Team:Paris Bettencourt/Project/Foot Odor
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Revision as of 23:22, 17 October 2014
BACKGROUND Isovaleric acid has a pungent smell associated with both foot odor and strong cheese. A major source of this molecule on feet is leucine degradation by Bacillus strains, including the well-known lab strain B. subtilis. |
AIMS We explore the possibility of using B. subtilis mutants to reduce foot odor. Strains of B. subtilis deleted in leucine degradation pathways should produce less odor, yet fill established ecological niches on human feet and socks. |
RESULTS Demonstrated that mutant strains of B. subtilis produce less odor. Measured growth and viability of mutants in synthetic sweat media and on socks. |
Aims and Achievement | Introduction | Results | Methods | References |
Fig. 1. B. subtilis is gram positive bacterium which is commonly found in the human foot flora, which degrades the leucine aminoacid present in the sweat to produce isovaleric acid. Our strategy is to perturb the leucine degradation pathway by knocking out the vital enzymes in the pathway. The leucine dehydrogenase knock out mutants lacks the capability to produce leucine and prevents the conversion of leucine to 4-methyl 2-oxopentanoate. The isovaleryl-coA dehydrogenase α and β subunit knock mutants lacks the capability of conversion of 4-methyl 2-oxopentanoate to isovaleryl-coA.
Aims and Achievement
Foot odor is generally perceived as socially awkward and negative. Although there are a many commercially available solutions for this problem, current products indiscriminately target bacteria on the foot skin microbiome. These type of products can have negative effects on skin health and microbiome dynamics. We aim to develop a targeted approach to prevent foot odor, by selectively killing microbes responsible for the biosynthesis of volatile compounds which compose the characteristic stinky feet smell, without destroying the beneficial microbes.
Introduction
Isovaleric acid is the characteristic odorant of foot odor. It is produced primarily from leucine, found in the sweat, via the leucine degradation pathway (Fig. 1). Of the many bacterial species found on the foot, only Bacillus frequency correlates with foot odor intensity (Ara et al., 2006). We therefore chose to focus our project on the leucine degradation pathway of the model microbe B. subtilis. We hypothesize that a leucine degradation mutant of B. subtilis will produce less odor, yet still survive and replicate on the foot. A large population of mutants on the foot would exclude the wild-type strain and therefore attenuate odor. If the mutant strain can persist in the foot ecosystem, bacterial foot deodorants could provide a cheap alternative to traditional chemical deodorizers. .
Figure 2. Diffusion model of isovaleric acid through air. This animation shows the concentration of isovaleric acid diffusing through air from a foot over a time period of 0 to 1000 hours. From the graph on the left of the animation, you can see that the odor threshold is reached very early in the model, given that the concentration of isovaleric acid at the skin surface is kept at a constant concentration of 1.1*10-6 M.
Figure 3. The B. subtilis wt and mutant strains were grown overnight in M9 minimal medium. A double blind smell test was performed. The subjects were asked to rank the tubes in the order of 0 to 5.
An analysis with 95% confidence interval was made. Though there is variation observed
between the wt strain and the bcd knock out strain, it is not statistically significant. In the case of bkdaα
knock out strain and the wt strain there is a statistically significant variation observed. This confirms that the
bkdaα knock out strain produces less malodor compare to the wild type.
Results
We found ''B. subtilis'' mutants ΔBKDAa and ΔBKDAb to produce less odor than the wild type. We obtained 3 deletion strains from the Bacillus Genetic Stock Center (BGSC): ΔBCD, ΔBKDAa and ΔBKDAb. Each of these mutants blocks the metabolic pathway connecting leucine to Isovaleryl-CoA. Double-blind smell tests with human smellers revealed that cultures of ΔBKDAa and ΔBKDAb had signficantly less intense odor than wild type. No significant difference was detected for the ΔBCD strain. Because our smell tests used human noses, we built a model to estimate the sensitivity of our instruments (Fig. X). Using COMSOL Multiphysics, we simulated odor diffusion as a system of differential equations. Isovaleric acid can be smelled at a concentration of 80 parts per trillion (Nagata, 1993). After diffusion equilibrium, this corresponds to a liquid phase concentration of 10 mg/L at a distance of 5 cm, comparable to the leucine concentration in human sweat (Callewaert et al., 2014). Our model confirms that human noses are able to detect isovaleric acid at physiologically relevant concentrations. We next investigated the leucine-dependance of odor production in the B. subtilis and mutant strains. Strains were grown in M9 minimal media supplemented with 0%, 0.1% or 0.2% leucine. All strains produced detectable odor in all conditions, indicating that B. subtilis produces some odorant molecules independant of the leucine pathway. Odor production in the wild-type strain was strongly leucine dependant, suggesting leucine metabolism constributes significantly to odor. The odor of the BKDAb strain showed no leucine dependance, consistent with the successful inactivation of an odor pathway. If mutant B. subtilis are to exclude the wild type on the human foot, they must be able to grow on sweat. We found that growth of all 3 mutant strains was moderately impaired on LB media, and severely impaired on synthetic sweat, relative to wild type (Figure X). However, leucine-degradation mutant strains of B. subtilis showed robust survival on socks. We dipped cotton socks in dense M9 cultures of ΔBCD, ΔBKDAa, ΔBKDAb or wild-type strains. Socks were hung to dry and sampled daily for the density of B. subtilis CFUs. After 5 days, we detected no signifcant decline in population viability. This suggests that, once introduced to socks, a metabolic mutant strain could persist and modulate odor production for an extended time.
Methods
Synthetic sweat:
The chemical constituents present in the human sweat were analyzed with the aid of gas chromatography and mass spectroscopy. Synthetic sweat was prepared by diluting the exact concentration of all the amino acids and salts found in human sweat, the pH of the synthetic sweat was adjusted to 6.5 with the aid of a pH meter. The synthetic sweat was then autoclaved and stored at 4°C to avoid bacterial contamination.
M9 minimal media:
The minimal media was prepared by diluting
1ml of 50% glucose
1.1 ml of mgso4.3H20
2ml of 1% w/v casmino acids
2ml of 10mg/ml of tryptophan
in 100 ml of distilled water
The media is then filter sterilized under a laminar air flow cabinet.
Strain:
The leucine dehydrogenase, isovaleryl coA alpha subunit and isovaleryl coA beta subunit. The knockout strains were obtained from Bacillus Genetic Stock Centre, where the knockout library of the B. subtilis was generated by replacing each gene with the erythromycin cassette. The mutant strains are trp- so they require supplementation of tryptophan in the growth media. The knockout strains were validated with the PCR reaction.
Growth curve:
The growth kinetics of the wild type and the mutant strains of B. subtilis were studied with the aid of micro plate reader to have insights about the fitness advantage and disadvantage within the mutant and wild type strain.
Smell test:
The presence of isovaleric acid in the bacterial culture was sensed with double blind smell test, where neither the subject nor the experimenter is aware of the tube labels. In order to optimize this smell test we grew the B. subtilis in odorless M9 minimal media. The media was supplemented with 0.1% of leucine to study the influence of leucine in production of foot odor.
Sock experiment:
The bacterial cell culture is diluted in synthetic sweat till it reaches 0.1 OD. The sock was soaked in the synthetic sweat and hanged till it dry. After this step 2 cm2 of sock was cut and soaked in 5ml of 1% PBS. The tubes were stirred gently and supernatant is diluted in PBS to prepare 1X and 10X concentration of B. subtilis. The bacteria were then plated on LB agar.
Diffusion model of isovaleric acid:
The model is based on a 2D axisymmetric geometry, with the air modeled as the space 5 cm around the skin surface. Here, the skin surface is kept at a constant concentration, C0 = 1.1E-6 M. This value refers to the approximate amount of isovaleric acid in sweat (Harvey, 2010). The diffusivity of isovaleric acid through the air was calculated using the Chapman-Enskog theory of gas diffusivity given by the following equation:
D = [1.858*10-3* T-3/2*√(1/M1+1/M2)] / [p * s122 * w)]
- D is the diffusivity of the isovaleric acid
- T is the room temperature (298 K)
- p is the air pressure (1 atm)
- M1 is the mass of the isovaleric acid (102.13 g/mol)
- M2 is the mass of the air (29 g/mol).
- s12 is the average collision diameter, which is around 340 Angstroms for gas molecules in air.
- w is the dimensionless temperature-dependent collision integral, usually on the order of 1.
Thus, the diffusion coefficient of isovaleric acid was tabulated to be 1.7*10-9 m2 / s.
GC-MS analysis: For GC-MS analysis 1µl of the sample is injected in split mode in the instrument. Use a Rtx5MS- 30m column with 0.25-mm ID and 0.25µm df. Following are the parameters standardized for GC-MS run: • Injection temperature: 300°C, • Interface temperature: 300°C, • Ion source should be adjusted to 250°C. • Carrier gas: Helium (flow rate of 1 ml min-1). • Perform the analysis using the following temperature program: • 3 min. of isothermal heating at 50⁰C followed by heating at 350⁰C for 10 mins. • Mass spectra were recorded at 2 scan sec-1 with a scanning range of 40 to 850 m/z. Quantify each component based on peak areas and normalization based on the internal standard. • X caliber software is used for processing and analyzing the data.