ALKALINE PHOSPHATASE COMPOSITION, METHOD OF PRODUCING DEPHOSPHORYLATED NUCLEIC ACID AND METHOD OF PRODUCING LABELED NUCLEIC ACID

Information

  • Patent Application
  • 20210332337
  • Publication Number
    20210332337
  • Date Filed
    September 25, 2019
    5 years ago
  • Date Published
    October 28, 2021
    3 years ago
Abstract
A composition contains an alkaline phosphatase; and a peptide fragment group (A) composed of two or more peptide fragments, wherein each of the two or more peptide fragments consists of 5 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5, wherein a content ratio of the peptide fragment group (A) to the alkaline phosphatase satisfies formula (A): (XA/Y)×100≤4.4000 (A), wherein XA represents a peak area value of the peptide fragment group (A) calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y represents a peak area value of the alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis of the composition.
Description
TECHNICAL FIELD

This disclosure relates to a composition containing an alkaline phosphatase, a method of producing a dephosphorylated nucleic acid by using the composition and a method of producing a labeled nucleic acid by using the composition.


BACKGROUND

An alkaline phosphatase has a catalyst function that hydrolyzes phosphoric monoesters, and has been widely used in methods of measuring the amount of biological substances such as proteins and nucleic acids (e.g., the immunostaining method, ELISA, the nucleic acid microarray method or the like). For example, in the research field of genetic engineering, for pretreatment of labeling of nucleic acids such as DNA and RNA and prevention of self-ligation of vectors, dephosphorylation of the 5′ end and/or the 3′ end of a nucleic acid with an alkaline phosphatase has been performed.


As an industrial production method of an alkaline phosphatase, a production method in which bovine small intestine or large intestine is mainly used as a raw material has been widely adopted since the specific activity of the produced alkaline phosphatase is high. The specific activity of an alkaline phosphatase is generally evaluated by measuring the absorbance at 405 nm derived from p-nitrophenol produced when p-nitrophenylphosphate is decomposed.


The quality of an alkaline phosphatase has been evaluated based on the alkaline phosphatase specific activity. To obtain an alkaline phosphatase having a higher specific activity than that of an alkaline phosphatase derived from bovine intestine, an alkaline phosphatase having a high specific activity has been isolated in a purification process or has been produced by using recombinant Escherichia coli obtained by a genetic engineering method.


JP H10-262674 A discloses a method of producing an alkaline phosphatase having a high specific activity by using recombinant Escherichia coli into which an alkaline phosphatase-encoding gene derived from the genus Bacillus badius has been introduced. WO 2012/115023 discloses a method of producing an alkaline phosphatase having a high specific activity and heat resistance by using recombinant Escherichia coli into which an alkaline phosphatase-encoding gene derived from the genus Shewanella has been introduced.


A dephosphorylation reagent containing an alkaline phosphatase (e.g., a commercially available alkaline phosphatase product) is a composition containing other components in addition to the alkaline phosphatase. A quality of a dephosphorylation reagent containing an alkaline phosphatase is evaluated based on the alkaline phosphatase specific activity.


However, we found that, even if labeled nucleic acids prepared by using dephosphorylation reagents having almost the same alkaline phosphatase specific activity (labeled nucleic acids obtained by dephosphorylating the 5′ ends and/or the 3′ ends of nucleic acids with the dephosphorylation reagents, and then binding labeling substances to the 5′ ends and/or the 3′ ends of the dephosphorylated nucleic acids) are used for a nucleic acid detection method, a great difference in the detection sensitivity between the labeled nucleic acids may occur in the nucleic acid detection method. In other words, we found that the quality of a dephosphorylation reagent containing an alkaline phosphatase cannot be evaluated correctly by using the alkaline phosphatase specific activity as an index.


Thus, it could be helpful to provide a composition containing an alkaline phosphatase and having a high quality, a method of producing a dephosphorylated nucleic acid by using the composition and a method of producing a labeled nucleic acid by using the composition.


SUMMARY

We found that at least any one of the following impurities can coexist in a dephosphorylation reagent containing an alkaline phosphatase (e.g., a commercially available alkaline phosphatase product):


a peptide fragment group (A) composed of two or more peptide fragments, wherein each of the two or more peptide fragments consists of 5 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5 (which corresponds to an amino acid sequence of a bovine-derived alkaline phosphatase);


a peptide fragment group (B) composed of two or more peptide fragments, wherein each of the two or more peptide fragments consists of 13 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5 and contains positions 516 to 528 of the amino acid sequence set forth in SEQ ID NO: 5;


a peptide fragment group (C) composed of two or more peptide fragments, wherein each of the two or more peptide fragments consists of 12 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5 and contains positions 534 to 545 of the amino acid sequence set forth in SEQ ID NO: 5;


a first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1;


a second peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 2;


a third peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 3; and


a fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4.


In addition, we found that, by reducing, in a dephosphorylation reagent which is used to prepare a labeled nucleic acid (a labeled nucleic acid obtained by dephosphorylating the 5′ end and/or the 3′ end of a nucleic acid with the dephosphorylation reagent, and then binding a labeling substance to the 5′ end and/or the 3′ end of the dephosphorylated nucleic acid) for a nucleic acid detection method,


the content of the peptide fragment group (A),


the content of the peptide fragment group (B),


the content of the peptide fragment group (C),


the content of the second peptide fragment (preferably, the content of the second peptide fragment, and the content(s) of one, two or three peptide fragments selected from the first, third and fourth peptide fragments),


the content of the third peptide fragment (preferably, the content of the third peptide fragment, and the content(s) of one, two or three peptide fragments selected from the first, second and fourth peptide fragments), or


the content of the fourth peptide fragment (preferably, the content of the fourth peptide fragment, and the content(s) of one, two or three peptide fragments selected from the first, second and third peptide fragments),


it is possible to improve the detection sensitivity of the labeled nucleic acid in the nucleic acid detection method, thus completing this disclosure.


We thus provide:

  • [1] A composition containing:


an alkaline phosphatase; and


a peptide fragment group (A) composed of two or more peptide fragments, wherein each of the two or more peptide fragments consists of 5 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5,


wherein a content ratio of the peptide fragment group (A) to the alkaline phosphatase satisfies formula (A):





(XA/Y)×100≤4.4000   (A),


wherein XA represents a peak area value of the peptide fragment group (A) calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y represents a peak area value of the alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis of the composition.

  • [2] The composition according to [1], wherein the peptide fragment group (A) contains one, two, three or four peptide fragments selected from the group consisting of a first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1, a second peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 2, a third peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 3 and a fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4.
  • [3] The composition according to [2], wherein:


the peptide fragment group (A) contains the first peptide fragment; and


a content ratio of the first peptide fragment to the alkaline phosphatase satisfies formula (1):





(X1/Y)×100≤1.0000   (1),


wherein X1 represents a peak area value of the first peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.

  • [4] The composition according to [2] or [3], wherein:


the peptide fragment group (A) contains the second peptide fragment; and


a content ratio of the second peptide fragment to the alkaline phosphatase satisfies formula (2):





(X2/Y)×100≤1.6000   (2),


wherein X2 represents a peak area value of the second peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.

  • [5] The composition according to any one of [2] to [4], wherein:


the peptide fragment group (A) contains the third peptide fragment; and


a content ratio of the third peptide fragment to the alkaline phosphatase satisfies formula (3):





(X3/Y)×100≤0.2000   (3),


wherein X3 represents a peak area value of the third peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.

  • [6] The composition according to any one of [2] to [5], wherein:


the peptide fragment group (A) contains the fourth peptide fragment; and


a content ratio of the fourth peptide fragment to the alkaline phosphatase satisfies formula (4):





(X4/Y)×100≤0.3500   (4),


wherein X4 represents a peak area value of the fourth peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.

  • [7] A composition containing:


an alkaline phosphatase; and


a peptide fragment group (B) composed of two or more peptide fragments, wherein each of the two or more peptide fragments consists of 13 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5 and contains positions 516 to 528 of the amino acid sequence set forth in SEQ ID NO: 5,


wherein a content ratio of the peptide fragment group (B) to the alkaline phosphatase satisfies formula (B):





(XB/Y)×100≤3.4000   (B),


wherein XB represents a peak area value of the peptide fragment group (B) calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y represents a peak area value of the alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis of the composition.

  • [8] The composition according to [7], wherein the peptide fragment group (B) contains one or two peptide fragments selected from the group consisting of a first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1 and a second peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 2.
  • [9] The composition according to [8], wherein:


the peptide fragment group (B) contains the first peptide fragment; and


a content ratio of the first peptide fragment to the alkaline phosphatase satisfies formula (1):





(X1/Y)×100≤1.0000   (1),


wherein X1 represents a peak area value of the first peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.

  • [10] The composition according to [8] or [9], wherein:


the peptide fragment group (B) contains the second peptide fragment; and


a content ratio of the second peptide fragment to the alkaline phosphatase satisfies formula (2):





(X2/Y)×100≤1.6000   (2),


wherein X2 represents a peak area value of the second peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.

  • [11] A composition containing:


an alkaline phosphatase; and


a peptide fragment group (C) composed of two or more peptide fragments, wherein each of the two or more peptide fragments consists of 12 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5 and contains positions 534 to 545 of the amino acid sequence set forth in SEQ ID NO: 5,


wherein a content ratio of the peptide fragment group (C) to the alkaline phosphatase satisfies formula (C):





(XC/Y)×100≤1.0000   (C),


wherein XC represents a peak area value of the peptide fragment group (C) calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y represents a peak area value of the alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis of the composition.

  • [12] The composition according to [11], wherein the peptide fragment group (C) contains one or two peptide fragments selected from the group consisting of a third peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 3 and a fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4.
  • [13] The composition according to [12], wherein:


the peptide fragment group (C) contains the third peptide fragment; and


a content ratio of the third peptide fragment to the alkaline phosphatase satisfies formula (3):





(X3/Y)×100≤0.2000   (3),


wherein X3 represents a peak area value of the third peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.

  • [14] The composition according to [12] or [13], wherein:


the peptide fragment group (C) contains the fourth peptide fragment; and


a content ratio of the fourth peptide fragment to the alkaline phosphatase satisfies formula (4):





(X4/Y)×100≤0.3500   (4),


wherein X4 represents a peak area value of the fourth peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.

  • [15] A composition containing:


an alkaline phosphatase; and


a second peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 2,


wherein a content ratio of the second peptide fragment to the alkaline phosphatase satisfies formula (2):





(X2/Y)×100≤1.6000   (2),


wherein X2 represents a peak area value of the second peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y represents a peak area value of the alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis of the composition.

  • [16] The composition according to [15], wherein:


the composition further contains a first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1; and


a content ratio of the first peptide fragment to the alkaline phosphatase satisfies formula (1):





(X1/Y)×100≤1.0000   (1),


wherein X1 represents a peak area value of the first peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.

  • [17] The composition according to [15] or [16], wherein:


the composition further contains a third peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 3; and


a content ratio of the third peptide fragment to the alkaline phosphatase satisfies formula (3):





(X3/Y)×100≤0.2000   (3),


wherein X3 represents a peak area value of the third peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.

  • [18] The composition according to any one of [15] to [17], wherein:


the composition further contains a fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4; and


a content ratio of the fourth peptide fragment to the alkaline phosphatase satisfies formula (4):





(X4/Y)×100≤0.3500   (4),


wherein X4 represents a peak area value of the fourth peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.

  • [19] A composition containing:


an alkaline phosphatase; and


a third peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 3,


wherein a content ratio of the third peptide fragment to the alkaline phosphatase satisfies formula (3):





(X3/Y)×100≤0.2000   (3),


wherein X3 represents a peak area value of the third peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.

  • [20] The composition according to [19], wherein:


the composition further contains a first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1; and


a content ratio of the first peptide fragment to the alkaline phosphatase satisfies formula (1):





(X1/Y)×100≤1.0000   (1),


wherein X1 represents a peak area value of the first peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.

  • [21] The composition according to [19] or [20], wherein:


the composition further contains a fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4; and


a content ratio of the fourth peptide fragment to the alkaline phosphatase satisfies formula (4):





(X4/Y)×100≤0.3500   (4),


wherein X4 represents a peak area value of the fourth peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.

  • [22] A composition containing:


an alkaline phosphatase; and


a fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4,


wherein a content ratio of the fourth peptide fragment to the alkaline phosphatase satisfies formula (4):





(X4/Y)×100≤0.3500   (4),


wherein X4 represents a peak area value of the fourth peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.

  • [23] The composition according to [22], wherein:


the composition further contains a first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1; and


a content ratio of the first peptide fragment to the alkaline phosphatase satisfies formula (1):





(X1/Y)×100≤1.0000   (1),


wherein X1 represents a peak area value of the first peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.

  • [24] The composition according to any one of [1] to [23], wherein the composition has an alkaline phosphatase specific activity of 2,000 U/mg or more.
  • [25] The composition according to any one of [1] to [24], wherein the alkaline phosphatase is selected from the following (a) and (b):
  • (a) an alkaline phosphatase containing a protein molecule consisting of the amino acid sequence set forth in SEQ ID NO: 5; and
  • (b) an alkaline phosphatase containing a protein molecule consisting of an amino acid sequence that has 70% or more sequence identity to the amino acid sequence set forth in SEQ ID NO: 5 and comprises positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5.
  • [26] The composition according to any one of [1] to [25], wherein the composition further contains a nucleic acid.
  • [27] The composition according to [26], wherein the composition is a composition used for dephosphorylating the nucleic acid.
  • [28] The composition according to any one of [1] to [25], wherein the composition further contains a dephosphorylated nucleic acid.
  • [29] The composition according to [28], wherein the composition is a composition used for preparing a labeled nucleic acid containing the dephosphorylated nucleic acid and a labeling substance bound to the dephosphorylated nucleic acid.
  • [30] The composition according to any one of [1] to [25], wherein the composition further contains a labeled nucleic acid containing a dephosphorylated nucleic acid and a labeling substance bound to the dephosphorylated nucleic acid.
  • [31] The composition according to [30], wherein the composition is a nucleic acid sample to be subjected to a nucleic acid detection method.
  • [32] The composition according to [31], wherein the nucleic acid detection method is a nucleic acid detection method using a nucleic acid microarray.
  • [33] A method of producing a dephosphorylated nucleic acid, the method including the following steps of:


providing the composition according to any one of [1] to [25];


providing a nucleic acid; and


treating the nucleic acid with the composition to dephosphorylate the nucleic acid.

  • [34] A method of producing a labeled nucleic acid, the method including the following steps of:


providing the composition according to any one of [1] to [25];


providing a nucleic acid;


providing a labeling substance;


treating the nucleic acid with the composition to dephosphorylate the nucleic acid; and


binding the labeling substance to the dephosphorylated nucleic acid.


We thus provide a composition containing an alkaline phosphatase and having a high quality, a method of producing a dephosphorylated nucleic acid by using the composition and a method of producing a labeled nucleic acid by using the composition.





BRIEF DESCRIPTION OF THE DRAWINGS


FIG. 1 shows an extracted ion chromatogram on the first peptide fragment obtained by an LC-MS/MS analysis of the composition C2 in Comparative Example 2.



FIG. 2 shows an extracted ion chromatogram on the second peptide fragment obtained by an LC-MS/MS analysis of the composition C2 in Comparative Example 2.



FIG. 3 shows an extracted ion chromatogram on the third peptide fragment obtained by an LC-MS/MS analysis of the composition C2 in Comparative Example 2.



FIG. 4 shows an extracted ion chromatogram on the fourth peptide fragment obtained by an LC-MS/MS analysis of the composition C2 in Comparative Example 2.



FIG. 5 shows an extracted ion chromatogram on the first peptide fragment obtained by an LC-MS/MS analysis of the composition E1 (purified product of the composition C2) in Example 1.



FIG. 6 shows an extracted ion chromatogram on the second peptide fragment obtained by an LC-MS/MS analysis of the composition E1 (purified product of the composition C2) in Example 1.



FIG. 7 shows an extracted ion chromatogram on the third peptide fragment obtained by an LC-MS/MS analysis of the composition E1 (purified product of the composition C2) in Example 1.



FIG. 8 shows an extracted ion chromatogram on the fourth peptide fragment obtained by an LC-MS/MS analysis of the composition E1 (purified product of the composition C2) in Example 1.



FIG. 9 shows a chromatogram on an alkaline phosphatase obtained by an LC-UV analysis of the composition E1 (purified product of the composition C2) in Example 1.





DETAILED DESCRIPTION

Our compositions and methods will be described in detail below. It is possible to combine two or more of the aspects described below, and it is possible to combine two or more of the examples described below. This disclosure also encompasses such combinations. The expression “numerical value M to numerical value N” means a range of numerical value M or more and numerical value N or less.


We provide a composition containing an alkaline phosphatase and a peptide fragment group (A) as a first composition.


We provide a composition containing an alkaline phosphatase and a peptide fragment group (B) as a second composition.


We provide a composition containing an alkaline phosphatase and a peptide fragment group (C) as a third composition.


We provide a composition containing an alkaline phosphatase and a second peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 2 as a fourth composition.


We provide a composition containing an alkaline phosphatase and a third peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 3 as a fifth composition.


We provide a composition containing an alkaline phosphatase and a fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4 as a sixth composition.


The compositions above will be collectively expressed as the “composition.” Therefore, the descriptions of the “composition” apply to any of the above compositions unless otherwise specified.


Alkaline Phosphatase

The composition contains an alkaline phosphatase. The composition may contain one alkaline phosphatase or may contain two or more alkaline phosphatases.


The alkaline phosphatase contained in the composition is not particularly limited as long as it has alkaline phosphatase activity. The alkaline phosphatase activity is activity that hydrolyzes a phosphoric monoester bond in alkalinity (pH 8 to 11, e.g., pH 8 to 10 or pH 9 to 11), and the reaction form is classified into EC3.1.3.1.


The structure of the alkaline phosphatase contained in the composition (e.g., primary structure, secondary structure, tertiary structure, quaternary structure and the like) is not particularly limited. For example, the alkaline phosphatase may have a sugar chain or may not have a sugar chain. The alkaline phosphatase may be any isozyme that can exist based on differences in the structure of a protein molecule (e.g., amino acid sequence of a protein molecule), glycosylation and the like. The alkaline phosphatase may be a monomer that is formed from one subunit or may be an oligomer that is formed from two or more subunits (e.g., dimer, tetramer and the like). The oligomer may be a homooligomer or may be a heterooligomer.


The animal from which the alkaline phosphatase contained in the composition is derived is not particularly limited. Examples of the animal from which the alkaline phosphatase is derived include a bovine, a shrimp, a microorganism into which a gene encoding an alkaline phosphatase has been introduced and the like. Since a bovine-derived alkaline phosphatase has high alkaline phosphatase activity, the animal from which the alkaline phosphatase is derived is preferably a bovine. When the alkaline phosphatase is derived from a bovine, the organ from which the alkaline phosphatase is derived is preferably small intestine or large intestine.


The alkaline phosphatase contained in the composition may be wild-type or may be mutated. The mutated alkaline phosphatase contains, for example, a protein molecule consisting of an amino acid sequence obtained by introducing deletion, substitution, insertion or addition of one or more amino acids to an amino acid sequence of a protein molecule of a wild-type alkaline phosphatase. The amino acid sequence of the protein molecule of the mutated alkaline phosphatase has preferably 70% or more, more preferably 75% or more, still more preferably 80% or more, yet more preferably 85% or more, further preferably 90% or more, and still further preferably 95% or more sequence identity to the amino acid sequence of the protein molecule of the wild-type alkaline phosphatase.


Preferably, the alkaline phosphatase is selected from (a) and (b):

  • (a) an alkaline phosphatase containing a protein molecule consisting of the amino acid sequence set forth in SEQ ID NO: 5; and
  • (b) an alkaline phosphatase containing a protein molecule consisting of an amino acid sequence that has 70% or more sequence identity to the amino acid sequence set forth in SEQ ID NO: 5 and contains positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. In this example, the composition may contain one alkaline phosphatase selected from (a) and (b), or may contain two or more alkaline phosphatases selected from (a) and (b).


The amino acid sequence of the protein molecule of the alkaline phosphatase (a) (i.e., the amino acid sequence set forth in SEQ ID NO: 5) corresponds to an amino acid sequence of a protein molecule of a bovine-derived alkaline phosphatase. Therefore, a bovine-derived alkaline phosphatase falls within the alkaline phosphatase (a).


The amino acid sequence of the protein molecule of the alkaline phosphatase (b) has preferably 70% or more, more preferably 75% or more, still more preferably 80% or more, yet more preferably 85% or more, further preferably 90% or more, and still further preferably 95% or more sequence identity to the amino acid sequence set forth in SEQ ID NO: 5.


Both of a wild-type alkaline phosphatase (e.g., an alkaline phosphatase derived from an animal other than a bovine, a bovine-derived alkaline phosphatase having a polymorphism or the like) and a mutated alkaline phosphatase fall within the alkaline phosphatase (b). The position(s) at which one or more amino acids are deleted, substituted, inserted or added in the amino acid sequence set forth in SEQ ID NO: 5 is/are a position(s) other than positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5.


The alkaline phosphatases (a) and (b) can generate the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment, the fourth peptide fragment and the like, by decomposition of the alkaline phosphatases.


Peptide First Group (A)

The first composition may contain the peptide fragment group (A). The peptide fragment group (A) is composed of two or more peptide fragments, and each peptide fragment constituting the peptide fragment group (A) consists of 5 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. The peptide fragment group (A) is composed of, among peptide fragments contained in the first composition, all peptide fragments each corresponding to a peptide fragment consisting of 5 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. Preferably, the peptide fragment group (A) is composed of three or more peptide fragments. Further preferably, the peptide fragment group (A) is composed of four or more peptide fragments.


The amino acid sequence of each peptide fragment constituting the peptide fragment group (A) is a part (moiety consisting of a plurality of consecutive amino acid residues) of positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. In other words, the peptide fragment group (A) can be generated by decomposition of positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. This does not mean that the alkaline phosphatase contained in the first composition is required to contain positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. The alkaline phosphatase contained in the first composition may not contain positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. However, the alkaline phosphatase contained in the first composition preferably contains positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5.


The amino acid sequence of each peptide fragment constituting the peptide fragment group (A) is not particularly limited as long as the amino acid sequence is a part of positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. The amino acid sequence of each peptide fragment constituting the peptide fragment group (A) is preferably a part of positions 505 to 578 of the amino acid sequence set forth in SEQ ID NO: 5, more preferably a part of positions 511 to 578 of the amino acid sequence set forth in SEQ ID NO: 5, and still more preferably a part of positions 511 to 571 of the amino acid sequence set forth in SEQ ID NO: 5.


The number of amino acid residues constituting each peptide fragment constituting the peptide fragment group (A) is not particularly limited as long as the number is 5 to 50, and the number is preferably 5 to 45, more preferably 10 to 40, and still more preferably 10 to 30.


Preferably, the peptide fragment group (A) contains one, two, three or four peptide fragments selected from the group consisting of the first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1, the second peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 2, the third peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 3 and the fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4. In this example, the peptide fragment group (A) may or may not contain a peptide fragment other than the first to fourth peptide fragments.


The amino acid sequence set forth in SEQ ID NO: 1 (VPLASETHGGEDVAVF) corresponds to positions 516 to 531 of the amino acid sequence set forth in SEQ ID NO: 5. The amino acid sequence set forth in SEQ ID NO: 2 (VPLASETHGGEDV) corresponds to positions 516 to 528 of the amino acid sequence set forth in SEQ ID NO: 5. The amino acid sequence set forth in SEQ ID NO: 3 (GPQAHLVHGVQEETFVAH) corresponds to positions 534 to 551 of the amino acid sequence set forth in SEQ ID NO: 5. The amino acid sequence set forth in SEQ ID NO: 4 (GPQAHLVHGVQE) corresponds to positions 534 to 545 of the amino acid sequence set forth in SEQ ID NO: 5.


The peptide fragment group (A) can be generated by decomposition of an alkaline phosphatase containing positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. The peptide fragment group (A) may be one generated by decomposition of an alkaline phosphatase not contained in the first composition, but is usually one generated by decomposition of an alkaline phosphatase contained in the first composition. Therefore, preferably, the alkaline phosphatase contained in the first composition is an alkaline phosphatase that can generate the peptide fragment group (A). Preferably, the alkaline phosphatase that can generate the peptide fragment group (A) is selected from the alkaline phosphatases (a) and (b). In this example, the first composition contains one or two or more alkaline phosphatases selected from the alkaline phosphatases (a) and (b).


Peptide Second Group (B)

The second composition contains the peptide fragment group (B). The peptide fragment group (B) is composed of two or more peptide fragments, and each peptide fragment constituting the peptide fragment group (B) consists of 13 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5 and contains positions 516 to 528 (VPLASETHGGEDV) of the amino acid sequence set forth in SEQ ID NO: 5. The peptide fragment group (B) is composed of, among peptide fragments contained in the second composition, all peptide fragments each corresponding to a peptide fragment consisting of 13 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5 and containing positions 516 to 528 of the amino acid sequence set forth in SEQ ID NO: 5.


In the amino acid sequence of each peptide fragment constituting the peptide fragment group (B), the position at which positions 516 to 528 of the amino acid sequence set forth in SEQ ID NO: 5 are contained is not particularly limited. The position at which positions 516 to 528 of the amino acid sequence set forth in SEQ ID NO: 5 are contained may be any of the N terminal part of a peptide fragment, the C terminal part of a peptide fragment, and a part other than the N terminal part and the C terminal part of a peptide fragment.


The amino acid sequence of each peptide fragment constituting the peptide fragment group (B) is a part (moiety consisting of a plurality of consecutive amino acid residues) of positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. In other words, the peptide fragment group (B) can be generated by decomposition of positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. This does not mean that the alkaline phosphatase contained in the second composition is required to contain positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. The alkaline phosphatase contained in the second composition may not contain positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. However, the alkaline phosphatase contained in the second composition preferably contains positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5.


The amino acid sequence of each peptide fragment constituting the peptide fragment group (B) is not particularly limited as long as the amino acid sequence is a part of positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5 and contains positions 516 to 528 of the amino acid sequence set forth in SEQ ID NO: 5. The amino acid sequence of each peptide fragment constituting the peptide fragment group (B) is preferably a part of positions 501 to 570 of the amino acid sequence set forth in SEQ ID NO: 5, more preferably a part of positions 501 to 560 of the amino acid sequence set forth in SEQ ID NO: 5, and still more preferably a part of positions 501 to 555 of the amino acid sequence set forth in SEQ ID NO: 5.


The number of amino acid residues constituting each peptide fragment constituting the peptide fragment group (B) is not particularly limited as long as the number is 13 to 50, and the number is preferably 13 to 45, more preferably 13 to 40, and still more preferably 13 to 35.


Preferably, the peptide fragment group (B) contains one or two peptide fragments selected from the group consisting of the first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1 and the second peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 2. In this example, the peptide fragment group (B) may or may not contain a peptide fragment other than the first and second peptide fragments.


The amino acid sequence set forth in SEQ ID NO: 1 (VPLASETHGGEDVAVF) corresponds to positions 516 to 531 of the amino acid sequence set forth in SEQ ID NO: 5 and contains positions 516 to 528 of the amino acid sequence set forth in SEQ ID NO: 5 (the underlined part corresponds to positions 516 to 528 of the amino acid sequence set forth in SEQ ID NO: 5). The amino acid sequence set forth in SEQ ID NO: 2 (VPLASETHGGEDV) corresponds to positions 516 to 528 of the amino acid sequence set forth in SEQ ID NO: 5.


The peptide fragment group (B) can be generated by decomposition of an alkaline phosphatase containing positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. The peptide fragment group (B) may be one generated by decomposition of an alkaline phosphatase not contained in the second composition, but is usually one generated by decomposition of an alkaline phosphatase contained in the second composition. Therefore, preferably, the alkaline phosphatase contained in the second composition is an alkaline phosphatase that can generate the peptide fragment group (B). Preferably, the alkaline phosphatase that can generate the peptide fragment group (B) is selected from the alkaline phosphatases (a) and (b). In this example, the second composition contains one or two or more alkaline phosphatases selected from the alkaline phosphatases (a) and (b).


Peptide Third Group (C)

The third composition contains a peptide fragment group (C). The peptide fragment group (C) is composed of two or more peptide fragments, and each peptide fragment constituting the peptide fragment group (C) consists of 12 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5 and contains positions 534 to 545 (GPQAHLVHGVQE) of the amino acid sequence set forth in SEQ ID NO: 5. The peptide fragment group (C) is composed of, among peptide fragments contained in the third composition, all peptide fragments each corresponding to a peptide fragment consisting of 12 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5 and containing positions 534 to 545 of the amino acid sequence set forth in SEQ ID NO: 5.


In the amino acid sequence of each peptide fragment constituting the peptide fragment group (C), the position at which positions 534 to 545 of the amino acid sequence set forth in SEQ ID NO: 5 may be any of the N terminal part of a peptide fragment, the C terminal part of a peptide fragment, and a part other than the N terminal part and the C terminal part of a peptide fragment.


The amino acid sequence of each peptide fragment constituting the peptide fragment group (C) is a part (moiety consisting of a plurality of consecutive amino acid residues) of positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. In other words, the peptide fragment group (C) can be generated by decomposition of positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. This does not mean that the alkaline phosphatase contained in the third composition is required to contain positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. The alkaline phosphatase contained in the third composition may not contain positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. However, the alkaline phosphatase contained in the third composition preferably contains positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5.


The amino acid sequence of each peptide fragment constituting the peptide fragment group (C) is not particularly limited as long as the amino acid sequence is a part of positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5 and contains positions 534 to 545 of the amino acid sequence set forth in SEQ ID NO: 5. The amino acid sequence of each peptide fragment constituting the peptide fragment group (C) is preferably a part of positions 506 to 578 of the amino acid sequence set forth in SEQ ID NO: 5, more preferably a part of positions 511 to 578 of the amino acid sequence set forth in SEQ ID NO: 5, and still more preferably a part of positions 521 to 578 of the amino acid sequence set forth in SEQ ID NO: 5.


The number of amino acid residues constituting each peptide fragment constituting the peptide fragment group (C) is not particularly limited as long as the number is 12 to 50, and the number is preferably 12 to 45, more preferably 12 to 40, and still more preferably 12 to 35.


Preferably, the peptide fragment group (C) contains one or two peptide fragments selected from the group consisting of the third peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 3 and the fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4. In this example, the peptide fragment group (C) may or may not contain a peptide fragment other than the third and fourth peptide fragments.


The amino acid sequence set forth in SEQ ID NO: 3 (GPQAHLVHGVQEETFVAH) corresponds to positions 534 to 551 of the amino acid sequence set forth in SEQ ID NO: 5 and contains positions 534 to 545 of the amino acid sequence set forth in SEQ ID NO: 5 (the underlined part corresponds to positions 534 to 545 of the amino acid sequence set forth in SEQ ID NO: 5). The amino acid sequence set forth in SEQ ID NO: 4 (GPQAHLVHGVQE) corresponds to positions 534 to 545 of the amino acid sequence set forth in SEQ ID NO: 5.


The peptide fragment group (C) can be generated by decomposition of an alkaline phosphatase containing positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. The peptide fragment group (C) may be one generated by decomposition of an alkaline phosphatase not contained in the third composition, but is usually one generated by decomposition of an alkaline phosphatase contained in the third composition. Therefore, preferably, the alkaline phosphatase contained in the third composition is an alkaline phosphatase that can generate the peptide fragment group (C). Preferably, the alkaline phosphatase that can generate the peptide fragment group (C) is selected from the alkaline phosphatases (a) and (b). In this example, the third composition contains one or two or more alkaline phosphatases selected from the alkaline phosphatases (a) and (b).


First Peptide Fragment

Preferably, the first, second, third, fourth, fifth or sixth compositions contain the first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1.


The first peptide fragment can be generated by decomposition of an alkaline phosphatase containing positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. The first peptide fragment may be one generated by decomposition of an alkaline phosphatase not contained in the first, second, third, fourth, fifth or sixth compositions, but is usually one generated by decomposition of an alkaline phosphatase contained in the first, second, third, fourth, fifth or sixth compositions. Therefore, preferably, the alkaline phosphatase contained in the first, second, third, fourth, fifth or sixth compositions is an alkaline phosphatase that can generate the first peptide fragment. Preferably, the alkaline phosphatase that can generate the first peptide fragment is selected from the alkaline phosphatases (a) and (b). In this example, the first, second, third, fourth, fifth or sixth compositions contain one or two or more alkaline phosphatases selected from the alkaline phosphatases (a) and (b).


Second Peptide Fragment

The fourth composition contains the second peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 2. Preferably, the fourth composition further contains one, two or three peptide fragments selected from the group consisting of the first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1, the third peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 3 and the fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4. In this example, the fourth composition may or may not contain a peptide fragment other than the first to fourth peptide fragments.


The second peptide fragment can be generated by decomposition of an alkaline phosphatase containing positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. The second peptide fragment may be one generated by decomposition of an alkaline phosphatase not contained in the fourth composition, but is usually one generated by decomposition of an alkaline phosphatase contained in the fourth composition. Therefore, preferably, the alkaline phosphatase contained in the fourth composition is an alkaline phosphatase that can generate the second peptide fragment. Preferably, the alkaline phosphatase that can generate the second peptide fragment is selected from the alkaline phosphatases (a) and (b). In this example, the fourth composition contains one or two or more alkaline phosphatases selected from the alkaline phosphatases (a) and (b).


Third Peptide Fragment

The fifth composition contains the third peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 3. Preferably, the fifth composition further contains one, two or three peptide fragments selected from the group consisting of the first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1, the second peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 2 and the fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4. In this example, the fifth composition may or may not contain a peptide fragment other than the first to fourth peptide fragments.


The third peptide fragment can be generated by decomposition of an alkaline phosphatase containing positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. The third peptide fragment may be one generated by decomposition of an alkaline phosphatase not contained in the fifth composition, but is usually one generated by decomposition of an alkaline phosphatase contained in the fifth composition. Therefore, preferably, the alkaline phosphatase contained in the fifth composition is an alkaline phosphatase that can generate the third peptide fragment. Preferably, the alkaline phosphatase that can generate the third peptide fragment is selected from the alkaline phosphatases (a) and (b). In this example, the fifth composition contains one or two or more alkaline phosphatases selected from the alkaline phosphatases (a) and (b).


Fourth Peptide Fragment

The sixth composition contains the fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4. Preferably, the sixth composition further contains one, two or three peptide fragments selected from the group consisting of the first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1, the second peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 2 and the third peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 3. In this example, the sixth composition may or may not contain a peptide fragment other than the first to fourth peptide fragments.


The fourth peptide fragment can be generated by decomposition of an alkaline phosphatase containing positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5. The fourth peptide fragment may be one generated by decomposition of an alkaline phosphatase not contained in the sixth composition, but is usually one generated by decomposition of an alkaline phosphatase contained in the sixth composition. Therefore, preferably, the alkaline phosphatase contained in the sixth composition is an alkaline phosphatase that can generate the fourth peptide fragment. Preferably, the alkaline phosphatase that can generate the fourth peptide fragment is selected from the alkaline phosphatases (a) and (b). In this example, the sixth composition contains one or two or more alkaline phosphatases selected from the alkaline phosphatases (a) and (b).


Content Ratio of Peptide Fragment Group (A) to Alkaline Phosphatase

In the first composition, the content ratio of the peptide fragment group (A) to the alkaline phosphatase satisfies formula (A):





(XA/Y)×100≤4.4000   (A).


In formula (A), XA represents a peak area value of the peptide fragment group (A) calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the first composition, and Y represents a peak area value of the alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis of the first composition. The “peak area value of the peptide fragment group (A)” means a total peak area value of all peptide fragments constituting the peptide fragment group (A). The “peak area value of the alkaline phosphatase” means, when the first composition contains one alkaline phosphatase, a peak area value of the one alkaline phosphatase, and, when the first composition contains two or more alkaline phosphatases, a total peak area value of the two or more alkaline phosphatases (i.e., total peak area value of all alkaline phosphatases contained in the first composition).


The LC-MS/MS analysis and the LC-UV analysis are performed by using a sample in which the content ratio of the peptide fragment group (A) to the alkaline phosphatase is the same as that of the first composition. The LC-MS/MS analysis and the LC-UV analysis can be performed, for example, by using an aqueous solution prepared from the first composition and with an alkaline phosphatase concentration of 10% by weight.


The LC-MS/MS analysis is one of the hyphenated methods. The hyphenated method is a method of analyzing by connecting a chromatograph such as a gas chromatograph and a liquid chromatograph to a mass spectrometer. The LC-MS/MS analysis is a method of analyzing by connecting a liquid chromatograph (LC) to a tandem mass spectrometer (MS/MS). In the LC-MS/MS analysis, analyte components separated by the liquid chromatograph are ionized, the ions thus produced are separated by the tandem mass spectrometer, and specific mass ions are fragmented and detected.


In the hyphenated method, an extracted ion chromatogram is a chromatogram expressed as a function of time obtained by measuring a mass spectrum at a certain time interval and storing it in a computer, followed by reading a relative intensity at a specific (not necessarily one type) m/z value. The m/z value of an ion of each peptide fragment constituting the peptide fragment group (A) used for detecting a peak of each peptide fragment constituting the peptide fragment group (A) is preferably 50 to 2,200, more preferably 200 to 1,500, and still more preferably 300 to 1,200. Regarding an ion of a peptide fragment with an m/z value being specified, it is possible to create an extracted ion chromatogram of the ion of the peptide fragment based on the m/z value. The m/z value of the first peptide fragment is 814.4018, the m/z value of the second peptide fragment is 655.8148, the m/z value of the third peptide fragment is 652.6623, and the m/z value of the fourth peptide fragment is 636.3282. Regarding a peptide fragment with an m/z value not being specified, after whether a certain peak corresponds to a peak of a predetermined peptide fragment or not is confirmed by an amino acid sequence analysis of a peptide fragment showing the peak, it is possible to create an extracted ion chromatogram of the peptide fragment based on the m/z value of the peak.


The LC-UV analysis is a method of analyzing by connecting a liquid chromatograph (LC) to an ultraviolet detector (UV detector). In the LC-UV analysis, an alkaline phosphatase is detected as a component having absorption at 214 nm.


Conditions of the LC-MS/MS analysis are as follows.


Conditions of LC-MS/MS Analysis
Apparatus Configuration

Mass spectrometer: maXis impact (manufactured by Bruker Daltnics, Inc.)


Conditions of Mass Spectrometry

Ionization method: ESI


Measured ion: cation


Capillary voltage: 4,500 V


Nebulizer: 2.0 bar


Dry gas: 8.0 L/min


Detector voltage: 1,823 V


Measuring span (MS): m/z 50 to 2,200


MS/MS Conditions

Measuring span (MS): m/z 50 to 2,200


Collision gas: nitrogen


Conditions of LC-UV Analysis
Apparatus Configuration

Liquid chromatograph: LC-30A system (manufactured by Shimadzu Corporation)


Detector: UV-Vis (190 to 900 nm, manufactured by Shimadzu Corporation)


Conditions of Liquid Chromatography

Column: Acquity BEH C18 1.7 μm (manufactured by Waters Corporation)


Column size: 2.1 mm×100 mm


Column temperature: 50° C.


Mobile phase flow rate: 0.2 mL/min


Mobile phase A: mixed solution of water/formic acid (1000:1)


Mobile phase B: mixed solution of acetonitrile/water/formic acid (900:100:1)


Injection volume: 20 μL


Gradient program:













TABLE 1







Times (min)
Mobile phase A (vol %)
Mobile phase B (vol %)




















0
100
0



10
100
0



40
35
65



40.1
0
100



50
0
100



50.1
100
0



60
100
0










The value of (XA/Y)×100 is not particularly limited as long as it is 4.4000 or less, and the smaller the value is, the more preferable it is. The value of (XA/Y)×100 is preferably 4.0000 or less, more preferably 3.5000 or less, and still more preferably 3.0000 or less. The lower limit of (XA/Y)×100 is a detection limit. In terms of obtaining an effect that matches an effort to decrease the value of (XA/Y)×100 (e.g., removal and separation of the peptide fragment group (A) by purification), the value of (XA/Y)×100 is preferably 0.0800 or more, more preferably 0.1000 or more, and still more preferably 0.1500 or more.


The smaller the peak area value of the peptide fragment group (A), which is calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis performed by using an aqueous solution prepared from the first composition and with an alkaline phosphatase concentration of 10% by weight, is, the more preferable it is. The peak area value of the peptide fragment group (A) is preferably 10,000 or less, more preferably 8,000 or less, and still more preferably 7,000 or less. The lower limit of the peak area value of the peptide fragment group (A) is a detection limit. In terms of obtaining an effect that matches an effort to decrease the peak area value of the peptide fragment group (A) (e.g., removal and separation of the peptide fragment group (A) by purification), the peak area value of the peptide fragment group (A) is preferably 600 or more, more preferably 800 or more, and still more preferably 1,000 or more.


The peak area value of an alkaline phosphatase, which is calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis performed by using an aqueous solution prepared from the first composition and with an alkaline phosphatase concentration of 10% by weight, is preferably 200,000 or more, more preferably 220,000 or more, and still more preferably 240,000 or more. The upper limit of the peak area value of an alkaline phosphatase is not particularly limited. The peak area value of an alkaline phosphatase is preferably 500,000 or less, more preferably 400,000 or less, and still more preferably 350,000 or less.


Content Ratio of Peptide Fragment Group (B) to Alkaline Phosphatase

In the second composition, the content ratio of the peptide fragment group (B) to the alkaline phosphatase satisfies formula (B):





(XB/Y)×100≤3.4000   (B).


In formula (B), XB represents a peak area value of the peptide fragment group (B) calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the second composition, and Y represents a peak area value of the alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis of the second composition. The “peak area value of the peptide fragment group (B)” means a total peak area value of all peptide fragments constituting the peptide fragment group (B). The “peak area value of the alkaline phosphatase” means, when the second composition contains one alkaline phosphatase, a peak area value of the one alkaline phosphatase, and, when the second composition contains two or more alkaline phosphatases, a total peak area value of the two or more alkaline phosphatases (i.e., total peak area value of all alkaline phosphatases contained in the second composition). The descriptions on formula (A) (including the descriptions on the LC-MS/MS analysis and the LC-UV analysis) also apply to formula (B) unless otherwise specified.


The m/z value of an ion of each peptide fragment constituting the peptide fragment group (B) used to detect a peak of each peptide fragment constituting the peptide fragment group (B) is preferably 50 to 2,200, more preferably 200 to 1,500, and still more preferably 300 to 1,200.


The value of (XB/Y)×100 is not particularly limited as long as it is 3.4000 or less, and the smaller the value is, the more preferable it is. The value of (XB/Y)×100 is preferably 3.0000 or less, more preferably 2.8000 or less, and still more preferably 2.5000 or less. The lower limit of (XB/Y)×100 is a detection limit. In terms of obtaining an effect that matches an effort to decrease the value of (XB/Y)×100 (e.g., removal and separation of the peptide fragment group (B) by purification), the value of (XB/Y)×100 is preferably 0.0800 or more, more preferably 0.1000 or more, and still more preferably 0.1500 or more.


The smaller the peak area value of the peptide fragment group (B), which is calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis performed by using an aqueous solution prepared from the second composition and with an alkaline phosphatase concentration of 10% by weight, is, the more preferable it is. The peak area value of the peptide fragment group (B) is preferably 7,500 or less, more preferably 7,000 or less, and still more preferably 6,000 or less. The lower limit of the peak area value of the peptide fragment group (B) is a detection limit. In terms of obtaining an effect that matches an effort to decrease the peak area value of the peptide fragment group (B) (e.g., removal and separation of the peptide fragment group (B) by purification), the peak area value of the peptide fragment group (B) is preferably 500 or more, more preferably 600 or more, and still more preferably 800 or more.


The peak area value of an alkaline phosphatase, which is calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis performed by using an aqueous solution prepared from the second composition and with an alkaline phosphatase concentration of 10% by weight, is preferably 200,000 or more, more preferably 220,000 or more, and still more preferably 240,000 or more. The upper limit of the peak area value of an alkaline phosphatase is not particularly limited. The peak area value of an alkaline phosphatase is preferably 500,000 or less, more preferably 400,000 or less, and still more preferably 350,000 or less.


In an example in which the second composition a peptide fragment consisting of 5 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5 other than the peptide fragment group (B), the second composition may or may not satisfy formula (A).


Content Ratio of Peptide Fragment Group (C) to Alkaline Phosphatase

In the third composition, the content ratio of the peptide fragment group (C) to the alkaline phosphatase satisfies formula (C):





(XC/Y)×100≤1.0000   (C).


In formula (C), XC represents a peak area value of the peptide fragment group (C) calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the third composition, and Y represents a peak area value of the alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis of the third composition. The “peak area value of the peptide fragment group (C)” means a total peak area value of all peptide fragments constituting the peptide fragment group (C). The “peak area value of the alkaline phosphatase” means, when the third composition contains one alkaline phosphatase, a peak area value of the one alkaline phosphatase, and, when the third composition contains two or more alkaline phosphatases, a total peak area value of the two or more alkaline phosphatases (i.e., total peak area value of all alkaline phosphatases contained in the third composition). The descriptions on formula (A) (including the descriptions on the LC-MS/MS analysis and the LC-UV analysis) also apply to formula (C) unless otherwise specified.


The m/z value of an ion of each peptide fragment constituting the peptide fragment group (C) used to detect a peak of each peptide fragment constituting the peptide fragment group (C) is preferably 50 to 2,200, more preferably 200 to 1,500, and still more preferably 300 to 1,200.


The value of (XC/Y)×100 is not particularly limited as long as it is 1.0000 or less, and the smaller the value is, the more preferable it is. The value of (XC/Y)×100 is preferably 0.9000 or less, more preferably 0.8000 or less, and still more preferably 0.7000 or less. The lower limit of (XC/Y)×100 is a detection limit. In terms of obtaining an effect that matches an effort to decrease the value of (XC/Y)×100 (e.g., removal and separation of the peptide fragment group (C) by purification), the value of (XC/Y)×100 is preferably 0.0800 or more, more preferably 0.1000 or more, and still more preferably 0.1500 or more.


The smaller the peak area value of the peptide fragment group (C), which is calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis performed by using an aqueous solution prepared from the third composition and with an alkaline phosphatase concentration of 10% by weight, is, the more preferable it is. The peak area value of the peptide fragment group (C) is preferably 2,400 or less, more preferably 2,000 or less, and still more preferably 1,500 or less. The lower limit of the peak area value of the peptide fragment group (C) is a detection limit. In terms of obtaining an effect that matches an effort to decrease the peak area value of the peptide fragment group (C) (e.g., removal and separation of the peptide fragment group (C) by purification), the peak area value of the peptide fragment group (C) is preferably 200 or more, more preferably 300 or more, and still more preferably 400 or more.


The peak area value of an alkaline phosphatase, which is calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis performed by using an aqueous solution prepared from the third composition and with an alkaline phosphatase concentration of 10% by weight, is preferably 200,000 or more, more preferably 220,000 or more, and still more preferably 240,000 or more. The upper limit of the peak area value of an alkaline phosphatase is not particularly limited. The peak area value of an alkaline phosphatase is preferably 500,000 or less, more preferably 400,000 or less, and still more preferably 350,000 or less.


In an example in which the third composition contains a peptide fragment consisting of 5 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5 other than the peptide fragment group (C), the third composition may or may not satisfy formula (A).


Content Ratio of First Peptide Fragment to Alkaline Phosphatase

In an example in which the first, second, third, fourth, fifth or sixth compositions contain the first peptide fragment, the content ratio of the first peptide fragment to the alkaline phosphatase preferably satisfies formula (1):





(X1/Y)×100≤1.0000   (1).


In formula (1), X1 represents a peak area value of the first peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the first, second, third, fourth, fifth or sixth composition, and Y represents a peak area value of the alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis of the first, second, third, fourth, fifth or sixth composition. The descriptions of formula (A) (including the descriptions on the LC-MS/MS analysis and the LC-UV analysis) also apply to formula (1) unless otherwise specified.


The value of (X1/Y)×100 is not particularly limited as long as it is 1.0000 or less, and the smaller the value is, the more preferable it is. The value of (X1/Y)×100 is preferably 0.9000 or less, more preferably 0.8000 or less, and still more preferably 0.7000 or less. The lower limit of (X1/Y)×100 is a detection limit. In terms of obtaining an effect that matches an effort to decrease the value of (X1/Y)×100 (e.g., removal and separation of the first peptide fragment by purification), the value of (X1/Y)×100 is preferably 0.0500 or more, more preferably 0.0600 or more, and still more preferably 0.0700 or more.


The smaller the peak area value of the first peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis performed by using an aqueous solution prepared from the first, second, third, fourth, fifth or sixth compositions and with an alkaline phosphatase concentration of 10% by weight is, the more preferable it is. The peak area value of the first peptide fragment is preferably 3,000 or less, more preferably 2,500 or less, and still more preferably 2,000 or less. The lower limit of the peak area value of the first peptide fragment is a detection limit. In terms of obtaining an effect that matches an effort to decrease the peak area value of the first peptide fragment (e.g., removal and separation of the first peptide fragment by purification), the peak area value of the first peptide fragment is preferably 100 or more, more preferably 150 or more, and still more preferably 200 or more.


The peak area value of an alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis performed by using an aqueous solution prepared from the first, second, third, fourth, fifth or sixth compositions and with an alkaline phosphatase concentration of 10% by weight is preferably 200,000 or more, more preferably 220,000 or more, and still more preferably 240,000 or more. The upper limit of the peak area value of an alkaline phosphatase is not particularly limited. The peak area value of an alkaline phosphatase is preferably 500,000 or less, more preferably 400,000 or less, and still more preferably 350,000 or less.


Content Ratio of Second Peptide Fragment to Alkaline Phosphatase

In the fourth composition, the content ratio of the second peptide fragment to the alkaline phosphatase satisfies formula (2):





(X2/Y)×100≤1.6000   (2).


In an example in which the first, second, third, fifth or sixth compositions contain the second peptide fragment, the content ratio of the second peptide fragment to the alkaline phosphatase preferably satisfies formula (2):





(X2/Y)×100≤1.6000   (2).


In formula (2), X2 represents a peak area value of the second peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the first, second, third, fourth, fifth or sixth compositions, and Y represents a peak area value of the alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis of the first, second, third, fourth, fifth or sixth compositions. The descriptions on formula (A) (including the descriptions on the LC-MS/MS analysis and the LC-UV analysis) also apply to formula (2) unless otherwise specified.


The value of (X2/Y)×100 is not particularly limited as long as it is 1.6000 or less, and the smaller the value is, the more preferable it is. The value of (X2/Y)×100 is preferably 1.5000 or less, more preferably 1.2000 or less, and still more preferably 1.0000 or less. The lower limit of (X2/Y)×100 is a detection limit. In terms of obtaining an effect that matches an effort to decrease the value of (X2/Y)×100 (e.g., removal and separation of the second peptide fragment by purification), the value of (X2/Y)×100 is preferably 0.0500 or more, more preferably 0.0600 or more, and still more preferably 0.0700 or more.


The smaller the peak area value of the second peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis performed by using an aqueous solution prepared from the first, second, third, fourth, fifth or sixth compositions and with an alkaline phosphatase concentration of 10% by weight is, the more preferable it is. The peak area value of the second peptide fragment is preferably 4,500 or less, more preferably 3,000 or less, and still more preferably 2,500 or less. The lower limit of the peak area value of the second peptide fragment is a detection limit. In terms of obtaining an effect that matches an effort to decrease the peak area value of the second peptide fragment (e.g., removal and separation of the second peptide fragment by purification), the peak area value of the second peptide fragment is preferably 100 or more, more preferably 150 or more, and still more preferably 200 or more.


The peak area value of an alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis performed by using an aqueous solution prepared from the first, second, third, fourth, fifth or sixth compositions and with an alkaline phosphatase concentration of 10% by weight is preferably 200,000 or more, more preferably 220,000 or more, and still more preferably 240,000 or more. The upper limit of the peak area value of an alkaline phosphatase is not particularly limited. The peak area value of an alkaline phosphatase is preferably 500,000 or less, more preferably 400,000 or less, and still more preferably 350,000 or less.


Content Ratio of Third Peptide Fragment to Alkaline Phosphatase

In the fifth composition, the content ratio of the third peptide fragment to the alkaline phosphatase satisfies formula (3):





(X3/Y)×100≤0.2000   (3).


In an example in which the first, second, third, fourth or sixth compositions contain the third peptide fragment, the content ratio of the third peptide fragment to the alkaline phosphatase preferably satisfies formula (3):





(X3/Y)×100≤0.2000   (3).


In formula (3), X3 represents a peak area value of the third peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the first, second, third, fourth, fifth or sixth compositions, and Y represents a peak area value of the alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis of the first, second, third, fourth, fifth or sixth compositions. The descriptions of formula (A) (including the descriptions on the LC-MS/MS analysis and the LC-UV analysis) also apply to formula (3) unless otherwise specified.


The value of (X3/Y)×100 is not particularly limited as long as it is 0.2000 or less, and the smaller the value is, the more preferable it is. The value of (X3/Y)×100 is preferably 0.1800 or less, more preferably 0.1700 or less, and still more preferably 0.1500 or less. The lower limit of (X3/Y)×100 is a detection limit. In terms of obtaining an effect that matches an effort to decrease the value of (X3/Y)×100 (e.g., removal and separation of the third peptide fragment by purification), the value of (X3/Y)×100 is preferably 0.0500 or more, more preferably 0.0600 or more, and still more preferably 0.0700 or more.


The smaller the peak area value of the third peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis performed by using an aqueous solution prepared from the first, second, third, fourth, fifth or sixth compositions and with an alkaline phosphatase concentration of 10% by weight is, the more preferable it is. The peak area value of the third peptide fragment is preferably 500 or less, more preferably 450 or less, and still more preferably 400 or less. The lower limit of the peak area value of the third peptide fragment is a detection limit. In terms of obtaining an effect that matches an effort to decrease the peak area value of the third peptide fragment (e.g., removal and separation of the third peptide fragment by purification), the peak area value of the third peptide fragment is preferably 100 or more, more preferably 150 or more, and still more preferably 200 or more.


The peak area value of an alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis performed by using an aqueous solution prepared from the first, second, third, fourth, fifth or sixth compositions and with an alkaline phosphatase concentration of 10% by weight is preferably 200,000 or more, more preferably 220,000 or more, and still more preferably 240,000 or more. The upper limit of the peak area value of an alkaline phosphatase is not particularly limited. The peak area value of an alkaline phosphatase is preferably 500,000 or less, more preferably 400,000 or less, and still more preferably 350,000 or less.


Content Ratio of Fourth Peptide Fragment to Alkaline Phosphatase

In the sixth composition, the content ratio of the fourth peptide fragment to the alkaline phosphatase satisfies formula (4):





(X4/Y)×100≤0.3500   (4).


In an example in which the first, second, third, fourth or fifth compositions contain the fourth peptide fragment, the content ratio of the fourth peptide fragment to the alkaline phosphatase preferably satisfies formula (4):





(X4/Y)×100≤0.3500   (4).


In formula (4), X4 represents a peak area value of the fourth peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the first, second, third, fourth, fifth or sixth compositions, and Y represents a peak area value of the alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis of the first, second, third, fourth, fifth or sixth compositions. The descriptions of formula (A) (including the descriptions on the LC-MS/MS analysis and the LC-UV analysis) also apply to formula (4) unless otherwise specified.


The value of (X4/Y)×100 is not particularly limited as long as it is 0.3500 or less, and the smaller the value is, the more preferable it is. The value of (X4/Y)×100 is preferably 0.3200 or less, more preferably 0.3000 or less, and still more preferably 0.2800 or less. The lower limit of (X4/Y)×100 is a detection limit. In terms of obtaining an effect that matches an effort to decrease the value of (X4/Y)×100 (e.g., removal and separation of the fourth peptide fragment by purification), the value of (X4/Y)×100 is preferably 0.0800 or more, more preferably 0.1000 or more, and still more preferably 0.1500 or more.


The smaller the peak area value of the fourth peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis performed by using an aqueous solution prepared from the first, second, third, fourth, fifth or sixth compositions and with an alkaline phosphatase concentration of 10% by weight is, the more preferable it is. The peak area value of the fourth peptide fragment is preferably 1000 or less, more preferably 900 or less, and still more preferably 800 or less. The lower limit of the peak area value of the fourth peptide fragment is a detection limit. In terms of obtaining an effect that matches an effort to decrease the peak area value of the fourth peptide fragment (e.g., removal and separation of the fourth peptide fragment by purification), the peak area value of the fourth peptide fragment is preferably 100 or more, more preferably 150 or more, and still more preferably 200 or more.


The peak area value of an alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis performed by using an aqueous solution prepared from the first, second, third, fourth, fifth or sixth compositions and with an alkaline phosphatase concentration of 10% by weight is preferably 200,000 or more, more preferably 220,000 or more, and still more preferably 240,000 or more. The upper limit of the peak area value of an alkaline phosphatase is not particularly limited. The peak area value of an alkaline phosphatase is preferably 500,000 or less, more preferably 400,000 or less, and still more preferably 350,000 or less.


Alkaline Phosphatase Specific Activity

Our compositions preferably have an alkaline phosphatase specific activity of 2,000 U/mg or more. The alkaline phosphatase specific activity of the compositions is more preferably 2,500 U/mg or more, and still more preferably 3,000 U/mg or more. The alkaline phosphatase specific activity of the compositions is measured as follows. By measuring the absorbance at 405 nm derived from p-nitrophenol produced by adding an alkaline phosphatase to an aqueous solution of p-nitrophenylphosphate, it is possible to calculate the specific activity of the alkaline phosphatase.


Other Components

Our compositions can contain one or two or more other components. Examples of the other components include aqueous vehicles such as water, metal salts such as a magnesium salt and a sodium salt, surfactants, organic acids, glycerin and the like.


Our compositions can be used for various applications requiring an alkaline phosphatase activity, and can contain one or two or more other components selected according to the applications.


In one example, the composition contains a protein such as an antigen and an antibody. In this example, the composition can be used for labeling a protein such as an antigen and an antibody with the alkaline phosphatase. In other words, in one example, the composition is a composition used to label a protein with the alkaline phosphatase. Labeling of a protein with the alkaline phosphatase can be performed by reacting a succinimide ester of the alkaline phosphatase, which is obtained by esterifying a carboxyl group of the alkaline phosphatase with succinimide, with an amino group of the protein.


In one example, the composition contains a substrate for the alkaline phosphatase. In this example, the composition can be used to dephosphorylate a substrate for the alkaline phosphatase. In other words, in one example, the composition is used to dephosphorylate a substrate for the alkaline phosphatase. The substrate for the alkaline phosphatase is not particularly limited as long as the substrate is a compound having a phosphoric monoester bond. Examples of the substrate for the alkaline phosphatase include a nucleic acid, a phospholipid, pyrophosphoric acid and the like. When the substrate for the alkaline phosphatase is treated with the composition, the phosphoric monoester bond of the substrate for the alkaline phosphatase is hydrolyzed by the alkaline phosphatase, resulting in dephosphorylation of the substrate for the alkaline phosphatase.


Preferably, the composition contains a nucleic acid. In this example, the composition can be used to dephosphorylate a nucleic acid. In other words, preferably, the composition is used to dephosphorylate a nucleic acid. The peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment coexisting in the alkaline phosphatase has a possibility of adversely influencing when the nucleic acid is dephosphorylated by the alkaline phosphatase. In this regard, in the composition, the content ratio of the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment to the alkaline phosphatase satisfies the above predetermined formula. In other words, in the composition, the relative content of the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment has been reduced. Therefore, by using the composition, it is possible to reduce the adverse influence of the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment that can occur when the nucleic acid is dephosphorylated by the alkaline phosphatase, thus enabling improvement in the dephosphorylation efficiency of the nucleic acid. By treating the nucleic acid with the composition, the 5′ end and/or the 3′ end of the nucleic acid can be dephosphorylated. By dephosphorylating the 5′ end and/or the 3′ end of the nucleic acid, it is possible to improve the labeling efficiency when the 5′ end and/or the 3′ end of the nucleic acid is/are labeled with the labeling substance. Particularly, when 32P is used as the labeling substance, this effect is remarkable. By dephosphorylating the 5′ end and/or the 3′ end of a vector used for DNA cloning, self-ligation of the vector can be prevented, thus enabling a reduction in the background of a transformed cell.


Examples of the nucleic acid include nucleic acids such as DNA, RNA, peptide nucleic acid (PNA) and locked nucleic acid (LNA) or a nucleic acid derivative. Examples of the nucleic acid derivative include a nucleic acid derivative containing a modified nucleotide (e.g., a nucleotide that has undergone reconstitution of a nucleotide or base containing a halogen group, an alkyl group such as a methyl group, an alkoxy group such as a methoxy group, a thio group and a carboxymethyl group and the like, saturation of a double bond, deamination, substitution of an oxygen molecule with a sulfur molecule and the like). The nucleic acid may be single-stranded or double-stranded. Examples of the DNA include chromosomal DNA, viral DNA, DNA of a bacterium, a fungus and the like, cDNA, fragments thereof and the like. Examples of the RNA include mRNA, rRNA, small RNA, fragments thereof and the like. The nucleic acid may be chemically synthesized DNA, RNA and the like. Specific examples of the nucleic acid include a gene of a pathogen, a virus and the like, or a part thereof, a causative gene for genetic disease or a part thereof and the like.


The nucleic acid can be prepared by an extraction by a conventional method from, for example, a biomaterial, a virus, a bacterium, a fungus, a food and drink and the like. Examples of the biomaterial include body fluids such as blood, serum, plasma, urine, stool, spinal fluid, saliva, swab and tissue fluid, a cell, a tissue and the like. The biomaterial may be animal-derived or plant-derived.


The amount of the nucleic acid contained in the composition can be appropriately adjusted according to the intended use of the composition (e.g., detection of the target nucleic acid) and the like. For example, when a certain nucleic acid (i.e., a target nucleic acid) among nucleic acids contained in the composition is intended to be detected, it is possible to amplify the target nucleic acid by performing a nucleic acid amplification method such as PCR, by using the nucleic acids contained in the composition as a template. This enables improvement in the detection sensitivity of the target nucleic acid.


The length (number of bases) of the nucleic acid can be appropriately adjusted according to the intended use of the composition (e.g., detection of the target nucleic acid) or the like. For example, when the nucleic acid is intended to be detected, the length of the nucleic acid is usually 10 to 300 bases, preferably 10 to 100 bases, and more preferably 15 to 100 bases. The length of the nucleic acid can be appropriately adjusted by fragmentation treatment. The length of the nucleic acid is, for example, a length at which the nucleic acid can be hybridized with a probe. When the nucleic acid is long (e.g., 1,500 bases or more, particularly 4,000 bases or more), it is preferable to perform fragmentation treatment of the nucleic acid and to adjust the length of the nucleic acid to an appropriate length. When fragmentation treatment is performed, it is not necessarily that a specific nucleic acid fragment is selected from the generated nucleic acid fragments, and the fragmentation product can be used as it is.


Examples of a method of cleaving the nucleic acid for fragmentation include a method of cleaving by irradiation with ultrasonic waves, a method of cleaving with an enzyme, a method of cleaving with a restriction enzyme, a method using a nebulizer, a method of cleaving with an acid or an alkali and the like. In the method of cleaving with ultrasonic waves, by controlling the output intensity and the irradiation time of the ultrasonic waves with which the nucleic acid is irradiated, it is possible to cleavage the nucleic acid into a desired length.


Preferably, the composition contains a dephosphorylated nucleic acid. The descriptions on the nucleic acid are the same as mentioned above. The dephosphorylated nucleic acid has a 5′ end and/or a 3′ end, each of which has been dephosphorylated by the alkaline phosphatase. In this example, the composition can be used to prepare a labeled nucleic acid containing the dephosphorylated nucleic acid and a labeling substance bound to the dephosphorylated nucleic acid. In other words, preferably, the composition is a composition used to prepare a labeled nucleic acid containing the dephosphorylated nucleic acid and a labeling substance bound to the dephosphorylated nucleic acid. The peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment coexisting in the alkaline phosphatase has a possibility of adversely influencing when the nucleic acid is dephosphorylated by the alkaline phosphatase and/or when the labeling substance is bound to the dephosphorylated nucleic acid. In this regard, in the composition, the content ratio of the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment to the alkaline phosphatase satisfies the above predetermined formula. In other words, in the composition, the relative contents of the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment has been reduced. Therefore, by using the composition, it is possible to reduce the adverse influence of the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment that can occur when the nucleic acid is dephosphorylated by the alkaline phosphatase and/or when the labeling substance is bound to the dephosphorylated nucleic acid, thus enabling improvement in the dephosphorylation efficiency of the nucleic acid and/or the labeling efficiency of the dephosphorylated nucleic acid.


Preferably, the composition contains a labeled nucleic acid containing a dephosphorylated nucleic acid and a labeling substance bound to the dephosphorylated nucleic acid. The descriptions on the nucleic acid are the same as mentioned above. The dephosphorylated nucleic acid has a 5′ end and/or a 3′ end, each of which has been dephosphorylated by the alkaline phosphatase. The labeling substance is bound to the 5′ end and/or the 3′ end of the dephosphorylated nucleic acid.


As the labeling substance, for example, a fluorescent dye, a fluorescent protein, a chemiluminescent body, a metal complex, a metal fine particle, biotin, a radioisotope or the like can be used. The reaction conditions when the target nucleic acid is labeled can be appropriately adjusted according to the type of the labeling substance. When the labeling substance is a fluorescent dye, the fluorescent dye can be detected by using a fluorescence microscope, a fluorescence scanner and the like.


Examples of the fluorescent dye include organic fluorescent dyes such as a fluorescein-based dye, a rhodamine-based dye, an Alexa Fluor (manufactured by Invitrogen)-based dye, a BODIPY (manufactured by Invitrogen)-based dye, a cascade-based dye, a coumarin-based dye, an eosin-based dye, an NBD-based dye, a pyrene-based dye, a Texas Red-based dye and a cyanine-based dye.


Specific examples of the organic fluorescent dye include 5-carboxy-fluorescein, 6-carboxy-fluorescein, 5,6-dicarboxy-fluorescein, 6-carboxy-2′,4,4′,5′,7,7′-hexachloro-fluorescein, 6-carboxy-2′,4,7,7′-tetrachloro-fluorescein, 6-carboxy-4′,5′-dichloro-2′,7′-dimethoxy-fluorescein, naphtho-fluorescein, 5-carboxy-rhodamine, 6-carboxy-rhodamine, 5,6-dicarboxy-rhodamine, rhodamine 6G, tetramethylrhodamine, X-rhodamine, Alexa Fluor 350, Alexa Fluor 405, Alexa Fluor 430, Alexa Fluor 488, Alexa Fluor 500, Alexa Fluor 514, Alexa Fluor 532, Alexa Fluor 546, Alexa Fluor 555, Alexa Fluor 568, Alexa Fluor 594, Alexa Fluor 610, Alexa Fluor 633, Alexa Fluor 635, Alexa Fluor 647, Alexa Fluor 660, Alexa Fluor 680, Alexa Fluor 700, Alexa Fluor 750, BODIPY FL, BODIPY TMR, BODIPY 493/503, BODIPY 530/550, BODIPY 558/568, BODIPY 564/570, BODIPY 576/589, BODIPY 581/591, BODIPY 630/650, BODIPY 650/665 (all of which are manufactured by Invitrogen), methoxycoumarin, eosin, NBD, pyrene, Cy5, Cy5.5, Cy7 and the like.


In the example in which the composition contains a labeled nucleic acid containing a dephosphorylated nucleic acid and a labeling substance bound to the dephosphorylated nucleic acid, the composition can be used as a nucleic acid sample to be subjected to a nucleic acid detection method. In other words, preferably, the composition is a nucleic acid sample to be subjected to the nucleic acid detection method. The labeled nucleic acid can contain a target nucleic acid to be detected and a nucleic acid other than the target nucleic acid. In the nucleic acid detection method, the target nucleic acid contained in the nucleic acid sample can be detected by using the labeling substance of the target nucleic acid as an index. The nucleic acid detection method is not particularly limited, and can be appropriately selected from known nucleic acid detection methods. The target nucleic acid can be detected, for example, by using the hybridization method. In one example of the hybridization method, the target nucleic acid can be detected by using a probe that can be hybridized with the target nucleic acid. In one example of the nucleic acid detection method using a probe, the probe is brought into contact with the nucleic acid sample containing the target nucleic acid to hybridize the probe with the target nucleic acid, and the target nucleic acid hybridized with the probe can be detected by using the labeling substance of the target nucleic acid as an index. When a nucleic acid other than the target nucleic acid is contained in the sample, it is preferable that, after the target nucleic acid is brought into contact with the probe, the nucleic acid that was not hybridized with the probe is removed by washing or the like.


The reaction conditions when the target nucleic acid is hybridized with the probe can be appropriately adjusted according to chain length of the target nucleic acid, the chain length of the probe and the like. The reaction time is usually 30 to 1,200 minutes, and preferably 60 to 360 minutes. The reaction temperature is usually 25 to 60° C., and preferably 30 to 40° C. The reaction is usually performed in an aqueous vehicle such as water.


The amount of the target nucleic acid or probe used is not particularly limited as long as the hybridization between the target nucleic acid and the probe can occur and the labeling substance bound to the target nucleic acid can be detected, and the amount can be appropriately adjusted according to the chain length of the target nucleic acid, the chain length of the probe, the type of the labeling substance and the like.


As the probe, for example, nucleic acids such as DNA, RNA, peptide nucleic acid (PNA) and locked nucleic acid (LNA) or a nucleic acid derivative can be used. Examples of the nucleic acid derivative include a nucleic acid derivative containing a modified nucleotide (e.g., a nucleotide that has undergone reconstitution of a nucleotide or base containing a halogen group, an alkyl group such as a methyl group, an alkoxy group such as a methoxy group, a thio group and a carboxymethyl group and the like, saturation of a double bond, deamination, substitution of an oxygen molecule with a sulfur molecule and the like).


The probe has a base sequence complementary to at least a part of the base sequence of the target nucleic acid, and can be hybridized with the target nucleic acid. When the target nucleic acid is double-stranded, the probe may be hybridized with a sense strand or may be hybridized with an antisense strand. The base sequence of the probe may be complementary to any part of the base sequence of the target nucleic acid, and is preferably complementary to a highly-specific part of the base sequence of the target nucleic acid. In other words, the base sequence of the probe is preferably complementary to a base sequence which other nucleic acids contained in the sample do not have, of the base sequence of the target nucleic acid.


Of the base sequence of the probe, the length (number of bases) of the part complementary to the base sequence of the target nucleic acid is not particularly limited, and is usually 10 to 150 bases, preferably 20 to 100 bases, and more preferably 20 to 70 bases. The probe may be composed of a base sequence complementary to the base sequence of the target nucleic acid, or may include a base sequence not complementary to the base sequence of the target nucleic acid. The full length (total number of bases) of the probe is usually 10 to 300 bases, preferably 20 to 200 bases, and more preferably 15 to 100 bases.


The probe may be any of a commercially available product, a synthetic product, a prepared product from a living body and the like. A nucleic acid having a length of up to 200 bases, which is referred to as an oligonucleic acid, can be easily artificially synthesized with a synthesizer.


The probe is preferably fixed to a support. In other words, preferably, the nucleic acid detection method is a nucleic acid detection method using a nucleic acid microarray. The nucleic acid microarray has a support and a plurality of probes fixed to the surface of the support. In the nucleic acid detection method using a nucleic acid microarray, the labeled target nucleic acid is brought into contact with a nucleic acid microarray provided with a probe that can be hybridized with the target nucleic acid, and the target nucleic acid hybridized with the probe can be detected by using the labeling substance bound to the target nucleic acid as an index. When a nucleic acid other than the target nucleic acid is contained in the sample, it is preferable that, after the target nucleic acid is brought into contact with the nucleic acid microarray, the nucleic acid that has not been hybridized with the probe on the nucleic acid microarray is removed by washing or the like. By using a nucleic acid microarray provided with a plurality of probes, two or more target nucleic acids can be simultaneously detected.


The support is not particularly limited as long as it can fix the probe. Examples of the support include a slide, a membrane, a bead and the like. Examples of the material of the support include inorganic materials such as glass, ceramic and silicon, and polymers such as polyethylene terephthalate, cellulose acetate, polycarbonate, polystyrene, polymethyl methacrylate and silicone rubber and the like.


Fixation of the probe to the support can be performed in accordance with a conventional method. As a method of fixing the probe to the support, a method of synthesizing an oligonucleic acid on the top surface of the support, a method of adding dropwise an oligonucleic acid synthesized in advance to the top surface of the support to fix and the like are known. Examples of the former method include the method by U.S. Pat. No. 5,705,610 A, the method by U.S. Pat. No. 6,142,266 A, the method by U.S. Pat. No. 7,037,659 A and the like. In those methods, since an organic solvent is used during DNA synthesis reaction, the support is desirably a material that is resistance to an organic solvent. For example, it is possible to use a glass support having an irregular structure fabricated by using the method disclosed in JP H10-503841 A. Particularly, in the method by U.S. '659, since the back of the support is irradiated with light to control DNA synthesis, the support is preferably a material having translucency. Examples of the latter method include the method by JP 3922454 B2, a method using a glass capillary and the like. As an example of the glass capillary, it is possible to use a self-made glass capillary, commercially available products such as a micropipette (manufactured by Micro Support Co., Ltd.; MP-005) and the like.


As a method of detecting the target nucleic acid, the sandwich hybridization method can be used. In the sandwich hybridization method, a first probe (capture probe) fixed to the support and a second probe (detection probe) not fixed to the support are used. The capture probe and the detection probe each have a base sequence complementary to different parts of the target nucleic acid, and can be hybridized with different parts of the target nucleic acid. The target nucleic acid is hybridized with the detection probe and the capture probe, thus forming a complex. By detecting a labeling substance contained in this complex, the target nucleic acid can be detected.


The sequence identity between the base sequence of the detection probe and the base sequence of the capture probe is preferably low. The sequence identity is preferably 20% or less, and more preferably 10% or less. In this regard, the identity between two base sequences is a numerical value obtained by aligning two sequences (inserting a gap, if necessary) so that bases are matched as many as possible, and then by dividing the number of matched bases by total number of bases (the higher number of bases when the number of bases of two base sequences is different), and the identity can be easily calculated with commercially available software such as FASTA and BLAST (also provided via the internet).


The signal detected in the method of detecting the target nucleic acid (e.g., intensity of the detected labeling substance) is compared with a surrounding noise. Specifically, the signal value obtained from a position on the support at which a probe is fixed is compared with the signal value (noise value) obtained from a position of the support at which no probe is fixed, and a ratio of the former numerical value to the noise value is defined as an S/N ratio. The detection accuracy can be represented by the S/N ratio. In other words, the larger the S/N ratio is, the higher the detection accuracy is, and the smaller the S/N ratio is, the lower the detection accuracy is.


In the example in which the composition contains a labeled nucleic acid containing a dephosphorylated nucleic acid and a labeling substance bound to the dephosphorylated nucleic acid, by using the composition as a nucleic acid sample in the nucleic acid detection method, it is possible to improve the detection sensitivity of the target nucleic acid. This effect is remarkable in a nucleic acid detection method using an extremely small amount (preferably 5 to 1,000 μL, more preferably 5 to 500 μL) of a nucleic acid sample. In the nucleic acid detection method using an extremely small amount of a nucleic acid sample, the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment contained in the nucleic acid sample has a possibility of adversely influencing the detection sensitivity. In this regard, in the composition, the content ratio of the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment to the alkaline phosphatase satisfies the above predetermined formula. In other words, in the composition, the relative content of the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment has been reduced. Therefore, in the nucleic acid detection method using an extremely small amount of a nucleic acid sample, by using the composition as the nucleic acid sample, it is possible to reduce the adverse influence of the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment, thus enabling remarkable improvement in the detection sensitivity of the target nucleic acid.


Preferably, the nucleic acid detection method is a nucleic acid detection method using a nucleic acid microarray. In the nucleic acid detection method using a nucleic acid microarray, an extremely small amount (preferably 5 to 1,000 μL, more preferably 5 to 500 μL) of a nucleic acid sample is used. Therefore, in the nucleic acid detection method using a nucleic acid microarray, by using the composition as the nucleic acid sample, it is possible to reduce the adverse influence of the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment, thus enabling remarkable improvement in the detection sensitivity of the target nucleic acid.


Production Method

The composition can be produced by separating the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment from an alkaline phosphatase extract from an organ of a bovine, a shrimp or the like, an alkaline phosphatase extract from a microorganism into which a gene encoding an alkaline phosphatase has been introduced, a bacterial cell homogenate of a microorganism into which a gene encoding an alkaline phosphatase has been introduced, a commercially available alkaline phosphatase product and the like. Examples of the method of separating the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment include dialysis, salting out, gel filtration, ultrafiltration, membrane separation, ion exchange, column chromatography, electrophoresis and the like. Regarding the method of separating the peptide fragment, one separation method may be used alone, or two or more separation methods may be used in combination. For example, by purifying a commercially available alkaline phosphatase product by column chromatography or the like, it is possible to make the content of the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment to the alkaline phosphatase be to a desired range. The column chromatography is, for example, liquid chromatography. The column and the mobile phase used in liquid chromatography is not particularly limited as long as the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment can be separated, and it is preferable to use a C18-supported reverse-phase column.


Use

The composition can be used for various methods requiring an alkaline phosphatase activity.


In one example, the composition is used for a method of producing a dephosphorylated nucleic acid, the method including the steps of:


providing the composition;


providing a nucleic acid; and


treating the nucleic acid with the composition to dephosphorylate the nucleic acid. The peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment coexisting in the alkaline phosphatase has a possibility of adversely influencing when the nucleic acid is dephosphorylated by the alkaline phosphatase. In this regard, in the composition, the content ratio of the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment to the alkaline phosphatase satisfies the above predetermined formula. In other words, in the composition, the relative content of the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment has been reduced. Thus, by treating the nucleic acid with the composition, it is possible to improve the dephosphorylation efficiency of the nucleic acid.


In one example, the composition is used for a method of producing a labeled nucleic acid, the method including the steps of:


providing the composition;


providing a nucleic acid;


providing a labeling substance;


treating the nucleic acid with the composition to dephosphorylate the nucleic acid; and


binding the labeling substance to the dephosphorylated nucleic acid. The peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment coexisting in the alkaline phosphatase has a possibility of adversely influencing when the nucleic acid is dephosphorylated by the alkaline phosphatase and/or when the labeling substance is bound to the dephosphorylated nucleic acid. In this regard, in the composition, the content ratio of the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment to the alkaline phosphatase satisfies the above predetermined formula. In other words, in the composition, the relative content of the peptide fragment group (A), the peptide fragment group (B), the peptide fragment group (C), the second peptide fragment, the third peptide fragment or the fourth peptide fragment has been reduced. Thus, by treating the nucleic acid with the composition, it is possible to improve the dephosphorylation efficiency of the nucleic acid and/or the labeling efficiency of the dephosphorylated nucleic acid.


In the step of treating the nucleic acid with the composition to dephosphorylate the nucleic acid, the reaction conditions can be appropriately adjusted. The reaction time is usually 10 to 60 minutes, and preferably 20 to 50 minutes. The reaction temperature is usually 20 to 60° C., and preferably 25 to 45° C. The reaction is usually performed in an aqueous vehicle such as water. The nucleic acid is, for example, DNA, RNA and the like. When the nucleic acid is treated with the composition, the 5′ end and/or the 3′ end of the nucleic acid is dephosphorylated.


In the step of binding the labeling substance to the dephosphorylated nucleic acid, as the labeling substance, for example, a fluorescent dye, a fluorescent protein, a chemiluminescent body, a metal complex, a metal fine particle, biotin, a radioisotope, and the like can be used. The reaction conditions can be appropriately adjusted according to the type of the labeling substance. The dephosphorylated nucleic acid has a 5′ end and/or a 3′ end, each of which has been dephosphorylated by the alkaline phosphatase, and the labeling substance can be bound to the dephosphorylated 5′ end and/or 3′ end.


EXAMPLES

Our compositions and methods will be described in detail by way of Examples, but this disclosure is not limited to the following Examples.


Conditions of LC-MS/MS Analysis

Conditions of the LC-MS/MS analysis used in Examples and Comparative Examples were as follows.


Apparatus Configuration

Mass spectrometer: maXis impact (manufactured by Bruker Daltnics, Inc.)


Conditions of Mass Spectrometry

Ionization method: ESI


Measured ion: cation


Capillary voltage: 4,500 V


Nebulizer: 2.0 bar


Dry gas: 8.0 L/min


Detector voltage: 1,823 V


Measuring span (MS): m/z 50 to 2,200


MS/MS Conditions

Measuring span (MS): m/z 50 to 2,200


Collision gas: nitrogen


Conditions of LC-UV Analysis

Conditions of the LC-UV analysis used in Examples and Comparative Examples were as follows.


Apparatus Configuration

Liquid chromatograph: LC-30A system (manufactured by Shimadzu Corporation)


Detector: UV-Vis (190 to 900 nm, manufactured by Shimadzu Corporation)


Conditions of Liquid Chromatography

Column: Acquity BEH C18 1.7 μm (manufactured by Waters Corporation)


Column size: 2.1 mm×100 mm


Column temperature: 50° C.


Mobile phase flow rate: 0.2 mL/min


Mobile phase A: mixed solution of water/formic acid (1000:1)


Mobile phase B: mixed solution of acetonitrile/water/formic acid (900:100:1)


Injection volume: 20 μL


Gradient program:













TABLE 2







Times (min)
Mobile phase A (vol %)
Mobile phase B (vol %)




















0
100
0



10
100
0



40
35
65



40.1
0
100



50
0
100



50.1
100
0



60
100
0










Nucleic Acid Detection Method

The nucleic acid detection method used in Examples and Comparative Examples was as follows.


The detection method of a nucleic acid was performed by using a DNA chip (DNA microarray). Specifically, detection was performed by using “3D-Gene” human miRNA oligo chip (compatible with miRBase release 21) manufactured by Toray Industries, Inc.


Comparative Examples 1 to 8

Eight alkaline phosphatase products purchased from five companies (hereinafter referred to as “composition C1” to “composition C8”) were used as the alkaline phosphatase compositions of Comparative Examples 1 to 8. The alkaline phosphatase contained in each of the compositions C1 to C8 was an alkaline phosphatase derived from the intestinal tract of a bovine. When the alkaline phosphatase specific activities of the compositions C1 to C8 were measured, they were 2,238 U/mg for the composition C1, 2,492 U/mg for the composition C2, 2,431 U/mg for the composition C3, 2,519 U/mg for the composition C4, 2,411 U/mg for the composition C5, 2,552 U/mg for the composition C6, 2,448 U/mg for the composition C7, and 2,490 U/mg for the composition C8. The alkaline phosphatase specific activities were measured by a method using p-nitrophenylphosphate. Specifically, the method was as follows.


The following solutions A and B were provided:


Solution A: 1M diethanolamine buffer (pH 9.8)


Solution B: aqueous 0.67M p-nitrophenolphosphate solution.


2.9 mL of the solution A and 0.1 mL of the solution B were prepared in a cuvette (optical path length=1 cm), and warmed at 37° C. for 5 minutes. Then, 0.1 mL of an aqueous alkaline phosphatase solution was added, and the absorbance change at 405 nm (37° C.) was measured with a spectrophotometer for 3 to 5 minutes to obtain an absorbance change per unit time (ΔOD). By using as a control, a sample to which water was added in place of the aqueous alkaline phosphatase solution, the absorbance change was obtained (ΔOD blank). The alkaline phosphatase activity (U/mL) was calculated from the formula:





Alkaline phosphatase activity (U/mL)=(ΔOD−ΔOD blank)×3.1/(18.2×0.1×1.0).


The concentration of the alkaline phosphatase in the aqueous alkaline phosphatase solution was calculated by measuring the absorbance at 214 nm. The aqueous alkaline phosphatase solution was diluted with distilled water so that the absorbance at 214 nm became 0.1 to 1.0, and 1 Abs was approximated to 1 mg/mL, and then the value obtained by multiplying by the dilution rate was regarded as the concentration of the alkaline phosphatase. The specific activity represents an activity (U/mg) per 1 mg of the alkaline phosphatase, and was calculated by the abovementioned measurement method.


An aqueous 10% by weight alkaline phosphatase solution was prepared from each of the compositions C1 to C8, and by using this aqueous solution, an LC-UV analysis and an LC-MS/MS analysis were performed. Based on the extracted ion chromatogram obtained by the LC-MS/MS analysis, the peak area value of each of the first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1 (VPLASETHGGEDVAVF), the second peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 2 (VPLASETHGGEDV), the third peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 3 (GPQAHLVHGVQEETFVAH) and the fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4 (GPQAHLVHGVQE) was calculated by an automatic integration method. Based on the chromatogram obtained by the LC-UV analysis, the peak area value of the alkaline phosphatase was calculated by an automatic integration method. In the LC-UV analysis, the alkaline phosphatase was detected as a component having absorption at 214 nm.



FIG. 1 shows an extracted ion chromatogram on the first peptide fragment obtained by an LC-MS/MS analysis of the composition C2 in Comparative Example 2.



FIG. 2 shows an extracted ion chromatogram on the second peptide fragment obtained by an LC-MS/MS analysis of the composition C2 in Comparative Example 2.



FIG. 3 shows an extracted ion chromatogram on the third peptide fragment obtained by an LC-MS/MS analysis of the composition C2 in Comparative Example 2.



FIG. 4 shows an extracted ion chromatogram on the fourth peptide fragment obtained by an LC-MS/MS analysis of the composition C2 in Comparative Example 2.


By using each of the alkaline phosphatase compositions of Comparative Examples 1 to 8, a nucleic acid was dephosphorylated, and the obtained dephosphorylated nucleic acid was labeled with a cyanine-based organic fluorescent dye. Specifically, dephosphorylation reaction and labeling reaction were performed as follows.


Whole blood collected from a healthy individual was centrifuged to obtain 1 mL of serum. From the serum, microRNA was extracted by using the “3D-Gene” RNA extraction reagent from liquid sample kit (manufactured by Toray Industries, Inc.). The obtained extracted microRNA was regarded as a mother liquor and was labeled by using “3D-Gene” miRNA labeling kit (manufactured by Toray Industries, Inc.). Specifically, 5 μL of the obtained extracted microRNA was added to a mixed solution of 0.4 μL of AP buffer and 1.0 μL of Spike Control of the abovementioned kit, and 0.4 μL of the composition C1 was further added to prepare a solution. Then, the prepared solution was incubated at 37° C. for 40 minutes, followed by allowing to stand on ice for 2 minutes. Then, 1.2 μL of LE Buffer, 3.0 μL of 3D-Gene Fluorescent Label, 2.5 μL of Nuclease free water and 1.0 μL of Labeling enzyme were added, and the obtained solution was incubated at 16° C. for 1 hour, followed by incubation at 65° C. for 15 minutes to obtain a labeled nucleic acid. Dephosphorylation reaction and labeling reaction were performed by using the same method as mentioned above, in which the compositions C2 to C8 and the same extracted microRNA mother liquor were used.


By using the obtained labeled nucleic acid, detection of a nucleic acid was performed. Specifically, for the labeled sample RNA, hybridization was performed by using a DNA chip (“3D-Gene” miRNA chip, manufactured by Toray Industries, Inc.) in accordance with the standard protocol thereof. The DNA chip after hybridization was subjected to a microarray scanner (manufactured by Toray Industries, Inc.) to measure the fluorescence intensity. Regarding the setting of the scanner, the laser output was set at 100%, and the voltage setting of the photomultiplier was set at AUTO setting. Detection of a nucleic acid was performed by using a DNA chip (DNA microarray) as mentioned above. The number of valid spots in the DNA chip was determined to calculate the detection rate (%). Specifically, of a total of 2,588 spots on the DNA chip, spots with a value obtained by subtracting the noise (signal value at a site having no spot) from the detection signal value being 100 or more were regarded as valid spots, and the value obtained by dividing the number of valid spots by the number of all spots and by multiplying by 100 was regarded as the detection rate. The results are shown in Table 4-2.


Examples 1 to 4

The alkaline phosphatase compositions of Comparative Examples 2 to 4 and 8 (compositions C2 to C4 and C8) were purified by the following method to obtain alkaline phosphatase compositions of Examples 1 to 4 (hereinafter referred to as “composition E1” to “composition E4”). The purification method was as follows.


Dialysis Step

The composition C2 (30 μL) was dialyzed three times with a dialysis buffer (1 mL, 50 mM Tris-HCl, 2 mM MgCl2, 0.2 mM ZnCl2) by using a dialysis cup (cutoff molecular weight of 3.5 K), and the concentrate was collected.


Gel Filtration Step

The concentrate after dialysis treatment was collected by filtration with a buffer (2.5 mL, 10 mM Tris-HCl, 1 mM MgCl2, 0.1 mM ZnCl2, 50 mM KCl, 55% by weight glycerin) by using a gel filtration column.


Hydrophobic Column Step

From the collected solution after gel filtration, the alkaline phosphatase fraction was collected by using a hydrophobic column under the following conditions.


Mobile phase flow rate: 1.0 mL/min


Mobile phase A: 20 mM disodium hydrogenphosphate, 3M ammonium sulfate (50/50)


Mobile phase B: 20 mM disodium hydrogenphosphate


Detector: UV 214 nm


Gradient program:













TABLE 3







Times (min)
Mobile phase A (vol %)
Mobile phase B (vol %)




















0
100
0



3
100
0



40
0
100



50
0
100



55
100
0



65
100
0










Dialysis Step

The collected alkaline phosphatase fraction was dialyzed three times under the same conditions as for the abovementioned dialysis, and the concentrate was collected.


Ultrafiltration Step

The collected concentrate was collected by filtration with a buffer (2.5 mL, 10 mM Tris-HCl, 1 mM MgCl2, 0.1 mM ZnCl2, 50 mM KCl, 55% by weight glycerin) by using an ultrafiltration column (cutoff molecular weight of 10 K) to obtain the composition E1.


The compositions E2, E3 and E4 were also obtained from the compositions C3, C4 and C8, respectively, by using the same method as mentioned above.


When the alkaline phosphatase specific activities of the alkaline phosphatase compositions of Examples 1 to 4 were measured, they were 2,490 U/mg for the composition E1, 2,420 U/mg for the composition E2, 2,522 U/mg for the composition E3, and 2,470 U/mg for the composition E4. The alkaline phosphatase specific activities were measured in the same manner as mentioned above.


An aqueous 10% by weight alkaline phosphatase solution was prepared from each of the compositions E1 to E4, and by using this aqueous solution, an LC-UV analysis and an LC-MS/MS analysis were performed. Based on the extracted ion chromatogram obtained by the LC-MS/MS analysis, the peak area value of each of the first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1 (VPLASETHGGEDVAVF), the second peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 2 (VPLASETHGGEDV), the third peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 3 (GPQAHLVHGVQEETFVAH) and the fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4 (GPQAHLVHGVQE) was calculated by an automatic integration method. Based on the chromatogram obtained by the LC-UV analysis, the peak area value of the alkaline phosphatase was calculated by an automatic integration method. In the LC-UV analysis, the alkaline phosphatase was detected as a component having absorption at 214 nm.



FIG. 5 shows an extracted ion chromatogram on the first peptide fragment obtained by an LC-MS/MS analysis of the composition E1 (purified product of the composition C2) in Example 1.



FIG. 6 shows an extracted ion chromatogram on the second peptide fragment obtained by an LC-MS/MS analysis of the composition E1 (purified product of the composition C2) in Example 1.



FIG. 7 shows an extracted ion chromatogram on the third peptide fragment obtained by an LC-MS/MS analysis of the composition E1 (purified product of the composition C2) in Example 1.



FIG. 8 shows an extracted ion chromatogram on the fourth peptide fragment obtained by an LC-MS/MS analysis of the composition E1 (purified product of the composition C2) in Example 1.



FIG. 9 shows a chromatogram on an alkaline phosphatase obtained by an LC-UV analysis of the composition E1 (purified product of the composition C2) in Example 1. A chromatogram on an alkaline phosphatase obtained by an LC-UV analysis of each of the composition in Examples 2 to 4 and Comparative Examples 1 to 8 was the same as FIG. 9.


By using the alkaline phosphatase compositions of Examples 1 to 4, a nucleic acid was dephosphorylated, and the obtained dephosphorylated nucleic acid was labeled with a cyanine-based organic fluorescent dye. Dephosphorylation reaction and labeling reaction were performed in the same manner as mentioned above.


By using the obtained labeled nucleic acid, detection of a nucleic acid was performed. Detection of a nucleic acid was performed by using a DNA chip (DNA microarray) as mentioned above. The number of valid spots in the DNA chip was determined to calculate the detection rate (%). The results are shown in Table 4-1.











TABLE 4-1









Examples












1
2
3
4














Peak area value of First
1783
517
2416
246


peptide fragment (X1)






Peak area value of Second
1766
949
1769
585


peptide fragment (X2)






Peak area value of Third
226
226
360
200


peptide fragment (X3)






Peak area value of Fourth
668
367
736
278


peptide fragment (X4)






Peak area value of
263754
268264
267135
258635


Alkaline phosphatase (Y)






(X1/Y) × 100
0.6762
0.1928
0.9044
0.0951


(X2/Y) × 100
0.6697
0.3536
0.6624
0.2262


(X3/Y) × 100
0.0856
0.0843
0.1346
0.0773


(X4/Y) × 100
0.2534
0.1367
0.2756
0.1075


((X1 + X2)/Y) × 100
1.3459
0.5463
1.5668
0.3213


((X3 + X4)/Y) × 100
0.3390
0.2210
0.4102
0.1848


((X1 + X2 +
1.6849
0.7673
1.9770
0.5061


X3 + X4)/Y) × 100






Number of valid spots
1632
1582
1577
1693


Detection rate (%)
63
61
61
65

















TABLE 4-2








Comparative Examples
















1
2
3
4
5
6
7
8


















Peak area value of First peptide fragment (X1)
7534
23335
125531
1405
16063
1406
37705
33511


Peak area value of Second peptide fragment (X2)
4536
2811195
5945
124326
17235
6523
118914
672270


Peak area value of Third peptide fragment (X3)
5580
637579
37977
78293
2662
481
12520
107131


Peak area value of Fourth peptide fragment (X4)
1050
564467
2922
22250
1197
2012
18566
464618


Peak area value of Alkaline phosphatase (Y)
268197
288388
245377
208272
232234
232042
272193
276191


(X1/Y) × 100
2.8091
8.0915
51.1585
0.6746
6.9167
0.6061
13.8523
12.1333


(X2/Y) × 100
1.6913
974.7951
2.4228
59.6940
7.4215
2.8110
43.6874
243.4081


(X3/Y) × 100
2.0806
221.0835
15.4770
37.5917
1.1462
0.2073
4.5999
38.7888


(X4/Y) × 100
0.3915
195.7316
1.1908
10.6831
0.5153
0.8669
6.8208
168.2237


((X1 +X2)/Y) × 100
4.5004
982.8866
53.5813
60.3686
14.3382
3.4171
57.5397
255.5414


((X3 +X4)/Y) × 100
2.4721
416.8151
16.6679
48.2748
1.6615
1.0742
11.4206
207.0126


((X1 +X2 +X3 +X4)/Y) × 100
6.9725
1399.7017
70.2492
108.6435
15.9997
4.4912
68.9604
462.5539


Number of valid spots
1442
1080
1259
1241
1211
1153
1245
1205


Detection rate (%)
56
42
49
48
47
45
48
47









As shown in Tables 4-1 and 4-2, when each of the nucleic acid samples prepared by using the alkaline phosphatase compositions of Comparative Examples 1 to 8 was used in the nucleic acid detection method, the number of valid spots was less than 1,500, while, when each of the nucleic acid samples prepared by using the alkaline phosphatase compositions of Examples 1 to 4 was used in the nucleic acid detection method, the number of valid spots was 1,500 or more. The detection rates in Comparative Examples 1 to 8 were different although the alkaline phosphatase specific activities of the alkaline phosphatase compositions were almost the same, while the detection rates in Examples 1 to 4 were almost the same and were higher than the detection rates in Comparative Examples 1 to 8.


As shown in Tables 4-1 and 4-2, the value of ((X1+X2+X3+X4)/Y)×100, which represents the content ratio of a total of the first to fourth peptide fragments to the alkaline phosphatase, was more than 4.4000 for each of the alkaline phosphatase compositions of Comparative Examples 1 to 8 (the minimum value was 4.4912 in the alkaline phosphatase composition of Comparative Example 6), while the value was 4.4000 or less for each of the alkaline phosphatase compositions of Examples 1 to 4. This is considered as one of the primary causes of the difference in the effect between Examples 1 to 4 and Comparative Examples 1 to 8.


As shown in Tables 4-1 and 4-2, the value of ((X1+X2)/Y)×100, which represents the content ratio of a total of the first and second peptide fragments to the alkaline phosphatase, was more than 3.4000 for each of the alkaline phosphatase compositions of Comparative Examples 1 to 8 (the minimum value was 3.4171 in the alkaline phosphatase composition of Comparative Example 6), while the value was 3.4000 or less for each of the alkaline phosphatase compositions of Examples 1 to 4. This is considered as one of the primary causes of difference in the effect mentioned above between Examples 1 to 4 and Comparative Examples 1 to 8.


As shown in Tables 4-1 and 4-2, the value of ((X3+X4)/Y)×100, which represents the content ratio of a total of the third and fourth peptide fragments to the alkaline phosphatase, was more than 1.0000 for each of the alkaline phosphatase compositions of Comparative Examples 1 to 8 (the minimum value was 1.0742 in the alkaline phosphatase composition of Comparative Example 6), while the value was 1.0000 or less for each of the alkaline phosphatase compositions of Examples 1 to 4. This is considered as one of the primary causes of the difference in the effect between Examples 1 to 4 and Comparative Examples 1 to 8.


As shown in Tables 4-1 and 4-2, the value of (X2/Y)×100, which represents the content ratio of the second peptide fragment to the alkaline phosphatase, was more than 1.6000 for each of the alkaline phosphatase compositions of Comparative Examples 1 to 8 (the minimum value was 1.6913 in the alkaline phosphatase composition of Comparative Example 1), while the value was 1.6000 or less for each of the alkaline phosphatase compositions of Examples 1 to 4. This is considered as one of the primary causes of the difference in the effect between Examples 1 to 4 and Comparative Examples 1 to 8.


As shown in Tables 4-1 and 4-2, the value of (X3/Y)×100, which represents the content ratio of the third peptide fragment to the alkaline phosphatase, was more than 0.2000 for each of the alkaline phosphatase compositions of Comparative Examples 1 to 8 (the minimum value was 0.2073 in the alkaline phosphatase composition of Comparative Example 6), while the value was 0.2000 or less for each of the alkaline phosphatase compositions of Examples 1 to 4. This is considered as one of the primary causes of the difference in the effect between Examples 1 to 4 and Comparative Examples 1 to 8.


As shown in Tables 4-1 and 4-2, the value of (X4/Y)×100, which represents the content ratio of the fourth peptide fragment to the alkaline phosphatase, was more than 0.3500 for each of the alkaline phosphatase compositions of Comparative Examples 1 to 8 (the minimum value was 0.3915 in the alkaline phosphatase composition of Comparative Example 1), while the value was 0.3500 or less for each of the alkaline phosphatase compositions of Examples 1 to 4. This is considered as one of the primary causes of the difference in the effect between Examples 1 to 4 and Comparative Examples 1 to 8.


As shown in Tables 4-1 and 4-2, the value of (X1/Y)×100, which represents the content ratio of the first peptide fragment to the alkaline phosphatase, was more than 1.0000 for each of the alkaline phosphatase compositions of Comparative Examples 1 to 3, 5, 7 and 8 (but 1.0000 or less for each of Comparative Examples 4 and 6), while the value was 1.0000 or less for each of the alkaline phosphatase compositions of Examples 1 to 4. This is considered as one of the secondary causes of the difference in the effect between Examples 1 to 4 and Comparative Examples 1 to 3, 5, 7 and 8.

Claims
  • 1-14. (canceled)
  • 15. A composition comprising: an alkaline phosphatase; anda peptide fragment group (A) composed of two or more peptide fragments, wherein each of the two or more peptide fragments consists of 5 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5,wherein a content ratio of the peptide fragment group (A) to the alkaline phosphatase satisfies formula (A): (XA/Y)×100≤4.4000   (A),wherein XA represents a peak area value of the peptide fragment group (A) calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y represents a peak area value of the alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis of the composition.
  • 16. A composition comprising: an alkaline phosphatase; anda peptide fragment group (B) composed of two or more peptide fragments, wherein each of the two or more peptide fragments consists of 13 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5 and comprises positions 516 to 528 of the amino acid sequence set forth in SEQ ID NO: 5,wherein a content ratio of the peptide fragment group (B) to the alkaline phosphatase satisfies formula (B): (XB/Y)×100≤3.4000   (B),wherein XB represents a peak area value of the peptide fragment group (B) calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y represents a peak area value of the alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis of the composition.
  • 17. A composition comprising: an alkaline phosphatase; anda peptide fragment group (C) composed of two or more peptide fragments, wherein each of the two or more peptide fragments consists of 12 to 50 consecutive amino acid residues selected from positions 501 to 578 of the amino acid sequence set forth in SEQ ID NO: 5 and comprises positions 534 to 545 of the amino acid sequence set forth in SEQ ID NO: 5,wherein a content ratio of the peptide fragment group (C) to the alkaline phosphatase satisfies formula (C): (XC/Y)×100≤1.0000   (C),wherein XC represents a peak area value of the peptide fragment group (C) calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y represents a peak area value of the alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis of the composition.
  • 18. A composition comprising: an alkaline phosphatase; anda second peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 2,wherein a content ratio of the second peptide fragment to the alkaline phosphatase satisfies formula (2): (X2/Y)×100≤1.6000   (2),wherein X2 represents a peak area value of the second peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y represents a peak area value of the alkaline phosphatase calculated by an automatic integration method from a chromatogram obtained by an LC-UV analysis of the composition.
  • 19. The composition according to claim 4, wherein: the composition further comprises a first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1; anda content ratio of the first peptide fragment to the alkaline phosphatase satisfies formula (1): (X1/Y)×100≤1.0000   (1),wherein X1 represents a peak area value of the first peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.
  • 20. The composition according to claim 18, wherein: the composition further comprises a third peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 3; anda content ratio of the third peptide fragment to the alkaline phosphatase satisfies formula (3): (X3/Y)×100≤0.2000   (3),wherein X3 represents a peak area value of the third peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.
  • 21. The composition according to claim 18, wherein: the composition further comprises a fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4; anda content ratio of the fourth peptide fragment to the alkaline phosphatase satisfies formula (4): (X4/Y)×100≤0.3500   (4),wherein X4 represents a peak area value of the fourth peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.
  • 22. A composition comprising: an alkaline phosphatase; anda third peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 3,wherein a content ratio of the third peptide fragment to the alkaline phosphatase satisfies formula (3): (X3/Y)×100≤0.2000   (3),wherein X3 represents a peak area value of the third peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.
  • 23. The composition according to claim 22, wherein: the composition further comprises a first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1; anda content ratio of the first peptide fragment to the alkaline phosphatase satisfies formula (1): (X1/Y)×100≤1.0000   (1),wherein X1 represents a peak area value of the first peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.
  • 24. The composition according to claim 22, wherein: the composition further comprises a fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4; anda content ratio of the fourth peptide fragment to the alkaline phosphatase satisfies formula (4): (X4/Y)×100≤0.3500   (4),wherein X4 represents a peak area value of the fourth peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.
  • 25. A composition comprising: an alkaline phosphatase; anda fourth peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 4,wherein a content ratio of the fourth peptide fragment to the alkaline phosphatase satisfies formula (4): (X4/Y)×100≤0.3500   (4),wherein X4 represents a peak area value of the fourth peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.
  • 26. The composition according to claim 25, wherein: the composition further comprises a first peptide fragment consisting of the amino acid sequence set forth in SEQ ID NO: 1; anda content ratio of the first peptide fragment to the alkaline phosphatase satisfies formula (1): (X1/Y)×100≤1.0000   (1),wherein X1 represents a peak area value of the first peptide fragment calculated by an automatic integration method from an extracted ion chromatogram obtained by an LC-MS/MS analysis of the composition, and Y is the same as defined above.
  • 27. A method of producing a dephosphorylated nucleic acid, the method comprising: providing the composition according to claim 15;providing a nucleic acid; andtreating the nucleic acid with the composition to dephosphorylate the nucleic acid.
  • 28. A method of producing a labeled nucleic acid, the method comprising: providing the composition according to claim 15;providing a nucleic acid;providing a labeling substance;treating the nucleic acid with the composition to dephosphorylate the nucleic acid; andbinding the labeling substance to the dephosphorylated nucleic acid.
Priority Claims (1)
Number Date Country Kind
2018-179561 Sep 2018 JP national
PCT Information
Filing Document Filing Date Country Kind
PCT/JP2019/037520 9/25/2019 WO 00