HU209802B - Deodorant composition with increased effect - Google Patents

Abstract

An improved efficiency deodorant prepn. contains at least 0.01 wt.% of 2,4,4,'-tri:chloro-2'-hydroxy -di:phenyl-ether (IRGASAN DP300) AND M-n-di:methyl-thio- carboxylic-acid-o- 2-naphthyl)-ester pref. in 2:1 ratio(Dwg.0/0)

Description

FIELD OF THE INVENTION The present invention relates to a broad-spectrum deodorant composition having an enhanced action.

It is known that unpleasant body (sweat) odor is caused by bacterial enzymatic decomposition of secretions produced by sweat separation. Decomposition products are odorous and / or odorous. containing unpleasant strong odor components such as hydrogen sulphide, aliphatic and aromatic amines, justified, ammonia and mercaptan.

Decomposing bacteria and many other microorganisms are released from the large sweat glands through the hair follicles and sebaceous glands, and from the environment (clothing, air, etc.).

The unpleasant odor of the body can be reduced with the help of deodorizing agents. eliminated. The mechanism of action of the known deodorants falls into the following main groups:

- reduction of the function of sweat glands with adrenaline

- killing bacteria and microorganisms on the skin surface with broad spectrum agents

- inhibition of bacterial metabolism or function by at least inhibiting enzyme blocking agents

- the use of anti-enzymatic additives (like enzyme blockers) that intervene in the bacterial cycle.

Of the known deodorants with various mechanisms of action, bactericidal and bacteriostatic agents have the consequence that they are effective on a broad spectrum, gram positive and gram negative microbes.

Well known materials of this type are e.g. hexachlorophen, similar halogenated phenol derivatives (Raluben TL, Actamer, Bithinol), non-photosensitive non-chlorinated phenol derivative are TMTD (tetramethylthiuram disulfide). Based on their mechanism of action, this includes chloramine, chlorhexidine, which is used in aerosols or in the form of relatively insoluble chlorohydrate in powders. The disadvantage of broad spectrum drugs is that they cannot be used on sensitive skin and can cause dermatitis.

A widely used chlorinated aromatic compound of good stability is IRGASAN (Ciba Geigy). Irgasan DP 300 (2,4,4'-trichloro-2'-hydroxy diphenyl ether) is a deodorant used in cosmetic products as it inhibits the development and growth of gram positive and negative microorganisms at low concentrations. Its advantage is that it is proven to work well in people with sensitive skin and does not cause unpleasant side effects.

Despite the relatively broad spectrum of action of Irgasan DP 300, it is barely effective against Pseudomonas species and yeast and other fungi, so its use as an antiperspirant is limited.

On the other hand, tolnaftate (m-N-dimethylthiocarbanyl acid-O- (2-naphthyl) ester) is known to have antifungal activity, is unsuitable in itself and is not used in deodorant formulations.

The development of deodorant formulations must pursue two basic goals, one of which is to reduce the concentration of the active ingredient in the formulations and thus eliminate the side effects caused by the deodorant, and secondly, to increase the spectrum of action, to induce enzymatic degradation by sweat bacteria and fungi.

It is therefore an object of the present invention to provide deodorant compositions which achieve their desired effect over a wide spectrum at relatively low drug concentrations. The deodorant composition of the present invention is at least 0.01% by weight, based on the total weight of the composition, of 2,4,4'-trichloro-2'-hydroxydiphenyl ether (IRGASAN DP 3000), in addition to the usual liquid, solid or gaseous carriers and / or excipients used. ) and a mixture of mN-dimethylthiocarbanilic acid O- (2-naphthyl) ester, (TOLNAPHTAT), preferably in a 2: 1 weight ratio, in the form of an aerosol, powder, lotion, lotion, solution, solid bar (stick, ball-stick) preparation. form. The deodorant composition of the present invention optionally contains stabilizing agents (antioxidants), skin protecting conditioners, and surfactants (TWEEN, EMULGIN).

The antimicrobial activity of the two active substances is different in the spectrum of action, but when used in the appropriate ratio, the spectrum of action can be broadened, while the concentration of the active ingredient in the composition can be reduced.

The process of the present invention for preparing a deodorant composition using a liquid or gaseous carrier and / or excipient conventionally used in a cosmetic composition is characterized in that a mixture of 0.1-10 tr Irgasan DP 300 and Tolnaphtat is suitably 2: 1 in an excess solvent, preferably 35- Dissolve in 90 liters of ethyl alcohol, add volatile material and propylene glycol to the solution, and fill the vessel with or without propellant. To form a solid preparation, the active ingredient mixture is added to an alcoholic solution of sodium stearate together with the fragrance and then, after dissolution, allowed to solidify.

The preparation and activity of the composition according to the invention are illustrated by the following examples:

Example 1

Tolnaphtat 0.03 tr

ORION Corporation

Espoo, Finland Irgasan DP 300 0,07 tr Ciba Geigy, Switzerland

Fragrance 0.02 tr

Propylene glycol 14.00 tr

Ethyl alcohol 35.90 tr

Propulsion gas 50.00 tr

The active compounds are dissolved in alcohol and then the perfume and propylene glycol are added to the solution. The solution thus prepared is filled with propellant into aerosol cans by a known method.

HU 209 802 Β

Example 2

Tolnaphtat 0.025 tr (Example 1) Irgasan DP 300 0.050 tr (Example 1) fragrance 0.025 tr Propylene glycol 10,000 tr Ethyl alcohol 89,900 tr

The active compounds are dissolved in ethyl alcohol and the perfume and propylene glycol are added to the solution. The solution thus prepared is disposed of in a manual pressure pump container by a conventional method. The composition can also be used as a face tonic.

Example 3

Tolnaphtat 0.025 tr (Example 1) Irgasan DP 300 0.050 tr (Example 1) fragrance 0.075 tr Ethyl alcohol 91,000 tr Sodium stearate 8,000 tr

Dissolve the sodium stearate in ethyl alcohol with warm reflux and stir in ca. After cooling to 40 ° C, the active ingredients and finally the perfume are mixed. After dissolution, allow the solution to solidify by pouring into a mold.

The effect of the compositions of the invention was demonstrated by the following test method. The purpose of the studies is to investigate the antimicrobial activity of Irgasan and Tolnaphtat in the following composition:

Tolnaphtat 0.35 g = 0.35 tr (Example 1) Irgasan 0.70 g = 0.70 tr (Example 1) Emulgin-L (Tensides) 5.0 g = 5.0 tr (sorbetane) propylene 24.0 g = 24.0 tr ethanol 70.0 g = 70.0 tr Altogether: 100.0 g Test organisms used: Staphylococcus aureus - HNXMB-110003 Escherichia coli - NHCMB-33 001 Pseudomonas aeruginosa - HNCMB-170003 Bacillus subtilis -ATCC-6633

Method used: half dilution method in liquid medium.

Short description:

Composition and indication of culture medium:

CM-3 Soup:

meat extract 3.0 g glucose 1.0 g trypsin 10.0 g Aqua dest. ad 1000 ml of sodium chloride 3.0 g pH: 7.2 (± 0.1) dipotassium hydrogen phosphate 2.0 g sterilization: 121 ° C20min 55

2.02.0 ml of CM-3 broth were pipetted into a sufficient number of sterile stoppered tubes. For the meat extract, 100 g of horse or beef is minced and topped with 1000 g of distilled water and left to stand overnight. The next day we filter through a canvas, squeeze it and make up to 1 60 liters. The meat broth is cooked in an autoclave at 121 ° C for 30 minutes, the weight loss is corrected, then sterilized at 121 ° C for 30 minutes and stored in a refrigerator. 2.0 ml of the pre-prepared stock solutions (also using CM-3 broth for preparation of stock solutions) were pipetted into the first test tube and carefully homogenized. From this first test tube, 2.0 ml was pipetted into a second test tube, homogenized, and again, 2.0 ml was pipetted into a third test tube. Thus, dilution was continued until the end of the series. Each tube contained half or twice the amount of material. Separate dilution series were prepared for each test organism from the same stock solution. Subsequently, the previously prepared and defined above vegetative culture of test organisms fresh 10 ⁴ -10 ⁵ -fold dilution series of each tube 0.1 ml is pipetted also made the same amount of sterile vials containing only medium (control bacteria). An additional 2 tubes containing sterile medium alone were added to the series (medium control). The so-filled series were incubated for 18-28 hours in a 37 ° C thermostat. At the end of the incubation period, evaluation was performed. Non-turbid tubes with a '-' sign, bacterial control turbidity tubes and the same turbidity tubes with a '++++' sign, other tubes depending on their turbidity '+', '++' and '+++' marked with.

The tests were performed under sterile conditions.

TESTS PERFORMED AND THEIR RESULTS

To determine the independent antimicrobial activity of the substances in the above formulation, a separate study was first performed.

Preparation of stock solutions

EMULGIN L

To 0.1 ml of Emulgin-L, 9.90 ml of CM-3 broth was pipetted40. The resulting solution contained 10,000 pg / ml Emulgin-L.

Propylene glycol

To 0.1 ml of propylene glycol, 9.90 ml of CM-3 broth was pipetted. The concentration of the solution is 10,000 µg / ml of pro45 pilene glycol.

CONTROL SOLUTION Composition:

Emulgin-L 5.0 g

Propylene glycol 24.0 g

Ethanol 70.0 g

To 0.1 ml of this solution was pipetted 9.90 ml of CM-3 broth. The concentration of the solution is 10,000 g / ml of control solution.

IRGASAN DP 300

Irgasan DP 300 (500 mg) was dissolved in 50.0 ml of propylene glycol in a water bath at 60 ° C. To 0.1 ml of the solution was pipetted 19.90 ml of CM-3 broth. The concentration of the resulting solution in Irgasan is 500 μg / ml.

TOLNAPHTAT

Dissolve 500 mg of Tolnaphtat in 50.0 ml of acetone3

HU 209 802 B us. To 0.1 ml of the solution was added 19.90 ml of CM / 3 broth using pipette A stock solutions and the method described. The Tolnaphtat concentration of the resulting solution was tested. The results obtained are 1,500 pg / ml. and Tables 3.

Table 1

EMULGIN L propylene Glycol Conc., In pg / ml (Λ 3 Ü u> □ CO CZ5 □ υ u She 8 -C cl co GO Escherichia coli Pseudomonas aeruginosa I Bacillus subtilis Staphylococcus aureus Escherichia coli Pseudomonas aeruginosa Bacillus subtilis 10000.0 - ++++ + - ++++ ++++ ++++ ++++ 5000.0 - ++++ + - ++++ ++++ ++++ ++++ 2500.0 - ++++ + - ++++ ++++ ++++ ++++ 1250.0 - ++++ + - ++++ ++++ ++++ ++++ 625.0 - ++++ + - ++++ ++++ ++++ ++++ 312.50 - ++++ + - ++++ ++++ ++++ ++++ 156.25 - +++ Ψ + - ++++ ++++ ++++ ++++ 78.12 - ++++ + - ++++ ++++ ++++ ++++ 39.06 - ++++ +++ - ++++ ++++ ++++ ++++ 19.53 - ++++ ++++ - ++++ ++++ ++++ ++++ 9.76 - ++++ ++++ ++ ++++ ++++ ++++ ++++ 4.88 - ++++ ++++ ++++ ++++ ++++ ++++ ++++ 2.44 ++ ++++ ++++ ++++ ++++ ++++ ++++ ++++ 1.22 ++++ ++++ ++++ ++++ ++++ ++++ ++++ ++++ 0.61 ++++ ++++ ++++ ++++ ++++ ++++ ++++ ++++ Tapto. k. - - - - - - - - Bact. k. ++++ ++++ ++++ ++++ ++++ ++++ ++++ ++++

The following can be deduced from Tables 1:

1. Propylene glycol is ineffective on all four test organisms.

2. Emulgin-L is inactive against Escherichia coli but inhibits Staphylococcus aureus at a concentration of 4.88 pg / ml and Bacillus subtilis at a concentration of 19.53 pg / ml. Pseudomonas aeruginosa has a very significant but not complete inhibitory effect.

The control solution was also ineffective against Escherichia coli, since the components of the control solution were ineffective individually. In contrast, the inhibitory effect on the test organisms of Pseudomonas aeruginosa and Bacillus subtilis varies in proportion of the components in the control solution compared to the data in Table 1. Only Staphylococcus aureus shows an increase in effect of approximately 20 fold (0.24 pg / ml Emulgin-L in the control solution at 4.88 pg / ml).

Table 3

Irgasan TOLNAPHTAT Conc., pg / ml Staphylococcus aureus Escherichia coli Pseudomonas aeruginosa Bacillus subtilis Staphylococcus aureus Escherichia coli Pseudomonas aeruginosa Bacillus subtilis 500.0 - - + - - ++++ ++++ ++++ 250.0 - - ++++ - - ++++ ++++ ++++ 125.0 - - ++++ - - ++++ ++++ ++++

HU 209 802 Β

Irgasan TOLNAPHTAT Conc., pg / ml Staphylococcus aureus Γ Escherichia coli Pseudomonas aeruginosa Bacillus subtilis Staphylococcus aureus Escherichia coli Pseudomonas aeruginosa Bacillus subtilis 62.50 - - ++++ - - ++++ ++++ ++++ 31.25 - - ++++ - - ++++ ++++ ++++ 15.62 - - ++++ - - ++++ ++++ ++++ 7.81 - - ++++ - - ++++ ++++ ++++ 3.90 - - ++++ - - ++++ ++++ ++++ 1.95 - - ++++ - - ++++ ++++ ++++ 0,976 - - ++++ - - ++++ ++++ ++++ 0.488 - - ++++ + - ++++ ++++ ++++ 0,244 - - ++++ ++++ - ++++ ++++ ++++ 0.122 - - ++++ ++++ - ++++ ++++ ++++ 0.061 - - ++++ ++++ - ++++ ++++ ++++ 0,030 - ++++ ++++ ++++ - ++++ ++++ ++++ Tapto. k. - - - - - - - - Bact. k. ++++ ++++ ++++ ++++ ++++ ++++ ++++ ++++

Table 3 summarizes the independent antibacterial activity data of Irgasan DP 300 and Tolnaphtat.

According to the results, Tolnaphtat has a significant inhibitory effect only on Staphylococcus aureus. It is inactive against Escherichia coli, Pseudomonas aeruginosa and Bacillus subtilis. Irgasan DP 300 has a significant antibacterial effect. Staphylococcus aureus is less than 0.03 pg / ml, Escherichia coli 0.061 μg / ml and Bacillus subtilis 0.97 g / ml. Only pseudomonas aeruginosa has a weaker effect. At 250 μg / ml it is still ineffective, but at 500 μg / ml it is almost complete inhibition.

Table 4

total active substance concentration only the Irgasan concentration only Tolnaphtat concentration Staphylococcus aureus Escherichia coli Pseudomonas aeruginosa Bacillus subtilis pg / ml pg / ml pg / ml 525.0 350.0 175.0 - - - - 262.5 175.0 87.5 - - + - 131.25 87.5 43.75 - - ++++ - 65.62 43.75 21.87 - - ++++ - 32.81 21.87 10.93 - - ++++ - 16.40 10.93 5.46 - - ++++ - 8.20 5.46 2.73 - - ++++ - 4.10 2.73 1.36 - - ++++ - 1.05 1.3 0.93 - - ++++ -

HU 209 802 Β

total active substance concentration only on Irgasan concentration only Tolnapht concentration Staphylococcus aureus Escherichia coli Pseudomonas aeruginosa i Bacillus subtilis pg / ml pg / ml pg / ml 1,025 0.68 0.34 - - ++++ - 0.512 0.34 0.17 - - ++++ - .256 0.17 0,085 - - ++++ ++++ 0.128 0,085 0.042 - - ++++ ++++ 0,064 0.042 0,021 - ++++ ++++ ++++ 0.032 0,021 0,010 - ++++ ++++ ++++ Media Control - - - - Bacterial control ++++ ++++ ++++ ++++

Table 4 summarizes the antibacterial activity data for the composition of the invention. The tests were carried out by first diluting the resulting solution 20 times with CM-3 broth (0.5 ml solution with 25 + 9.5 ml CM-3 broth). This diluted solution was serially diluted. The diluted solution contained a total of 525 pg / ml of the active substance, of which 350 pg / ml was Irgasan DP 300 and 175 pg / ml Tolnaphtat.

Table 4 shows that the effect of the 30 solutions tested on Staphylococcus aureus, Escherichia coli and Bacillus subtilis is limited to Irgasan DP 300. However, the results obtained with Pseudomonas aeruginosa differ from the data in Table 3. In particular, inhibition is observed at lower Irgasan concentrations. This can only be explained by the synergistic effect of Irgasan and Tolnaphtat. The experiment was repeated at higher concentrations to more accurately determine the difference in effect and its results are summarized in Table 5.

Table 5

Irgasan concentration Pseudomonas aeruginosa Tolnaphtat concentration Pseudomonas aeruginosa Irgasan concentration Tolnaphtat concentration Joint Concentration Irgasan + Tolnaphtat Pseudomonas aeruginosa pg / ml pg / ml pg / ml 2000.0 - 1000.0 ++++ 1000.0 + 500.0 = 1500.0 - 1000.0 - 500.0 ++++ 500.0 + 250.0 = 750.0 - 500.0 + 250.0 ++++ 250.0 + 125.0 = 375.0 - 250.0 ++++ 125.0 ++++ 125.0 + 62.5 = 187.5 ++++ 125.0 ++++ 62.5 ++++ 62.5 + 31.2 = 93.7 ++++ 62.5 ++++ 31.2 ++++ 31.2 + 15.6 = 46.8 ++++ 31.2 ++++ 15.6 ++++ 15.6 + 7.8 = 23.4 ++++ Tapto. k. - - - Bact. k. ++++ ++++ ++++

HU 209 802 Β

Based on the table, the following can be determined:

1. Irgasan alone has significant inhibitory activity against Staphylococcus aureus (pus), Escherichia coli (gut) and Bacillus subtilis (spore bacterium). For Pseudomonas aeruginosa, this inhibitory effect is significantly reduced.

2. Tolnaphtat alone has an inhibitory effect only on Staphylococcus aereus. It is ineffective against other test organisms tested.

3. The combined effect of Irgasan and Tolnaphtat in a 2: 1 ratio is that the effect of the solution on Pseudomonas aeruginosa is more than doubled, unlike Irgasan's original action. As this effect cannot be demonstrated individually, the excess effect can only be explained by synergism.

4. Tolnaphtat primarily has antifungal effect. It is also known that Irgasan has antibacterial activity, but also that Pseudomonas have a significantly weaker effect. Furthermore, its antifungal effect is also reduced.

The appropriate combination of Irgasan and Tolnaphtat provides the following two benefits:

- On the one hand, the antibacterial activity of their common solutions increases by increasing their anti-Pseudomonas activity.

- On the other hand, they complement each other's effect areas, that is, their joint solutions have a broad antibacterial and broad antifungal activity at the same time.

Recognition of the synergistic effect between the two compounds allowed a broad spectrum deodorant effect to be produced at minimal, less than the drug effect. The mixture should be used as a known formulated deodorant cosmetic product (aerosol, stick, powder, solution, cream, ball stick, shampoo, lotion, tonic, etc.). The significance of the combined action of the two agents in the field of deodorants is a new discovery not apparent from the state of the art.

Claims (2)

PATIENT INDIVIDUAL POINTS 1. An enhanced deodorant composition comprising, as active ingredient, at least 0.01% by weight of the composition, 2,4,4'-trichloro-2'-hydroxy-diphenyl ether and mN-dimethylthiocarbonylic acid 0- A mixture of (2-naphthyl) ester, preferably 2: 1 by weight, with the usual used liquid, solid or gaseous carrier and / or excipients in the form of an aerosol, powder, cream, lotion, solution, solid rod (rod, ball-stick) preparation . Composition according to claim 1, characterized in that it contains stabilizing, preferably antioxidant, skin protection conditioners and surfactants.