Embodiments relate to a screening culture medium and a screening method which enable the identification and screening of Candida auris.
There are more than 400 species of Candida bacteria, known as the causative bacteria of candidiasis, of which 20 of them are clinically important. Many of them have similar morphological and biochemical properties and are generally difficult to be discriminated.
Studies have been carried out on a method of identifying species with respect to the existing species of Candida bacteria. For example, Patent Document 1 discloses a culture medium for simple identification of Candida, which is obtained by adding 2,3,5-triphenyltetrazolium chloride (TTC) and yeast extract to a dye-added Sabouraud's culture medium. This culture medium for simple identification of Candida is intended to be a culture medium for carrying out discrimination between two species of Candida bacteria, Candida albicans and Candida glabrata, according to the colony color tone by using the difference in redox ability of these bacterial species on the culture medium.
Patent Document 2 discloses a method of detecting the presence of a specific microorganism bacterial strain in a culture medium, which is a method in which at least one chromogen that is a substrate for the enzyme of the bacterial strain and at least one compound of a high concentration, selected from carbohydrates, are added to a culture medium, and after the hydrolysis of the chromogen, an induced color different from the basic color of the chromophore is obtained. This method is intended to be one in which, for an enzyme that is produced by each of the bacteria including Candida albicans and Candida tropicalis, two chromogens, which are substrates of the enzyme, are added to a culture medium, and after the hydrolysis of the chromogens, colors different from the basic color of the chromophore are obtained to carry out distinguishment between the two strains.
[Patent Document 1] Japanese Unexamined Patent Application, First Publication No. H06-78793
[Patent Document 2] Published Japanese Translation No. H09-500790 of the PCT international Publication
Among the Candida bacteria, Candida auris, discovered and named by the inventors of the present invention have acquired multiple drug resistance and exhibited a high mortality rate, which has posed a global threat. There is a particular need for a means for conveniently and quickly examining whether or not this bacterial species, among the Candida bacteria, is present in a specific environment (for example, a certain closed space such as a hospital room).
For identifying Candida auris with respect to other bacteria, such as other bacterial species of Candida of the Candida bacteria, the identification can be carried out, for example, by analyzing the genes of the bacteria. However, this analysis requires equipment which may be inconvenient, and requires time and cost as well.
In the detection technique using the ability to degrade an enzyme substrate such as Patent Document 2 described above, it is possible to carry out detection with relatively convenient equipment and operation in a short culture time, and in the above technique and a detection method applying the above technique, other Candida bacteria such as Candida albicans and Candida tropicalis can be detected. However, according to the above technique, a method of distinguishing Candida auris from other Candida bacteria has not been found, and thus Candida auris cannot be detected by this technique.
For this reason, a technique for conveniently and quickly examining the existence of Candida auris has not yet been found.
The present invention has been made in consideration of the above circumstances, and an object thereof is to provide a screening culture medium that enables a convenient and quick examination for the presence of Candida auris, and a screening method using the screening culture medium.
In order to solve the above object, the present invention has the following aspects.
According to an embodiment, there is provided a screening culture medium containing an enzyme substrate, in which the screening culture medium is used for screening Candida auris based on an ability to degrade the enzyme substrate, the enzyme substrate including raffinose and xylose.
According to at least one embodiment, any of the above screening culture mediums, in which the Candida auris is an East Asian strain of Candida auris, and the enzyme substrate further includes N-acetylglucosamine
According to at least one embodiment, any of the above screening culture mediums, in which the Candida auris is an East Asian strain of Candida auris, and the enzyme substrate further includes potassium gluconate.
According to at least one embodiment, any of the above screening culture mediums, in which the enzyme substrate further includes glycerol.
According to at least one embodiment, any of the above screening culture mediums, in which the enzyme substrate further includes D-glucosamine hydrochloride.
According to at least one embodiment, any of the above screening culture mediums, in which each of the enzyme substrates is labeled such that a different color is developed in a case of being degraded.
According to another embodiment, there is provided a screening method including screening a microorganism based on an ability to degrade an enzyme substrate, in which in a case where the enzyme substrate includes raffinose and the microorganism has a positive ability to degrade raffinose, and in a case where the enzyme substrate includes xylose and the microorganism has a negative ability to degrade xylose, the microorganism is determined to be Candida auris.
According to at least one embodiment, any of the above screening methods, in which in a case where the enzyme substrate further includes N-acetylglucosamine, and the microorganism has a negative ability to degrade N-acetylglucosamine, the microorganism is determined to be an East Asian strain of Candida auris.
According to at least one embodiment, any of the above screening methods, in which in a case where the enzyme substrate further includes potassium gluconate, and the microorganism has a negative ability to degrade potassium gluconate, the microorganism is determined to be an East Asian strain of Candida auris.
According to at least one embodiment, any of the above screening methods, in which in a case where the enzyme substrate further includes glycerol, and the microorganism has an ability to degrade glycerol by more than 0% and 20% or less, which is negative, the microorganism is determined to be an East Asian strain of Candida auris.
According to at least one embodiment, any of the above screening methods, in which in a case where the enzyme substrate further includes glycerol, and the microorganism has a positive ability to degrade glycerol, the microorganism is determined to be a South American, African, or South Asian strain of Candida auris.
According to at least one embodiment, any of the above screening methods, in which in a case where the enzyme substrate is D-glucosamine hydrochloride, and the microorganism has a negative ability to degrade D-glucosamine hydrochloride, the microorganism is determined to be an East Asian strain of Candida auris.
According to at least one embodiment, any of the above screening methods, in which in a case where the enzyme substrate is D-glucosamine hydrochloride, and the microorganism has an ability to degrade D-glucosamine hydrochloride by 80% or more and less than 100%, which is positive, the microorganism is determined to be a South American strain of Candida auris.
According to at least one embodiment, any of the above screening methods, in which in a case where the enzyme substrate is D-glucosamine hydrochloride, and the microorganism has a positive ability to degrade D-glucosamine hydrochloride, the microorganism is determined to be an African or South Asian strain of Candida auris.
According to at least one embodiment, any of the above screening methods, further including a step of inoculating a sample in a screening culture medium containing the enzyme substrate; a step of culturing a microorganism contained in the sample in the screening culture medium; and a step of detecting the microorganism in the screening culture medium.
According to at least one embodiment, any of the above screening methods, in which a screening culture medium is used, where the screening culture medium enables detection of an ability of the microorganism to degrade the enzyme substrate, by allowing each enzyme substrate to develop a different color.
According to at least one embodiment, any of the above screening methods, in which in the step of culturing the microorganism, the culture is carried out at 35° C. or higher.
According to the present invention, it is possible to obtain a screening culture medium that enables a convenient and quick examination for the presence of Candida auris, and a screening method using the screening culture medium.
Hereinafter, a screening culture medium and a screening method according to the present invention will be described with reference to embodiments. However, the present invention is not limited to the following embodiments.
The screening culture medium according to the present embodiment contains an enzyme substrate, where the screening culture medium is used for screening Candida auris based on the ability to degrade the enzyme substrate, the enzyme substrate including raffinose and xylose.
Screening broadly refers to an operation of sorting out a microorganism. It broadly refers to an operation of sorting out a sample to be screened containing a microorganism, from the stage of the presence or absence of the possibility, by the presence or absence of a certain microorganism. The screening also refers to a step of obtaining more information for determining the possibility that a sample contains a certain microorganism (for example, determining the possibility from the results of a plurality of screenings).
The screening operation may be carried out one time or a plurality of times. Alternatively, the same screening operation may be carried out a plurality of times, and this series of operations may be collectively referred to as screening.
The screening culture medium according to the present embodiment is used for screening Candida auris.
There are various strains of Candida auris, which are classified into clades such as a South American clade, an African clade, an East Asian (Japanese and Korean) clade, and a South Asian (Indian) clade, depending on the origin thereof. According to the screening culture medium according to the present embodiment, any strain belonging to any cladecan be screened as long as it is Candida auris.
According to the screening culture medium according to the present embodiment, it is possible to carry out screening for the presence or absence of a certain bacterium or the bacterium classification (the classification on whether or not a microorganism is a certain bacterium), specifically, depending on whether or not a certain microorganism has an enzyme that degrades a specific compound as a substrate, that is, whether or not it has an ability to degrade a specific enzyme substrate. The degradation ability is also referred to as assimilation in a case where a microorganism uses an enzyme substrate as a nutrient. Examples of the enzyme substrate that is degraded by a bacterium include various carbohydrates (sugars) that are used in the present embodiment.
As such a screening culture medium, it is possible to use, for example, a known enzyme substrate culture medium. The enzyme substrate culture medium is a culture medium in which an enzyme substrate labeled with a chromogen (a color-developing substance) is contained, where the enzyme substrate is a substrate specifically metabolized (degraded and assimilated) by a target microorganism (a bacterial species). In a case where an enzyme substrate is incorporated and metabolized by a target bacterial species, a chromogen dissociates and the condensed chromogen develops a color (is colored). As a result, it is possible to screen a bacterial species having an ability to degrade the enzyme substrate.
As the chromogen with which an enzyme substrate is labeled, it is possible to use, for example, a compound that releases by hydrolysis two different chromophores that are capable of causing a coupling reaction. As such a compound, it is possible to use, for example, an indoxyl derivative. In a case where a culture medium contains a plurality of enzyme substrates, it is preferable to use a chromogen that exhibits a different color for each enzyme substrate, for example, a chromogen of a different compound.
The screening culture medium according to the present embodiment contains raffinose (RAF) and xylose (XYL) among the enzyme substrates.
Candida auris exhibits a positive ability to degrade raffinose and a negative ability to degrade xylose. Specifically, all of the 44 strains of Candida auris, including each of the above clades, exhibit positivity to raffinose (positive rate: 100%) and negativity to xylose (positive rate: 0%). As a result, in a case where a microorganism cultured in the screening culture medium of the present embodiment exhibits a positive ability to degrade raffinose and a negative ability to degrade xylose, there is a high possibility that such a microorganism is Candida auris. In addition, the combination of the positive ability to degrade raffinose and the negative ability to degrade xylose is not found in major pathogenic bacteria other than Candida auris. As a result, the culture medium of the present embodiment can be used for screening for Candida auris.
In a case where the screening culture medium is an enzyme substrate culture medium, it is preferable that the culture medium contain raffinose and xylose each labeled with a chromogen that exhibits a different color at the time of degradation.
According to the above configuration, it is possible to carry out screening such that, among the colonies of microorganisms cultured on the solid culture medium, a colony that exhibits a color obtained in a case where raffinose is degraded and does not exhibit a color obtained in a case where xylose is degraded is Candida auris, and a colony that exhibits only the color obtained in a case where xylose is degraded or both the colors obtained in a case where raffinose and xylose are degraded is not Candida auris.
The enzyme substrate contained in the screening culture medium of the present embodiment may further contain another enzyme substrate in addition to raffinose and xylose. As the enzyme substrate, enzyme substrates that are used in the related art for identifying a bacterial species can be appropriately selected. As a preferred example thereof, the screening culture medium may contain N-acetylglucosamine (NAG), potassium gluconate (GNT), glycerol (GLY), or D-glucosamine hydrochloride (GLN). As will be described later regarding the screening method, in a case where the screening culture medium contains these enzyme substrates in addition to raffinose and xylose, it is possible to obtain the information on which clade of strain a microorganism belongs to, in addition to the information on whether it is Candida auris.
In a case where the screening culture medium is the enzyme substrate culture medium described above and contains another enzyme substrate other than raffinose and xylose, the other enzyme substrate is preferably labeled to develop a color different from those of raffinose and xylose. According to this above configuration, it is possible to obtain the information on which clade of strain a cultured microorganism belongs to, concurrently with the information on whether or not it is Candida auris, based on the coloration that exhibits an ability to degrade each of raffinose, xylose, and another enzyme substrate (such as N-acetylglucosamine).
In a case where the screening culture medium of the present embodiment is an enzyme substrate culture medium, other configurations thereof may be those that are used for the existing culture medium. For example, components can be appropriately selected from the compositions of known enzyme substrate culture mediums, for example, a color-developing medium. The enzyme substrate culture medium may contain nutrients such as peptone, yeast extract, sugar, minerals, and vitamins As the nutrient, peptone is suitably used. The enzyme substrate culture medium may contain a thickening agent, a pH-adjusting agent, or the like. Further, it may contain an additive for improving the color development of the enzyme substrate, for example, a redox reagent.
The enzyme substrate culture medium may contain an antibacterial agent for suppressing the growth of microorganisms other than the target microorganism for screening. Examples of the antibacterial agent include an aminoglycoside-based antibiotic, a broad-spectrum antibiotic such as chloramphenicol or tetracycline, and cephalosporins or penicillin. Chloramphenicol is suitably used as an antibiotic for screening Candida auris.
The enzyme substrate culture medium may take an existing form as appropriate, such as liquid, semi-fluid, or solid; however, for example, in a case where a solid culture medium, particularly a flat plate solid culture medium (having a plate shape) is used, culture and detection are easy. A solidifying agent that is used in the related art, such as agar, carrageenan, or locust bean gum can be used to form a solid culture medium, and in the present embodiment, agar is used.
It is to be noted that a case where the screening culture medium contains a plurality of enzyme substrates may be a case of a combination of a plurality of culture media containing one or more of the plurality of enzyme substrates, in addition to a case where one culture medium contains all the enzyme substrates. For example, in a case where one kind of microorganism has been isolated in advance and a sample contains only that microorganism, and in a case where the information on whether the microorganism is Candida auris or the information on other clades of the microorganism is to be obtained, the present embodiment also includes an aspect in which the sample is cultured in different culture media each containing a different enzyme substrate and the information on the ability to degrade each enzyme substrate is obtained.
The screening method of the present embodiment is a screening method including screening a microorganism based on an ability to degrade an enzyme substrate, in which in a case where the enzyme substrate includes raffinose and the microorganism has a positive ability to degrade raffinose, and in a case where the enzyme substrate includes xylose and the microorganism has a negative ability to degrade xylose, the microorganism is determined to be Candida auris. Specifically, the screening is carried out by culturing a target microorganism using the above-described screening culture medium.
According to the screening method of the present embodiment, it is possible to carry out screening for whether or not a sample contains Candida auris, where the sample contains a plurality of microorganisms, or it is possible to carry out screening for whether or not a certain microorganism has a high possibility of being Candida auris.
As the sample containing a plurality of microorganisms, a sample collected from a specific space in which microorganisms might be present can be conceived.
Specifically, the screening method of the present embodiment further includes a step of inoculating a sample in a screening culture medium containing the enzyme substrate; a step of culturing a microorganism contained in the sample in the screening culture medium; and a step of detecting the microorganism in the screening culture medium.
For example, a method of carrying out screening for whether a sample containing a plurality of microorganisms contains Candida auris by using the above-described enzyme substrate culture medium will be described.
First, a step of inoculating a sample in a screening culture medium containing the enzyme substrate is carried out. Inoculation may be appropriately carried out according to the cell culture method in the related art.
Then, a step of culturing the microorganisms contained in the sample is carried out. Specifically, by culturing the microorganisms in the enzyme substrate culture medium inoculated with the sample, colonies of the microorganisms are formed on the enzyme substrate culture medium.
The conditions for carrying out culture in the enzyme substrate culture medium can be appropriately selected from the conditions for culturing microorganisms, known in the related art. In the present embodiment, it is preferable to carry out the culture at 35° C. or higher. In a case of carrying out the culture at 35° C. or higher, it is possible to culture pathogenic bacteria that grow under the conditions close to the human body temperature, thereby eliminating microorganisms that do not grow at lower temperatures. It is also preferable to carry out the culture at a temperature higher than 40° C. and lower than 42° C. Since Candida auris can grow even at 41° C., it is possible to eliminate other microorganisms that grow at a temperature up to 40° C. by carrying out culture under these temperature conditions.
The culture time can be appropriately selected from the conditions for culturing microorganisms, known in the related art; however, the culture is carried out for, for example, 24 hours or more and preferably 48 hours or more. In a case of carrying out culture for the above time, it is possible to form colonies sufficiently to the extent that coloration can be checked.
Then, a step of detecting the microorganisms in the screening culture medium is carried out. In the present embodiment, in a case of checking the coloration of the colonies of the microorganisms formed on the enzyme substrate culture medium, it is possible to carry out screening for whether the microorganism of the colony is Candida auris. Regarding the checking of the coloration, it is sufficient to visually check whether or not the color of the color-developing body with which the enzyme substrate is labeled is developed for each colony of the microorganism.
In the above-described enzyme substrate culture medium, a screening culture medium is used, where the screening culture medium enables the detection of the ability of the microorganism to degrade the enzyme substrate, by allowing each enzyme substrate to develop a different color. That is, in the enzyme substrate culture medium of the present embodiment, the enzyme substrates raffinose and xylose are each labeled to develop a different color in a case of being degraded. As described above, Candida auris exhibits an ability to degrade raffinose but does not exhibit an ability to degrade xylose. As a result, it can be determined that among the colonies of microorganisms cultured on the above culture medium, a colony that exhibits a color that is developed in a case where raffinose is degraded and does not exhibit a color that is not exhibited in a case where xylose is degraded is Candida auris. In a case where a sample containing a plurality of microorganisms has been inoculated in an enzyme substrate culture medium, and in a case where a colony that shows this coloration is included in the cultured colonies, it can be determined that the sample contains Candida auris.
In a case where the screening culture medium of the present embodiment further contains glucosamine (NAG), among the Candida auris strains, a strain of the East Asian clade exhibits negativity to N-acetylglucosamine, and strains of the South American, African, and South Asian clades exhibit positivity thereto. As a result, in a case of using this culture medium, it is possible to screen a strain of the East Asian clade of Candida auris.
Regarding the clades of Candida auris, it is known that other clades among these clades are more pathogenic than the East Asian clade. Regarding the East Asian clade, it is conceived that a fatal infection does not necessarily occur since the infection is limited to local infection that is basically limited to the inner ear and the outer ear.
That is, in a case of carrying out screening for whether or not a certain microorganism is Candida auris and also on whether or not it belongs to the East Asian clade, it is possible to obtain the information on the risk of the microorganism, or the sample containing the microorganism, or the environment in which the sample has been collected.
Further, in a case where the screening culture medium of the present embodiment contains potassium gluconate (GNT), among the Candida auris strains, a strain of the East Asian clade exhibits negativity to N-acetylglucosamine, and strains of the South American, African, and South Asian clades exhibit positivity thereto. As a result, in a case of using this culture medium, it is possible to obtain the information for screening a strain of the East Asian clade of Candida auris.
In addition, in a case where the screening culture medium of the present embodiment contains glycerol (GLY), among the Candida auris strains, only some of strains (roughly, more than 0% and less than 20%) of the East Asian clade exhibit positivity to glycerol, and strains of the South American, African, and South Asian clades exhibit positivity thereto. As a result, in a case of using this culture medium, it is possible to obtain the information for screening a strain of the East Asian clade of Candida auris and other strains.
In addition, in a case where the screening culture medium of the present embodiment contains D-glucosamine hydrochloride (GLN), among the Candida auris strains, a strain of the East Asian clade exhibits negativity to D-glucosamine hydrochloride, strains of the African and South American clades exhibit positivity thereto, and a large number of strains (roughly, more than 80% and less than 100%) of the South Asian clades exhibit positivity thereto. As a result, in a case of using this culture medium, it is possible to obtain the information for screening a strain of the East Asian clade of Candida auris and other strains.
In a case where the screening culture medium is the enzyme substrate culture medium described above and contains another enzyme substrate other than raffinose and xylose, and furthermore, the other enzyme substrate is labeled to develop a color different from those of raffinose and xylose, it is possible to carry out screening for whether or not a cultured microorganism is Candida auris and concurrently for whether or not it is the East Asian clade, based on the coloration that exhibits an ability to degrade each of raffinose, xylose, and another enzyme substrate (such as N-acetylglucosamine)
The screening based on such coloration can also be carried out by appropriately combining two or more substrates each providing different coloration. For example, in a case where a screening target is positive to two or more substrates, two or more types of coloration are exhibited, and a microorganism colony exhibits a color resulting from the mixed coloration, whereby it is possible to obtain the information on which substrate reacts with the screening target, that is, which strain of cladeamong Candida auris strains is included, based on the color tone and intensity of the colony.
The screening culture medium and screening method according to the present embodiment enables a convenient and quick examination for the presence of Candida auris. Specifically, for a sample containing a plurality of microorganisms, for example, a sample collected from a specific space, it is possible to carry out screening for the presence of Candida auris with a convenient operation of just inoculating and culturing the sample in a flat plate solid culture medium and in a short time of about 24 to 48 hours. For inoculation and culturing, it suffices that such equipment that enables culture in a flat plate solid culture medium is provided. Furthermore, the screening of microorganisms is carried out by only visual observation of the coloration, and thus special equipment or instrument is not required. Screening with a flat plate solid culture medium can be carried out at a very low cost as compared with gene analysis and the like.
As the sample to be screened in the present embodiment, for example, a sample collected from a specific indoor or outdoor space can be conceived. Examples of the specific space include places where Candida auris should be detected, and they include rooms in a hospital, particularly operating rooms or hospital rooms. In addition, those from various facilities or welfare facilities with elderly people and sick people can be used. In a case where the detection is carried out at an airport or a customhouse, it can be used for so-called border control measures.
The screening culture medium and the method of the present embodiment can be used to obtain information on the presence/absence of Candida auris or any clade of bacteria by combining a screening operation a plurality of times.
In addition, the screening culture medium and the method of the present embodiment can be used in combination with other means. For example, the screening culture medium and the method of the present embodiment can be used as a pre-stage screening for narrowing down the target to be subjected to further detailed gene analysis. Since the screening method of the present embodiment can be carried out conveniently and quickly, it is particularly effective in a case where the number or the like of samples to be screened (specific spaces where the presence is examined), clades, or the like is large.
The screening method of the present embodiment can also be used to carry out screening for one kind of microorganism on whether the bacterium is Candida auris. In that case, it is also possible to carry out screening using an enzyme substrate culture medium containing the above-described raffinose and xylose or containing another enzyme substrate. In addition, the present embodiment also includes an aspect in which the culture is carried out in different culture media each containing a different enzyme substrate and the information on the ability to degrade each enzyme substrate is obtained.
For the enzyme substrate culture medium, a plate-shaped culture medium is easy to use for culturing microorganisms; however, another form may be used. For example, a culture medium may be formed into a thin film shape. Since it is not difficult to simply install a film-shaped culture medium in various places and culture as is for carrying out screening, it is possible to install the film-shaped culture medium in the above-described specific space where Candida auris should be detected.
Hereinafter, Examples will be described. It is to be noted that the present invention is not limited to the following Examples.
The ability to degrade each enzyme substrate was examined for a plurality of bacterial strains including Candida auris. As Candida auris, 44 strains shown in Table 1 (as the bacterial species, 10 strains of the South American clade, 10 strains of the African clade, 10 strains of the East Asian clade, and 14 strains of the South Asian clade) were used. Other bacterial strains were selected from among the representative pathogenic yeast bacterial strains in Japan. The bacterial strains used as strains other than Candida auris are shown in Table 2.
As a kit that can identify the degradation ability as a positive rate, a plate of culture identification/fungus kit ID 32C API (Sysmex BioMérieux Co., Ltd.) was used for various enzyme substrates including raffinose (RAF), xylose (XYL), N-acetylglucosamine (NAG), potassium gluconate (GNT), glycerol (GLY), and D-glucosamine hydrochloride (GLN) among the enzyme substrates.
Bacterial solutions of the strains shown in Tables 1 and 2 were prepared with a suspension medium (a liquid culture medium) according to the protocol and taken into a positive rate detection cup of each enzyme substrate on a plate of ID 32C API and cultured for 48 hours. After culturing, wells that were transparent similar to the control were judged as negative (−), and wells that were opaque as compared with the control were judged as positive (+) by visual determination, and then the obtained positive data were analyzed using the database software 4.0 attached to ID 32C API.
C. auris #16
C. auris #17
C. auris #18
C. auris #19
C. auris #20
C. auris #21
C. auris #22
C. auris #23
C. auris #24
C. auris #25
C. auris #26
C. auris #27
C. auris #28
C. auris #29
C. auris #30
C. auris #31
C. auris #32
C. auris #33
C. auris #34
C. auris #35
C. auris #43
C. auris #44
C. auris 3540
C. auris 3541
C. auris 3435
C. auris 3436
C. auris 3449
C. auris 643
C. auris 3212
C. auris 3213
C. auris #52
C. auris #53
C. auris 3214
C. auris 3215
C. auris 3216
C. auris 3217
C. auris 3218
C. auris 3219
C. auris 3220
C. auris 3221
C. auris 3222
C. auris 3223
C. auris 3224
C. auris 3225
Candida albicans 1
Candida albicans 2
Candida dubliniensis
Candida famata
Candida glabrata
Candida globosa
Candida guilliermondii
Candida intermedia
Candida kefyr
Candida krusei
Candida lusitaniae
Candida parapsilosis
Candida sake
Candida tropicalis
Cryptococcus neoformans
Rhodotorula minuta
Candida auris
As shown in Table 1, all of the 44 strains of 4 clades of Candida auris had a positive ability to degrade RAF and a negative ability to degrade XYL.
Table 2 shows that all of the 44 strains of Candida auris (the bottom row of the table) had a positive ability (100%) to degrade RAF and a negative ability (0%) to degrade XYL. On the other hand, as shown in the other rows of Table 2, in the pathogenic bacterial strains other than Candida auris, the combination of a positive ability of 100% to degrade RAF and a negative ability (positive ability: 0%) to degrade XYL was not found.
That is, among the major pathogenic bacterial strains, only Candida auris had a positive ability of 100% to degrade RAF and a negative ability of 100% to degrade XYL. It was seen that it is possible to carry out screening for the presence or absence of Candida auris by detecting the ability to degrade RAF and the ability to degrade XYL.
As shown in the results shown in Table 1, among the 44 strains of Candida auris, the East Asian strain was positive to RAF and negative to XYL, as well as 100% negative to NAG.
That is, it was seen that in a case of detecting an ability of a Candida auris strain to degrade NAG in addition to RAF and XYL, it is possible to carry out screening for whether it is an East Asian strain or another strain.
Further, as shown in Table 1, the East Asian strain was 0% positive to GNT, whereas the strains other than the East Asian were 100% positive thereto.
The East Asian clade was 10% positive to GLY (that is, only one strain of the 10 East Asian strains was positive). From these results, it is conceived that the strains belonging to the East Asian clade include strains that are positive in a range of about 0 to 20% with respect to GLY. On the other hand, strains other than the East Asian were 100% positive thereto.
The East Asian clade was 0% positive to GLN, whereas the African and South Asian clades were 100% positive thereto, and the South American clade was 90% positive thereto. From this, it is conceived that the strains belonging to the South Asian clade include strains that are positive in a range of about 80% to 100% with respect to GLY.
That is, a strain having a low positive rate to GLY and a strain negative to GLN can be distinguished from other strains as the East Asian clade, and it is conceived that these combinations can be used for screening judgment of each of the strains.
According to the present invention, it is possible to obtain a screening culture medium that enables a convenient and quick examination for the presence of Candida auris, and a screening method using the screening culture medium.
Number | Date | Country | Kind |
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2020-017999 | Feb 2020 | JP | national |
This application claims the benefit of and priority to PCT/JP2021/003524, filed on Feb. 1, 2021, entitled (translation), “SCREENING CULTURE MEDIUM AND SCREENING METHOD,” which claims the benefit of and priority to Japanese Patent Application No. 2020-17999, filed on Feb. 5, 2020, which is hereby incorporated by reference in its entirety into this application.
Filing Document | Filing Date | Country | Kind |
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PCT/JP2021/003524 | 2/1/2021 | WO |