CA2112776C - Process for inhibiting activity of endotoxin - Google Patents

Process for inhibiting activity of endotoxin Download PDF

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Publication number
CA2112776C
CA2112776C CA002112776A CA2112776A CA2112776C CA 2112776 C CA2112776 C CA 2112776C CA 002112776 A CA002112776 A CA 002112776A CA 2112776 A CA2112776 A CA 2112776A CA 2112776 C CA2112776 C CA 2112776C
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Prior art keywords
solution
surfactant
endotoxin
aqueous
solutions
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CA2112776A1 (en
Inventor
Masakazu Tsuchiya
Kazuaki Harada
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Fujifilm Wako Pure Chemical Corp
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Wako Pure Chemical Industries Ltd
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    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K38/00Medicinal preparations containing peptides
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/579Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving limulus lysate
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K7/00Peptides having 5 to 20 amino acids in a fully defined sequence; Derivatives thereof
    • C07K7/50Cyclic peptides containing at least one abnormal peptide link
    • C07K7/54Cyclic peptides containing at least one abnormal peptide link with at least one abnormal peptide link in the ring
    • C07K7/60Cyclic peptides containing at least one abnormal peptide link with at least one abnormal peptide link in the ring the cyclisation occurring through the 4-amino group of 2,4-diamino-butanoic acid
    • C07K7/62Polymyxins; Related peptides
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/53Immunoassay; Biospecific binding assay; Materials therefor
    • G01N33/569Immunoassay; Biospecific binding assay; Materials therefor for microorganisms, e.g. protozoa, bacteria, viruses
    • G01N33/56911Bacteria

Abstract

By contacting a peptide derivative or a protein having a property of binding to endotoxin (ET) to inhibit the activity of ET, and at least one surfactant with a sample containing ET, the activity of ET can be inhibited, and even when an ET analogous substance having ET activity is present in the thus treated sample, it can be measured without influence of ET.

Description

. 2~1~;'~'~~

BACKGROUND OF THE INVENTION
This invention relates to a process for selective inhibition of properties of endotoxin (herein-after abbreviated as "ET"), such as a property of reacting with horseshoe crab hemocyte lysate (herein-after abbreviated as "AL solution") to cause activation reaction of an enzyme (e. g. protease) contained in said solution (hereinafter abbreviated as "enzyme activation reaction") or gelation reaction; arid a process for measuring at least one substance other than ET among substances having ET activity (hereinafter abbreviated as "activating substances for AL solution") (the substance other than ET is hereinafter abbreviated as "ET analogous substance"') which is contained in a sample treated by the above inhibiting process.
ET's are lipopolysaccharides (LPS) present in cell walls of Gram-negative bacteria and are known as potent pyrogens. Therefore, the detection of ET in parenteral drugs and the like is considered important, and test methods fox endotoxin are described in the U.S.
Pharmacopoeia and the Japanese Pharmacopoeia. ET is considered a main cause of shock in Gram-negative bacterial infections. In clinical diagnoses, the measurement of endotoxin in plasma is employed, for example, for diagnoses of Gram-negative bacterial infections, judgement of curative effect on and prognosis of Gram-negative bacterial infections, and early diagnosis of endotoxin shock. AL solution has a property of being activated by ET to cause activation reaction of an enzyme (e. g. protease) or gelation reaction. Simple, low-cost ET detecting methods utilizing this property, for example, so-called Limulus test including a method of measuring the degree of activation of the enzyme (e. g. protease) by a colori-metric method, or utilizing the gelation reaction (in the present invention, the "Limulus test" includes these methods mentioned above) are widely employed in the fields of medical science, pharmacy and micro-biology.
Reagents used for the Limulus test, however, have been disadvantageous in that since they react also with an ET analogous substances) such as (1-.3)-S-D-glucan and/or a derivative thereof (hereinafter abbreviated as "~G") (Kakinuma et al., Biochem. Biophys.
Res. Commun., vol. 101, 434-439 (1981), and Morita et al., FEBS Lett., vol. 129, 318-321 (1981)], the presence of SG together with ET in a sample for measurement causes positive errors in measured values.
Although, SG's are interfering substances which cause positive errors in ET measurement, the detection of SG by use of AL solution is considered utilizable for diagnoses of infectious diseases caused by Eumycetes, because they are components of cell wall 21~.~'~"~a of Eumycetes such as yeast and mold. Hence the development of a method for measurement of SG is investigated. However, since commercially available reagents usable for the Limulus test, of course, react with ET, there has been a problem in that when SG is measured using the reagents, ET in a sample affects measured values.
For solving the above problems, there have been reported, for example, a process for removing a factor which is present in AL solution and reacts with ET to cause activation reaction of an enzyme (e. g.
grotease) or gelation reaction (hereinafter abbreviated as "ET-sensitive factor°'), by treating AL solution by various chromatographies (Japanese Patent Unexamined Publication (JP-A) No. 59-27828, JP-A H2-138193 and JP-A
H4-76459), a process for inhibiting ET-sensitive factors by adding a peptide having affinity for ET to AL
solution (JP-A H2-207098), and a process for inhibiting ET-sensitive factors by adding antibodies against ET-sensitive factor to AL solution (JP-A H4-52558). All of these processes, however, are disadvantageous in that since they comprise treating AL solution itself, there is a strong fear that during the treatment, AL solution may be contaminated with ET or SG, which are widely present in a usual environment. Moreover, these processes require sterile facilities and complicated sterile operations for avoiding the contamination, and the peptide having affinity for ET and the antibodies zl~.~~~~
against ET-sensitive factor are difficult to obtain and are expensive. As is clear from these facts and the like, the processes involve many economical and technical problems.
For inactivating ET by treatment of not AL
solution but a sample for measurement, a process for heat-treating the sample has been reported (JP-A H2-141666). This process is free from the defects of the processes described above, but is disadvantageous in that a long treatment time is required for sufficient inactivation of ET. Therefore, it cannot be said to be a preferable process.
SUMMARY OF THE INVENTION
This invention was made in consideration of such conditions and is intended to provide a process for selective inhibition of ET activity which can be practiced by easy operations by use of easily available reagents; a process for measuring at least one ET
analogous substance in a sample by employing this inhibiting process; and a reagent for this measurement.
This invention provides a process for inhibit-ing the activity of ET which comprises contacting a peptide derivative or a protein, which has a property of binding to ET to inhibit the activity of ET (hereinafter abbreviated as "ET-inhibiting peptide") and at least one surfactant With a sample containing ET.
This invention also provides a process for 21~.2r~rl~~
measuring at least one ET analogous substance present in a sample which comprises reacting the sample treated by the above-mentioned inhibiting process with AL solution, and measuring the activity of an enzyme activated by enzyme activation reaction caused by the above reaction, or measuring the degree of turbidity change or gelation of the reaction solution which is due to gelation reaction caused by the above reaction, by means of a measuring instrument or with the naked eye.
In addition, this invention provides a pretreating solution for inhibiting the activity of ET
which is an aqueous solution containing an ET-inhibiting peptide and at least one surfactant, does not react with AL solution, and neither inhibits nor enhance the reaction of AL solution with an ET analogous substance.
Further, this invention provides a reagent for measuring at least one ET analogous substance which comprises an ET-inhibiting peptide, at least one surfactant and AL solution.
BRIEF DESCRIPTION OF THE DRAWINGS
Fig. 1 is a graph showing the influence of the concentration of a surfactant on the measurement of endotoxin (hereinafter abbreviated as "ET") (E. coli 055:85 LPS) in plasma, which was obtained in Example 1.
Fig. 2 is a graph showing the influence of the concentration of polymyxin B (hereinafter abbreviated as "Px B") on the measurement of ET (E. coli 055:85 LPS) in 1 ~. 2'~'Y 6 plasma, which was obtained in Example 1.
Fig. 3 is a graph showing the influence of the concentration of the surfactant on the measurement of ET
(E. coli 0128:B12 LPS) in plasma, which was obtained in Example 4.
Fig. 4 is a graph showing the influence of the concentration of Px B on the measurement of ET (E. coli 0128:B12 LPS) in plasma, which was obtained in Example 4.
Fig. 5 is a graph showing the influence of the concentration of Px B on the measurement of ET (E. coli 0128:B12 LPS) in plasma in the presence of the surfactant, which was obtained in Example 4.
Fig. 6 is a graph showing the influence of the concentration of the surfactant on the measurement of S-glucan in the presence of Px B, which was obtained in Example 9.
Fig. 7 is a graph showing the influence of the concentration of Px B on the measurement of the ET
concentration in an aqueous solution containing ET (E.
coli 055:B5 LPS), which was obtained in Example 10.
DESCRIPTION OF THE PREFERRED EMBODIMENTS
In the course of earnest study for finding a process for specific measurement of an AL solution activating substance such as ET, SG, etc. by use of AL
solution, the present inventors found that the presence of both a surfactant and an ET-inhibiting peptide in a sample or a reaction solution obtained at the time of measuring the AL solution activating substance inhibits only the activity of ET contained in the sample or the reaction solution and permits specific detection of an ET analogous substance such as ~G, whereby this invention has been accomplished.
In detail, it has been well known that surfactants and ET-inhibiting peptides represented by polymyxin and the like have a property of inhibiting ET
activity. But, for inhibiting ET activity completely by using a surfactant or an ET-inhibiting peptide alone, the addition of a large amount of the surfactant or the ET-inhibiting peptide has been necessary. Therefore, there has been a problem in that when an ET analogous substance in a sample treated using either the surfactant or the ET-inhibiting peptide alone is measured by the Limulus test, influences such as inhibition of activation of enzymes in AL solution are brought about, so that no exact measured value can be obtained. However. the present inventors found that simultaneous use of a surfactant and an ET-inhibiting peptide permits complete inhibition of ET activity in a sample even when they are added in such an amount that they do not affect the Limulus test, whereby this invention has been accomplished.
The surfactant used in this invention is not critical so long as it neither inhibits nor enhance the activation reactions (enzyme activation reaction, ~ 11 >'~'~ E~
-8_ gelation reaction, etc.) of AL solution by ET analogous substances and it does not cause appearance of non-specific turbidity during the reactions.
Specific examples of the surfactant are nonionic surfactants such as polyoxyethylene alkyl ethers (e. g. polyoxyethylene cetyl ether, polyoxy-ethylene lauryl ether, etc.), polyoxyethylene alkyl-phenyl ethers (e. g. polyoxyethylene octylphenyl ether, polyoxyethylene nonylphenyl ether, etc.), polyoxy-ethylene alkyl esters (e. g. polyoxyethyiene sorbitan monooleate, polyoxyethylene sorbitan monopalmitate, polyoxyethylene sorbitan monostearate, polyoxyethylene sorbitan triolate, etc.), methylglucamide derivatives (e. g, octanoyl-N-methylglucamide, nonanoyl-N-methyl-glucamide, decanoyl-N-methylglucamide, etc.), alkyl sugar derivatives (e.g. n-octyl-s-D-glucoside, etc.) and the like; anionic surfactants such as sodium dodecyl sulfate (SDS), laurylbenzenesulfonic acid, deoxycholic acid, cholic acid, tris(hydroxymethyl)aminomethane dodecyl sulfate (Tris DS) and the like; cationic surfactants such as alkylamine salts (e. g. octadecyl-amine acetic acid salt, tetradecylamine acetic acid salt, stearylamine acetic acid salt, laurylamine acetic acid salt, lauryldiethanolamine acetic acid salt, etc.), quaternary ammonium salts (e. g. octadecyltrimethyl-ammonium chloride, dodecyltrimethylammonium chloride, cetyltrimethylamrnonium chloride, cetyltrimethylammonium bromide, allyltrimethylammonium methylsulfate, 2112%~~

benzalkonium chloride, tetradecyldimethylbenzylammonium chloride, octadecyldimethylbenzylammonium chloride, lauryldimethylbenzylammonium chloride, etc.), alkyl-pyridinium salts (laurylpyridinium chloride, stearyl-amidomethylpyridinium chloride, etc.) and the like;
amphoteric surfactants such as 3-[(3-cholamidoamido-propyl)dimethylammonioJ-1-propane sulfonate, 3-[(3-cholamidoamidopropyl)dimethylammonio]-2-hydroxy-1-propane sulfonate and the like; and natural surfactants such as saponin (derived from soybean), digitonin and the like. In view of influences on enzyme systems and the like during the reaction, the nonionic surfactants or the amphoteric surfactants are preferable. The above-exemplified surfactants may be used singly or in proper combination of two or more thereof.
Although their using concentration is varied depending on their kind and a sample to be treated, it may be chosen without particular limitation so long as it is a concentration at which ET activity can be sufficiently inhibited in the presence of an ET-inhibiting peptide and the reactivity of ET analogous substances such as SG with AL solution is neither enhanced nor inhibited. More specifically, the concentration of the surfactants in an ET-containing sample or a reaction solution of said sample with AL
solution is properly chosen usually in the range of 0.005 to 5 w/v%, preferably 0.05 to 2.5 w/v%, more preferably 0.1 to 1 w/v%.

The ET-inhibiting peptide used in this invention is not critical so long as it is a peptide derivative (or a protein) which has a property of binding to ET to inhibit the activity of ET. The ET-inhibiting peptide preferably has properties of having strong basicity and/or having hydrophobic moieties.
Preferable examples of the ET-inhibiting peptide are polymyxin produced by Bacillus polymyxa or the like, and tachyplesin, polyphemusin, anti-LPS factor and the like which are derived from AL solution. Since tachyplesin, polyphemusin, anti-LPS factor and the like are usually difficult to obtain and expensive, employment of polymyxin is economically advantageous. The polymyxin is not particularly limited and polymyxins A, B, C, D, E, K, M, P and the like may be used as a single purified component, a mixture of two or more of them, or a salt of any of them. Sulfate of polymyxin B is preferable in view of commercial availability.
Although the using concentration of the ET-inhibiting peptide is varied depending on the kind of the ET-inhibiting peptide and a sample to be treated, it may be chosen without particular limitation so long as it is a concentration at which ET activity can be suffi-ciently inhibited in the presence of the surfactants) and the reactivity of ET analogous substances such as ~G
with AL solution is neither enhanced nor inhibited.
More specifically, the concentration of the ET-inhibit-ing peptide in an ET-containing sample or a reaction ~I1~?~'~6 solution of said sample with AL solution is properly chosen usually in the range of 0.00001 to 0.1 w/v~, preferably 0.0001 to 0.05 w/v~, more preferably 0.001 to 0.01 w/v~.
The inhibiting process of this invention is practiced, for example, as follow.
The word "contacting" means that the endotoxin-inhibiting peptide and surfactant contact with an ET-containing sample by means of addition, dilution, stirring, mixing, vibration, etc. For example, it is sufficient that the above-exemplified surfactants) and ET-inhibiting peptide are present in an ET-containing sample or at the time of the reaction of said sample with AL solution, at concentrations in the above-mentioned ranges. Needless to say, when an ET analogous substance is measured in a sample treated by the inhibiting process of this invention, the concentrations of the surfactants) and the ET-inhibiting peptide at the time of the reaction of said sample and AL solution may be below the above-mentioned ranges.
When the inhibiting process of this invention is employed for inhibiting ET activity in a sample which may be heated, the ET activity can be more efficiently inhibited by employing heat treatment together with the inhibiting process. Particularly when an ET analogous substance in a sample containing inhibiting factors or the like, such as plasma or serum is measured by the Limulus test, it is preferable to employ heat treatment 2~1~'~'~6 together with the inhibiting process as a pretreatment for removing the influences of the inhibiting factors or the like. Although the heat treatment may be carried out before or after the addition of both the surfac-tant(s) and the ET-inhibiting peptide, it is preferably carried out after the addition because a larger effect can be often obtained. Although not critical, the heat-ing temperature in the heat treatment is usually 60 -220°C, preferably approximately 70 - 100°C. Although not critical, the heating time is usually 3 - 60 minutes, preferably approximately 5 - 15 minutes. Any heating method may be employed so long as it permits heating of the sample under the above heating condi-tions. Preferable examples of heating method are heating in an incubator and heating in an autoclave.
For placing both the surfactants) and the ET-inhibiting peptide in an ET-containing sample or at the time of the reaction of said sample with AL solution, any method may be employed so long as it is such that the surfactants) and the ET-inhibiting peptide are added to said sample or AL solution to adjust their concentrations to values in the above-mentioned ranges before initiation of the activation of AL solution by ET. The following methods can be exemplified.
.. 1) A method in which an ET-containing sample is properly diluted with a solution containing proper amounts of the surfactants) and the ET-inhibiting peptide (or a solution containing a proper amount of the surfactants) and a solution containing a proper amount of the ET-inhibiting peptide) which does not activate AL
solution and neither inhibits nor enhance the reaction of AL solution with an ET analogous substance.
2) A method in which when an ET analogous substance is measured, proper amounts of the surfactants) and the ET-inhibiting peptide are previously incorporated into AL solution, and the thus treated AL solution is properly mixed with a sample for measurement.
When the above method 1) is employed. the degree of dilution of the sample is not critical, but when the sample is plasma or the like, the following problems are caused in some cases. When the degree of dilution is too low, an increase in viscosity or the formation of a precipitate is caused in the diluted plasma by denaturation of plasma protein during heating.
When the degree of dilution is too high, proper detec-tion of ET becomes impossible. Therefore, when the sample is plasma or the like, the degree of dilution is usually 5 to 20 times, preferably about 8 to about 12 times.
As the solution or solutions used in the above method 1), i.e., the solution containing the surfactants) and the ET-inhibiting peptide or the solutions containing them respectively, an aqueous solution of the above-exemplified surfactants) and ET-inhibiting peptide or aqueous solutions of them 21 ~ 2'~'~ ~
- l~ -respectively are prepared so as to have a proper con-centrations(s), and are used preferably after confirming that the aqueous solutions) does not activate AL
solution and neither enhance nor inhibits the reaction in the Limulus test. The solution containing the surfactants) and the ET-inhibiting peptide or the solutions containing them respectively may be autoclaved at 121°C for 20 minutes for sterilization. Although the concentration of the surfactants) in the solution is not critical so long as it is in a range in which the final concentration of the surfactants) in a dilution obtained by diluting an objective sample with the solutions) is in the range described above, it is usually 0.01 to 10 w/v%, preferably 0.1 to 5 w/v%, more preferably 0.2 to 2 w/v%, in view of ease of operations.
Although the concentration of the ET-inhibiting peptide in the solution is not critical so long as it is in a range in which the final concentration of the ET-inhibiting peptide in a dilution obtained by diluting an objective sample with the solutions) is in the range described above, it is usually 0.00002 to 0.2 w/v%, preferably 0.0002 to 0.1 w/v%, more preferably 0.002 to 0.02 w/v%, in view of ease of operations.
The AL solution containing predetermined amounts of the surfactants) and the ET-inhibiting peptide which is used in the above method 2) can, of course, be once freeze-dried, stored in the form of a reagent, redissolved in water containing no AL solution 2~~~~76 _ 15 _ activating substance, such as distilled water fox injection, and then used.
Since the inhibiting F>rocess of this invention makes it possible to inhibit ET activity in a sample completely by simultaneous use of small amounts of the surfactants) and the ET-inhibiting peptide, said process is very economical. A sample treated by the inhibiting process of this invention has low contents of the surfactants) and the ET-inhibiting peptide and hence can be used as a sample for measuring an ET
analogous substance by utilization of Limulus test, without considering the influences of the surfactants) and the ET-inhibiting peptide on Limulus test.
Depending on the kind (source) of ET, its ET
activity can be sufficiently inhibited using a low concentration of the ET-inhibiting peptide alone. Such inhibition is possible, for example, in the case of ET
derived from E. coli 0127:B8. However, when the inhibition of ET activity is necessary for measuring an ET analogous substance in a sample in which it is not clear what kind of ET is contained, application of the inhibiting process of this invention is, of course, preferable.
The process for inhibiting ET activity of the present invention can be applied, for example, in the following fields.
In the case of measuring the amount of ET
analogous substance such as S-glucan (more precisely (1-~3)-B-D-glucan) in a sample using the Limulus test, the ET activity inhibiting process can be used to inhibit influences of endotoxin present in the sample on the results of measurement.
Further, in the case of measuring endotoxin or endotoxin analogous substance such as S-glucan in a sample by adding an AL solution to the sample to bring about the activation of the AL solution, followed by addition of a synthetic substrate thereto, the ET
activity inhibiting process can be used to remove contamination of used reagents such as a synthetic substrate with endotoxin.
In addition, in an experiment using cultured cells, etc., when the cultured cells are susceptible to influences of endotoxin, the ET. activity inhibiting process can be used to remove the contamination of used reagents with endotoxin.
Ta measure an ET analogous substance in a sample treated by the inhibiting process of this invention, it is sufficient that the measurement is carried aut by a conventional method using AL solution, for example, the so-called Limulus test, i.e., a kinetic turbidimetric technique using an apparatus for exclusive use, such as Toxinometer ET-201 (mfd. by Wako Pure Chemical Industries, Ltd.), Toxinometer MT-251 (mfd. by Wako Pure Chemical Industries, Ltd.), LAL-5000 [mfd. by Associates of Cape Cod Inc. (ACC)] or the like; a chromogenic technique comprising measuring protease ~~.12'~~~j activity which arises owing to the activation of AL
solution, by use of a synthetic substrate; or a gel-clot technique comprising judging whether a gel is produced by the activation of AL solution or not with the naked eye.
The ET analogous substance according to this invention is not critical so long as it is other than ET
and reacts with AL solution to cause enzyme activation reaction or gelation reaction. Typical examples of the ET analogous substance are (1-~3)-s-D-glucan and derivatives thereof. As the (1-~3)-B-D-glucan and derivatives thereof, any polysaccharides can be exemplified without particular limitation so long as they contain (1-~3)-S-D-glucoside linkage. Preferable examples of the (1-~3)-S-D-glucan are natural poly-saccharides obtained from cell walls or other components of, for example, various bacteria (e. g. Alcaligenes genus. Agrobacterium genus, etc.), yeasts (e. g.
Saccharomyces genus, Candida genusr Crytrococcus genus, Trichosporon genus, Rhodotorula genus, etc.), molds (e. g. Aspergillus genus, Mucor genus, Penicillium genus, Trichaphyran genus, Sporothrix genus, Phialophora genus, etc.), actinomycetes (Actinomyces genus, Nocardia genus, etc.), and mushrooms (e. g. Cortinellus shiitake, Schizophyrum commune, Coriolus versicolor, etC.), specific examples of the natural polysaccharides being curdlan, pachyman, sclerotan, lentinan, schizophyllan, coriolan, etc.; storage polysaccharides of algae, e.g.

~~~.~'~'~v _ la _ brown algae, Euglena, diatoms, etc., specific examples of the storage polysaccharides being laminaran, paramylon, etc. Preferable examples of the (1;3)-B-D-glucan derivatives are polysaccharide derivatives obtained by introducing at least one group selected from the group consisting of a sulphonic group, carboxymethyl group, carboxyethyl group, methyl group, hydroxyethyl group, hydroxy propyl group, sulfopropyl group, etc.
into the natural polysaccharides or the storage polysaccharides according to a conventional method, for instance, any of the methods described, for example, in Munio Kotake °°Daiyukikagaku" vol. 19, 7th ed. Asakura Shoten, May 10. 1967, pp. 70-101; A.E. Clarke et al., Phytochemistry, vol. 1, 175-188 (1967); and T. Sasaki et al. Europ. J. Cancer, vol. 15, 211-215 (1967).
The AL solution usable in this invention is not critical so long as it can be used for usual measurement of ET. There may be used AL solutions prepared from freeze-dried products of AL solutions which are commercially available, fox example, from Associates of Cape Cod Inc. (ACC), HAEMACHEM, Inc., Hiowhittaker Inc., Endosafe Inc., Teikoku Hormon Mfg.
Co., Ltd., and Seikagaku Kogyo Co., Ltd. In addition, there can be exemplified any AL solution without pa-rticular limitation so long as it is prepared from hemocytes of horseshoe crab belonging to Limulus genus, Tachypleus genus or Carcinoscorpius genus and react with r 21~2'~'~u an AL solution activating substance to undergo enzyme (protease or the like) activation or gelation reaction.
This invention is illustrated below in further detail with reference to Examples, which are not by way of limitation but by wa.y of illustration.
Example 1 [Reagents]
~ ET solutions There were used solutions prepared by weighing 10 mg of Escherichia coli (E, coli) 055aB5 LPS
(available from Difco Laboratories), dissolving the same in 10 ml of distilled water for injection to prepare a 1 mg/ml solution as a starting solution, and diluting the starting solution properly with distilled water for injection.
~ AL solution A freeze-dried product of AL solution derived from horseshoe crab belonging to Limulus genus (hereinafter the freeze-dried product being abbreviated as "LAL"; available from Wako Pure Chemical Industries, Ltd.; for dissolution in 2 ml) was dissolved in a buffer solution for LAL reconstitution (HS) (mfd. by Wako Pure Chemical Industries, Ltd.), and the LAL solution thus obtained was used as AL solution.
~ Aqueous surfactant solutions Polyoxyethylene glycol p-t-octylphenyl ether (a nonionic surfactant, mfd. by Wako Pure Chemical Industries, Ltd.) was diluted to 10 w/v% with distilled water for injection, and the resulting dilution was autoclaved at 121°C for 20 minutes to obtain a starting solution. The starting solution was properly diluted with distilled water for injection, and the thus obtained diluted solutions were used as aqueous surfac-tant solutions after confirming that they did not acti-vate the AL solution and neither inhibited nor enhance the reaction for measuring ~G by the Limulus test.
. Aqueous polymyxin B (hereinafter abbreviated as "Px B") solutions Px B sulfate (mfd. by Wako Pure Chemical Industries, Ltd.) was diluted to 1.0 w/v% with distilled water for injection, arid the resulting dilution was autoclaved at 121°C for 20 minutes to obtain a starting solution. The starting solution was properly diluted with distilled Water for injection (or 0.2 w/v% aqueous surfactant solution prepared in the above), and the thus obtained dilutions were used as aqueous Px B solutions after confirming that they did not activate the AL
solution and neither inhibited nor enhance the reaction for measuring SG by the Limulus test.
[Procedure]
.. To 2.0 ml of normal human heparinized plasma was added 20 u1 of ET solution having a predetermined concentration, and 100 u1 of the resulting ET spiked plasma was diluted 10 times (i.e. 1/10) with 900 u1 of distilled water for injection, each of aqueous Px B
solutions having predetermined concentrations, or each of aqueous surfactant solutions having predetermined concentrations. Each of the thus obtained dilutions was heat-treated at 80°C for 5 minutes and then immediately cooled with ice (the final concentrations of ET, Px B
and the surfactant were 2 ng/ml, 0.0018 to 0.009 w/v%
and 0.09 to 0.45 w/v~, respectively). The ET
concentration in the diluted plasma thus obtained was measured as follows by a conventional method using an apparatus "Toxinometer MT--251" (mfd. by Wako Pure Chemical Industries, Ltd.).
To 0.1 ml of the LAL solution was added 0.1 ml of the aforesaid diluted plasma, and stirred, after which a time required for reducing the transmittance of the resulting mixture by 5$ (hereinafter abbreviated as "Tg") was measured while maintaining the temperature at 37°C. The ET concentration in the diluted plasma was determined an the basis of the thus obtained Tg value by use of a calibration curve showing the relationship between ET concentration and Tg which had been previously obtained by carrying out the same measurement as described above except for using ET solutions various in their concentrations as samples.
(Results?
Figs. 1 and 2 show the results obtained. Fig.
1 shows the results obtained for the plasma diluted with ~ x.12 '~ '~ c~

each surfactant solution and is a graph obtained by plotting the gelation time (Tg) of the diluted and heated plasma on the axis of ordinate corresponding to individual surfactant concentrations (at the time of the heat treatment) on the axis of abscissa. Fig. 2 shows the results obtained for the plasma diluted with each Px B solution and is a graph obtained by plotting the gelation time (Tg) of the diluted and heated plasma on the axis of ordinate corresponding to individual Px B
concentrations (at the time of the heat treatment) on the axis of abscissa. In Fig. 2, -D - shows the results obtained by use of the aqueous solutions containing Px B
alone, and -C7- shows the results obtained by use of the aqueous solutions containing both Px B and 0.2 w/v% of the surfactant (polyoxyethylene glycol p-t-octylphenyl ether) (the surfactant concentration at the time of the heat treatment was 0.18 w/v%). In Fig. 2, (D) indicates that Tg was 90 minutes or more, in other words. ET was not detected.
As is clear from the results shown in Fig. 1, the Tg value obtained from the plasma diluted with distilled water fox injection was 7.8 minutes, while the Tg values obtained from the plasma diluted with each of 0.1 to 0.5% aqueous surfactant solutions (the surfactant concentration at the time of the heat treatment was 0.09 to 0.45%) was as large as 16.3 to 33.7 minutes, indicating that the ability of ET to activate AL
solution (ET activity) was deteriorated (the smaller Tg, the higher the ET activity). As is clear from the results shown in Fig. 2, the Tg value obtained from the plasma diluted with distilled water for injection was 7.8 minutes, while the Tg values obtained from the plasma diluted with each of 0.002 to 0.01 w/v% aqueous Px B solutions (the Px B concentration at the time of the heat treatment was 0.0018 to 0.009 w/v%) was as large as 24.2 to 32.9 minutes, indicating that the ET
activity was lowered. Further, from the results shown in Fig. 2, it can be seen that when plasma was diluted with aqueous solution containing both 0.002 to 0.01 w/v%
of Px B and 0.2% of the surfactant (the concentrations of the surfactant and Px B at the time of the heat treatment were 0.18% and 0.0018 to 0.009 w/v%, respec-tively), ET was not detected (Tg became 90 minutes or more).
As is clear from the results described above, the ET activity of E. coli 0.55: B5 LPS spiked to plasma is completely inhibited by the simultaneous presence of the surfactant and Px B.
Example 2 [Reagents]
The same AL solution, aqueous surfactant solutions and aqueous Px B solutions as described in Example 1 were used.
~ ET solutions There were used solutions prepared by weighing ~~12'~'~~

mg of E. coli 0111: B4 LPS (available from Difco Laboratories), dissolving the same in 10 ml of distilled water for injection to prepare a 1 mg/ml solution as a starting solution, and diluting the starting solution 5 properly with distilled water for injection.
[Procedure]
To 0.6 ml of normal human heparinized plasma was added 12 u1 of ET solution having a predetermined concentration, and 100 u1 of the resulting ET spiked 10 plasma was diluted 10 times with 900 u1 of distilled water for injection, 0.04 w/v% aqueous surfactant solution, 0.2 w/v% aqueous surfactant solution, or 0.01 w/v% aqueous Px B solution [containing 0.2 w/v% of the surfactant (polyoxyethylene glycol p-t-octylphenyl ether)), respectively. Each of the thus obtained dilutions was heat-treated at 80°C for 5 minutes and then immediately cooled with ice (the final concentration of ET was 1.96 ng/ml). The ET
concentration in the diluted plasma thus obtained was measured in the same manner as in Example 1.
[Results) The results obtained are shown in Table 1.

2~.12'~7~i Table 1 Diluent Tg (min) concentration (pg/ml) Distilled water for 10.0 289.1 injection 0.04% Aqueous surfactant6.3 2363.0 solution 0.2% Aqueous surfactant 40.4 3.4 solution 0.01% Aqueous Px B >90 -solution (containing 0.2%

of the surfactant) As is clear from the results shown in Table 1, the Tg value obtained from the plasma diluted with distilled water for injection was 10.0 minutes, while the Tg value obtained from the plasma diluted with the 0.2 w/v% aqueous surfactant solution (the surfactant concentration at the time of the heat treatment was 0.18 w/v%) was as large as 40.4 minutes, indicating that the ET activity was lowered. It can also be seen that When plasma was diluted with the 0.01 w/v% aqueous Px B
solution (containing 0.2 w/v% of the surfactant) (the concentrations of Px B and the surfactant at the time of the heat treatment were 0.009 w/v% and 0.18 w/v%, respectively), ET was not detected (Tg became 90 minutes or more). In the case of the plasma diluted with the 0.04% aqueous surfactant solution, the Tg value was smaller (the ET activity was higher) than in the case of the plasma diluted with distilled water fox injection.
The reason can be presumed as follows: the influence of factors capable of inhibiting the reaction of ET with AL
solution which were present in plasma was reduced by the addition of the surfactant.
As is clear from the results described above, the ET activity of E. coli 0.111:84 LPS spiked to plasma is completely inhibited by the simultaneous presence of the surfactant and Px B.
Example 3 [Reagents]
The same AL solution, aqueous surfactant solutions and aqueous Px B solutions as described in Example 1 were used.
~ ET solutions There were used solutions prepared by weighing 10 mg of E. coli 0127: B8 LPS (available from Difco Laboratories), dissolving the same in 10 ml of distilled water for injection to prepare a 1 mg/ml solution as a starting solution, and diluting the starting solution properly with distilled water for injection.
[Procedure]
To 0.7 ml of normal human heparinized plasma was added 14 u1 of ET solution having a predetermined concentration, and 100 u1 of the resulting ET spiked plasma was diluted 10 times with 900 u1 of distilled water for injection, 0.04 w/v% aqueous surfactant solution, 0.2 wjv% aqueous surfactant solution, 0.01 ~~~2'~'~~

w/v% aqueous Px B solution, or 0.01 w/v% aqueous Px B
solution containing 0.2 w/v% of the surfactant (poly-oxyethylene glycol p-t-octylphenyl ether), respectively.
Each of the thus obtained diluted solutions was heat-treated at 80°C for 5 minutes and then immediately cooled with ice (the final concentration of ET was 1.96 ng/ml). The ET concentration in the diluted plasma thus obtained was measured in the same manner as in Example 1.
[Results]
The results obtained are shown in Table 2.
Table 2 Diluent Tg (min) Concentration (pg/ml) Distilled water for 10.6 221.2 injection 0.04% Aqueous surfactant6.6 2152.0 solution 0.2% Aqueous surfactant 28.6 6.3 solution 0.01% Aqueous Px B >90 -solution 0.01% Aqueous Px B >90 -solution (containing 0.2%

of the surfactant) As is clear from the results shown in Table 2, the Tg value obtained from the plasma diluted with distilled water far injection was 10.6 minutes, while 21~.~'~'~6 28 _ the Tg value obtained from the plasma diluted with the 0.2 w/v% aqueous surfactant solution (the surfactant concentration at the time of the heat treatment was 0.18 w/v%) was as large as 28.6 minutes, indicating that the ET activity was lowered. It can also be seen that when plasma was diluted with the 0.01 w/v% aqueous Px B solu-tion or the 0.01 w/v% aqueous Px B solution containing 0.2 w/v% of the surfactant (the concentrations of Px B
and the surfactant at the time of the heat treatment were 0.009 w/v% and 0.18 w/v%, respectively), ET was not detected (Tg became 90 minutes or more). In the case of the plasma diluted with the 0.04% aqueous surfactant solution, the Tg value was smaller (the ET activity was higher) than in the case of the plasma diluted with distilled water for injection. The reason can be presumed as follows: the influence of factors capable of inhibiting the reaction of ET with AL solution which were present in plasma was reduced by the addition of the surfactant.
As is clear from the results described above, the ET activity of E. coli 0.127:88 LPS spiked to plasma is completely inhibited by the simultaneous presence of the surfactant and Px B.
Example 4 [Reagents) The same AL solution, aqueous surfactant solutions and aqueous Px B solutions as described in ~11~"~'~~

Example 1 were used.
~ ET solutions There were used solutions prepared by weighing mg of E. coli 0128:B12 LPS (available from Difco Laboratories), dissolving the same in 10 ml of distilled water for injection to prepare a 1 mg/ml solution as a starting solution, and diluting the starting solution properly with distilled water for injection.
[Procedure]
10 To 1.3 ml of normal human heparinized plasma was added 13 u1 of ET solution having a predetermined concentration, and 100 u1 of the resulting ET spiked plasma was diluted 10 times with 900 u1 of distilled water for injection, each of aqueous surfactant solu-tions having predetermined concentrations, each of aqueous Px B solutions having predetermined concentra-tions, or each of aqueous Px B solutions having pre-determined concentrations and containing 0.1 w/v% or 0.2 w/v% of the surfactant (polyoxyethylene glycol p-t-octylphenyl ether), respectively. Each of the thus obtained dilutions was heat-treated at 80°C for 5 minutes and then immediately cooled with ice (the final concentrations of ET, Px B and the surfactant were 2 ng/ml, 0.00009 to 0.009 w/v%, and 0.09 to 0.9 w/v%, respectively). The ET concentration in the diluted plasma thus obtained was measured in the same manner as in Example 1.

-.. 2:~~2'~"~ci [Results]
Figs. 3 to 5 show the results obtained. Fig.
3 shows the results obtained from the plasma diluted with each surfactant solution and is a graph obtained by plotting the gelation time (Tg) of the diluted and heated plasma on the axis of ordinate corresponding to individual surfactant concentrations (at the time of the heat treatment) on the axis of abscissa. Fig. 4 shows the results obtained from the plasma diluted with each Px B solution and is a graph obtained by plotting the gelation time (Tg) of the diluted and heated plasma on the axis of ordinate corresponding to individual Px B
concentrations (at the time of the heat treatment) on the axis of abscissa. Fig. 5 shows the results obtained from the p7.asma diluted with each aqueous solution containing the surfactant and Px B and is a graph obtained by plotting the gelation time (Tg) of the diluted and heated plasma on the axis of ordinate corresponding to individual Px B concentrations (at the time of the heat treatment) on the axis of abscissa. In Fig. 5, -~ - shows the results obtained by use of aqueous solutions containing 0.1 w/v% of the surfactant (the surfactant concentration at the time of the heat treatment was 0.09 w/v%). and -x- shows the results obtained by use of aqueous solutions containing 0.2 w/v%
of the surfactant (the surfactant concentration at the time of the heat treatment was 0.18 w/v%). All of (O) in Fig. 4 and (O) and (x) in Fig. 5 indicate that Tg ~1.~ ~'~'~~

was 90 minutes or more, in other words, ET was not detected.
As is clear from the results shown in Figs. 3 to 5, the ET activity in plasma can be completely inhibited by the presence of 0.009 w/v~ of Px B or the simultaneous presence of the surfactant and Px B. It can also be seen that when the ET activity is inhibited by the inhibiting process of this invention, the amount of Px B used can be reduced (to one hundredth that required in the case of using Px B alone), in other words, the process of this invention is economically superior to conventional processes using Px B alone.
Example 5 [Reagents]
The same AL solution, aqueous surfactant solutions and aqueous Px B solutions as described in Example 1 were used.
~ ET solutions There were used solutions prepared by weighing 10 mg of Salmonella typhimurium LPS (available from Difco Laboratories), dissolving the same in 10 ml of distilled water for injection to prepare a 1 mg/ml solution as a starting solution, and diluting the starting solution properly with distilled water for injection.

~1~2'~7f~

[Procedure]
To 1.0 ml of normal human heparinized plasma was added 10 u1 of ET solution having a predetermined concentration, and 100 u1 of the resulting ET spiked plasma was diluted 10 times with 900 ~1 of distilled water for injection, 0.2 w/v% aqueous surfactant solution, 0.01 w/v% aqueous Px B solution, or 0.01 w/v%
aqueous Px B solution containing 0.2 w/v% of the surfactant (polyoxyethylene glycol p-t-octylphenyl ether), respectively. Each of the thus obtained dilutions was heat-treated at 80°C far 5 minutes and then immediately cooled with ice (the final concentra-tion of ET was 2 ng/ml). The ET concentration in the diluted plasma thus obtained was measured in the same mariner as in Example 1.
[Results]
The results obtained are shown in Table 3.
Table 3 Diluent Tg (min) Concentration (pg/ml) Distilled water for 8.2 453.6 injection 0.2% Aqueous surfactant 12.3 77.9 solution 0.01% Aqueous Px B 13.4 55.7 solution 0.01% Aqueous Px B >90 -solution (containing 0.2%

of the surfactant) As is clear from the results shown in Table 3, the ET activity of S. typhimurium LPS spiked to plasma is completely inhibited by the simultaneous presence of the surfactant and Px H.
Example 6 [Reagents]
The same AL solution, aqueous surfactant solutions and aqueous Px B solutions as described in Example 1 were used.
~ Aqueous S-glucan solutions There were used solutions prepared by weighing 100 mg of carboxymethylated curdlan [a linear (1+3)-S-D-glucan derivative, mfd. by Wako Pure Chemical Industries, Ltd.], dissolving the same in 10 ml of distilled water for injection to prepare a 10 mg/ml solution as a starting solution, and diluting the starting solution properly with distilled water for injection.
[Procedure]
By diluting 100 u1 of 50 ng/ml aqueous glucan solution 10 times with 900 ~1 of 0.2 w/v% aqueous surfactant solution, 0.01 w/v% aqueous Px B solution, or 0.01 w/v% aqueous Px B solution containing 0.2 w/v% of polyoxyethylene glycol p-t-octylphenyl ether, solutions containing spiked ~-glucan (the final concentration of ~-glucan was 5 ng/ml) were prepared. The S-glucan concentration in each of the prepared solutions was measured as follows by a conventional method using an apparatus "Toxinometer MT-251" (mfd. by Wako Pure Chemical Industries, Ltd.). To 0.1 ml of the LAL
solution was added 0.1 ml of each of the above-mentioned diluted solutions, and stirred, after which a time required for reducing the transmittance of the resulting mixture by 5% (hereinafter abbreviated as "Tg") was measured while maintaining the temperature at 37°C. The g-glucan concentration was determined on the basis of the thus obtained Tg value by use of a calibration curve showing the relationship between S-glucan concentration and Tg which had been previously obtained by carrying out the same measurement as described above except for using S-glucan solutions various in their concentrations as samples. On the basis of the results of the measurement, the recovery of S-glucan was calculated.
[Results]
The results obtained are shaven in Table 4.
Table 4 Diluent Recovery of ~-glucan (%)' 0.2% Aqueous surfactant 100 solution 0.01% Aqueous Px B solution112 0.01% Aqueous Px B solution (containing 0.2% of the 8g surfactant) ~1 , v As is clear from the results shown in Table 4, the recovery of S-glucan was as high as about 90~ to about 110, whichever diluted solution was used.
Therefore, it can be seen that none of the diluted solutions either inhibit or enhance the reaction of AL
solution with ~-glucan.
Example 7 [Reagents]
The same AL solution, aqueous surfactant solutions and aqueous Px B solutions as described in Example 1 were used.
~ ET solutions There were used solutions prepared by weighing 10 mg of E. coli 026: B6 LPS (available from Difco Laboratories), dissolving the same in 10 ml of distilled water for injection to prepare a 1 mg/ml solution as a starting solution, and diluting the starting solution properly with distilled water for injection.
~ Aqueous surfactant solutions Various aqueous surfactant solutions were prepared in the same manner as described in Example 1 except for using as surfactants, sodium deoxycholate (an anionic surfactant, mfd. by Wako Pure Chemical Industries, Ltd.), Emalgen 709 (a nonionic surfactant (a polyoxyethylene higher alcohol ether), a trade name, Kao Corp.] and Amphitol 20N (an amphoteric surfactant, a trade name, Kao Corp.; main constituent: lauryldimethyl-amine oxide).
[Procedure) To 1.7 ml of normal human heparinized plasma was added 17 u1 of ET solution having a predetermined concentration, and 100 u1 of the resulting ET spiked plasma was diluted 10 times with 900 u1 of distilled water for injection, 0.1 w/v% aqueous sodium deoxy-cholate solution, 0.2 w/v% aqueous Emalgen 709 solution, 0,4 w/v% aqueous Amphitol 20N solution, 0.01 w/v%
aqueous Px B solution, 0.1 w/v% aqueous sodium deoxy-cholate solution containing 0.01 w/v% of Px B, 0.2 w/v%
aqueous Emalgen 709 solution containing 0.01 w/v% of Px B, or 0.4 w/v% aqueous Amphitol 20N solution containing 0.01 w/v% of Px B. Each of the thus obtained dilutad solutions was heat-treated at 80°C for 5 minutes and then immediately Gaoled with ice (the final concentration of ET was 4 ng/ml). The ET concentration in the diluted plasma thus obtained was measured in the same manner as in Example 1 .
[Results) The results obtained are shown in Table 5.

~~~~~~~i Table 5 Diluent Tg (min) concentration (pg/ml) Distilled water 9.0 1019.0 for injection 0.1% Aqueous sodium 7.5 2287.0 deoxycholate solution 0.2% Aqueous Emalgen709 27.3 22.7 solution 0.4% Aqueous Amphitol20N 52.6 4.3 solution 0.01% Aqueous Px 30.8 16.2 B

solution 0.1% Aqueous sodium >90 -deoxycholate solution (containing 0.01% Px of B) 0.2% Aqueous Emalgen709 >90 -solution (containing0.01%

of Px B) 0.4% Aqueous Amphitol20N >90 -solution (containing0.01%

of Px B ) As is clear from the results shown in Table 5, the ET activity of E. coli 0.26:86 LPS spiked to plasma is completely inhibited by the simultaneous presence of each surfactant and Px B.
5, Example 8 [Reagents]
The same AL solution, aqueous surfactant solutions and aqueous Px B solutions as described in Example 1 were used.

~ Aqueous surfactant solutions Various aqueous surfactant solutions were prepared in the same manner as described in Example 1 except for using as surfactants, polyoxyethylene glycol p-t-octylphenyl ether (a nonionic surfactant, mfd. by Wako Pure Chemical Industries, Ltd.), Emalgen 709 [a nonionic surfactant (a polyoxy~thylene higher alcohol ether), a trade name, Kao Corp.] and Amphitol 20N (an amphoteric surfactant, a trade name, Kao Corp.; main constituent: lauryldimethylamine oxide).
~ ET solutions There were used solutions prepared by weighing ZO mg of Salmonella typhosa 0901 LPS (available from Difco Laboratories), dissolving the same in 10 ml of distilled water for injection to prepare a 1 mg/ml solution as a starting solution, and diluting the starting solution properly with distilled water for injection.
[Procedure]
To 1.0 ml of normal human heparinized plasma was added 10 u1 of ET solution having a predetermined concentration, and 100 u1 of the resulting ET spiked plasma was diluted 10 times with 900 u1 of distilled water for injection, 0.2 w/v% aqueous polyoxyethylene glycol p-t-octylphenyl ether solution containing 0.01 w/v% of Px B, 0.2 w/v% aqueous Emalgen 709 solution containing 0.01 w/v% of Px B, or 0.4 w/v% aqueous ~1.~~'~7 Amphitol 20N solution containing 0.01 w/v% of Px B.
Each of the thus obtained diluted solutions was heat-treated at 80°C for S minutes and then immediately cooled with ice (the final concentration of ET was 4 ng/ml). The ET concentration in the diluted plasma thus obtained was measured in the same manner as in Example 1.
[Results]
The results obtained are shown in Table 6.
Table 6 Diluent Tg (min) Concentration (pg/ml) Distilled water for 7.8 910.9 injection 0.2% Aqueous polyoxyethylene>90 -glycol p-t-octylphenyl ether solution (containing 0.01%

of Px B) 0.2% Aqueous Emalgen 709 >90 solution (containing 0.01%

of Px B) 0.4% Aqueous Amphitol 20N >90 -solution (containing 0.01%

of Px B) As is clear from the results shown in Table 6, the ET activity of S. typhosa 0901 LPS spiked to plasma is completely inhibited by the simultaneous presence of each surfactant and Px B.

~1~2'~"l~

Example 9 [Reagents]
The same AL solution, aqueous surfactant solutions and aqueous Px B solutions as described in Example 1 were used.
~ Aqueous S-gluten solutions After 108 mg of curdlan [a linear (1-~3)-S-D-glucan derivative, mfd by Wako Pure Chemical Industries, Ltd.] was weighed, ZO ml of distilled water for injection and then 800 u1 of 1N NaOH were added to dissolve the curdlan, whereby a 10 mg/ml solution was prepared. This solution was diluted 10 times with distilled water for injection to obtain a starting solution, which was properly diluted with distilled water for injection. The thus obtained solutions were used as aqueous ~-gluten solutions.
[Procedure]
By diluting 100 u1 of 10 ng/ml aqueous S-glucan solution 10 times with 900 u1 of each of aqueous surfactant solutions having predetermined concentrations and containing 0.01 w/v% of Px B, there were prepared solutions containing spiked S-glucan (the final concentration of ~-gluten was 1 ng/ml, and the final concentrations of Px B and the surfactant in the S-gluten spiked solutions were 0.009 w/v$ and 0.9 to 4.5 w/v~, respectively). The recovery of ~-gluten from the ~.1~~~~b various B-glucan spiked solutions was determined in the same manner as described in Example 6.
[Results]
The results obtained are shown in Fig. 6.
Fig. 6 is a graph obtained by plotting the recovery of ~-glucan on the axis of ordinate corresponding to individual surfactant concentrations (in the S-glucan spiked solutions containing 0.009 w/v~ of Px B) on the axis of abscissa.
As is clear from the results shown in Fig. 6, the recovery of S-glucan was kept constant at about 90~
even when the surfactant concentration was increased.
From this fact, it can be judged that in the above surfactant concentration range, the surfactant (poly-i5 oxyethylene glycol p-t-octylphenyl ether) neither inhibits nor enhance the reaction of AL solution with S-glucan.
Example 10 [Reagents]
There were used the same AL solution, aqueous surfactant solutions and aqueous Px B solutions as described in Example 1.
[Procedure]
By diluting 100 u1 of ET solution having a predetermined concentration 10 time with 900 ~1 of ,~ .~ ;~ ; ~ ~i distilled water for injection, 0.2 w/v~ aqueous surfactant (polyoxyethylene glycol p-t-octylphenyl ether) solution, each of 0.002 to 0.01 w/v~ aqueous Px B
solutions, or each of 0.2 w/v~ aqueous surfactant (polyoxyethylene glycol p-t-octylphenyl ether) solutions containing 0.002 to 0.01 w/v~ of Px B, there were prepared solutions containing spiked ET (the final concentration of ET was 2 ng/ml, and the final concentrations of Px B and the surfactant in the ET
spiked solutions were 0.0018 to 0.009 w/v~ and 0.18 w/v~, respectively). The ET concentration in the ET
spiked solutions was measured in the same manner as in Example 1.
(Results]
The results obtained are shown in Fig. 7.
Fig. 7 is a graph obtained by plotting the gelation time (Tg) of the ET spiked solutions on the axis of ordinate corresponding to individual Px B concentrations in the ET spiked solutions on the axis of abscissa. In Fip. 7, -D - shows the results obtained for the ET spiked solutions prepared by use of the aqueous Px B solutions various in their concentrations, and -O - shows the results obtained for the ET spiked solutions prepared by use of the aqueous Px B solutions containing 0.2 w/v~ of the surfactant.
As is clear from the results shown in Fig. 7, the ET activity of E. coli 0.55: B5 LPS in the ET spiked ~:~1~'~~~

solutions is completely inhibited by the simultaneous presence of the surfactant and Px B.
Example 11 [Reagents]
There were used the same AL solution, aqueous surfactant solutions and aqueous Px B solutions as described in Example 1, the same ET solutions as described in Example 8, and the same S-glucan solutions as described in Example 9.
[Procedure]
To 1.0 ml of normal human heparinized plasma was added 10 u1 of 4 g/ml ET solution and 10 u1 or 100 ng/ml s-glucan solution, and 100 u1 of the obtained plasma containing spiked ET and spiked S-glucan was diluted 10 times with 900 u1 of distilled water for injection, 0.2 w/v% aqueous surfactant (polyoxyethylene glycol p-t-octylphenyl ether) solution, 0.01 w/v% aque-ous Px B solution, or 0.2 w/v% aqueous surfactant (poly-oxyethylene glycol p-t-octylphenyl ether) solution con-taining 0.01 w/v% of Px B. Each of the thus obtained diluted solutions was heat-treated at 80°C for 5 minutes and then immediately cooled with ice (the final concent-rations of ET and S-glucan were 3.92 ng/ml and 196 pg/ml). The S-glucan concentration in the diluted plasma thus obtained was measured in the same manner as in Example 6. The same procedure as described above was carried out for a mixture prepared by adding 10 u1 of distilled water for injection and 10 u1 of 20 ng/ml S-glucan solution to the same plasma as used in the above, and the s-glucan concentration in the mixture was measured.
Further, on the basis of the measurement results. the recovery of s-glucan was calculated.
[Results]
The results obtained are shown in Table 7.
Table 7 Recovery of S-glucan (%) Diluent ET spikedPlasma without plasma spiked ET

Distilled water for 54200 107 injection 0.2% Aqueous surfactant 3540 98 solution 0.01% Aqueous Px B 893 105 solution 0.01% Aqueous Px B 117 112 solution (containing 0.2%

of the surfactant) As is clear from the results shown in Table 7, S-glucan can be measured without the influence (the influence of causing positive errors in measured values) of ET present in a sample only when the surfactant and Px B are present during the measurement of s-glucan.

As is clear from the above, this invention provides a process for inhibiting ET activity in a sample effectively. The process of this invention is effective in that it permits easier and more certain inhibition of ET activity than do conventional processes, so that it makes it possible to measure an ET analogous substance without the influence of ET.
Therefore, this invention contributes greatly to the art.

Claims (17)

1. ~A process for inhibiting the activity of endotoxin which comprises contacting an endotoxin-inhibiting peptide having a property of binding to endotoxin to inhibit the activity of endotoxin and selected from peptide derivatives and proteins, and at least one surfactant with a sample containing endotoxin.
2. ~A process according to Claim 1, wherein a heat treatment is employed simultaneously.
3. ~A process according to Claim 1, wherein said sample is heat-treated after the endotoxin-inhibiting peptide and the surfactant are contacted with the sample.
4. ~A process according to Claim 1, wherein the concentration of the surfactant is 0.005 to 5.0 w/v% and the concentration of the endotoxin-inhibiting peptide is 0.00001 to 0.1 w/v%.
5. ~A process according to Claim 2, wherein the heat treatment is carried out by heating at 60 - 220°C
for 3 to 60 minutes.
6. ~A process according to Claim 1, wherein the endotoxin-inhibiting peptide is polymyxin.
7. ~A process according to Claim 1, wherein the surfactant is a nonionic surfactant or an amphoteric surfactant.
8. ~A process for measuring at least one endotoxin analogous substance present in a sample and having a property of reacting with a horseshoe crab hemocyte lysate to cause enzyme activation reaction or gelation reaction, which comprises reacting the sample treated by the process of Claim 1 with horseshoe crab hemocyte lysate, and measuring the activity of an enzyme activated by enzyme activation reaction caused by the above reaction, or measuring the degree of turbidity change or gelation of the reaction solution which is due to gelation reaction caused by the above reaction, by means of a measuring instrument or with the naked eye.
9. ~A process according to Claim 8, wherein the endotoxin analogous substance(s) is (1.fwdarw.3)-.beta.-D-glucan and/or a derivative thereof.
10. ~A pretreating aqueous solution for inhibiting the activity of endotoxin comprising an endotoxin-inhibiting peptide and at least one surfactant, said solution being unable to react with a horseshoe crab hemocyte lysate, to inhibit and to enhance the reaction of horseshoe crab hemocyte lysate with an endotoxin analogous substance.
11. ~A pretreating solution according to Claim 10, wherein the concentration of the surfactant is 0.01 to 10.0 w/v% and the concentration of the endotoxin-inhibiting peptide is 0.00002 to 0.2 w/v%.
12. ~A pretreating solution according to Claim 10, wherein the endotoxin-inhibiting peptide is polymyxin.
13. ~A pretreating solution according to Claim 10, wherein the surfactant is a nonionic surfactant or an amphoteric surfactant.
14. ~A reagent for measuring at least one endotoxin analogous substance which comprises an endotoxin-inhibiting peptide, at least one surfactant and AL
solution.
15. A reagent according to Claim 14, wherein the endotoxin-inhibiting peptide is polymyxin.
16. A reagent according to Claim 14, wherein the surfactant is a nonionic surfactant or an amphoteric surfactant.
17. A reagent according to Claim 14, wherein the endotoxin analogous substance is (1.fwdarw.3)-.beta.-D-glucan and/or a derivative thereof.
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CA2112776C (en) * 1993-01-21 2002-11-12 Masakazu Tsuchiya Process for inhibiting activity of endotoxin
JP2003528619A (en) * 2000-03-24 2003-09-30 ソシエテ デ プロデユイ ネツスル ソシエテ アノニム Β-glucan derived from filamentous fungi
WO2002101836A1 (en) * 2001-06-12 2002-12-19 Hitachi, Ltd. Semiconductor device and method of producing the same
WO2004045636A1 (en) * 2002-11-18 2004-06-03 Vicuron Pharmaceuticals Inc. Methods of administering dalbavancin for treatment of bacterial infections
EP1606414B1 (en) 2003-03-17 2009-12-23 Charles River Laboratories, Inc. Methods and compositions for the detection of microbial contaminants
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EP1842069A2 (en) 2004-12-02 2007-10-10 Charles River Laboratories, Inc. Methods and compositions for the detection and/or quantification of gram positive bacterial contaminants
EP1836492B1 (en) * 2005-01-13 2008-12-31 Charles River Laboratories, Inc. Method for classifying a microorganism in a biological sample
WO2009137244A1 (en) * 2008-04-15 2009-11-12 Charles River Laboratories, Inc. Cartridge and method for sample analysis
NZ593892A (en) 2008-12-23 2013-11-29 Biosource Pharm Inc Antibiotic compositions for the treatment of gram negative infections
WO2010151751A2 (en) * 2009-06-26 2010-12-29 Charles River Laboratories, Inc. Heat-treated limulus amebocyte lysates
US8415307B1 (en) 2010-06-23 2013-04-09 Biosource Pharm, Inc. Antibiotic compositions for the treatment of gram negative infections
US20130078665A1 (en) * 2012-07-18 2013-03-28 Deepika Bodapati Test strip, a test kit and a method for detection of endotoxin in food
CN103592442B (en) * 2013-10-29 2016-01-20 王明丽 A kind of method detecting bacteria endotoxin content in Recombinant Swine Interferon α1 freeze drying powder injection
CN108387739A (en) * 2018-01-23 2018-08-10 福州启新生物技术有限公司 The reagent and preparation method thereof of fungi in a kind of specific detection serum
CN109142760B (en) * 2018-07-04 2021-02-02 中国农业大学 Kit for rapidly and accurately detecting colistin in feed

Family Cites Families (26)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JPS5648897A (en) * 1979-09-25 1981-05-02 Nitsusui Seiyaku Kk Selective isolation medium for cholera bacillus
US4276050A (en) * 1980-01-10 1981-06-30 Abbott Laboratories Method for systemic endotoxin detection
US4322217A (en) * 1980-06-27 1982-03-30 Mallinckrodt, Inc. Process for preparing Limulus lysate
JPS5813519A (en) * 1981-07-16 1983-01-26 Seikagaku Kogyo Co Ltd Endotoxin adsorbent and removing method of endotoxin using the same
JPS5967210A (en) * 1982-10-09 1984-04-16 Nissan Chem Ind Ltd Nematocide
JPS60184100A (en) * 1984-03-02 1985-09-19 Toray Ind Inc Method of immobilization of physiologically active substance containing amino group
EP0634656B1 (en) * 1986-12-03 2000-01-12 Wako Pure Chemical Industries, Ltd. Processes for collecting body fluid from insects
US4803314A (en) * 1986-12-22 1989-02-07 Carlingswitch, Inc. Momentary rotary switch
DK255887D0 (en) * 1987-05-20 1987-05-20 Claus Koch IMMUNOASSAY
CA1337781C (en) * 1987-08-21 1995-12-19 Takanori Nakamura Polypeptide from horseshoe crab exhibiting affinity for lipopolysaccharide and method of preparation
US4808314A (en) * 1987-09-18 1989-02-28 Scripps Clinic And Research Foundation Method for reducing bacterial endotoxin contamination in solutions of macromolecules
JPH0715474B2 (en) * 1988-02-27 1995-02-22 和光純薬工業株式会社 Endotoxin assay
JPH0711523B2 (en) * 1988-03-16 1995-02-08 和光純薬工業株式会社 Reagent preparation method
US5594113A (en) * 1988-06-23 1997-01-14 Associates Of Cape Cod, Inc. Endotoxin binding and neutralizing protein and uses thereof
JP2688773B2 (en) * 1988-11-24 1997-12-10 和光純薬工業株式会社 Endotoxin inactivation method
JP2701916B2 (en) * 1989-02-08 1998-01-21 マルハ株式会社 Amebosite lysate having high specificity for β-glucan and method for preparing the same
US5234912A (en) * 1989-02-14 1993-08-10 Incyte Pharmaceuticals, Inc. Pharmaceutical compositions comprising recombinant BPI proteins and a lipid carrier and uses thereof
US5177059A (en) * 1989-11-15 1993-01-05 Sandoz Ltd. Polymyxin B conjugates
JP3085310B2 (en) * 1990-04-26 2000-09-04 日本バイリーン株式会社 Microbial removal material
CA2037727A1 (en) * 1991-03-07 1992-09-08 Burton W. Blais Removing lps pyrogen from aqueous solution
JP2944709B2 (en) * 1990-06-21 1999-09-06 生化学工業株式会社 (1 → 3) -β-D-glucan measuring agent
US5198339A (en) * 1990-07-13 1993-03-30 Board Of Regents, The University Of Texas System Method for detection of gram-negative bacterial lipopolysaccharides in biological fluids
CA2085448C (en) * 1991-12-24 2003-11-18 Masakazu Tsuchiya Process for extracting endotoxin
EP0549102B1 (en) * 1991-12-25 1996-07-03 Maruha Corporation Beta-glucans detection reagents and methods of detecting beta-glucans
US5552294A (en) * 1992-10-20 1996-09-03 Children's Medical Center Corporation Rapid detection of virulence-associated factors
CA2112776C (en) * 1993-01-21 2002-11-12 Masakazu Tsuchiya Process for inhibiting activity of endotoxin

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EP0608982B1 (en) 1997-09-17
EP0608982A2 (en) 1994-08-03
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KR940018097A (en) 1994-08-16
US5622833A (en) 1997-04-22
CN1120370C (en) 2003-09-03
US5750500A (en) 1998-05-12
CN1379248A (en) 2002-11-13
CN1109598A (en) 1995-10-04
DE69405594T2 (en) 1998-03-19
US5616557A (en) 1997-04-01
KR100255993B1 (en) 2000-05-01
CA2112776A1 (en) 1994-07-22
ES2107124T3 (en) 1997-11-16
DE69405594D1 (en) 1997-10-23

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