RU2367454C1 - Intime hygiene product "femivit" - Google Patents

Abstract

FIELD: medicine.

SUBSTANCE: feminine hygiene product contains metabolites of probiotic cells Bacillus subtilis strain 3/28 (All Russian Collection of Industrial Microorganisms B 3679), metabolites of probiotic cells Lactobacillus plantarum strain 8P-A3, sage essence, lavender essence, propolis, sodium benzoate and water in specified ratio.

EFFECT: higher vaginal cleanness and recovery of normal flora, discomfort elimination, improvement of vaginal hygienics ensured by inhibition of pathogenic and opportunistic vaginal flora providing antiinflammatory and immunocorrelating action.

4 ex, 1 tbl

Description

The invention relates to medicine, in particular to dosage forms of bacterial preparations.

Known probiotic preparation for the treatment of bacterial vaginosis, containing as an active principle a microbial mass of living bacteria, namely lactobacilli and one or more genera of eubiotic bacteria selected from the group: bifidobacteria, streptococci and lactococci, in the amount of 10 ⁵ -10 ⁹ microbial cells per dose, sorbent in the ratio of it to the microbial mass of bacteria (9-1) :( 9-1), a protective environment, a biologically active additive in an amount of 0.05-3.0 wt.% relative to the mass of the preparation and a fat base containing no more than 5 wt.% water and having a pH of 4.5-7.0 (RF application No. 2002134006, MKI A61K 35/74, 2004).

The disadvantages of the known drug are: the presence in the composition of viable microorganisms that carry a potential threat of the development of an infectious process; the presence of a fatty base, which causes the lack of good solubility of the components of the drug and, therefore, the inability to fully pass the biologically active substances that produce the bacteria that make up the drug through the mucous or cell wall in the case of intracellular sexually transmitted infection.

Known vaginal composition comprising viable microorganisms of lactobacilli and / or bifidobacteria, preferably Lactobacillus bifidus, non-viable cultures of saccharomycetes, preferably Saccharomyces cerevisiae, saccharide (s), vitamin A (retinol) and zinc (RF application No. 200413612058, MKI A 2006, 2006610058, MKI g.). The use of the vaginal composition for the care of the vaginal mucosa and for the prevention of its defeat by bacteria, fungi and / or viruses is proposed.

However, the known composition has a number of significant disadvantages. Firstly, a high concentration of viable microorganisms can lead to the development of an infectious process, especially against the background of a reduced immune status. Secondly, the lactic acid bacteria that make up the composition can act as a recipient of genes from pathogenic microorganisms also contained in the bacterial microflora of the vagina, thereby assuming their virulent properties.

Thus, the authors were faced with the task of developing a tool that, along with high effectiveness, lacks undesirable side effects.

The problem is solved by applying the proposed means of intimate hygiene "Femivit", characterized in that it contains metabolites of probiotic cells of hay bacillus, metabolites of probiotic cells of sour milk bacteria, essential oil of sage, essential oil of lavender, propolis, sodium benzoate and water in the following ratios of components, wt. .%:

metabolites of probiotic hay bacillus cells 3 ÷ 5; metabolites of probiotic cells sour milk bacteria 3 ÷ 5; sage essential oil 0.5 ÷ 1; lavender essential oil 0.03 ÷ 0.05; propolis 3 ÷ 5; sodium benzoate 0.1 ÷ 1; distilled water - the rest.

Moreover, as metabolites of probiotic hay bacillus cells, the product contains metabolites produced by Bacillus subtilis strain 3/28 (VKPM B-3679)

And as metabolites of probiotic sour-milk bacteria, the product contains metabolites produced by Lactobacillus plantarum strain 8P-A3.

Currently, the composition of the means of intimate hygiene for women is not known from the patent and scientific literature containing the totality of the proposed components within the claimed limits of their content.

Probiotics - drugs or biologically active additives that contain more often bifidobacteria or lactobacilli. Probiotics, unlike antibiotics, do not have a detrimental effect on the normal microflora, so their use for the treatment of various infectious diseases has a definite advantage over antimicrobials. An important feature of probiotics is their ability to increase the anti-infective resistance of the body, to provide anti-allergenic effect.

Metabolites (proteins, amino acids, enzymes, antibiotic substances) produced by probiotic bacteria of the species Bacillus subtilis (hay bacillus) are characterized by polyenzymatic properties. Bacillus cells include a set of enzymes of various classes: oxidoreductases, transferases, hydrolases, lyases. The system of hydrolases, enzymes that catalyze the hydrolytic cleavage of molecules, is especially well developed in hay bacillus.

The main function of proteolytic enzymes is the breakdown of proteins contained in the environment, and their transformation into a form that can easily penetrate into the cell.

Proteolytic enzymes are used in medical practice to treat inflammatory processes, to cleanse purulent and necrotic wounds, burns, frostbite, to dissolve blood clots and to treat certain oncological diseases.

Lytic enzymes are a complex complex consisting of enzymes with different substrate specificity. They are used as antimicrobial agents.

Bacteriolytic enzymes are highly active against the cell walls of microorganisms of such species as: P.aeruginosa, E.coli, S.typhimurium, S.aureus, St.pyogenes, etc.

The essential amino acids produced by hay bacillus (lysine, phenylalanine, cystine, tryptophan) are an important component and an integral part in the process of regeneration of dystrophically altered tissues.

Antibiotic substances produced by bacteria of the species Bacillus subtilis have high bacteriostatic and bactericidal properties against numerous representatives of the normal microflora of the vagina.

The metabolites of probiotic lactic acid bacteria, in particular the species Lactobacillus, are bactericidal substances, including bacteriocins, organic acids and hydrogen peroxide.

Bacteriocins are compounds produced by bacteria that promote the proliferation of biologically active proteins that have bactericidal activity.

Organic acids are some of the end products of lactic acid metabolism, the most famous examples of this group are lactic and acetic acids. The effectiveness of organic acids largely depends on the pH of the medium. At low pH, these acids are in an undissociated form, which is bactericidal.

Hydrogen peroxide (a solution of hydrogen peroxide) quickly decomposes under the influence of light, when heated, in contact with alkali, oxidizing or reducing substances, releases atomic oxygen. The application finds a 3% solution of hydrogen peroxide as a disinfectant and deodorizing agent for washing and rinsing with stomatitis, tonsillitis, gynecological diseases.

The healing properties of propolis have been known to people since ancient times. In medicine, propolis is used primarily in surgery, dermatology, otorhinolaryngology, pediatrics and dentistry. Propolis is successfully used to treat non-healing trophic ulcers, erosions and wounds of various etiologies, burn disease, etc. Given the antimicrobial, antipruritic, epithelizing properties of propolis, propolis-containing drugs have been widely used in dermatology, venereology and gynecology. There is rich experience in the use of propolis preparations in dermatology in case of trichophytosis, epidermophytosis and foot hyperkeratosis, verocosis-infiltrative forms of skin tuberculosis, nest and total hair loss, pyoderma, furunculosis, burns, eczema. A significant amount of information is available in the specialized literature on the use of propolis drugs in diseases of the digestive tract. In the treatment of stomatitis, gingivitis, glossitis, glossalgia, periodontal disease, moniliasis, candidomycosis. There is evidence of a positive experience with propolisotherapy for respiratory diseases of both infectious and non-infectious etiology (pneumonia, inflammatory diseases of the upper respiratory tract, bronchial asthma, tracheitis, pharyngitis, etc.). The healing properties of propolis and its pharmacological effect are explained by the presence in its composition of a large number of biologically active substances, trace elements, vitamins, enzymes, fructose, glucose, phytoncides.

Sage is a plant in the family of Lamiaceae, using leaves containing essential oil, which includes cineole, borneol, camphor, tannins, triterpene acids, alcohols. The highest content of essential oil in the fruiting phase. Sage is used as an antiseptic, as well as anti-inflammatory, antispasmodic, hemostatic, expectorant, astringent, wound healing. It has been established that sage essential oil actively suppresses the development of dysenteric bacteria and E. coli bacteria, moderately inhibits the development of Staphylococcus aureus, as well as some other pathogenic and conditionally pathogenic microorganisms. Sage has an astringent effect primarily in the oral cavity (with stomatitis and gingivitis), it is used to rinse with inflammation of the upper respiratory tract. Sage is a good remedy for asthma, cough, sore throat. It is widely used in the form of inhalations.

Lavender belongs to the family Labiaceae. It is used as a disinfectant, anti-inflammatory and sedative. Lavender essential oil is produced from the flowers of a plant by distillation. Lavender oil has a relaxing effect and gives a mild sedative effect. Lavender helps to overcome the decline in physical strength and overcome a sense of anxiety and anxiety. She soothes the nerves. Massage with lavender oil relaxes and serves as an excellent remedy for insomnia. Due to its mild analgesic effect, lavender oil is prescribed for the treatment of headaches and muscle pains. It can be applied to the skin in a concentrated form.

Studies conducted by the authors showed good compatibility of all active components of the proposed tool and allowed us to identify the limits of their quantitative content, providing the manifestation of the maximum therapeutic effect. At the same time, the authors experimentally managed to obtain a quantitative ratio of the components, in which not only the individual healing properties of each component are preserved, but their combination ensures the combined effect of the properties of the active components, while no adverse side effects are observed. So, when the content of metabolites of probiotic bacterial cells of hay bacillus (proteins, amino acids, enzymes, vitamins, antibiotic substances) is less than 3 wt.%; metabolites of sour milk bacteria less than 3 wt.%; carbohydrates, enzymes and trace elements propolis less than 3 wt.%; sage essential oil less than 0.5 wt.%, lavender essential oil less than 0.03 wt.%; sodium benzoate less than 0.1 wt.% there is a slowdown in the manifestation of anti-inflammatory, antitoxic and immunocorrection effect due to a decrease in the intensity of suppression of pathogenic and conditionally pathogenic vaginal microflora. In addition, due to the low content of sodium benzoate as a preservative, the shelf life of the drug is sharply reduced. An increase in the content of metabolites of bacterial cells of hay bacillus (proteins, amino acids, enzymes, antibiotic substances) more than 5 wt.%, Metabolites of sour milk bacteria more than 5 wt.%; carbohydrates, enzymes and trace elements propolis more than 5 wt.%; sage essential oil more than 1 wt.%, lavender essential oil more than 0.05 wt.%; sodium benzoate more than 1 wt.% is impractical, since the viability of the natural microflora of the vagina is violated due to a significant change in the normal functioning of the mucous membrane and other tissues of the vagina.

The proposed tool can be obtained as follows. Cultures of probiotic cells of hay bacillus strain Bacillus subtilis 3/28 (VKPM B 3679) and sour-milk bacteria Lactobacillus plantarum strain 8P-A3 are grown in a deep way in liquid nutrient media. For the cultivation of hay bacillus, a medium based on hydrochloric acid hydrolysates of casein or fish bone meal is used. Cultivation is carried out at a temperature of (37 ± 1) ° C. Monitoring the development of cultures is carried out visually, by microscopy of smears stained according to Ziehl-Nielsen. After 16-18 hours of cultivation, which corresponds to the end of the exponential growth phase, the biosynthesis process is stopped, the culture fluid is cooled to a temperature of (12 ± 3) ° С, and then transferred to separation.

The cultivation of lactobacilli is carried out in liquid cabbage or liquid nutrient medium MRS-2 under static conditions at a temperature of (37 ± 1) ° C for 10-12 hours. The sowing dose of L. plantarum 8P-A3 should be at least

1.2 · 10 ⁷ cells · cm ^-3 . The control is carried out by microcopying smears. The concentration of lactobacilli in the culture fluid reaches 1-2 · 10 ⁹ cells · cm ^-3 . After cooling the culture fluid to a temperature of (12 ± 3) ° C, it is also transferred to separation.

The obtained concentrated microbial masses of vegetative cells of Bacillus subtilis and Lactobacillus plantarum are subjected to destruction on an ultrasonic disintegrator.

The finished composition is obtained by mixing in the ratio 1: 1 of the starting components: biologically active substances (metabolites) of probiotic bacterial cells of hay bacillus and sour-milk bacteria obtained after separation of the culture fluid and ultrasonic disintegration of concentrated microbial mass. Then add sodium benzoate and distilled water. Everything is thoroughly mixed at a temperature of (12 ± 3) ° C for 10 min in a rotary mixer. Then, the essential oils of sage and lavender, propolis are successively added, after which distilled water is again added to the required volume. The resulting solution was again thoroughly mixed for 15 minutes. A light gray (light yellow) color liquid is obtained with a pH value of 6.5-7.0; in the following ratio of components, wt.%: metabolites of probiotic bacterial cells of hay bacillus (proteins, amino acids, enzymes, antibiotic substances) 3-5; metabolites of sour-milk bacteria 3-5; carbohydrates, enzymes and trace elements propolis 3-5; sage essential oil 0.5-1, lavender essential oil 0.03-0.05; distilled water - the rest. Certification of the obtained product is carried out by chemical-analytical method.

The proposed technical solution is illustrated by the following examples.

Example 1. Prepare a mixture of powder of sodium benzoate 1 g (0.1 wt.%) And suspension containing metabolites of probiotic bacterial cells of hay bacillus 30 g (3 wt.%) And metabolites of sour-milk bacteria 30 g (3 wt.%) . The mixture is thoroughly mixed at a temperature of (12 ± 3) ° C for 10 min in a rotary mixer with the addition of distilled water. Then sage essential oils of 5 g (0.5 wt.%), Lavender 0.3 g (0.03 wt.%) And 30 g (3 wt.%) Propolis are successively added, after which distilled water is added up to 1000 g. The resulting solution was again thoroughly mixed for 15 minutes. A light yellow liquid is obtained with a pH value of 6.5-7.0; in the following ratio of components, wt.%: metabolites of probiotic bacterial cells of hay bacillus (proteins, amino acids, enzymes, antibiotic substances) 3; metabolites of sour-milk bacteria 3; sodium benzoate 0.1; propolis 3; essential oils: sage 0.5; lavender 0.03; distilled water 90.37.

Example 2. Prepare a mixture of powder of sodium benzoate 1 g (0.1 wt.%) And a suspension containing metabolites of probiotic bacterial cells of hay bacillus 40 g (4 wt.%) And metabolites of sour-milk bacteria 40 g (4 wt.%) . The mixture is thoroughly mixed at a temperature of (12 ± 3) ° C for 10 min in a rotary mixer with the addition of distilled water. Then sage essential oils of 7.5 g (0.75 wt.%), Lavender 0.4 g (0.04 wt.%) And 40 g (4 wt.%) Propolis are added sequentially, after which distilled water is added up to 1000 d. The resulting solution was again thoroughly mixed for 15 minutes A light yellow liquid is obtained with a pH value of 6.5-7.0; in the following ratio of components, wt.%: metabolites of probiotic bacterial cells of hay bacillus (proteins, amino acids, enzymes, antibiotic substances) 4; metabolites of sour-milk bacteria 4; sodium benzoate 0.1; propolis 4; essential oils: sage 0.75; lavender 0.04; distilled water 87.11.

Example 3. Prepare a mixture of powder of sodium benzoate 10 g (1.0 wt.%), Followed by the addition of essential oils of sage 10 g (1 wt.%), Lavender 0.5 g (0.05 wt.%) And 50 g ( 5 wt.%) Propolis and distilled water. The mixture is thoroughly mixed for 15 minutes in a rotary mixer. Distilled water is then added. A suspension is prepared containing metabolites of probiotic bacterial cells of hay bacillus 50 g (5 wt.%) And metabolites of sour-milk bacteria 5 g (50 wt.%). The suspension is added to the resulting solution and still thoroughly mixed at a temperature of (12 ± 3) ° C for 10 minutes, after which distilled water is added up to 1000 g. A light yellow liquid is obtained with a pH value of 6.5-7 0; in the following ratio of components, wt.%; metabolites of probiotic bacterial cells of hay bacillus (proteins, amino acids, enzymes, antibiotic substances) 5; metabolites of sour-milk bacteria 5; sodium benzoate 1; propolis 5; essential oils: sage 1; lavender 0.05; distilled water 82.95.

Preclinical studies of feminine intimate hygiene products for women

The purpose of preclinical studies was to conduct experimental clinical and laboratory studies to assess the safety indicators of the proposed tool.

We studied an intimate hygiene product for women, obtained in the form of a light yellow liquid with a pH value of 6.5-7.0; in the following ratio of components, wt.%: metabolites of probiotic bacterial cells of hay bacillus (proteins, amino acids, enzymes, antibiotic substances) 4; metabolites of sour-milk bacteria 4; sodium benzoate 0.1; propolis 5; essential oils: sage 1; lavender 0.05; distilled water - up to 1000 (corresponds to example 2, see above).

The studies were conducted at the departments of pharmacology and histology, with the participation of the morphological department of the Central Research Institute of Ural State Medical Academy.

The experimental animals used in the studies were kept in a conventional vivarium on a generally accepted diet.

Studies were performed on the following types of laboratory animals: white mice, white Vistar rats, guinea pigs and rabbits. The toxicity study was carried out in accordance with the requirements set out in the Methodological materials for the experimental and clinical study of new drugs (Official Edition, M., 1986) and set out in the Guide to the experimental (preclinical) study of new pharmacological substances (M., 2006).

As a result of studies on the detection of acute toxicity, it was found that during intragastric and cutaneous application of the developed product, the state of experimental animals did not differ from that of intact animals: behavior, appetite, physiological functions, functions of the cardiovascular and respiratory systems, weight gain were identical in the control and intact animals. Total protein, blood sugar, residual nitrogen remained within acceptable limits. No destructive, necrobiotic and dystrophic changes in the liver, kidneys, adrenal glands, heart, spleen, lungs, thyroid gland, stomach and skin were detected in any experimental animal during histological examination of internal organs and tissues. The weights of the internal organs of the experimental animals did not differ from those of intact animals. There were no cases of complications and death.

In the process of studying chronic toxicity, which lasted for 56 days, examining the tissues and organs of animals of different groups who received the drug in various doses once daily by skin or through a probe into the stomach, showed the absence of pathological changes, which confirms the non-toxicity of the drug. The results of an experimental study suggest that the proposed tool is non-toxic, belongs to the "low-hazard substances" - 4th hazard class according to GOST (12.097.76).

During pathomorphological studies, the skin, liver, kidneys, adrenal and thyroid glands, heart, lungs, and stomach of experimental animals were taken for various observation periods after oral administration of this drug. The results of pathomorphological studies of organs and tissues of experimental animals allow us to conclude that with the introduction of the studied means pathological changes in the studied histological samples were not detected.

The study of the allergic effect was carried out by the method of cutaneous applications, conjunctival tests, the reaction of specific lysis of leukocytes, and the provocation of anaphylactic shock. The experiment was performed on white Vistar rats weighing 196.4 ± 6.9 g and guinea pigs weighing 365 ± 8.4 g (conjunctival test and anaphylactic shock). The results of studies of the proposed drug in a therapeutic dose and a dose that is 10 times higher than the therapeutic dose, did not reveal an allergenic effect. The proposed tool is not a potential allergen.

The blood test data in accordance with the micronuclear test when exposed to experimental animals intraperitoneally and with a cutaneous application of a 50% solution of the drug indicate that when applied topically, it does not have a mutagenic effect. Given the close relationship of mutagenesis and carcinogenesis, the composition of the drug and the method of its use, a carcinogenic effect seems unlikely.

Based on the results of the study of histological material, we can conclude that the proposed tool does not cause a negative effect at the level of its use in experimental conditions in laboratory animals: with short-term and long-term contact with the tool, the mucous sclera of the eyes and oral cavity remain unchanged. Long-term exposure (12-14 days, one application per day) of the product to the genitals of female white rats and guinea pigs and rabbits also does not cause negative manifestations.

Thus, the results of experimental studies of the proposed tool give reason to believe that it is non-toxic, quickly excreted from the body, does not have cumulative and local irritating effects (when studying the skin-resorptive effect, no intoxication effects were observed in any animal), it does not have an allergenic effect, as well as mutagenic activity, and therefore carcinogenic properties. Morphological changes in the genitals in white rats, guinea pigs and rabbits under the influence of the drug have not been established.

The method of application of intimate hygiene products for women of the proposed composition is as follows. Before using the product, it is recommended to shake the contents of the bottle thoroughly. Take a horizontal position, insert the tip and 3-5 times pressing the bottle head to evenly distribute the hygiene product in the vaginal cavity. Apply at least 3-4 times a day.

Evaluation of the effectiveness of local use of intimate hygiene products in patients with bacterial vaginosis was carried out on the basis of the obstetric and gynecological hospital of Municipal Clinical Hospital No. 40 of Yekaterinburg.

The data of clinical and laboratory studies are illustrated by the following results.

Under observation were 40 patient volunteers. The criterion for the effectiveness of the proposed means of intimate hygiene was the clinical and laboratory recovery and the absence of relapse 1 month after its use. To verify the diagnosis and evaluate the effectiveness of Femivita, the following examination methods were performed for all patients in the study group:

- clinical examination (collection of complaints, medical history, general examination, special gynecological examination);

- laboratory examination (microscopy of a vaginal smear stained according to Gram, smear for purity, pH meter of vaginal secretion, amino test, culture of vaginal discharge from the vagina and its sensitivity to antibiotics, smear for chronic urogenital infection using PIF methods (direct immunofluorescence ) and PCR (polymerase chain reaction) depending on the causative agent. The diagnosis of bacterial vaginosis was made by the definition of Nugent scores [Information from Nugent RP, Krohn MA, Hillier SL. Reliability of diagnosing bacterial vaginosis is improved by a sta ndardized method of Gram stain interpretation J Clin Microbiol 1991].

The proposed tool was used as a hygienic drug by introducing into the vagina three times with an interval of 8 hours for 10 days.

The results obtained during the studies are presented in the table.

Table The effectiveness of femivitis in bacterial vaginosis Diagnosis criteria Normal criteria The presence of clinical symptoms for different periods of observation from the start of treatment, the number of patients Before treatment After 1 day In 2 weeks After 1 month Complaints no 32 thirty 0 0 Whites no 37 35 0 0 pH meter Slightly acidic 5 eighteen 40 40 Amino test negative 0 12 38 39 Gram smear “key cells” no 40 34 0 0 Note: a total of 40 patients with a confirmed diagnosis of bacterial vaginosis were observed

Example 4. Patient M., 40 years old. The diagnosis is bacterial vaginosis, IV degree of purity of the vagina. The treatment was prescribed - three times the introduction of the composition, wt.%: Metabolites of probiotic bacterial cells of hay bacillus 5; metabolites of sour-milk bacteria 5; sodium benzoate 0.5; propolis 5; essential oils: sage 1; lavender 0.05; distilled water 83.45; into the vaginal cavity every 6 hours 4 times for 7 days.

After the treatment, the majority of patients found that there were no complaints, there was no leucorrhoea, the vaginal environment was weakly acidic, the amino test was negative, “key cells” were not observed in a Gram smear.

Analysis of the results of the use of Femivitis in bacterial vaginosis in the studied group of patients allows us to recommend the proposed tool as a drug for the treatment of infectious and inflammatory diseases of the genital area.

Thus, the proposed means of intimate hygiene for women helps to increase the degree of purity of the vagina and restore its normal microflora, eliminate discomfort, improve the hygienic condition of the vagina by suppressing pathogenic and conditionally pathogenic microflora of the vagina, and have anti-inflammatory and immunocorrelation effects.

Claims (1)

An intimate hygiene product for women, characterized in that it contains metabolites of probiotic cells of Bacillus subtilis strain 3/28 (VKPM B 3679), metabolites of probiotic cells of Lactobacillus plantarum strain 8P-A3, sage essential oil, lavender essential oil, propolis, sodium benzoate and water in the following ratio of components, wt.%:
metabolites of probiotic cells Bacillus subtilis strain 3/28 (VKPM B 3679) 3 ÷ 5 metabolites of probiotic cells Lactobacillus plantarum strain 8P-AZ 3 ÷ 5 sage essential oil 0.5 ÷ 1 lavender essential oil 0.03 ÷ 0.05 propolis 3 ÷ 5 sodium benzoate 0.1 ÷ 1; distilled water rest