prepared from a sample not containing erythrocyte and having a known concentration of hemoglobins to be measured is also measured. Examples of the sample not containing erythrocyte and having a known concentration of hemoglobins to be measured include a standard substance for hemoglobins to be measured (hemoglobins to be measured having a known concentration), and a hemoglobin substance for measurement control to be measured (hemoglobins to be measured having a known concentration; multiple concentrations such as a low concentration, a medium concentration, and a high concentration are preferably measured). The standard substance for hemoglobins and the hemoglobin substance for measurement control are preferably a sample prepared at time of use, a freeze-dried sample, or a frozen sample. The standard substance for hemoglobins and the hemoglobin substance for measurement control are commercially available as a freeze-dried product or a frozen product.

In the method for measuring hemoglobins, the concentration of hemoglobins is preferably determined, for example, as follows. (1) The erythrocyte-containing sample and the reagent for measuring hemoglobins are mixed to obtain a mixed solution. (2) The mixed solution is measured by cation exchange liquid chromatography. (3) The ratio of the peak area of hemoglobins to be measured to the total of the peak areas of hemoglobins (the peak area of hemoglobins to be measured/the total of the peak areas of hemoglobins) is taken as the hemoglobin value (the concentration of hemoglobins) to be measured. For example, when the value of hemoglobin A1c is determined, in the above (3), the ratio of the peak area of hemoglobin A1c to the total of the peak areas of hemoglobins (the peak area of hemoglobin A1c/the total of the peak areas of hemoglobins) is taken as the value of hemoglobin A1c.

In the method for measuring hemoglobins, the concentration of hemoglobins can also be determined, for example, as follows. (1) The erythrocyte-containing sample and the reagent for measuring hemoglobins are mixed to obtain a first mixed solution. (2) A hemoglobin-containing sample having a known concentration of hemoglobins to be measured and the reagent for measuring hemoglobins are mixed to obtain a second mixed solution. (3) The first mixed solution and the second mixed solution are measured by cation exchange liquid chromatography. (4) The measurement value obtained by measuring the mixed solution containing the hemoglobin-containing sample having a known concentration of hemoglobins to be measured by cation exchange liquid chromatography, and the measurement value obtained by measuring the mixed solution containing the erythrocyte-containing sample are compared to determine the concentration of hemoglobins in the erythrocyte-containing sample.

From the viewpoint of even more satisfactorily causing hemolysis, the reagent for measuring hemoglobins is preferably mixed in an amount of preferably 25 mL or more, more preferably 50 mL or more, and preferably 400 mL or less, more preferably 200 mL or less relative to 1 mL of the erythrocyte-containing sample.

In the cation exchange liquid chromatography, measurement is preferably performed by a salt concentration gradient or a pH gradient. The gradient can be a linear gradient or a step gradient.

Two or more eluents are preferably used in the gradient measurement. When measurement is performed by the salt concentration gradient, as the eluent, an eluent having a low salt concentration and an eluent having a high salt concentration (for example, an eluent having an NaCl concentration of 50 mM and an eluent having an NaCl concentration of 200 mM) can be used. When measurement is performed by the pH gradient, two types of eluents having different pHs (for example, an eluent at pH 5.4 and an eluent at pH 8.0) can be used. A commercially available product can also be used as the eluent. Examples of the commercially available product of the eluent include “Eluent 80A”, “Eluent 80B”, “Eluent 60A-VP/TP”, “Eluent 60B-VP/TP”, and “Eluent 60C-VP” manufactured by ARKRAY, Inc.

As the cation exchange column used in the cation exchange liquid chromatography, a conventionally known cation exchange column can be used. The cation exchange column is preferably a column packed with a packing material having a cation exchange group such as a carboxyl group, a sulfonic acid group, or a phosphoric acid group. Examples of the commercially available product of the cation exchange column include “COLUMN UNIT 80” and “COLUMN UNIT HSVI-VP” manufactured by ARKRAY, Inc.

Hereinafter, the present invention will be specifically described by giving Examples, Reference Example, and Comparative Examples. The present invention is not limited to the following Examples.

Examples 1 to 30, Reference Example A, and Comparative Examples 1 to 69

Preparation of reagent for measuring hemoglobins: Potassium dihydrogen phosphate, dipotassium hydrogen phosphate, sodium chloride, sodium azide, and water were mixed to obtain a first composition. Each surfactant shown in Tables 2 to 6 was added to the obtained first composition and the mixture was mixed to prepare a reagent for measuring hemoglobins. The composition of the obtained reagent for measuring hemoglobins is shown in Table 1 below. The type, the content, the HLB value, and the clouding point of the surfactant in Table 1 are shown in Tables 2 to 6. The HLB value of the surfactant is the value measured by the above-mentioned method.

TABLE 1

Content in 100% by

weight of reagent

for measuring

hemoglobins

Potassium dihydrogen phosphate
% by weight
0.013

Dipotassium hydrogen phosphate
% by weight
0.052

Sodium chloride
% by weight
0.233

Sodium azide
% by weight
0.02

Surfactant *
% by weight
*

Water
% by weight
Remainder

Total
% by weight
100

* Type and content of surfactants are shown in Tables 2 to 6.

(Evaluation)
(1) Solubility of Surfactant

The solubility of the surfactant when the surfactant was added to the first composition and the mixture was mixed was visually checked. The solubility of the surfactant was judged based on the following criteria.

[Criteria for Judging Solubility of Surfactant]

◯◯: Surfactant is completely dissolved in less than 15 minutes

◯: Surfactant is completely dissolved in 15 minutes or more and less than 30 minutes

Δ: Surfactant is completely dissolved in 30 minutes or more and less than 1 hour

x: Surfactant is completely dissolved in 1 hour or more, or is not dissolved

(2) Measurement by Cation Exchange Liquid Chromatography

Whole blood (erythrocyte-containing sample) contained in a blood collection tube (manufactured by SEKISUI MEDICAL CO., LTD.) was prepared. The obtained reagent for measuring hemoglobins (100 mL) was mixed with whole blood (1 mL) to obtain a mixed solution. The obtained mixed solution was measured under the following conditions. The reagent for measuring hemoglobins that had the judgement result of x in “(1) Solubility of surfactant” was not measured by cation exchange liquid chromatography.

Cation exchange chromatography conditions:

HPLC instrument: glycohemoglobin analyzer (“HA-8180” manufactured by ARKRAY, Inc.)

Cation exchange column: COLUMN UNIT 80 (manufactured by ARKRAY, Inc.)

Eluent A: ELUENT 80A (manufactured by ARKRAY, Inc.)

Eluent B: ELUENT 80B (manufactured by ARKRAY, Inc.)

The measurement was performed by the measurement method installed in the HPLC instrument.

(2-1) Peak Separation Pattern

The following i) to iii) were checked for the chromatogram obtained by measuring the mixed solution. In Reference Example A, a peak pattern of a chromatogram shown in FIG. 2 was obtained. In the obtained chromatogram, the peak detected at about 19 seconds is the peak of hemoglobin A1c, and the peak detected at about 40 seconds is the peak of hemoglobin A0.

i) Separation of Peak of Hemoglobin A1c

The peak height of hemoglobin A1c obtained in Reference Example A was compared with the peak height of hemoglobin A1c obtained in Examples and Comparative Examples. When the obtained peak height of hemoglobin A1c was decreased 50 or more based on absorbance compared with the peak height of hemoglobin A1c obtained in Reference Example A, the separation of the peak of hemoglobin A1c was judged to be good, and when it was decreased more than 50, it was judged to be bad.

ii) Shape of Peak of Hemoglobin A0

In Reference Example A, no peak was detected in the peak tail part of the peak of hemoglobin A0. The shape of the peak tail of the peak of hemoglobin A0 obtained in Examples and Comparative Examples was checked. In this peak tail part, when no peak was detected, the shape of the peak of hemoglobin A0 was judged to be good, and when a peak was detected, it was judged to be bad.

An example of a chromatogram judged to be good is shown in FIG. 3(a), and an example of a chromatogram judged to be bad is shown in FIG. 3(b).

iii) Peak Shape of First Fraction

In Reference Example A, no shoulder peak was detected in the peak of the first fraction. The peak shape of the fast fraction obtained in Examples and Comparative Examples was checked. In the peak of the first fraction, when no shoulder peak was detected, the peak shape of the first fraction was judged to be good, and when a shoulder peak was detected, it was judged to be bad.

An example of a chromatogram judged to be good is shown in FIG. 4(a), and an example of a chromatogram judged to be bad is shown in FIG. 4 (b). The peak indicated by the arrow in FIG. 4(b) is the shoulder peak.

[Criteria for Judging Peak Separation Pattern]

◯: All judgments in i) to iii) are good

x: Any of judgments in i) to iii) is bad

(2-2) Carryover

Following the measurement of the mixed solution obtained by mixing whole blood and the reagent for measuring hemoglobins, only the reagent for measuring hemoglobins was continuously measured 5 times. The following i) to iii) were checked for the obtained chromatogram.

i) Height of Peak of Hemoglobin A0

In the first measurement of the reagent for measuring hemoglobins, the peak height of hemoglobin A0 obtained in Reference Example A was compared with the peak height of hemoglobin A0 obtained in Examples and Comparative Examples. When the obtained peak height of hemoglobin A0 was not increased 100 or more based on absorbance compared with the peak height of hemoglobin A0 obtained in Reference Example A, the judgement of good was given, and when it was increased more than 100, the judgement of bad was given.

An example of the chromatogram obtained in Reference Example A is shown in FIG. 5(a), an example of a chromatogram judged to be good is shown in FIG. 5(b), and an example of a chromatogram judged to be bad is shown in FIG. 5(c).

ii) Presence or Absence of Peak of Hemoglobin A1c

In the first measurement of the reagent for measuring hemoglobins, the presence or absence of the peak of hemoglobin A1c was checked. When no peak of hemoglobin A1c was observed, the judgement of good was given, and when the peak of hemoglobin A1c was observed, the judgement of bad given.

iii) Presence or Absence of Drift Occurrence

In the first measurement of the reagent for measuring hemoglobins, the presence or absence of the drift of the peak of hemoglobin A0 was checked. When no drift was observed, the judgement of good was given, and when the drift was observed, the judgement of bad was given.

[Criteria for Judging Carryover]

◯: All judgments in i) to iii) are good

x: Any of judgments in i) to iii) is bad

(3) pH

The pH of the reagent for measuring hemoglobins obtained in Reference Example A and Examples was measured using a pH meter (“F-52” manufactured by HORIBA, Ltd.).

(4) Osmotic Pressure

The osmotic pressure of the reagent for measuring hemoglobins obtained in Reference Example A and Examples was measured using an osmometer (“Osmometer 3250” manufactured by Advanced Instruments, Inc.).

The compositions and results are shown in Tables 2 to 6 below. In Tables 2, 3, and 5, the value represented by “E.O.” means the average number of moles of an oxyethylene group added.

TABLE 2

Product

name
Manufacturer
Name of component

Reference
Nonionic
Component
Triton
NACALAI
Polyoxyethylene octyl phenyl ether

Example A
surfactant
X
X-100
TESQUE, INC.
(10 E.O.)

Comparative

Brij35
Sigma-
Polyoxyethylene lauryl ether

Example 1

Aldrich
(23 E.O.)

Comparative

EMULGEN
Kao
Polyoxyethylene lauryl ether

Example 2

103
Corporation
(3E.O.)

Comparative

EMULGEN
Kao
Polyoxyethylene lauryl ether

Example 3

104P
Corporation
(4E.O.)

Comparative

EMULGEN
Kao
Polyoxyethylene lauryl ether

Example 4

105
Corporation
(4E.O.)

Comparative

EMULGEN
Kao
Polyoxyethylene lauryl ether

Example 5

106
Corporation
(5E.O.)

Comparative

EMULGEN
Kao
Polyoxyethylene lauryl ether

Example 6

108
Corporation
(6E.O.)

Example 1

Component
EMULGEN
Kao
Polyoxyethylene lauryl ether

A1
109P
Corporation
(9E.O.)

Example 2

Component
EMULGEN
Kao
Polyoxyethylene lauryl ether

A1
120
Corporation
(12E.O.)

Example 3

Component
EMULGEN
Kao
Polyoxyethylene lauryl ether

A1
120
Corporation
(12E.O.)

Example 4

Component
EMULGEN
Kao
Polyoxyethylene lauryl ether

A1
147
Corporation
(19E.O.)

Comparative

EMULGEN
Kao
Polyoxyethylene lauryl ether

Example 7

123P
Corporation
(23 E.O.)

Comparative

EMULGEN
Kao
Polyoxyethylene lauryl ether

Example 8

130K
Corporation
(41E.O.)

Comparative

EMULGEN
Kao
Polyoxyethylene lauryl ether

Example 9

150
Corporation
(47E.O.)

Comparative

EMULGEN
Kao
Polyoxyethylene cetyl ether

Example 10

210P
Corporation
(7E.O.)

Example 5

Component
EMULGEN
Kao
Polyoxyethylene cetyl ether

A1
220
Corporation
(13E.O.)

Example 6

Component
EMULGEN
Kao
Polyoxyethylene cetyl ether

A1
220
Corporation
(13E.O.)

Example 7

Component
Brij58
Sigma-
Polyoxyethylene cetyl ether

A1

Aldrich
(20E.O.)

Comparative

EMULGEN
Kao
Polyoxyethylene stearyl ether

Example 11

306P
Corporation
(6E.O.)

Comparative

EMULGEN
Kao
Polyoxyethylene stearyl ether

Example 12

320P
Corporation
(12E.O.)

Example 8

Component
EMULGEN
Kao
Polyoxyethylene stearyl ether

A2
350
Corporation
(50E.O.)

Evaluation

Clouding

Peak

Osmotic

point
HLB

Solu-
separation
Carry-

pressure

(° C.)
value
Content
bility
pattern
over
pH
(mOsm)

Reference
66
13.5
0.1%
∘
∘
∘
7.50
100

Example A

Comparative
—
—
0.5%
Δ
x
x
—
—

Example 1

Comparative
—
8.1
0.5%
x
—
—
—
—

Example 2

Comparative
—
9.6
0.5%
x
—
—
—
—

Example 3

Comparative
—
9.7
0.5%
x
—
—
—
—

Example 4

Comparative
—
10.5
0.5%
x
—
—
—
—

Example 5

Comparative
40
12.1
0.5%
∘
x
x
—
—

Example 6

Example 1
83
13.6
0.5%
∘∘
∘
∘
7.26
101

Example 2
98
15.3
0.5%
∘
∘
∘
7.35
103

Example 3
98
15.3
0.1%
∘
∘
∘
7.35
103

Example 4
>100
16.3
0.5%
∘
∘
∘
7.32
104

Comparative
>100
16.9
0.5%
∘
x
x
—
—

Example 7

Comparative
>100
18.1
0.5%
∘
x
x
—
—

Example 8

Comparative
>100
18.4
0.5%
∘
x
x
—
—

Example 9

Comparative
—
10.7
0.5%
x
—
—
—
—

Example 10

Example 5
98
14.2
0.5%
Δ
∘
∘
7.36
100

Example 6
98
14.2
0.1%
Δ
∘
∘
7.36
100

Example 7
—
—
0.5%
Δ
∘
∘
7.34
101

Comparative
—
9.4
0.5%
x
—
—
—
—

Example 11

Comparative
91
13.9
0.5%
x
—
—
—
—

Example 12

Example 8
>100
17.8
0.5%
Δ
∘
∘
7.41
101

TABLE 3

Product

name
Manufacturer
Name of component

Comparative
Nonionic

EMULGEN 404
Kao
Polyoxyethylene oleyl ether

Example 13
surfactant

Corporation
(4E.O.)

Comparative

EMULGEN 408
Kao
Polyoxyethylene oleyl ether

Example 14

Corporation
(8E.O.)

Example 9

Component
EMULGEN
Kao
Polyoxyethylene oleyl ether

A3
409PV
Corporation
(9E.O.)

Example 10

Component
EMULGEN 420
Kao
Polyoxyethylene oleyl ether

A3

Corporation
(13E.O.)

Example 11

Component
EMULGEN 420
Kao
Polyoxyethylene oleyl ether

A3

Corporation
(13E.O.)

Comparative

EMULGEN 430
Kao
Polyoxyethylene oleyl ether

Example 15

Corporation
(30E.O.)

Comparative

EMULGEN 705
Kao
Polyoxyethylene-sec-alkyl ether

Example 16

Corporation
(carbon number of an alkyl group of

11 or more and 15 or less, 5E.O.)

Example 12

Component
EMULGEN 707
Kao
Polyoxyethylene-sec-alkyl ether

A4

Corporation
(carbon number of an alkyl group of

11 or more and 15 or less, 7E.O.)

Example 13

Component
EMULGEN 707
Kao
Polyoxyethylene-sec-alkyl ether

A4

Corporation
(carbon number of an alkyl group of

11 or more and 15 or less, 7E.O.)

Example 14

Component
EMULGEN 709
Kao
Polyoxyethylene-sec-alkyl ether

A4

Corporation
(carbon number of an alkyl group of

11 or more and 15 or less, 9E.O.)

Example 15

Component
EMULGEN 709
Kao
Polyoxyethylene-sec-alkyl ether

A4

Corporation
(carbon number of an alkyl group of

11 or more and 15 or less, 9E.O.)

Comparative

EMULGEN
Kao
Polyoxyethylene alkyl ether

Example 17

1108
Corporation
(carbon number of an alkyl group of

11, 8 E.O.)

Comparative

EMULGEN
Kao
Polyoxyethylene myristyl ether

Example 18

4085
Corporation
(80E.O.)

Comparative

EMULGEN
Kao
Polyoxyethylene octyldodecyl ether

Example 19

2020G-HA
Corporation
(20 E.O.)

Comparative

EMULGEN
Kao
Polyoxyethylene octyldodecyl ether

Example 20

2025G
Corporation
(25 E.O.)

Example 16

Component
LEOCOL
Lion
Polyoxyethylene tridecyl ether

A5
TD-150
Corporation
(15 E.O.)

Example 17

Component
LEOCOL
Lion
Polyoxyethylene tridecyl ether

A5
TD-150
Corporation
(15 E.O.)

Evaluation

Clouding

Peak

Osmotic

point
HLB

Solu-
separation
Carry-

pressure

(° C.)
value
Content
bility
pattern
over
pH
(mOsm)

Comparative
—
8.8
0.5%
x
—
—
—
—

Example 13

Comparative
—
10
0.5%
x
—
—
—
—

Example 14

Example 9
55
12
0.5%
Δ
∘
∘
7.39
100

Example 10
91
13.6
0.5%
∘∘
∘
∘
7.38
101

Example 11
91
13.6
0.1%
∘∘
∘
∘
7.38
101

Comparative
>100
16.2
0.5%
Δ
x
x
—
—

Example 15

Comparative
—
10.5
0.5%
x
—
—
—
—

Example 16

Example 12
33
12.1
0.5%
∘∘
∘
∘
7.31
104

Example 13
33
12.1
0.1%
∘∘
∘
∘
7.31
104

Example 14
56
13.3
0.5%
∘∘
∘
∘
7.22
103

Example 15
56
13.3
0.1%
∘∘
∘
∘
7.22
103

Comparative
66
13.5
0.5%
∘
x
x
—
—

Example 17

Comparative
>100
18.9
0.5%
∘
x
x
—
—

Example 18

Comparative
—
13
0.5%
∘
x
x
—
—

Example 19

Comparative
—
15.7
0.5%
∘
x
x
—
—

Example 20

Example 16
75
15.4
0.5%
∘
∘
∘
7.33
103

Example 17
75
15.4
0.1%
∘
∘
∘
7.33
103

TABLE 4

Clouding

point

Product name
Manufacturer
Name of component
(° C.)

Comparative
Nonionic
EMULGEN A-60
Kao Corporation
Polyoxyethylene
—

Example 21
surfactant

distyrenated phenyl ether

Comparative

EMULGEN A-90
Kao Corporation
Polyoxyethylene
—

Example 22

distyrenated phenyl ether

Comparative

EMULGEN 3-66
Kao Corporation
Polyoxyethylene tribenzyl
—

Example 23

phenyl ether

Comparative

TWEEN20
Tokyo Chemical
Polyoxyethylene sorbitan
—

Example 24

Industry Co., Ltd.
monolaurate

Comparative

TWEEN40
Tokyo Chemical
Polyoxyethylene sorbitan
—

Example 25

Industry Co., Ltd.
monopalmitate

Comparative

TWEEN60
Tokyo Chemical
Polyoxyethylene sorbitan
—

Example 26

Industry Co., Ltd.
monostearate

Comparative

TWEEN80
Tokyo Chemical
Polyoxyethylene sorbitan
—

Example 27

Industry Co., Ltd.
monooleate

Comparative

TWEEN85
Tokyo Chemical
Polyoxyethylene sorbitan
—

Example 28

Industry Co., Ltd.
trioleate

Comparative

RHEODOL
Kao Corporation
Polyoxyethylene sorbitan
—

Example 29

TW-IS399C

triisostearate

Comparative

RHEODOL SP-L10
Kao Corporation
Sorbitan monolaurate
—

Example 30

Comparative

RHEODOL SP-P10
Kao Corporation
Sorbitan monopalmitate
—

Example 31

Comparative

RHEODOL
Kao Corporation
Sorbitan monostearate
—

Example 32

SP-S10V

Comparative

RHEODOL
Kao Corporation
Sorbitan tristearate
—

Example 33

SP-S30V

Comparative

RHEODOL
Kao Corporation
Sorbitan monooleate
—

Example 34

SP-O10V

Comparative

RHEODOL
Kao Corporation
Sorbitan trioleate
—

Example 35

SP-O30V

Comparative

RHEODOL AO-15V
Kao Corporation
Sorbitan sesquioleate
—

Example 36

Comparative

EMANON 1112
Kao Corporation
Polyethylene glycol
—

Example 37

monolaurate

Comparative

EMANON 3199V
Kao Corporation
Polyethylene glycol
—

Example 38

monostearate

Comparative

EMANON 3299VB
Kao Corporation
Polyethylene glycol
—

Example 39

distearate

Comparative

EMANON 3299RV
Kao Corporation
Polyethylene glycol
—

Example 40

distearate

Comparative

AMINON PK-02S
Kao Corporation
Alkyl alkanolamide
—

Example 41

Comparative

AMIET 105
Kao Corporation
Polyoxyethylene alkylamine
—

Example 42

Comparative

AMIET 320
Kao Corporation
Polyoxyethylene alkylamine
—

Example 43

Evaluation

Peak

Osmotic

HLB

Solu-
separation
Carry-

pressure

value
Content
bility
pattern
over
pH
(mOsm)

Comparative
—
0.5%
∘
x
x
—
—

Example 21

Comparative
—
0.5%
∘
x
x
—
—

Example 22

Comparative
—
0.5%
x
—
—
—
—

Example 23

Comparative
—
0.5%
∘
x
x
—
—

Example 24

Comparative
—
0.5%
x
—
—
—
—

Example 25

Comparative
—
0.5%
x
—
—
—
—

Example 26

Comparative
—
0.5%
∘
x
x
—
—

Example 27

Comparative
—
0.5%
∘
x
x
—
—

Example 28

Comparative
—
0.5%
∘
x
x
—
—

Example 29

Comparative
—
0.5%
x
—
—
—
—

Example 30

Comparative
—
0.5%
x
—
—
—
—

Example 31

Comparative
—
0.5%
x
—
—
—
—

Example 32

Comparative
—
0.5%
x
—
—
—
—

Example 33

Comparative
—
0.5%
x
—
—
—
—

Example 34

Comparative
—
0.5%
x
—
—
—
—

Example 35

Comparative
—
0.5%
x
—
—
—
—

Example 36

Comparative
13.7
0.5%
∘
x
∘
—
—

Example 37

Comparative
19.4
0.5%
x
—
—
—
—

Example 38

Comparative
18.9
0.5%
x
—
—
—
—

Example 39

Comparative
19.2
0.5%
x
—
—
—
—

Example 40

Comparative
—
0.5%
x
—
—
—
—

Example 41

Comparative
—
0.5%
∘
x
x
—
—

Example 42

Comparative
—
0.5%
∘
x
x
—
—

Example 43

TABLE 5

Product

name
Manufacturer
Name of component

Example 18
Nonionic
Component
EMULGEN
Kao Corporation
Polyoxyethylene

surfactant
A6
LS-106

polyoxypropylene alkyl ether

Example 19

Component
EMULGEN
Kao Corporation
Polyoxyethylene

A6
LS-106

polyoxypropylene alkyl ether

Example 20

Component
EMULGEN
Kao Corporation
Polyoxyethylene

A6
LS-114

polyoxypropylene alkyl ether

Example 21

Component
EMULGEN
Kao Corporation
Polyoxyethylene

A6
LS-114

polyoxypropylene alkyl ether

Example 22

Component
EMULGEN
Kao Corporation
Polyoxyethylene

A6
MS-100

polyoxypropylene alkyl ether

Example 23

Component
EMULGEN
Kao Corporation
Polyoxyethylene

A6
MS-100

polyoxypropylene alkyl ether

Comparative

LATEMUL
Kao Corporation
Polyoxyalkylene alkenyl ether

Example 44

PD-420

Comparative

LATEMUL
Kao Corporation
Polyoxyalkylene alkenyl ether

Example 45

PD-430

Comparative

LATEMUL
Kao Corporation
Polyoxyalkylene alkenyl ether

Example 46

PD-450

Comparative

MEGA-8
Dojindo Molecular
n-octanoyl-N-methyl-D-glucamine

Example 47

Technologies, Inc.

Example 24

Component
MEGA-9
Dojindo Molecular
n-nonanoyl-N-methyl-D-glucamine

A7

Technologies, Inc.

Comparative

MEGA-10
Dojindo Molecular
n-decanoyl-N-methyl-D-glucamine

Example 48

Technologies, Inc.

Example 25

Component
—
Dojindo Molecular
n-octyl-β-D-glucopyranoside

A8

Technologies, Inc.

Example 26

Component
Saponin
NACALAI TESQUE,
Soybean-derived saponin having

A9

INC.
structure of formula (9)

Comparative

EMANON
Kao Corporation
Polyoxyethylene hydrogenated

Example 49

CH-40

castor oil (40E.O.)

Comparative

EMANON
Kao Corporation
Polyoxyethylene hydrogenated

Example 50

CH-60K

castor oil (60E.O.)

Comparative

EMANON
Kao Corporation
Polyoxyethylene hydrogenated

Example 51

CH-80

castor oil (80E.O.)

Comparative

RHEODOL
Kao Corporation
Tetraoleic acid polyoxyethylene

Example 52

430V

sorbit (30E.O.)

Comparative

RHEODOL
Kao Corporation
Tetraoleic acid polyoxyethylene

Example 53

440V

sorbit (40E.O.)

Comparative

RHEODOL
Kao Corporation
Tetraoleic acid polyoxyethylene

Example 54

460V

sorbit (60E.O.)

Comparative

RHEODOL
Kao Corporation
Self-emulsifying glycerin

Example 55

MS165V

monostearate

Evaluation

Clouding

Peak

Osmotic

point
HLB

Solu-
separation
Carry-

pressure

(° C.)
value
Content
bility
pattern
over
pH
(mOsm)

Example 18
34
12.5
0.5%
∘∘
∘
∘
7.34
101

Example 19
34
12.5
0.1%
∘∘
∘
∘
7.34
101

Example 20
88
14
0.5%
∘
∘
∘
7.39
101

Example 21
88
14
0.1%
∘
∘
∘
7.39
101

Example 22
55
12.7
0.5%
∘∘
∘
∘
7.36
102

Example 23
55
12.7
0.1%
∘∘
∘
∘
7.36
102

Comparative
—
—
0.5%
∘
x
x
—
—

Example 44

Comparative
—
—
0.5%
∘
x
x
—
—

Example 45

Comparative
—
—
0.5%
∘
x
x
—
—

Example 46

Comparative
—
—
0.5%
∘
x
x
—
—

Example 47

Example 24
—
—
0.5%
∘
∘
∘
7.28
117

Comparative
—
—
0.5%
x
—
—
—
—

Example 48

Example 25
—
—
0.5%
∘∘
∘
∘
7.28
120

Example 26
—
—
0.5%
∘
∘
∘
6.32
123

Comparative
—
—
0.5%
x
—
—
—
—

Example 49

Comparative
—
—
0.5%
x
—
—
—
—

Example 50

Comparative
—
—
0.5%
x
—
—
—
—

Example 51

Comparative
—
—
0.5%
x
—
—
—
—

Example 52

Comparative
—
—
0.5%
x
—
—
—
—

Example 53

Comparative
—
—
0.5%
x
—
—
—
—

Example 54

Comparative
—
—
0.5%
x
—
—
—
—

Example 55

TABLE 6

Product

name
Manufacturer
Name of component

Comparative
Nonionic

EMULGEN
Kao
Polyoxyethylene

Example 56
surfactant

PP-290
Corporation
polyoxypropylene glycol

Comparative

Pluronic
ADEKA
Polyoxyethylene

Example 57

L-31

polyoxypropylene glycol

Comparative

Pluronic
ADEKA
Polyoxyethylene

Example 58

L-71

polyoxypropylene glycol

Comparative

Pluronic
ADEKA
Polyoxyethylene

Example 59

F-108

polyoxypropylene glycol

Comparative

Pluronic
ADEKA
Polyoxyethylene

Example 60

P-85

polyoxypropylene glycol

Comparative

Pluronic
ADEKA
Ethylenediamine

Example 61

TR-704

tetrapolyoxyethylene

polyoxypropylene

Comparative

Pluronic
ADEKA
Ethylenediamine

Example 62

TR-913R

tetrapolyoxyethylene

polyoxypropylene

Comparative
Anionic

—
—
Sodium lauryl sulfate

Example 63
surfactant

Comparative

—
—
Sodium taurocholate

Example 64

Comparative

—
—
Sodium deoxycholate

Example 65

Example 27
Amphoteric
Component
CHAPS
Dojindo Molecular
3-[(3-cholamidopropyl)

surfactant
B1

Technologies, Inc.
dimethylammonio]propane

sulfonate

Example 28

Component
CHAPSO
Dojindo Molecular
3-[(3-cholamidopropyl)

B2

Technologies, Inc.
dimethylammonio]-2-

hydroxypropane sulfonate

Comparative

AMPHITOL
Kao Corporation
Lauryl dimethylamino acetic

Example 66

20BS

acid betaine

Comparative

AMPHITOL
Kao Corporation
Stearyl dimethylamino acetic

Example 67

86B

acid betaine

Example 29

Component
AMPHITOL
Kao Corporation
Lauryl dimethylamine oxide

B3
20N

Example 30

Component
AMPHITOL
Kao Corporation
Lauryl dimethylamine oxide

B3
20N

Comparative

AMPHITOL
Kao Corporation
2-alkyl-N-carboxymethyl-N-

Example 68

20Y-B

hydroxyethyl imidazolinium

betaine

Comparative
—

—
—
No surfactant added

Example 69

Evaluation

Clouding

Peak

Osmotic

point
HLB

Solu-
separation
Carry-

pressure

(° C.)
value
Content
bility
pattern
over
pH
(mOsm)

Comparative
—
—
0.5%
∘
x
x
—
—

Example 56

Comparative
—
—
0.5%
∘
x
x
—
—

Example 57

Comparative
—
—
0.5%
x
—
—
—
—

Example 58

Comparative
—
—
0.5%
∘
x
x
—
—

Example 59

Comparative
—
—
0.5%
∘
x
x
—
—

Example 60

Comparative
—
—
0.5%
∘
x
x
—
—

Example 61

Comparative
—
—
0.5%
∘
x
x
—
—

Example 62

Comparative
—
—
0.5%
∘
x
x
—
—

Example 63

Comparative
—
—
0.5%
∘
x
x
—
—

Example 64

Comparative
—
—
0.5%
∘
x
x
—
—

Example 65

Example 27
—
—
0.5%
∘
∘
∘
7.44
116

Example 28
—
—
0.5%
∘
∘
∘
7.41
110

Comparative
—
—
0.5%
x
—
—
—
—

Example 66

Comparative
—
—
0.5%
x
—
—
—
—

Example 67

Example 29
—
—
0.5%
∘∘
∘
∘
7.37
103

Example 30
—
—
0.1%
∘∘
∘
∘
7.37
103

Comparative
—
—
0.5%
x
—
—
—
—

Example 68

Comparative
—
—

0%
—
x
x
—
—

Example 69

It can be understood that the reagents for measuring hemoglobins obtained in Examples 1 to 30 are capable of satisfactorily causing hemolysis and measuring hemoglobins with high accuracy.

Reference Example A and Examples 31 to 38

A reagent for measuring hemoglobins was prepared in the same manner as in Example 1 except that the compositions were changed to those shown in Table 7.

(5) Storage Stability of Reagent for Measuring Hemoglobins

The reagent for measuring hemoglobins obtained in Reference Example A and each reagent for measuring hemoglobins obtained in Examples 32, 34, 36 to 38 having a concentration of a surfactant of 0.5% by weight were respectively sealed in a glass vial and stored at 60° C. for 7 days. After the storage, properties of the reagent for measuring hemoglobins were visually checked.

Generally, a reagent for measuring hemoglobins is stored at room temperature. In this evaluation item, the reagent for measuring hemoglobins was stored and evaluated under a temperature condition severer than that in a normal storage condition.

[Criteria for Judging Storage Stability of Reagent for Measuring Hemoglobins (60° C., 7 Days)]

A: Phase separation does not occur

B: Phase separation occurs

(6) Storage Stability of Mixed Solution

(6-1) Storage Stability of Mixed Solution with Whole Blood

Whole blood (erythrocyte-containing sample) was prepared. Each reagent for measuring hemoglobins obtained in Reference Example A and Examples 31 to 36 was prepared. Whole blood was diluted 101-fold with the reagent for measuring hemoglobins to obtain a mixed solution. The obtained mixed solution was placed in a glass vial and stored at 4° C. Before the storage, and on the 1st day, the 2nd day, the 5th day, the 7th day, and the 9th day after the storage, the mixed solution was repeatedly measured 3 times under the measurement conditions described in “(2) Measurement by cation exchange liquid chromatography”, and the value of hemoglobin A1c and the variation in the value of the hemoglobin A1c were determined from the average.

Value of hemoglobin A1c (%)=peak area of hemoglobin A1c/total peak area of hemoglobins

Variation in value of hemoglobin A1c (%)=value of hemoglobin A1c before storage−value of hemoglobin A1c after storage

FIG. 6(a) is a figure showing the relationship between the number of storage days and the value of hemoglobin A1c in a mixed solution with whole blood. FIG. 6(b) is a figure showing the relationship between the number of storage days and the variation in the value of hemoglobin A1c in a mixed solution with whole blood.

[Criteria for Judging Mixed Solution with Whole Blood]

◯: For the variation in the value of hemoglobin A1c on the 5th day, the absolute value of the difference from the value of Reference Example A is 0.2% or less

Δ: For the variation in the value of hemoglobin A1c on the 5th day, the absolute value of the difference from the value of Reference Example A is more than 0.2% and 0.4% or less.

ΔΔ: For the variation in the value of hemoglobin A1c on the 5th day, the absolute value of the difference from the value of Reference Example A is more than 0.4% and 0.7% or less.

x: For the variation in the value of hemoglobin A1c on the 5th day, the absolute value of the difference from the value of Reference Example A is more than 0.7%.

(6-2) Storage Stability of Mixed Solution with Hemoglobin A1c Substance for Measurement Control (Low Concentration) (IRC-L)

A hemoglobin A1c substance for measurement control having a value of hemoglobin A1c of 5.8% (low concentration) (IRC-L) was prepared. Each reagent for measuring hemoglobins obtained in Reference Example A and Examples 31 to 36 was prepared. The hemoglobin A1c substance for measurement control (low concentration) (IRC-L) was diluted 101-fold with the reagent for measuring hemoglobins to obtain a mixed solution. The obtained mixed solution was placed in a glass vial and stored at 4° C. Before the storage, and on the 1st day, the 2nd day, the 3rd day, the 9th day, and the 14th day after the storage, the mixed solution was repeatedly measured 3 times under the measurement conditions in “(2) Measurement by cation exchange liquid chromatography”, and the value of hemoglobin A1c and the variation in the value of the hemoglobin A1c were determined from the average in the same manner as above.

FIG. 7(a) is a figure showing the relationship between the number of storage days and the value of hemoglobin A1c in a mixed solution with a hemoglobin A1c substance for measurement control (low concentration) (IRC-L). FIG. 7(b) is a figure showing the relationship between the number of storage days and the variation in the value of hemoglobin A1c in a mixed solution with a hemoglobin A1c substance for measurement control (low concentration) (IRC-L).

[Criteria for Judging Storage Stability of Mixed Solution with Hemoglobin A1c Substance for Measurement Control (Low Concentration) (IRC-L)]

◯: For the variation in the value of hemoglobin A1c on the 14th day, the absolute value of the difference from the value of Reference Example A is 0.2% or less

Δ: For the variation in the value of hemoglobin A1c on the 14th day, the absolute value of the difference from the value of Reference Example A is more than 0.2% and 0.4% or less.

ΔΔ: For the variation in the value of hemoglobin A1c on the 14th day, the absolute value of the difference from the value of Reference Example A is more than 0.4% and 0.7% or less.

x: For the variation in the value of hemoglobin A1c on the 14th day, the absolute value of the difference from the value of Reference Example A is more than 0.7%.

(6-3) Storage Stability of Mixed Solution with Hemoglobin A1c Substance for Measurement Control (High Concentration) (IRC-H)

The value of hemoglobin A1c and the variation in the value of hemoglobin A1c were determined in the same manner as in “(6-2) Storage stability of mixed solution with hemoglobin A1c substance for measurement control (low concentration) (IRC-L)” except that the hemoglobin A1c substance for measurement control (low concentration) (IRC-L) was changed to the hemoglobin A1c substance for measurement control having a value of hemoglobin A1c of 10.4% (high concentration) (IRC-H).

FIG. 8(a) is a figure showing the relationship between the number of storage days and the value of hemoglobin A1c in a mixed solution with a hemoglobin A1c substance for measurement control (high concentration) (IRC-H). FIG. 8(b) is a figure showing the relationship between the number of storage days and the variation in the value of hemoglobin A1c in a mixed solution with a hemoglobin A1c substance for measurement control (high concentration) (IRC-H).

[Criteria for Judging Storage Stability of Mixed Solution with Hemoglobin A1c Substance for Measurement Control (High Concentration) (IRC-H)]

◯: For the variation in the value of hemoglobin A1c on the 14th day, the absolute value of the difference from the value of Reference Example A is 0.25% or less

Δ: For the variation in the value of hemoglobin A1c on the 14th day, the absolute value of the difference from the value of Reference Example A is more than 0.25% and 0.45% or less

ΔΔ: For the variation in the value of hemoglobin A1c on the 14th day, the absolute value of the difference from the value of Reference Example A is more than 0.45% and 0.75% or less

x: For the variation in the value of hemoglobin A1c on the 14th day, the absolute value of the difference from the value of Reference Example A is more than 0.75%

The compositions and results are shown in Tables 7 below.

TABLE 7

Reference

Product

Exam-
Exam-
Exam-
Exam-
Exam-

name
Name of component

ple A
ple 31
ple 32
ple 33
ple 34

Potassium dihydrogen phosphate
% by weight
0.013
0.013
0.013
0.013
0.013

Dipotassium hydrogen phosphate
% by weight
0.052
0.052
0.052
0.052
0.052

Sodium chloride
% by weight
0.233
0.233
0.233
0.233
0.233

Sodium azide
% by weight
0.02
0.02
0.02
0.02
0.02

Component
Triton
Polyoxyethylene octyl phenyl
% by weight
0.1

X
X-100
ether (10 E.O.)

Component
EMULGEN
Polyoxyethylene lauryl ether
% by weight

0.1
0.5

A1
120
(12 E.O.)

Component
EMULGEN
Polyoxyethylene cetyl ether
% by weight

0.1
0.5

A1
220
(13 E.O.)

Component
EMULGEN
Polyoxyethylene oleyl ether
% by weight

A3
420
(13 E.O.)

Component
EMULGEN
Polyoxyethylene
% by weight

A6
LS-114
polyoxypropylene alkyl ether

Component
EMULGEN
Polyoxyethylene
% by weight

A6
MS-100
polyoxypropylene alkyl ether

Water
% by weight
Remainder
Remainder
Remainder
Remainder
Remainder

Total
% by weight
100
100
100
100
100

Evaluation
Storage stability of reagent for
Judgement
A
—
A
—
A

measuring hemoglobins (60° C., 7 days)

Storage
Mixed solution with whole blood
Judgement
—
∘
∘
∘
Δ

stability
(4° C., 5 days)

of mixed
Mixed solution with hemoglobin
Judgement
—
∘
Δ
∘
Δ

solution
A1c substance for measurement

control (low concentration)

(IRC-L) (4° C., 14 days)

Mixed solution with hemoglobin
Judgement
—
Δ
ΔΔ
∘
ΔΔ

A1c substance for measurement

control (high concentration)

(IRC-H) (4° C., 14 days)

Product

Exam-
Exam-
Exam-
Exam-

name
Name of component

ple 35
ple 36
ple 37
ple 38

Potassium dihydrogen phosphate
% by weight
0.013
0.013
0.013
0.013

Dipotassium hydrogen phosphate
% by weight
0.052
0.052
0.052
0.052

Sodium chloride
% by weight
0.233
0.233
0.233
0.233

Sodium azide
% by weight
0.02
0.02
0.02
0.02

Component
Triton
Polyoxyethylene octyl phenyl
% by weight

X
X-100
ether (10 E.O.)

Component
EMULGEN
Polyoxyethylene lauryl ether
% by weight

A1
120
(12 E.O.)

Component
EMULGEN
Polyoxyethylene cetyl ether
% by weight

A1
220
(13 E.O.)

Component
EMULGEN
Polyoxyethylene oleyl ether
% by weight
0.1
0.5

A3
420
(13 E.O.)

Component
EMULGEN
Polyoxyethylene
% by weight

0.5

A6
LS-114
polyoxypropylene alkyl ether

Component
EMULGEN
Polyoxyethylene
% by weight

0.5

A6
MS-100
polyoxypropylene alkyl ether

Water
% by weight
Remainder
Remainder
Remainder
Remainder

Total
% by weight
100
100
100
100

Evaluation
Storage stability of reagent for
Judgement
—
A
B
B

measuring hemoglobins (60° C., 7 days)

Storage
Mixed solution with whole blood
Judgement
Δ
ΔΔ
—
—

stability
(4° C., 5 days)

of mixed
Mixed solution with hemoglobin
Judgement
∘
∘
—
—

solution
A1c substance for measurement

control (low concentration)

(IRC-L) (4° C., 14 days)

Mixed solution with hemoglobin
Judgement
∘
∘
—
—

A1c substance for measurement

control (high concentration)

(IRC-H) (4° C., 14 days)

Each reagent for measuring hemoglobins obtained in Examples 31 to 36 successfully increased its storage stability compared with each reagent for measuring hemoglobins obtained in Examples 37 and 38. Each reagent for measuring hemoglobins obtained in Examples 31 to 36 also successfully increased the storage stability of a mixed solution obtained by mixing the reagent and the substance to be tested. Each reagent for measuring hemoglobins obtained in Examples 31 to 36 can measure hemoglobins with high accuracy even after the mixed solution obtained by mixing the reagent for measuring hemoglobins and the substance to be tested is stored for a long time.

(7) Column Durability

Whole blood (erythrocyte-containing sample), a hemoglobin A1c substance for measurement control having a value of hemoglobin A1c of 10.4% (high concentration) (IRC-H), and each reagent for measuring hemoglobins obtained in Reference Example A and Example 32 were prepared. Whole blood was diluted 101-fold with the reagent for measuring hemoglobins to obtain Liquid (1). The hemoglobin A1c substance for measurement control was diluted 101-fold with the reagent for measuring hemoglobins to obtain Liquid (2). Liquid (1) is a measurement sample for applying a load to the column, and Liquid (2) is a measurement sample for checking the variation in the value of hemoglobin A1c and the variation in the number of theoretical plates. The obtained Liquid (1) and Liquid (2) were measured according to the following procedures under the following conditions.

First, the obtained Liquid (2) was measured 3 times. Then, every time the obtained Liquid (1) was passed through the column multiple times (tens of times to 200 times), Liquid (2) was measured 3 times. Liquid (1) and Liquid (2) were repeatedly measured according to the above procedure until the number of samples loaded on the column reached about 3000.

Cation Exchange Chromatography Conditions:

HPLC instrument: glycohemoglobin analyzer (“HA-8160VP” manufactured by ARKRAY, Inc.)

Cation exchange column: COLUMN UNIT HSVI-VP (manufactured by ARKRAY, Inc.)

Eluent A: ELUENT 60A-VP/TP (manufactured by ARKRAY, Inc.)

Eluent B: ELUENT 60B-VP/TP (manufactured by ARKRAY, Inc.)

Eluent C: ELUENT 60C-VP (manufactured by ARKRAY, Inc.)

The measurement was performed by the measurement method installed in the HPLC instrument.

FIG. 9(a) is a figure showing the relationship between the number of samples loaded on the column and the variation in the value of hemoglobin A1c. FIG. 9(b) is a figure showing the relationship between the number of samples loaded on the column and the variation in the number of theoretical plates.

In FIG. 9(a), the vertical axis shows the difference between the value of hemoglobin A1c in Liquid (2) measured first and the value of hemoglobin A1c in Liquid (2) measured at each number of samples loaded (value of hemoglobin A1c in Liquid (2) measured first—value of hemoglobin A1c in Liquid (2) measured at each number of samples loaded). In FIG. 9(b), the vertical axis shows the difference between the number of theoretical plates in Liquid (2) measured first and the number of theoretical plates in Liquid (2) measured at each number of samples loaded (number of theoretical plates in Liquid (2) measured first—number of theoretical plates in Liquid (2) measured at each number of samples loaded).

The reagent for measuring hemoglobins obtained in Example 32 was superior to the reagent for measuring hemoglobins obtained in Reference Example A in column durability.

Number	Date	Country	Kind
2018-170562	Sep 2018	JP	national
2018-170563	Sep 2018	JP	national

REAGENT AND METHOD FOR MEASURING HEMOGLOBINS

Information

Publication Number

Date Filed

Date Published

Inventors

Original Assignees

CPC

International Classifications

Abstract

Description

Claims

Priority Claims (2)

PCT Information