EP3615654A1 - Dispositif de culture microbiologique comprenant un feuillet d'hydrogel polysaccharidique deshydrate - Google Patents

Dispositif de culture microbiologique comprenant un feuillet d'hydrogel polysaccharidique deshydrate

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Publication number
EP3615654A1
EP3615654A1 EP18728205.8A EP18728205A EP3615654A1 EP 3615654 A1 EP3615654 A1 EP 3615654A1 EP 18728205 A EP18728205 A EP 18728205A EP 3615654 A1 EP3615654 A1 EP 3615654A1
Authority
EP
European Patent Office
Prior art keywords
dehydrated
culture device
microbiological culture
hydrogel
polysaccharide hydrogel
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Pending
Application number
EP18728205.8A
Other languages
German (de)
English (en)
French (fr)
Inventor
Marie-Pierre MONTET
Christine ROZAND
Jean-Pierre Flandrois
Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)
Biomerieux SA
Original Assignee
Biomerieux SA
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by Biomerieux SA filed Critical Biomerieux SA
Publication of EP3615654A1 publication Critical patent/EP3615654A1/fr
Pending legal-status Critical Current

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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12MAPPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
    • C12M33/00Means for introduction, transport, positioning, extraction, harvesting, peeling or sampling of biological material in or from the apparatus
    • C12M33/02Means for introduction, transport, positioning, extraction, harvesting, peeling or sampling of biological material in or from the apparatus by impregnation, e.g. using swabs or loops
    • CCHEMISTRY; METALLURGY
    • C08ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
    • C08BPOLYSACCHARIDES; DERIVATIVES THEREOF
    • C08B37/00Preparation of polysaccharides not provided for in groups C08B1/00 - C08B35/00; Derivatives thereof
    • C08B37/0006Homoglycans, i.e. polysaccharides having a main chain consisting of one single sugar, e.g. colominic acid
    • C08B37/0024Homoglycans, i.e. polysaccharides having a main chain consisting of one single sugar, e.g. colominic acid beta-D-Glucans; (beta-1,3)-D-Glucans, e.g. paramylon, coriolan, sclerotan, pachyman, callose, scleroglucan, schizophyllan, laminaran, lentinan or curdlan; (beta-1,6)-D-Glucans, e.g. pustulan; (beta-1,4)-D-Glucans; (beta-1,3)(beta-1,4)-D-Glucans, e.g. lichenan; Derivatives thereof
    • C08B37/0033Xanthan, i.e. D-glucose, D-mannose and D-glucuronic acid units, saubstituted with acetate and pyruvate, with a main chain of (beta-1,4)-D-glucose units; Derivatives thereof
    • CCHEMISTRY; METALLURGY
    • C08ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
    • C08BPOLYSACCHARIDES; DERIVATIVES THEREOF
    • C08B37/00Preparation of polysaccharides not provided for in groups C08B1/00 - C08B35/00; Derivatives thereof
    • C08B37/006Heteroglycans, i.e. polysaccharides having more than one sugar residue in the main chain in either alternating or less regular sequence; Gellans; Succinoglycans; Arabinogalactans; Tragacanth or gum tragacanth or traganth from Astragalus; Gum Karaya from Sterculia urens; Gum Ghatti from Anogeissus latifolia; Derivatives thereof
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12MAPPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
    • C12M1/00Apparatus for enzymology or microbiology
    • C12M1/16Apparatus for enzymology or microbiology containing, or adapted to contain, solid media
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12MAPPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
    • C12M25/00Means for supporting, enclosing or fixing the microorganisms, e.g. immunocoatings
    • C12M25/02Membranes; Filters
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12MAPPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
    • C12M41/00Means for regulation, monitoring, measurement or control, e.g. flow regulation
    • C12M41/30Means for regulation, monitoring, measurement or control, e.g. flow regulation of concentration
    • C12M41/36Means for regulation, monitoring, measurement or control, e.g. flow regulation of concentration of biomass, e.g. colony counters or by turbidity measurements

Definitions

  • the present invention belongs to the field of microbiology and culture of microorganisms on solid and semi-solid media. It relates more specifically to alternative solutions proposed to traditional agar culture media, intended in particular for culturing, detecting and / or identifying microorganisms present in a sample to be analyzed.
  • solid and semi-solid culture media more commonly referred to as agar or agar media nutritious - are valuable tools for the detection and study of potentially pathogenic and / or infectious microorganisms.
  • microorganism isolation techniques on agar medium, which are still widely used today in many microbiological analysis methods, given their great simplicity of execution. These are mainly techniques of isolation, exhaustion or the technique of dials.
  • isolation techniques on agar medium consist in dispersing, on the surface of the solid culture medium, the cells of a biological sample deposit to be analyzed. This dispersion is performed, for example, thanks to mechanical means / tools that are slid on the surface of the culture medium along a particular path. AT the outcome of this dispersion process, the cells arriving at the end of the spreading course are found individualized, separated from each other. Each of these individualized cells then develops to form ultimately a colony of pure culture, that is to say a cell cluster containing microorganisms, all genetically identical. Each colony can then be the subject of a morphological analysis (examination of the shape of the colony, its elevation, the regularity of the edges ...), directly on this same culture medium or on other environments. These cells may also be collected for conservation purposes and / or for subsequent complementary analyzes.
  • gelled / solidified culture media In addition to providing microorganisms with a support adapted to their growth and development, gelled / solidified culture media, conventionally based on agar, have the advantage of being able to present levels of hardness and surface conditions that make them perfectly adapted to cell isolation and spreading operations, and in particular to the pressure and friction forces exerted by the tools and instrumentations developed for this purpose (see, for example, EP 0 242 114, WO 2005/071055) .
  • Agar culture media however, have some major disadvantages. As such, we note a preparation, which when it is artisanal, requires time (at least one hour) and many operations (weighing ingredients, dissolutions, autoclaving, pouring, distribution in Petri dishes). Also, as is the case for liquid culture media, these solid or semi-solid media are extremely sensitive to any form of biological contamination. Finally, because of the great difficulty in ensuring sterility, "artisanal" agar media must be prepared extemporaneously or almost extemporaneously.
  • Petrifilm TM industrial microbiological culture devices
  • EP 0 070 310, EP 0 620 844 or EP 0 832 180 are formed of two waterproof films affixed to one another. At the interface, the inner face of each of the two films is covered with an adhesive composition for adhering a thin layer of powder (s) water soluble (s) cold.
  • one of the inner faces of the films is covered with a first powder, which corresponds to a dehydrated and micronized culture medium composition.
  • the other internal face is in turn covered with a second powder, which corresponds to a gelling agent (such as guar gum and / or xanthan gum) micronized.
  • a gelling agent such as guar gum and / or xanthan gum
  • the two inner faces are coated with the same powder, formed by a mixture of a dehydrated and micronized culture medium composition, and a micronized gelling agent.
  • Petrifilm TM devices are intended for the detection and / or enumeration of microorganisms present in a sample to be analyzed.
  • the culture device is opened by lifting the upper film, transparent.
  • the upper film is repositioned on the lower film.
  • the gelling agent forms a hydrogel with a high water content, having a gelatinous and viscous appearance, coming to swallow the cells present in the sample to be analyzed.
  • This same water present in the sample to be analyzed also makes it possible to solubilize and activate the culture medium.
  • the microbiological culture device is finally incubated at the temperature and for the prescribed time before reading the results.
  • Petrifilm TM devices if they effectively allow a good fixation of the cells, the hydrogel formed creates a surface, very gelatinous and viscous not suitable for operations of isolation and / or spreading cells as it could be done on an agar culture medium, and moreover is not compatible with the tools and instrumentations developed for this purpose (see, for example, EP 0 242 114, WO 2005/071055).
  • Compact Dry cultivation devices developed by the company NISSUI PHARMACEUTICAL (Japan), whose microbiological culture support is formed by a sheet of absorbent fibrous material, incorporating in its mass a dehydrated nutritive composition, optionally also selective, and / or or discriminant (see, for example, EP 1 179 586).
  • an alcoholic suspension is prepared by mixing, in ethanol, a composition of culture medium, an adhesive dissolved in both water and ethanol (e.g. ethylene] and hydroxypropylcellulose) and a water-soluble but ethanol-insoluble gelling agent (eg, locust bean gum, guar gum, carrageenan, hydroxyethylcellulose).
  • a composition of culture medium e.g. ethylene] and hydroxypropylcellulose
  • a water-soluble but ethanol-insoluble gelling agent eg, locust bean gum, guar gum, carrageenan, hydroxyethylcellulose.
  • Compact Dry TM devices are intended for the detection and / or enumeration of microorganisms present in a sample to be analyzed.
  • a volume of sample to be analyzed (liquid or previously made liquid) of a high fluidity, possibly previously diluted, is seeded with a pipette on the culture medium covering a maximum area.
  • the culture device is then incubated for the prescribed time and temperature, before reading the results.
  • This type of culture medium does not lend itself to isolation techniques implemented by spreading ⁇ samples to be analyzed. Indeed, because of their fibrous nature, these culture media have an irregular surface, with numerous asperities that hinder the continuous and regular sliding tools and instruments usually used to spread and disperse the cells on the surface of an agar medium classic. Also, the cells tend to develop in depth in the thickness of the porous support, which can make it difficult to visualize / identify the colonies formed.
  • microbiological culture devices ready for use, dedicated to the detection, identification and / or enumeration of microorganisms. These devices are also based on a culture support of fibrous and absorbent material, incorporating in its thickness a culture medium composition. The incorporation of the dehydrated culture medium composition into the thickness of the culture support is carried out by a dry impregnation technique. As for Compact Dry TM devices, because of their fibrous nature, these culture media have an irregular surface with many asperities; these devices are therefore not compatible with the techniques and tools developed so far for the isolation and spreading of cells on the surface of a conventional agar medium.
  • the cells grow deep in the thickness of the porous support.
  • Applicant proposes to cover this fibrous surface with a surface layer able to perfect the surface state.
  • a pore (micro) filtration membrane that is sufficiently narrow to prevent the cells from diffusing towards the underlying layers, and at the same time to form a relatively smooth rendering surface.
  • Said (micro) filtration membrane can be made based on one or more materials chosen from latex, polytetrafluoroethylene, poly (vinylidene) fluoride, polycarbonate, polystyrene, polyamide, polysulfone, polyethersulfone, cellulose, nitrocellulose.
  • a covering by a porous layer of composition comprising a mixture of kaolin pigments, talc, titanium dioxide, and / or calcium carbonate, and a binder of styrene butadiene latex type, acrylic styrene latex or carboxyl methyl cellulose.
  • the object of the present invention is therefore to propose a microbiological culture device which, while offering a long shelf life, including at room temperature, provides a real alternative to traditional agar culture media, both in terms of fertility and on the compatibility with the mechanical operations of spreading and dispersion of the cells.
  • Another objective of the present invention is to be able to propose a microbiological culture device that is compatible with the constraints of an industrial and commercial exploitation, particularly in terms of production cost and profitability.
  • the present invention aims at providing a microbiological culture device of design and manufacturing adapted to the facilities and means of production currently used in the industry of media and microbiological culture devices.
  • the present invention therefore proposes a microbiological culture device comprising:
  • a piece of absorbent material having an upper face at least substantially flat and incorporating in its thickness a dehydrated culture medium composition (dry or dried),
  • a polysaccharide hydrogel sheet dehydrated and rehydratable at room temperature in particular at temperatures between 5 ° C and 40 ° C; said dehydrated hydrogel sheet being affixed directly to the upper face of said piece of absorbent material, or indirectly through a permeable interlayable membrane.
  • said dehydrated polysaccharide hydrogel sheet has been previously prepared by dehydrating a hydrogel layer of water-based composition and at least one polysaccharide gelling agent. This dehydrated hydrogel sheet has the particularity of being rehydratable at room temperature.
  • hydrogel properties by simple absorption of an aqueous composition, without requiring any additional heat treatment and while retaining characteristics of shape, texture, hardness / rigidity and surface state very close to those a polysaccharide hydrogel slip constituting a microbiological culture device according to the invention would show if it had not been dehydrated after pouring (or after display / coating) but simply hardened.
  • the dehydrated polysaccharide hydrogel film restores a monoblock hydrogel layer, having a consistency and hardness / rigidity very comparable to those of a traditional agar culture medium ready to use.
  • said one-piece hydrogel layer has a hardness of between 500 and 2000 g. cm "2 , preferably between 700 and 1400 g cm -2 .
  • the hardness of said hydrogel layer can be measured by means of a texture analyzer, for example of the TA.XT plus type from STABLE MICRO SYSTEMS LTD (Great Britain).
  • a microbiological culture device In use, a microbiological culture device according to the invention must be hydrated to be activated. To do this, the piece of absorbent material is soaked with a quantity of water or an aqueous composition. The culture medium composition, initially present in a dry state, is thus solubilized and activated. In contact with the piece of absorbent material, or through a permeable interlayable membrane, the dehydrated polysaccharide hydrogel sheet rehydrates in turn, almost instantaneously and at room temperature. By rehydrating liquid from the absorbent material part, the hydrogel sheet regains flexibility and provides a thin layer of one-piece hydrogel (or hydrogel film) soaked with a solubilized and activated culture medium composition.
  • Seeding of the sample to be analyzed on the polysaccharide hydrogel slip can be performed both before and after rehydration of the latter.
  • the surface of the polysaccharide hydrogel film, before or after rehydration, is sufficiently smooth and rigid / hard to lend itself to cell isolation and spreading operations, and in particular to withstand the pressure and friction forces exerted by the tools and instrumentations developed for this purpose.
  • the polysaccharide hydrogel layer provides the surface of the microbiological culture device with a lubricating effect which facilitates the mechanical operations of spreading and dispersing the cells. Also, by its consistency agar, it promotes the implantation of microorganisms closer to the nutritive ingredients and active agents of the culture medium. As for the piece of absorbent material, in addition to its role in the preservation and distribution of the composition of medium its structure contributes to the rigidity and overall firmness of the surface of the microbiological culture device, ensuring its compatibility with regard to the pressure and friction forces exerted by the tools and instrumentations used to spread and disperse the cells .
  • culture medium refers to a nutrient composition allowing the growth and development of cells, more particularly bacteria, molds and / or yeasts. These media can meet the nutritional needs of microorganisms to grow. Schematically, we find in their composition:
  • At least one carbohydrate as a carbon source and energy
  • nutrients in particular, amino acids, growth factors, vitamins, minerals, trace elements, iron salts, sodium citrate, sodium chloride, etc.
  • chemically complex compositions such as mixtures of peptones (milk, meat and / or potato starch, corn ...), yeast extracts, serum, and / or animal or vegetable tissue extracts.
  • a culture medium within the meaning of the present invention may optionally demonstrate a certain selectivity with regard to target microorganisms, that is to say that it promotes the development of these target microorganisms rather than that of the annex flora, and / or that it inhibits and / or slows the development of the annex flora.
  • This selective effect can in particular be obtained through the use of agents with an inhibitory effect for the subsidiary flora or of agents with an activating effect for the target microorganisms.
  • a culture medium within the meaning of the present invention can possibly demonstrate discriminating abilities that make it possible to differentiate and visually distinguish the different categories of microorganisms growing on the same culture medium.
  • the culture medium advantageously incorporates a chromogenic and / or fluorogenic component allowing a visual observation of the microorganisms in function of particular metabolic activities that they express.
  • composition and formulation of many culture media are described in particular in HANDBOOK OF MICROBIOLOGICAL MEDIA (2010; 4th Edition).
  • sample refers to a sample taken for analysis or a small or small portion of that sample.
  • the invention more specifically relates to biological samples containing or suspected of containing microorganisms to be detected and / or analyzed.
  • biological samples can be of human, animal, plant or environmental origin. They can also have an industrial origin and come from withdrawals operated on a manufactured product or a product in the course of manufacture, or on instruments, installations encountered in an industrial environment.
  • the industrial sectors targeted here are more particularly the agro-food, pharmaceutical, cosmetic and veterinary industries, medical devices, microbiology of environmental controls (water, air, surfaces).
  • microorganisms and “cells” are used here equivalently and refer to bacteria, yeasts, molds and / or amoebae.
  • isolation / spreading means / tools means mechanical instruments suitable for use in the implementation of isolation techniques (for example, the technique of exhaustion, the technique of striations or dials), spreading techniques or cell layering techniques (for example, for cell counting or antibiotic susceptibility testing), such as those commonly used on traditional agar culture media.
  • These mechanical instruments used manually or in an automated manner, make it possible to produce one or more point deposits of microorganisms on the surface of the culture medium, and by sliding on this surface, they spread out the cells.
  • the proposed microbiological culture device is essentially formed of the combination between a piece of absorbent material incorporating in its thickness a composition of dehydrated culture medium, and a sheet of dehydrated polysaccharide hydrogel, having the ability to rehydrate at temperature room.
  • the dehydrated polysaccharide hydrogel sheet covers all or part of the upper face of the piece of absorbent material.
  • the absorbent material part which composes the inner / deep layer of the microbiological culture device according to the invention and serves as a reservoir for a composition of dehydrated culture medium
  • its structure, its design and its dimensions are largely described or suggested by EP 1 179 586, WO 2015/104501, WO 2014/013089, WO 2015/107228.
  • said piece of absorbent material is made from a nonwoven short fiber substrate, constituting an assembly having a structural integrity and a mechanical coherence.
  • Particularly suitable substrates are natural cellulosic fiber (such as cotton) or synthetic fiber (such as rayon), modified cellulosic fiber (for example, carboxymethylcellulose, nitrocellulose), absorbent chemical polymer fiber (such as polyacrylate salts). acrylate / acrylamide copolymers).
  • said piece of absorbent material is nonwoven fabric made of cellulose fiber, especially cotton.
  • liquid phase impregnation techniques see, for example, CN 102337324 or WO 2005/061013. These techniques involve imbibing an absorbent material from a culture medium composition formulated in solution in a volatile solvent (for example, water, an alcohol). Once well soaked, the drying of the absorbent material is achieved by evaporation of the solvent.
  • a volatile solvent for example, water, an alcohol
  • the amount of solution of the activated (hydrated) culture medium and the concentration of its constituents determine, on the one hand, the choice of material of the absorbent material part (especially in view of its retention capacity of water) and that of the dimensions of this piece of absorbent material and, secondly, the amount of culture medium powder to be incorporated, and vice versa.
  • said piece of absorbent material has a weight per unit area of between 50 gm "2 and 150 gm “ 2 , and preferably between 90 gm "2 and 110 gm “ 2 , for a thickness advantageously still between 0.5 mm and 10 mm, and more preferably between 1 mm and 4 mm.
  • the absorbent material part is advantageously subjected to a calendering operation.
  • the calendering by the pressure and the heating temperature generated, improves the retention of the composition of the dehydrated culture medium in the thickness of the absorbent material part, as well as its stability over time.
  • the calendering also has the advantage of improving the flatness of the surface of the piece of absorbent material, and to increase the capillary power of the latter.
  • the calendering is advantageously at a recommended temperature included between 30 ° C and 60 ° C. A temperature below 60 ° C makes it possible not to denature thermolabile compounds.
  • the piece of absorbent material incorporating in its thickness a dehydrated culture medium composition advantageously incorporates the technical characteristics of the dry-impregnated porous support described by WO 2015/104501.
  • the amount of culture medium composition formulated powder and incorporated in the thickness of the piece of absorbent material is between 0.01 g.cm "3 and 0.1 g. Cm" 3, preferably between 0 , 02 g. cm “3 and 0.09 g. cm” 3, more preferably between 0.03 g.cm "3 and 0.06 g.cm" 3.
  • this sheet of dehydrated polysaccharide hydrogel forms a hyperabsorbent and rehydratable material at room temperature, in particular at temperatures of between 5 ° C.
  • the spreading operations are often traumatic for the cells, they are generally displaced despite their adhesion to the culture medium, with a microbiological culture device according to the invention, thanks to a good surface quality of the hydrogel (possibly thixotropic properties), the cells are not abruptly detached from their support but are driven in motion with the hydrogel micro-fraction surrounding them.
  • the dehydrated polysaccharide hydrogel sheet is advantageously a dehydrated hydrogel sheet of gellan, xanthan, gallactomannan, starch and / or a mixture of these hydrogels.
  • Said dehydrated hydrogel sheet is obtained by dehydrating a hydrogel layer of water-based composition and at least one polysaccharide gelling agent.
  • Said polysaccharide gelling agent is preferably chosen from a gellan gum, a xanthan gum, a galactomannan gum (for example, a locust bean gum or a guar gum), starch and a mixture thereof.
  • the dehydrated polysaccharide hydrogel sheet is obtained by dehydration of a polysaccharide hydrogel layer previously prepared by mixing with one liter of water, 0.1 to 30 g of at least one polysaccharide gelling agent. .
  • the dehydrated polysaccharide hydrogel film is obtained by dehydration of a layer of gellan hydrogel, previously prepared by mixing with one liter of water, 10 to 20 g of gellan gum and, preferably, 13 to 15 g of gellan gum.
  • the dehydrated polysaccharide hydrogel sheet is obtained by dehydration of a layer of xanthan hydrogel, previously prepared by mixing with one liter of water, 0.2 to 10 g of xanthan gum, preferably of the order of 0.5 g of xanthan gum.
  • the hydrogel sheet Dehydrated polysaccharide is obtained by dehydrating a layer of xanthan hydrogel and gallactomannan, previously prepared from a mixture of xanthan gum and locust bean gum.
  • the weight ratio [xanthan gum] / [locust bean gum] is advantageously between 1: 2 and 2: 1, preferably of the order of 1: 1.
  • the dehydrated polysaccharide hydrogel sheet is obtained by dehydration of a layer of starch hydrogel, preferably of potato starch, previously prepared by mixing with one liter of water, 0.5 to 15 g of starch.
  • the dehydrated polysaccharide hydrogel sheet is obtained by dehydrating a layer of gellan hydrogel and starch, preferably potato starch, previously prepared from a mixture of gellan gum and starch.
  • the weight ratio [gellan gum] / [starch] is advantageously between 40: 1 and 2: 3.
  • a dehydrated polysaccharide slip can be prepared in multiple ways.
  • the hydrogel may be cast or spread in a continuous layer on a non-adherent surface. This continuous layer can also be obtained by a coating method.
  • the hydrogel layer is then dried / dewatered and then cut to the desired shape and size.
  • the preparation of the dehydrated polysaccharide hydrogel sheet can also be carried out by a molding method, followed by a dehydration step.
  • the dehydrated polysaccharide hydrogel sheet is advantageously structurally strengthened chemically by means of a reinforcing additive chosen from glycerol, ethylene glycol and polyethylene glycol.
  • a reinforcing additive chosen from glycerol, ethylene glycol and polyethylene glycol.
  • the addition of said reinforcing additive is carried out during the preparation of the polysaccharide hydrogel composition.
  • this addition is carried out at the step of mixing the gelling agent and the water, prior to the dehydration step.
  • a sheet of dehydrated polysaccharide hydrogel according to the invention further comprises at least one reinforcing additive selected from glycerol, ethylene glycol and polyethylene glycol.
  • said reinforcing additive is glycerol.
  • said dehydrated polysaccharide hydrogel sheet is a dehydrated gellan hydrogel sheet further comprising glycerol.
  • Such a dehydrated polysaccharide hydrogel slip is prepared from gellan gum and glycerol.
  • the weight ratio [gellan gum] / glycerol used in this preparation is advantageously between 2: 1 and 1: 8, preferably between 2: 7 and 2: 9, and is typically of the order of 1: 4.
  • said dehydrated polysaccharide hydrogel sheet further comprises at least one hardening agent chosen from divalent cation salts.
  • the curing agent is selected from magnesium chloride (MgCl 2 ), calcium chloride (CaCl 2 ), magnesium sulfate (MgSO 4) and manganese chloride (MnCl 2 ).
  • the curing agent is MgCl 2 .
  • said dehydrated polysaccharide hydrogel sheet is a dehydrated gellan hydrogel sheet further comprising at least one curing agent selected from MgCl 2 , CaCl 2 , MgSC 4 and MnCl 2 .
  • the curing agent is advantageously MgCl 2 .
  • the gellan / MgCl 2 weight ratio is advantageously between 100: 1 and 3: 2, preferably between 30: 1 and 1: 3, and is typically of the order of 15: 1.
  • the dehydrated polysaccharide hydrogel sheet is prepared from gellan gum and MgCl 2 .
  • the weight ratio [gellan gum] / MgCl 2 used in this preparation is advantageously between 100: 1 and 3: 2, preferably between 30: 1 and 1: 3, and is typically of the order of 15: 1.
  • the dehydrated polysaccharide hydrogel sheet is prepared from gellan gum and MgSC.
  • the weight ratio [gellan gum] / MgSO4 used in this preparation is advantageously between 100: 1 and 3: 2, preferably between 30: 1 and 1: 3, and is typically of the order of 15: 1.
  • said dehydrated polysaccharide hydrogel sheet is a dehydrated gellan hydrogel sheet comprising, in addition, at least one plasticizing agent such as, for example, a silicone oil.
  • a plasticizer makes it possible to obtain dehydrated hydrogels of greater flexibility and flexibility. The advantage is thus to be able to prepare large surfaces of dehydrated hydrogel, for example in long strips that can be rolled and thus preserved until they are cut into sheets of dimensions appropriate to the microbiological culture devices according to the invention.
  • incorporation of the plasticizer is performed during the preparation of the polysaccharide hydrogel composition.
  • this incorporation is carried out at the step of mixing the gelling agent and the water, prior to obtaining the dehydrated polysaccharide sheet.
  • the dehydrated polysaccharide hydrogel sheet incorporates in its thickness chromogenic and / or fluorogenic compounds allowing a visual observation of the microorganisms as a function of the particular metabolic activities that they express.
  • These compounds may be, for example, synthetic substrates for the demonstration of defined enzymatic activities, colored pH indicators.
  • incorporation of the chromogenic and / or fluorogenic compounds is carried out during the preparation of the polysaccharide hydrogel composition.
  • this incorporation is carried out at the step of mixing the gelling agent and the water, prior to obtaining the dehydrated polysaccharide sheet.
  • a microbiological culture device in addition to the piece of absorbent material and the dehydrated polysaccharide hydrogel sheet, may also comprise an intermediate permeable membrane disposed between said piece of absorbent material and said sheet of Dehydrated polysaccharide hydrogel.
  • the composition, the design and the thickness of this intermediate permeable membrane are chosen so that the latter impedes as little as possible the transfer of the liquids between the absorbent material part and the dehydrated polysaccharide hydrogel sheet or the polysaccharide hydrogel layer. rehydrated.
  • it can be made from a substrate of natural cellulosic fiber (such as cotton) or synthetic (such as rayon), of modified cellulosic fiber (for example, carboxymethylcellulose, nitrocellulose), of polymer fiber absorbent chemicals (such as polyacrylate salts, acrylate / acrylamide copolymers) or stable protein fibers (such as silk, wool).
  • natural cellulosic fiber such as cotton
  • synthetic such as rayon
  • modified cellulosic fiber for example, carboxymethylcellulose, nitrocellulose
  • polymer fiber absorbent chemicals such as polyacrylate salts, acrylate / acrylamide copolymers
  • stable protein fibers such as silk, wool
  • this optional permeable permeable membrane can be used for a very wide variety of purposes, for example:
  • said intermediate permeable membrane is used to improve the contrast and observation of colonies growing on the surface of the microbiological culture device.
  • it is chosen sufficiently opaque to light and of a great whiteness (for example, a CIE whiteness of at least 65).
  • the design of the biological culture devices according to the invention and the methods of use thereof allow the main constituent elements, such as in particular: the piece of absorbent material,
  • microbiological culture device can be packaged and marketed in various forms, in particular:
  • a microbiological culture device composite, previously assembled and assembled, wherein the piece of absorbent material is surmounted by a sheet of dehydrated polysaccharide hydrogel, optionally with a permeable membrane interlayers;
  • a microbiological culture device in a kit, which the user will assemble by himself; such a kit comprises at least one piece of absorbent material, at least one dehydrated hydrogel sheet, optionally at least one intermediate permeable membrane.
  • microbiological culture device is packaged preassembled or conditioned so that it can be assembled extemporaneously by a user, to facilitate handling thereof:
  • a blocking system disposed within a receptacle (for example, the receptacle of a petri dish) specifically adapted to receive said microbiological culture device;
  • the different constituent elements of the microbiological culture device according to the invention are, in this case, of shape and dimensions adapted to those of said receptacle, and the rim of said receptacle is provided on its internal face (s) mechanical retention members, type pins, projecting out of the surface.
  • the invention also relates to a microbiological culture device as previously described, and presented in the form of a kit to be assembled.
  • a microbiological culture device in a kit to be assembled, according to the invention thus comprises:
  • At least one piece of absorbent material having an upper face which is at least substantially flat and incorporates in its thickness a composition of dehydrated culture medium
  • At least one polysaccharide hydrogel sheet that is dehydrated and rehydratable at ambient temperature, in particular at temperatures between 5 ° C. and 40 ° C., and optionally
  • At least one permeable membrane spacer is provided.
  • a polysaccharide hydrogel slip dehydrated and rehydratable at room temperature particularly at temperatures between 5 ° C and 40 ° C.
  • the said dehydrated and rehydratable polysaccharide hydrogel sheet at room temperature is intended to be used as a microbiological culture support.
  • a dehydrated and rehydratable polysaccharide hydrogel sheet according to the invention is characterized by all or part of the technical characteristics listed below:
  • said dehydrated polysaccharide hydrogel sheet is a dehydrated hydrogel sheet of gellan, xanthan, galactomannan, starch or a mixture thereof,
  • said dehydrated polysaccharide hydrogel sheet has been prepared by dehydrating a hydrogel layer of water-based composition and at least one polysaccharide gelling agent chosen from a gellan gum, a xanthan gum, a galactomannan gum, starch and a mixture thereof,
  • said dehydrated polysaccharide hydrogel sheet is obtained by dehydration of a polysaccharide hydrogel layer prepared by mixing with one liter of water 0.1 to 30 g of at least one of the above-mentioned polysaccharide gelling agents,
  • said dehydrated polysaccharide hydrogel sheet is obtained by dehydration of a layer of gellan hydrogel, previously prepared by mixing with one liter of water, 10 to 20 g of gellan gum and, preferably, 13 to 15 g of gellan gum,
  • said dehydrated polysaccharide hydrogel sheet is obtained by dehydration of a layer of xanthan hydrogel, previously prepared by mixing with one liter of water, 0.2 to 10 g of xanthan gum,
  • said dehydrated polysaccharide hydrogel sheet is obtained by dehydration of a layer of xanthan hydrogel and gallactomannan, previously prepared from a mixture of xanthan gum and locust bean gum,
  • said dehydrated polysaccharide hydrogel sheet is obtained by dehydration of a starch hydrogel layer, previously prepared by mixing with one liter of water, 0.5 to 15 g of starch,
  • said dehydrated polysaccharide hydrogel sheet is obtained by dehydration of a layer of gellan and starch hydrogel, prepared from a mixture of gellan gum and of starch, with a weight ratio of gellan gum ] / [starch] of between 40: 1 and 2: 3,
  • said dehydrated polysaccharide hydrogel sheet is structurally reinforced chemically by means of a reinforcing additive chosen from glycerol, ethylene glycol and polyethylene glycol,
  • said dehydrated polysaccharide hydrogel sheet further comprises at least one hardening agent chosen from divalent cation salts, in particular MgCl 2 , CaCl 2 , MgSO 4 and MnCl 2 ,
  • said dehydrated polysaccharide hydrogel sheet further comprises at least one plasticizing agent such as, for example, a silicone oil.
  • FIG. 1 is a schematic representation of a microbiological culture device according to the invention, and its general principle of use;
  • FIG. 2 is a photograph showing an example of dehydrated polysaccharide hydrogel leaflets at the end of the drying / dehydration process
  • FIGS. 3 to 13 show photographs of cultures and isolations of bacterial strains carried out on microbiological culture devices according to the invention.
  • a microbiological culture device consists, in the first place, of a piece of absorbent material 1, more or less thick and a sheet of dehydrated polysaccharide hydrogel 2, of lesser thickness.
  • these two elements 1 and 2 are substantially square shape.
  • the absorbent material part 1 made of hydrophilic and non-water-soluble material, incorporates in its thickness a composition of dehydrated culture medium.
  • the dehydrated polysaccharide hydrogel sheet 2 is itself formed by drying / dehydration of a polysaccharide hydrogel layer, and its mechanical structure can be reinforced by means of a fibrous reinforcement, for example a woven fabric.
  • the piece of absorbent material 1 and the dehydrated polysaccharide hydrogel sheet 2 can be provided already preassembled, joined together, or else in the form of two mechanically independent elements.
  • the design and manufacture of this piece of absorbent material 1 and this dehydrated polysaccharide hydrogel sheet 2 will be described in more detail in the following examples.
  • a receptacle 4 is associated with the microbiological culture device to facilitate handling thereof, in particular for the rehydration and activation stage of the device, and for any displacement (for example, a transfer from the bench to the incubator).
  • the use of a microbiological culture device according to the invention requires activation of the device through hydration by the absorbent material part 1, with water 4.
  • the microbiological culture device is placed inside the receptacle 4, with the dehydrated polysaccharide hydrogel sheet 2 facing upwards. Since the receptacle 4 is larger than that of the culture device, the water 5 is poured into the receptacle 4, taking care not to pour directly onto the dehydrated polysaccharide hydrogel sheet 2.
  • the volume of water used is more or less calibrated to be able to sufficiently wet the absorbent material part 1 and solubilize the composition of culture medium it contains.
  • Another way to operate is to pour into the bottom of the receptacle 4, the appropriate volume of water, then to deposit the piece of absorbent material 1, topped with the sheet of dehydrated polysaccharide hydrogel 2.
  • the hydration step can then be carried out in a third way.
  • the piece of absorbent material 1 is then placed inside the receptacle 4.
  • a sufficient quantity of water is poured in order to thoroughly soak the piece of absorbent material 1 Then we come cover the surface with dehydrated polysaccharide hydrogel sheet 2.
  • the hydration by the absorbent material part 1 makes it possible, initially, to solubilize the composition of culture medium contained in the thickness of the absorbent material part 1.
  • this activation is continued by the hydration of the dehydrated polysaccharide hydrogel sheet 2, applied to the surface of the absorbent material part 1.
  • This rehydration of the dehydrated polysaccharide hydrogel sheet 2 on the surface of the piece of absorbent material 1, a rehydrated polysaccharide hydrogel layer 2 ' is shown and swollen, not simply by the water coming from the piece of absorbent material 1 but rather by a solution of culture medium. from the absorbent material part 1.
  • the cell culture device is ready to receive the sample to be analyzed.
  • the sample is inoculated on the device, in particular by spreading and dispersing the cells, for example by means of an oesse 6, the whole is incubated at a temperature and for a fixed duration, before reading. results.
  • the layer / film of rehydrated polysaccharide hydrogel 2 'of a microbiological culture device makes it possible to create a culture surface, both lubricated and adherent for the cells, capable of to receive the microorganisms and allow their isolation by operations and mechanical means usually used to spread the cells on the surface of a conventional agar medium.
  • this layer / film of polysaccharide hydrogel 2 ' will be able to self-regenerate, throughout the period incubating continuously, the culture medium solution from the piece of absorbent material 1.
  • the microbiological culture device may also incorporate an intermediate permeable membrane 3 interposed between the absorbent material part 1 and the dehydrated polysaccharide hydrogel sheet 2.
  • this membrane permeable insert 3 can be used for a variety of purposes, for example: to provide mechanical reinforcement and / or additional rigidity to the entire system, or only to the dehydrated polysaccharide hydrogel sheet 2 and the rehydrated polysaccharide hydrogel layer 2 ',
  • the piece of absorbent material 1 used in the constitution of a microbiological culture device according to the invention is shaped from a three-dimensional support, of open structure, porous, able to receive in its breast, both a liquid (in particular, an aqueous liquid) and solid particles of suitable particle size.
  • the microbiological culture devices tested comprise a piece of absorbent material incorporating a composition of culture medium, dry or dehydrated, made from the nonwoven Airlaid SCA95 N81, the company SCA ( Sweden).
  • This two-component PET / CoPET non-woven fabric (Polyester / coPolyester) has been specially treated to be tacky, by simple hot pressing (calendering), without adding glue. It is also characterized by a surface mass, before calendering (or non-calendered), of the order of 95 gm "2 for a thickness of 2 mm.From this non-woven, pieces of about 6 side cm were cut.
  • the nonwoven parts are calendered at 60 ° C. by applying a pressure of 3.10 5 Pa.cm -2 .
  • chromlD ® range media eg, chromlD ® CPS Elite, chromlD ® S. aureus, chromlD ® P. aeruginosa, chromlD ® VRE, chromlD ® Salmonella Elite.
  • microbiological culture devices according to the invention could then be tested for the detection and the isolation of bacteria such as Escherichia coli, Enterococcus faecalis, Staphylococcus aureus, Pseudomonas aeruginosa, Enterobacter cloacae, Clostridium freundii, Streptococcus agalactiae and Serratia marcescens.
  • bacteria such as Escherichia coli, Enterococcus faecalis, Staphylococcus aureus, Pseudomonas aeruginosa, Enterobacter cloacae, Clostridium freundii, Streptococcus agalactiae and Serratia marcescens.
  • the sheets of dehydrated polysaccharide hydrogel 2 which form part of the microbiological culture devices according to the invention, are designed above all so that, once rehydrated, they can offer microorganisms a support adapted to their growth and development. .
  • the composition and consistency of these sheets of dehydrated polysaccharide hydrogel 2 have also been specifically studied to obtain surfaces suitable for isolation and spreading operations. cells, that these polysaccharide hydrogel leaflets are in a rehydrated or dehydrated state.
  • Figure 2 is a photograph showing the dehydrated hydrogel leaflets at the oven outlet. As an indication, with 7 ml of hydrogel preparation poured into the Petri dishes, the thickness of the hydrogel pieces is of the order of 3 mm, before their preparation preparation in the oven or in the oven. After dehydration, the leaves are less than 1 mm thick.
  • the sheets of dehydrated polysaccharide hydrogel 2 of a microbiological culture device according to the invention have been declined in different versions, by varying, in particular: the nature of the polysaccharide gelling agent (for example, gellan gum, xanthan gum, galactomannan gums, starch, sodium alginate, pectin, methylcellulose and hydroxymethylcellulose),
  • the polysaccharide gelling agent for example, gellan gum, xanthan gum, galactomannan gums, starch, sodium alginate, pectin, methylcellulose and hydroxymethylcellulose
  • a light-fast and high-brightness membrane (for example, a CIE whiteness of at least 65) can be interposed between the piece of absorbent material and the dehydrated polysaccharide hydrogel sheet.
  • This permeable interlayable membrane may consist of a sheet of absorbent paper, of cellulosic composition.
  • bacterial cultures have been carried out in particular with strains of Escherichia coli, Enterococcus faecalis, Proteus mirabilis of Staphylococcus aureus, Serratia marcescens, Pseudomonas aeruginosa, Enterobacter cloacae, Clostridium freundii and Cronobacter sakazaki. .
  • the sheets of dehydrated polysaccharide hydrogel to be tested are associated with absorbent material parts incorporating in their thickness a particular dehydrated culture medium composition.
  • the peculiarity of this dehydrated culture medium composition lies in the fact that it has been chosen to be adapted to the growth and development of the bacteria of interest, and that they integrate chromogenic components facilitating the visual identification of these bacteria of interest.
  • the absorbent material parts which incorporate in their thickness a dehydrated culture medium composition, are placed in Petri dishes 90 mm in diameter, then wetted with 6-7 mL of sterile distilled water. These absorbent material parts are then overcome with a dehydrated polysaccharide hydrogel film. After hydration of the piece of absorbent material formed, the culture medium and the regenerated activated polysaccharide hydrogel layer, microbiological culture device is seeded with 10 ⁇ ⁇ a calibrated solution to a theoretical load of 10 bacterial 7 cfu / mL. The cell sample is deposited by means of a first oesse on the first dial of the hydrogel surface. The second dial is seeded with a new o ⁇ se by stretching several streaks from the first dial. The third dial is seeded like the second without changing o ⁇ se. The fourth dial is seeded by unstretched streaks from the second dial.
  • the boxes are placed in a jar with a little water so that the microbiological culture devices do not dry out. The whole is then incubated at 37 ° C. for 24 hours.
  • MgCl 2 at the rate of 1 g / L (that is to say 1 g of MgCl 2 per liter of water used in the preparation of the hydrogel) or
  • the gellan gum used here to prepare the dehydrated polysaccharide hydrogel leaflets is Gelrite ® , distributed by CARL ROTH GmbH, Germany.
  • the results obtained are very similar.
  • the colonies of E. coli grow on the surface of the hydrogel slip. They have a very nice size and a very beautiful color. Their morphotype corresponds to that of the colonies of E. coli growing on a reference chromogenic agar such as chromlD ® CPS Elite.
  • the gellan gum used here is Gelrite ® .
  • the gellan gum used here is Gelzan TM, distributed by CP KELCO, USA.
  • the gellan gum used here is Gelzan TM.
  • the colonies of E. faecalis growing on the surface of the hydrogel leaf are identical, in size, in color and in morphotype, to E. coli colonies. faecalis growing on chromogenic reference agar such as chromlD ® CPS Elite.
  • the gellan gum used here is Gelrite ® .
  • the P. mirabilis colonies growing on the surface of the hydrogel leaflet are identical in size, color and morphotype to colonies of P. mirabilis growing on chromogenic reference agar such as chromlD ® CPS Elite.
  • 8B, 8B ' gellan gum 13 g / L, CaCl 2 2 g / L,
  • 8C, 8C gellan gum 15 g / L, CaCl 2 1 g / L,
  • the gellan gum used here is Gelzan TM.
  • FIG. 9 a photograph of cultures and isolates of E. faecalis carried out on microbiological culture devices is presented, of which the dehydrated polysaccharide hydrogel sheets have been obtained from 15 g / L gellan hydrogels. of glycerol reinforced structure, at a rate of 43 ml / l, and hardened with:
  • the gellan gum used here is Gelzan TM.
  • the gellan gum used here is Gelrite ® .
  • a 2 gellan gum 30 g / L (Phytagel TM), glycerol 43mL / L, MgCl 2 1 g / L,
  • gellan gum 20 g / L (Gelrite ®), Glycerol 43ml / L, MgCl 2 1 g / L,
  • gellan gum 8 g / L (Gelrite ®), Glycerol 43ml / L, MgCl 2, 1 g / L,
  • gellan gum 6 g / L (Gelrite ® ), glycerol 43mL / L, MgCl 2 1 g / L,
  • 1 lCi gellan gum 20 g / L (Gelzan TM), glycerol 43mL / L, MgCl 2 1 g / L,
  • gellan gum 8 g / L Gellan TM
  • glycerol 43mL / L Gellan gum 8 g / L (Gelzan TM)
  • glycerol 43mL / L Gellan gum 8 g / L (Gelzan TM)
  • glycerol 43mL / L Gellan gum 8 g / L (Gelzan TM)
  • glycerol 43mL / L MgCl 2 1 g / L
  • FIG. 13 photographs of cultures and isolates of microorganisms conducted on microbiological culture devices are shown in which the dehydrated polysaccharide hydrogel sheets were obtained from a gelzan TM 15 g / L hydrogel, cured with MgCl 2 , at 1 g / L.
  • microbiological culture devices have also been successfully tested for the culture and detection of Streptococcus agalactiae (13A), Serratia marcescens, (13B), and for co-culture and co-detection of S. marcescens and S. aureus (13C).

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