RU2233173C1 - Method for prophylaxis and treatment of dermatomycosis, vaccine "poliderm" for its realization and method for preparing such vaccine - Google Patents

Abstract

FIELD: veterinary sciences, vaccines.

SUBSTANCE: invention relates to vaccine comprising inactivated field strains of dermatophytes and differs from the known mixed vaccines containing laboratory strains. In intramuscular administration the proposed vaccine has no reactivity and pathogenic effect and makes immunity in many species of sensitive animals against practically all basic pathogens of dermatophytosis in animals being independently of their areas inhabitation or geographic region of holding, i. e. it involves the complete set of exo-antigens and endo-antigens of dermatophyte cultures.

EFFECT: improved prophylactic and treatment method.

39 cl, 2 ex

Description

The invention relates to the field of veterinary medicine, in particular to the treatment and prevention of dermatomycosis - fungal skin diseases, in particular to vaccines against dermatomycoses containing antigenic material from dermatophyte cultures and methods for producing such vaccines. You can use the invention in the field of medicine for the treatment and prevention of human dermatomycosis.

There are various methods for the prevention and treatment of dermatomycosis with vaccines containing an immunologically effective amount of antigenic material from cultures of various dermatophytes. Known mocomponent vaccines against dermatomycoses of animals are used for the production of any one laboratory strain of a certain dermatophyte from the number of dermatophytes, which are one of the main causative agents of skin diseases, for example: Trichophyton equinum fungus strain No. 2251/71 is used in the vaccine for the prevention and treatment of horse trichophytosis [SU 548947, 1976]; strain of the fungus Trichophyton mentagrophytes VGNKI No. 27-DEPT - in the vaccine against trichophytosis of cattle, sheep, goats, rabbits [RU 2013445, 1994]: strain of the fungus Trichophyton verrucosum VGNKI No. TV-201 VGNKI-DEPT - in the vaccine against trichophytosis of cattle , rabbits [RU 2074251, 1997]. To obtain vaccines, the desired strain is grown in heat for about three weeks on a nutrient medium at a temperature of 26-28 ° C, the mushroom mass is removed, homogenized, and a number of operations are performed. Vaccination is carried out by double intramuscular injection of the finished vaccine with an interval of 10-14 days in doses of 1-2 ml.

Monocomponent vaccines do not provide immunity against microsporia and trichophytosis caused by other dermatophytes-pathogens.

Associated (or multicomponent) dermatomycosis vaccines are known, which partially eliminate the indicated disadvantage of monocomponent vaccines. Known vaccine against trichophytosis of cattle and other artiodactyls containing antigens from the strain of the fungus Trichophyton verrucosum VIEV No. 478 and from the strain of the fungus Trichophyton verrucosum VIEV No. 145, taken in equal proportions with a final concentration of 60-160 million microconidia in 1 ml of 4-5% saline solution of NaCl, and the adjuvant is aluminum hydroxide in an amount of 0.5-0.6 ml for every 100 ml of vaccine [RU 2093178, 1997]. The associated vaccine against trichophnia and microsporia of horses contains antigens from the strain of the fungus Microsporum canis VIEV No. 473 and the strain of the fungus Trichophyton equinum NL 2251/70, taken in equal proportions with the final concentration of each strain (1-8) · 10 ⁷ microconidia in 1 ml of the vaccine, and a protective environment based on sucrose and gelatin [RU 2097065, 1997]. Also known is the vaccine "Microderm" against dermatophytosis of animals, mainly carnivores and rodents, containing, wt.%: Antigen from the strain of the fungus Trichophyton mentagrophytes VGNKI No. 27 with a concentration of 70-90 million microconidia / cm ³ - 20.0-30.0; antigen from the strain of the fungus Microsporum canis VGNKI No. 2293 with a concentration of 70-90 million micronidium / cm ³ - 20.0-30.0; sucrose - 10.0-20.0: gelatin - 1.5-4.0; distilled water - the rest [RU 2084240, 1997].

As a prototype of the claimed vaccine, the well-known Polivak-TM vaccine was selected for the prevention and treatment of animal dermatophytosis, containing antigenic material in an amount of 40-120 million microconidia / 1 cm ³ from Trichophyton verrucosum VKPGF dermatophyte cultures No. 931/410 and / or Trichophyton mentagrophytes BKPGF No. 930/1032 and / or Trichophyton eguinum BKPGF No. 929/381 and / or Microsporum canis VKPGF No. 928/393 and / or Murosporum canis var. obesum. VKPGF No. 727/1311 and / or Microsporum canis var. ductortum No. 728/120 and / or Microsporum gypseum VKPG N 729/59, an inactivator (thimersal, formalin or 2-propiodactone) and a physiologically acceptable carrier.

As prototypes of the claimed method for producing the vaccine and the method of treatment and prevention, the technical solution according to the international application PCT / IB00 / 01196 [publication WO 01/15725 of 08.03.2001] was selected. Such an associated live vaccine for protecting vertebrates from fungal skin infectious diseases in particular contains an effective amount of immunostimulating material from several heat-inactivated dermatophyte cultures from the group: Candida; Eipidermophyton, including Epidermophyton floccusum: Keratinomyces (also known as Trichophyton ajelloi); Microsporum, including Microsporum canis strains DSM No. 13016 and DSM No. 13017: Trichophyton. including Trichophyton equinum DSM strain No. 13018. The specified material is suspended in the liquid phase in an amount of 10 ² -10 ¹⁰ microconidia in 1 ml. Dermatophyte cultures are contained in the vaccine alive and / or viable. The vaccine gives immune protection to vertebrates of the mammalian class: canine family, feline family, rabbits, ruminant family, horses, pigs, humans. The vaccine production method provides for the separate selection of immunological material of several dermatophyte cultures, which in combination can give immune protection to animals against dermatomycosis, combining selected dermatophyte cultures, inactivating the selected dermatophyte cultures by heat treatment at such a temperature and for such a time so as not to destroy the essential antigenic properties of the cultures dermatophytes. In particular, dermatophyte cultures are cooked at a temperature of 40-60 ° C. for 30-1440 minutes, preferably for about 60 minutes. A method for the prevention or treatment of dermatomycosis of vertebrates includes the use of an effective dose regimen of the vaccine, in particular intramuscular administration.

Known associated vaccines are used in an immunologically effective dose, preferably twice by intramuscular injection. Despite the fact that the known associated vaccines are quite effective against major skin diseases, they are not able to give immunity from other diseases, for example favus, because Recently, the number of dermatomycoses caused by other pathogens has increased: Achorion schoenleinii (also known as Trichophyton schoenleinii), Alternaria species. Moreover, the main pathogen dermatophytes are different for different climatic and geographical habitats or the geographical area where animals are kept, and the spectrum of dermatomycosis pathogens is expanding and more than 400 species of fungi causing diseases in humans and animals are currently known.

The technological process for preparing laboratory strains used in the above-mentioned known associated vaccines is relatively complicated and time-consuming, so only the technological stage of growing a laboratory strain requires a special nutrient medium, a special favorable thermal regime and takes 20-25 days.

The technical problem to which the group of inventions is directed: expanding the functionality and increasing the efficiency of the use of live vaccines containing dermatophyte cultures, reducing their cost and simplifying the process of obtaining such vaccines.

A method for the treatment and prevention of dermatomycosis of vertebrates is carried out by intramuscular administration of an immunologically effective amount of the vaccine in the form of a suspension of inactivated live and / or viable antigenic material from cultures of several different species in a physiologically acceptable carrier that is not pathogenic for the vaccinated vertebrate. New is that dermatophyte cultures are used as antigenic material, which are squeezed out of previously separated external appendages of the skin of vertebrates along with the liquid contained in the said external appendages of the skin, followed by inactivation of the resulting suspension.

As external appendages of the skin, you can use wool and / or hair (also claws, nails, feathers, scales) of a vertebrate animal: a) of the same and / or another class or subclass or order or family or subfamily or genus or species of vertebrate animals than vaccinated vertebrate; b) is better than living in the same geographical habitat or geographical area of detention as the vaccinated vertebrate, because the composition of dermatophytes in various animals from one geographic area practically coincides; c) separated from the skin of healthy vertebrates and / or vertebrates infected with dermatomycosis, and a healthy and sick animal from the same geographical area carries about the same composition of dermatophytes, and the sick animal simply contains more of those dermatophytes that caused the disease.

It is better when the antigenic material contains at least three dermatophyte cultures from the group: Achorion schoenleinii, Altemaria species, Candida species, Epidermophyton species, Microsporum species, Trichophyton species, which are the causative agents of major skin diseases in almost all geographical regions.

It is better when the vaccine is administered together with adjuvant in an effective amount.

It is better when the vaccine is administered twice with an interval of 10-14 days, and it is better to re-introduce the vaccine into another muscle of the vaccinated vertebrate.

It is better to introduce a vaccine containing antigenic material from dermatophyte cultures in an amount of 10 ² -10 ¹⁰ microconidia in 1 ml. In general, an effective amount of a vaccine is selected depending on the etiology of the skin disease, age, sex, condition of the animal, the presence of other diseases and the purpose of vaccination (treatment or prevention). Such a quantity for vertebrates is usually 0.25-2.00 ml.

A vaccine is also proposed for the treatment and prevention of dermatomycosis of vertebrates, containing an immunologically effective amount of live and or viable antigenic material from dermatophyte cultures in the form of a combination of several different types of dermatophytes (not a pathogenic combination), as well as an inactivator and a physiologically acceptable carrier. What is new is that, as dermatophyte cultures, the vaccine contains dermatophyte cultures squeezed out of its external appendages separated from the skin of vertebrate animals together with the liquid contained in the said external appendages of the skin, for example, in hair and / or hair (as well as claws, nails, feathers , scales).

It is better when the composition of the antigenic material includes at least three cultures of widespread pathogen dermatophytes from the group: Achorion schoenleinii, Alternaria species, Candida species, Epidermophyton species, Microsporum species, Trichophyton species.

It is better when the culture of dermatophytes is inactivated by pasteurization without destroying the essential antigenic properties of the cultures of dermatophytes, in particular at a temperature of 50-82 ° C for 30-240 minutes, preferably twice in 30-120 minutes with an interval of 12-48 hours.

It is better when the antigenic material of dermatophyte cultures is contained in an amount of 10 ² -10 ¹⁰ microconidia in 1 ml.

Formatin up to 1.5 wt.% Can be used as an inactivator. It is possible to use thimersal, 2-propiolactone in effective amounts.

At least part of a physiologically acceptable carrier may be a liquid squeezed out of the external appendages of vertebrates and / or physiological saline.

The vaccine is widely universal and can be intended for the treatment and prevention of dermatomycosis in birds and mammals. It is assumed that the vaccine can be used for fish, humans.

A method for producing a vaccine for the treatment and prevention of dermatomycosis of vertebrate animals is proposed, including the selection of antigenic material of several cultures of dermatophytes, which in combination are capable of conferring immune protection to vertebrates against dermatomycosis and are not pathogenic, and inactivation of selected cultures of dermatophytes so as not to destroy the essential antigenic properties of the selected cultures dermatophytes. What is new is that dermatophyte cultures are selected by extrusion from previously separated external appendages of the skin of vertebrate animals together with the liquid contained in the said external appendages of the skin, followed by inactivation of the resulting suspension.

As external appendages of the skin, it is better to use wool and / or hair (you can also claws, nails, feathers, scales), separated from the skin of vertebrates of the same and / or another class, or subclass, or detachment, or family, or subfamily or a genus or species of vertebrate animal than the vertebrate for which the vaccine is intended, and / or living in the same geographical habitat or geographical area as the vertebrate for which the vaccine is intended.

Wool and / or hair separated from the skin of healthy vertebrates and / or vertebrates infected with dermatomycosis are used as external appendages of the skin.

Pre-separated external skin appendages should be antiseptically treated, followed by washing with a physiologically acceptable liquid until the antiseptic residues are completely removed, for example, saline. After washing, the treated external skin appendages should be stored until extrusion in a physiologically acceptable liquid. Antiseptic treatment can be carried out with an aqueous solution of alkali in an effective amount, it is better to use a 2% aqueous solution of sodium hydroxide with a ratio of separated external skin appendages to an aqueous solution of 1 wt.h. : 5-9 parts by weight, carrying out antiseptic treatment, keeping the separated external skin appendages in the specified aqueous solution for 3-15 minutes at a temperature of 17-25 ° C.

Before extrusion, the separated external skin appendages are best crushed, in particular to a particle size of 2-4 mm.

For inactivation, you can use the heat treatment of the resulting suspension by pasteurization, in particular at a temperature of 50-82 ° C for 30-240 minutes, preferably twice but 30-120 minutes with an interval of 12-48 hours.

For inactivation, an inactivator can also be added to the resulting suspension in an effective amount, for example, formalin up to 1.5 wt.%.

To remove insoluble small particles of hair rods, etc. suspension inactivation is better to filter.

The proposed associated live vaccine obtained by the claimed method contains inactivated field strains of dermatophytes, in contrast to the known associated vaccines containing laboratory strains, which in itself determines the relative simplicity of the technological process for its preparation, which ultimately determines the lower cost of the vaccine. The higher efficiency of the proposed vaccine is determined by the presence of a more broadly selected set of antigens from dermatophyte cultures.

The above inventions of the group, as shown above, are connected by a single inventive concept and, in particular, any developing and / or clarifying set of essential features of one of the inventions of the group can be used to obtain or implement another invention of the group or is intended to use another invention of the group.

The invention is illustrated by examples of treatment in a veterinary clinic of domestic animals living in the Primorsky Territory.

In the examples described below, the Polyderm vaccine was prepared as follows.

Pre-harvested, shearing wool from several dogs and cats of different breeds, age, healthy and with various etiologies of skin fungal diseases contained in the Primorsky Territory. The collected wool in an amount of 100 g at normal humidity was previously subjected to antiseptic treatment with a 2% aqueous solution of sodium hydroxide in an amount of 700 ml for 5 minutes at normal temperature (18-22 ° C), and then at the same temperature it was washed 4 times with physiological solution. Wool treated in this way was stored in physiological saline, after which it was removed from it, the saline was allowed to drain and crushed, cutting to a particle size of 2-3 mm. The crushed particles were placed in a screw press, where liquid was squeezed out of them with a force sufficient to squeeze out most of the liquid contained in the wool. The resulting suspension, in particular containing saline, fragments of mycelium, spores and other fragments of fungi, was filtered through a double Davy mesh. The obtained filtrate was fixed with phenol to 0.5 wt.%, Poured into glass bottles with a capacity of 10-20 ml, which were hermetically sealed with rubber stoppers with aluminum caps, and pasteurized twice at 72-80 ° C for 1 hour with an interval of 24 hours, monitoring so that the suspension between cycles cools to a temperature not lower than normal (18-22 ° C). The finished vaccine was tested laboratory for sterility and the absence of pathogenicity. Laboratory tests showed the presence, both in the collected wool and in the finished vaccine, of more than 36 field strains of fungi, in particular: Achorion schoenleinii (also known as Trichophyton schoenleinii); Alternaria species, Candida species: Epidermophyton species, including Epidermophyton floccusum; Microsporum species, including Microsporum canis; Trichophyton species, including Trichophyton equinum; Trichophyton ajelloi. The vaccine concentration was about 10 ⁸ microconidia in 1 ml. To obtain the desired concentration, the vaccine can be diluted with saline. The vaccine was stored before use for up to 2 months in a dark place at a temperature of 0-4 ° C.

Example 1. Dog, Pekingese breed. Age - 4 years old, male. The diagnosis is sycosis (hair loss throughout the body, itching, the formation of asbestos-like crusts and abscesses with an unpleasant odor).

Prior to vaccination with the Polyderm vaccine, treatment with standard vaccines and an Ivomek injection were carried out for 3 years. There were short-term and fuzzy improvements. During the stay of the owners in Israel, they treated the dogs there, also almost to no avail.

Two doses of the Polyderm vaccine, 1 ml each, with 0.25 ml adjuvant (vitamin A, D ₃ , E concentrate) were injected intramuscularly into the femur muscles twice in two different paws with an interval of 14 days. After the first injection, itching disappeared, crusts formed on open lesions, and the cross section of the coat decreased. After the second injection, recovery occurred after 24 days. After this treatment with this animal to the veterinarian was not noted.

Example 2. Cat, breed Persian, age 2 years. The diagnosis is scab (yellow crusts on body parts, itching, peeling, partial hair loss).

Prior to vaccination with the Polyderm vaccine, standard vaccines were treated twice. There were short-term and fuzzy improvements.

Two doses of 0.8 ml Polyderm vaccine with 0.25 ml adjuvant (vitamin A, D ₃ , E concentrate) were injected intramuscularly into the femur muscles 2 times in two different paws with an interval of 10 days. After the first injection, itching disappeared, part of the yellow crusts disappeared, and the cross section of the coat decreased. After the second injection, recovery finally came in 20 days. A subsequent examination after one year showed no signs of scab and other dermatological diseases in the animal.

The described examples far from exhaust all the options for using the claimed invention. When administered intramuscularly, Polyderm live vaccine is areactogenic, non-pathogenic and creates immunity in many species of susceptible animals against almost all the main causative agents of dermatophytosis in animals, regardless of their habitat or geographical area of detention, because includes an almost complete set of exoantigens and endoantigens of dermatophyte cultures. In particular, the Polyderm vaccine was successfully used by the applicant for the treatment and prevention of dermatomycoses such as lichen, baldness, irreversible itching, persistent long-term unpleasant odor, in various animals: rabbits, guinea pigs, rats, mice, minks, cows, goats, marine seals, belugas, parrots, poultry. The vaccine was administered twice intramuscularly in doses of 0.25-2.00 ml with an interval of 10-14 days. Recovery occurred after 18-24 days. The technological process for obtaining the Polyderm vaccine is labor-intensive and takes a relatively short time, which in turn determines the low cost of the vaccine.

By analogy with the known vaccine described above [WO 01/15725, 2001] it is contemplated that the inventive vaccine prepared from human hair can be effectively used for the prevention and treatment of various dermatological diseases, such as dermatomycosis of the scalp, including favus (scab) , inguinal dermatomycosis, epidermophytosis of the foot, etc.

Claims (39)

1. A method for the treatment and prevention of dermatomycosis of vertebrates by intramuscular administration of an immunologically effective amount of a vaccine in the form of a suspension of inactivated live and / or viable antigenic material from cultures of several different species in a physiologically acceptable carrier that is not pathogenic for the vaccinated vertebrate, characterized in that it is antigenic The material used is a culture of dermatophytes, which are squeezed out of previously separated external appendages of the skin of the spinal farm animals together with the liquid contained in said external skin appendages, followed by inactivation of the resulting suspension. 2. The method according to claim 1, characterized in that as external appendages of the skin using wool and / or hair of a vertebrate animal of the same and / or another class, or subclass, or detachment, or family, or subfamily, or genus, or species vertebrates than vaccinated vertebrates. 3. The method according to claim 1, characterized in that the external appendages of the skin use wool and / or hair of vertebrates living in the same geographical habitat or geographical area of detention as the vaccinated vertebrate. 4. The method according to claim 1, characterized in that as external appendages of the skin using wool and / or hair, separated from the skin of healthy vertebrates and / or vertebrates infected with dermatomycosis. 5. The method according to claim 1, characterized in that the antigenic material contains at least three dermatophyte cultures from the group: Achorion schoenleinii, Alternaria species, Candida species, Epidermophyton species, Microsporum species, Trichophyton species. 6. The method according to claim 1, characterized in that the vaccine is administered together with the adjuvant in an effective amount. 7. The method according to claim 1, characterized in that the vaccine is administered twice with an interval of 10-14 days. 8. The method according to claim 7, characterized in that the vaccine is reintroduced into another muscle of the vaccinated vertebrate. 9. The method according to claim 1, characterized in that a vaccine is introduced containing antigenic material from dermatophyte cultures in an amount of 10 ² -10 ¹⁰ microconidia in 1 ml. 10. The method according to claim 9, characterized in that 0.25-2.00 ml of the vaccine is administered per administration. 11. A vaccine for the treatment and prevention of dermatomycosis of vertebrates, containing an immunologically effective amount of live and / or viable antigenic material from dermatophyte cultures in the form of a combination of several different types of dermatophytes, as well as an inactivator and physiologically acceptable carrier, characterized in that as dermatophyte cultures the vaccine contains dermatophyte cultures squeezed out of its external appendages separated from the skin of vertebrate animals along with the liquid contained in the aforementioned External Expansion skin appendages. 12. The vaccine according to claim 11, characterized in that it contains inactivated cultures of dermatophytes extruded from the hair and / or hair of vertebrates. 13. The vaccine according to claim 11, characterized in that it contains at least three dermatophyte cultures from the group: Achorion schoenleinii, Alternaria species, Candida species, Epidermophyton species, Microsporum species, Trichophyton species. 14. The vaccine according to claim 11, characterized in that it contains cultures of dermatophytes inactivated by pasteurization without destroying the essential antigenic properties of dermatophyte cultures. 15. The vaccine according to 14, characterized in that the pasteurization is carried out at a temperature of 50-82 ° C for 30-240 minutes 16. The vaccine according to clause 15, wherein the pasteurization is carried out twice for 30-120 minutes with an interval of 12-48 hours 17. The vaccine according to claim 11, characterized in that it contains antigenic material of dermatophyte cultures in an amount of 10 ² -10 ¹⁰ microconidia in 1 ml. 18. The vaccine according to claim 11, characterized in that as an inactivator contains formalin up to 1.5 wt.%. 19. The vaccine according to claim 11, characterized in that at least part of a physiologically acceptable carrier is a liquid squeezed out of the external appendages of vertebrates. 20. The vaccine according to claim 11, characterized in that at least part of a physiologically acceptable carrier is a physiological fluid. 21. The vaccine according to claim 11, characterized in that it is intended for the treatment and prevention of bird dermatomycosis. 22. The vaccine according to claim 11, characterized in that it is intended for the treatment and prevention of mammalian dermatomycosis. 23. A method of obtaining a vaccine for the treatment and prevention of dermatomycosis of vertebrates, including the selection of antigenic material of several cultures of dermatophytes, which in combination are able to give immune protection to vertebrates from dermatomycosis and are not pathogenic, inactivation of selected cultures of dermatophytes so as not to destroy the essential antigenic properties of the selected cultures dermatophytes, characterized in that cultures of dermatophytes are selected by extrusion from previously separated external appendages of the skin nocturnal animals with the liquid contained in said external skin appendages, followed by inactivation of the resulting suspension. 24. The method according to item 23, wherein the external appendages of the skin use wool and / or hair, separated from the skin of vertebrates of the same and / or another class, or subclass, or detachment, or family, or subfamily , or the genus or species of vertebrate animals than the vertebrate for which the vaccine is intended. 25. The method according to item 23, wherein the external appendages of the skin use wool and / or hair, separated from the skin of vertebrates living in the same geographical habitat or geographical area of detention as the vertebrate for which it is intended vaccine. 26. The method according to item 23, wherein the external appendages of the skin use wool and / or hair, separated from the skin of healthy vertebrates and / or vertebrates infected with dermatomycosis. 27. The method according to item 23, wherein the previously separated external skin appendages are subjected to antiseptic treatment, followed by washing with a physiologically acceptable liquid until the antiseptic residues are completely removed. 28. The method according to item 27, wherein the physiological solution is physiological saline. 29. The method according to item 27, wherein after washing the treated external skin appendages are stored until extrusion in a physiologically acceptable liquid. 30. The method according to item 27, wherein the antiseptic treatment is carried out with an aqueous solution of alkali in an effective amount. 31. The method according to p. 30, characterized in that as an aqueous solution of alkali using a 2% aqueous solution of sodium hydroxide with a ratio of separated external skin appendages to an aqueous solution of 1 parts by weight: 5-9 parts by weight, and antiseptic treatment with such a solution is carried out, keeping the separated external skin appendages in the specified aqueous solution for 3-15 minutes at a temperature of 17-25 ° C. 32. The method according to item 23, wherein the extruded external skin appendages are crushed before extrusion. 33. The method according to p, characterized in that the grinding is carried out to a particle size of 2-4 mm 34. The method according to item 23, wherein the inactivation using heat treatment of the resulting suspension by pasteurization. 35. The method according to clause 34, wherein the pasteurization of the suspension is carried out at a temperature of 50-82 ° C for 30-240 minutes 36. The method according to clause 35, wherein the pasteurization of the suspension is carried out twice for 30-120 minutes with an interval of 12-48 hours 37. The method according to item 23, wherein the inactivator is introduced into the resulting suspension in an effective amount for inactivation. 38. The method according to clause 37, characterized in that formalin up to 1.5 wt.% Is used as an inactivator. 39. The method according to item 23, wherein the suspension is filtered before inactivation.