Patent Grant
11124438
The present disclosure relates to the field of microbial technology, and more particularly to a strain of Alcaligenes faecalis capable of degrading ethylene oxide and uses thereof.
Incorporated by reference herein in its entirety is the Sequence Listing entitled “1211_CK05_ST25_PCT” created Jun. 9, 2020, size of 4.54 kilobytes.
Ethylene oxide (EO) is among the most important petrochemical products in the modern industries and plays a significant role in the medical sterilization industry thanks to its strong penetrability and ability to perform coupling reactions with biological macromolecules. In addition, ethylene oxide sterilization has a low cost and can be used for industrial-grade sterilization in a large scale, making it by far one of the most important low-temperature sterilizers. However, ethylene oxide is extremely active, flammable, explosive, and globally recognized as a carcinogen. Large quantities of ethylene oxide are found in wastewater from petrochemical industries and need to be decontaminated.
At present, oxidization of ethylene oxide with sulfuric acid is the primary way of ethylene oxide decontamination process in countries such as China. However, it fails to meet the requirements of full decontamination as, disadvantageously, a large amount of industrial wastewater containing ethylene oxide will be discharged after the chemical treatment.
There is an urgent and long-felt need to find a way of ethylene oxide decontamination. Microbial degradation of harmful substances plays an important role in the chemical industry. However, there are few studies on the use of microorganisms to degrade ethylene oxide and no reports of bacteria or their uses on effective degradation of ethylene oxide.
In view of this, the present disclosure provides an Alcaligenes faecalis strain that can effectively degrade ethylene oxide, which can be used to degrade ethylene oxide pollutants, e.g., in sewage, sludge, exhaust gas, or wastewater, especially industrial (such as industries related to petroleum and derivative products), medical treatment (such as ethylene oxide sterilant) and other sewage or wastewater. Therefore, it may greatly improve the decontamination processes of ethylene oxide and reduce environmental risks, such as public health risk.
In one of the aspects of the present disclosure, an Alcaligenes faecalis strain EO-05 with the Deposit Number of CGMCC No. 18435 is provided. The Alcaligenes faecalis EO-05 can effectively degrade ethylene oxide.
In one of the aspects of the present disclosure, an Alcaligenes faecalis strain comprising the 16S rDNA sequence of SEQ ID NO: 4 is provided. The Alcaligenes faecalis strain can effectively degrade ethylene oxide.
In one of the aspects of the present disclosure, it provides a degradation agent for degrading ethylene oxide, comprising the Alcaligenes faecalis strain EO-05 or the Alcaligenes faecalis strain comprising the 16S rDNA sequence of SEQ ID NO: 4.
In some of the embodiments, the degradation agent is prepared by culturing the Alcaligenes faecalis strain EO-05 or the Alcaligenes faecalis strain comprising the 16S rDNA sequence of SEQ ID NO: 4.
In some of the embodiments, a final concentration of the Alcaligenes faecalis strain EO-05 or the Alcaligenes faecalis strain comprising the 16S rDNA sequence of SEQ ID NO: 4 in the degradation agent is at least 108 cfu/mL, or from 108 cfu/mL to 1010 cfu/mL.
In one of the aspects of the present disclosure, it provides a method for preparing a degradation agent for degrading ethylene oxide, comprising: inoculating the Alcaligenes faecalis strain EO-05 or the Alcaligenes faecalis strain comprising the 16S rDNA sequence of SEQ ID NO: 4 and incubating the inoculated medium thereby obtaining the degradation agent. In some aspects, the strain is inoculated into tryptone soybean broth culture medium. In some aspects, the strain is incubated for 48 hours of incubation at 37° C. and 200 rpm.
In one of the aspects of the present disclosure, it provides a method for biodegrading ethylene oxide, comprising using the Alcaligenes faecalis strain EO-05, the Alcaligenes faecalis strain comprising the 16S rDNA sequence of SEQ ID NO: 4, or the aforementioned degradation agent to degrade ethylene oxide.
In one of the aspects of the present disclosure, it provides a method for decreasing the amount of ethylene oxide in material, comprising adding to a material comprising ethylene oxide an amount a pure culture of an Alcaligenes faecalis strain bacterium, allowing the bacterium to degrade the ethylene oxide, thereby decreasing the amount of ethylene oxide, wherein the 16S rDNA sequence of the Alcaligenes faecalis strain bacterium is SEQ ID NO: 4.
In a further aspect of the method, the Alcaligenes faecalis strain bacterium is capable of using ethylene oxide as a carbon source and is capable of growing normally with ethylene oxide as the sole carbon source in the culture.
In a further aspect of the method, the Alcaligenes faecalis strain bacterium is Alcaligenes faecalis strain EO-05 with the Deposit Number of CGMCC No. 18435.
The degradation rate in the methods is at least 10%, 15%, 20%, 25%, 30%, 35%, 40%, 50%, 60%, 70%, 75%, 80%, 90%, 95%, 100%, 125%, 150%, 200%, or 500% greater relative to the degradation rate of ethylene oxide in the absence of the Alcaligenes faecalis strain EO-05 or Alcaligenes faecalis strain comprising the 16S rDNA sequence of SEQ ID NO: 4.
In some of the embodiments, the method is used for degrading ethylene oxide in sewage, sludge, exhaust gas, or wastewater, and comprises: applying the Alcaligenes faecalis strain EO-05, the Alcaligenes faecalis strain comprising the 16S rDNA sequence of SEQ ID NO: 4 or the degradation agent aforementioned to the sewage or wastewater. The sewage or wastewater may be industrial (such as industries related to petroleum and derivative products), medical (such as ethylene oxide sterilant) or other sewage or wastewater.
In some embodiments, the method comprises incubating the strain in liquid TSB medium to a concentration from 1010 cfu/mL to 1012 cfu/mL, to obtain an activation liquid for degrading ethylene oxide.
In one embodiment, the method comprises a concentration of the strain for degrading ethylene oxide ranging from 108 cfu/mL to 1010 cfu/mL.
In some of the embodiments, the using an Alcaligenes faecalis of the invention to degrade ethylene oxide in the method comprises: inoculating the Alcaligenes faecalis strain EO-05 or the Alcaligenes faecalis strain comprising the 16S rDNA sequence of SEQ ID NO: 4 into tryptone soy broth culture medium for 48 hours of incubation at 37° C. and 200 rpm to obtain an Alcaligenes faecalis EO-05 culture; and using the Alcaligenes faecalis EO-05 culture to degrade ethylene oxide.
In one of the aspects of the present disclosure, it provides use of the Alcaligenes faecalis strain EO-05 the Alcaligenes faecalis strain comprising the 16S rDNA sequence of SEQ ID NO: 4, the degradation agents, or a degradation agent prepared according to the method aforementioned in degradation of ethylene oxide.
In one of the aspects of the present disclosure, it provides use of the Alcaligenes faecalis strain EO-05 or the Alcaligenes faecalis strain comprising the 16S rDNA sequence of SEQ ID NO: 4 in the preparation of a degradation agent for degrading ethylene oxide.
The present disclosure provides an Alcaligenes faecalis strain EO-05 or the Alcaligenes faecalis strain comprising the 16S rDNA sequence of SEQ ID NO: 4 that can degrade ethylene oxide, which can be used to treat pollution, for example, to treat industrial or medical sewage or wastewater containing ethylene oxide. The strain EO-05 or other strains of the invention can be cultivated in a very simple way and efficiently degrade high-concentration ethylene oxide in a short period of time without other carbon sources. Therefore, the present disclosure may greatly improve the decontamination processes of ethylene oxide.
In a further aspect of the present disclosure, there is also provided a method for purifying ethylene oxide-degrading potential bacteria, comprising:
In one embodiment, the method comprises mixing sewage or sludge containing the original strain with phosphate buffer, and filtering for removal of precipitate to obtain the suspension.
In one embodiment, the first enrichment medium is prepared as follows: sterilizing liquid TSB medium, cooling the medium to room temperature, and adding liquid ethylene oxide to the medium. The liquid TSB medium contains 17 g/L tryptone, 3 g/L soy peptone, 2.5 g/L of dipotassium hydrogen phosphate and 2.5 g/L of glucose, and has pH 7.4.
In one embodiment, the screening and purification medium is prepared as follows: sterilizing TSB agar medium, cooling the medium to 50° C. to 56° C., and adding liquid ethylene oxide to the medium. The TSB agar medium contains 2.5 g of dipotassium hydrogen phosphate, 2.5 g of glucose and 15 g/L agar, and has pH 7.4.
In one embodiment, the second enrichment medium is prepared as follows: sterilizing TSB medium, and cooling the medium to room temperature. The second enrichment medium does not contain ethylene oxide.
In one embodiment, the suspension is incubated in the first enriched enrichment medium having a low concentration of ethylene oxide for 24 to 48 hours, and the bacterial suspension is incubated on the screening and purification medium plate having a low concentration of ethylene oxide for at least 24 hours. The low concentration of ethylene oxide in the first enriched enrichment medium and the screening and purification medium plate may be range from 10 mg/L to 500 mg/L, e.g., 100 mg/L.
In further aspect of the present disclosure, there is also provided a method for producing a strain for degrading ethylene oxide, comprising:
In one embodiment, the concentration of carbon source serially decreases from 20 g/L to 0 mg/L during subculture.
In one embodiment, the concentration of the carbon source in the ethylene oxide-degradation acclimation mediums serially decreases from 50%, to 0% during subculture.
In one embodiment, the original strain is incubated at a temperature of 37° C. in the ethylene oxide-tolerance acclimation medium.
In one embodiment, the ethylene oxide-degrading predominant strain is incubated at a temperature of 37° C. in ethylene oxide-degradation acclimation mediums.
In one embodiment, the original strain is subcultured in ethylene oxide-tolerance acclimation mediums containing 0 mg/L to 100 mg/L, 100 mg/L to 200 mg/L, 200 mg/L to 500 mg/L, 500 mg/L to 800 mg/L ethylene oxide for 24 to 48 hours serially and respectively.
In one embodiment, the original strain is subcultured in the ethylene oxide-tolerance acclimation mediums containing 100 mg/L, 200 mg/L, 500 mg/L, 800 mg/L ethylene oxide serially and respectively.
In one embodiment, the ethylene oxide-degrading predominant strain is incubated in the second enrichment medium for at least 24 hours to obtain ethylene oxide-degrading potential bacteria.
In one embodiment, the ethylene oxide-degrading predominant strain is obtained by:
In one embodiment, the ethylene oxide-tolerance acclimation mediums are prepared as follows: adding liquid ethylene oxide into a sterilized Sabouraud's agar medium to a final concentration from 100 mg/L to 800 mg/L, wherein the ethylene oxide-tolerance acclimation mediums contain 10 g/L peptone, 40 g/L of glucose, and 15 g/L agar, and pH of 5.4 to 5.8.
In one embodiment, the sterilized Sabouraud's agar mediums are heated to melt, cooled to 50° C. to 56° C., and mixed with liquid ethylene oxide.
In one embodiment, the ethylene oxide-degrading predominant strain is serially and respectively subcultured in the ethylene oxide-degradation acclimation mediums containing 20 g/L, 12 g/L, 4 g/L, and 0 g/L the carbon source for 24 to 48 hours.
In one embodiment, the ethylene oxide-degradation acclimation mediums have glucose as the carbon source.
In one embodiment, the ethylene oxide-degrading predominant strain is inoculated into the ethylene oxide-degradation acclimation medium plates having 500 mg/L to 800 mg/L ethylene oxide and a carbon source with a serially decreasing concentration, and subcultured in an incubator at a temperature from 25° C. to 37° C. for 24 to 48 hours respectively and serially; and picking a single colony with a largest radius to obtain the strain for degrading ethylene oxide.
In one embodiment, the strain for degrading ethylene oxide is obtained as follows: inoculating the ethylene oxide-degrading predominant strain into the first ethylene oxide-degradation acclimation medium plate containing 800 mg/L ethylene oxide and 20 g/L carbon source, and incubating the first plate in an incubator at 37° C. for 24 to 48 hours; picking a first single colony with a largest radius on the first plate, inoculating the first single colony into the second ethylene oxide-degradation acclimation medium plate containing 800 mg/L ethylene oxide and 12 g/L carbon source, and incubating the second plate in an incubator at 37° C. for 24 to 48 hours; picking a second single colony with a largest radius on the second plate, inoculating the second single colony into the third ethylene oxide-degradation acclimation medium plate containing 800 mg/L ethylene oxide and 4 g/L carbon source, and incubating the third plate in an incubator at 37° C. for 24 to 48 hours; picking a third single colony with a largest radius on the third plate, inoculating the third single colony into the fourth ethylene oxide-degradation acclimation medium plate containing 800 mg/L ethylene oxide and 0 g/L carbon source, and incubating the fourth plate in an incubator at 37° C. for 24 to 48 hours; finally picking a fourth single colony with a largest radius on the fourth ethylene oxide-degradation acclimation medium plate containing 800 mg/L ethylene oxide and 0 g/L carbon source to obtain the strain for degrading ethylene oxide.
The Alcaligenes faecalis EO-05 strain was deposited on Aug. 29, 2019 at China General Microbiological Culture Collection Center, with the deposit number being CGMCC No. 18435 and the deposit address being Institute of Microbiology of Chinese Academy of Sciences, NO. 1 West Beichen Road, Beijing 100101, China.
Detailed description will be given below with referral to the accompanying figures to facilitate understanding of the present application. Preferred embodiments are shown in the figures. However, the present application may be implemented in various ways, without being limited to the examples presented in the description. The purpose of these embodiments is merely for illustration and better comprehension of the present disclosure.
Unless otherwise defined, all the technical and scientific terms herein shall be understood as the same meaning with those commonly accepted by a person skilled in the art. Such terms, as used herein, are for the purpose of describing specific embodiments of, without limiting, the present application. The term “and/or” as used herein refers to any and all combinations of one or more items recited.
This is an example of the screening and purification of bacteria strains with EO-degrading ability.
A sample of the sludge mixture was collected at the sewage outlet of a suburban sewage treatment plant in Guangzhou, Guangdong Province, and used for the screening and purification experiments of this example.
10.0 g of the sludge mixture sample was weighed, added with 100 mL of 0.03 mol/L phosphate buffer, well mixed, allowed to stand for 120 min for clarification, and filtered to remove large particles of sediment and obtain a suspension.
Liquid enrichment medium (also known as TSB medium) was prepared as follows: 17 g of tryptone, 3 g of soy peptone, 5 g of sodium chloride, 2.5 g of dipotassium hydrogen phosphate and 2.5 g of glucose were mixed, adjusted to a pH of 7.4, and added to 1000 mL of distilled water, thoroughly mixed. Portions of 250 ml of the prepared medium was added to 500 mL Erlenmeyer flasks, sterilized at 121° C. for 20 min, and cooled to room temperature. Pure ethylene oxide liquid was placed on an ice box and 28 μL of ethylene oxide liquid was taken and injected into the sterilized medium by a sealed syringe, providing 100 mg/L of ethylene oxide in the medium complying with the national emission standard.
1 mL of the suspension was added to each of 4 test tubes containing 10 mL of liquid enrichment medium and placed in a shaker for oxygen-consuming enrichment culture for 24-48 h (200 rpm, 37° C.).
Selection medium and selection culture plates were prepared as follows: 17 g of tryptone, 3 g of soy peptone, 5 g of sodium chloride, 2.5 g of dipotassium hydrogen phosphate, 2.5 g of glucose and 15 g of agar were mixed, adjusted to a pH of 7.4, and added to 1000 mL of distilled water, thoroughly mixed. Portions of 250 ml of the prepared selection medium was added into 500 mL Erlenmeyer flasks, sterilized at 121° C. for 20 minutes, and cooled to about 50-56° C. 28 μL of ethylene oxide liquid was injected into the sterilized medium by a sealed syringe to make a selection culture plate.
The dominant strains in the liquid enrichment medium were streaked on the selection culture plate for separation of the EO-degrading potential bacteria. As shown in
Single colonies were selected and cultured in the liquid enrichment medium without ethylene oxide for 24 hours to obtain EO-degrading potential bacteria, which were preserved at −80° C. using the glycerin preservation method (culture medium: 50% glycerol=1:
This is an example of characterization and identification of EO-degrading bacteria strains, using the following identification methods:
Morphological characterization: including observation of colony morphology, microscopic morphology, culture characteristics and Gram staining;
Physiological and biochemical characterization: including nutrition type, nitrogen and carbon source utilization capacity, and biochemical tests;
Molecular biological characterization (The DNA in the genome that produces the ribosomal RNA is called the “rRNA gene” or simply “rDNA.” 16s rDNA sequencing): including the procedure of bacterial culture, bacterial DNA extraction, PCR amplification, 16s rDNA sequencing and sequence alignment analysis, wherein the primer pair for PCR amplification was as follows:
The above characterization and identification methods are well known to those skilled in the art.
The characterization and identification results are as follows:
Morphological characteristics: gray-white colonies, uneven edges, spreading growth, colony diameter 4.0-6.0 mm, with blue-green fluorescent pigment. Under microscope, the bacterial cells were short rods or spherical-shaped, separately arranged and without spores. The Gram stain gave a negative result as shown in
Molecular biological characteristics: the sequencing result of 16s rDNA is shown in SEQ ID NO: 3; the 16S rDNA sequence was subjected to nucleotide sequence alignment analysis by BLAST and showed a 99% sequence homology with Alcaligenes faecalis. The phylogenetic tree of this strain is shown in
According to the characterization results of morphology, physiology, biochemistry, and molecular biology, EO-degrading potential bacteria strain obtained by screening and purification according to Example 1 was Alcaligenes faecalis.
This is an example of inductive acclimation of EO-degrading potential bacteria strains, including inductive acclimation of ethylene oxide tolerance and acclimation of ethylene oxide degradation ability.
Phase I: Inductive Acclimation of Ethylene Oxide Tolerance
The tolerance acclimation medium and culture plates were prepared as follows: 10 g of peptone, 40 g of glucose and 15 g of agar were mixed, adjusted to a pH of 5.4-5.8, and added to 1000 mL of distilled water, thoroughly mixed. The prepared culture medium was divided into portions of 250 mL and sterilized at 121° C. for 20 min. Before use, the medium was heated to melt, allowed to cool to about 50-56° C., and added with 25 mg, 50 mg, 125 mg or 200 mg of ethylene oxide respectively by a sealed syringe to make medium plates with four different concentrations of ethylene oxide (100 mg/L, 200 mg/L, 500 mg/L or 800 mg/L).
Using the method of plate streaking, the EO-degrading potential bacteria obtained from Example 1 was inoculated onto the tolerance acclimation medium with 100 mg/L ethylene oxide and incubated at a constant temperature of 37° C. for 48 h. Then the single colony with the largest radius was selected and subcultured onto the tolerance acclimation medium with 200 mg/L ethylene oxide and incubated at 37° C. for 48 h. Again, the single colony with the largest colony radius on the plate was selected and subcultured onto the tolerance acclimation medium with 500 mg/L ethylene oxide and incubated at a constant temperature of 37° C. for 48 h. The single colony with the largest colony radius on the plate was selected and subcultured onto the tolerance acclimation medium with 800 mg/L ethylene oxide and incubated at a constant temperature of 37° C. for 48 h. Then the single colony with the largest colony radius on the plate was selected as a strain with tolerance against high concentration of ethylene oxide.
Phase II: Inductive Acclimation of Ethylene Oxide Degradation Ability
The degradation acclimation medium and culture plates were prepared as follows: 10 g of peptone, glucose (20 g, 12 g, 4 g, or 0 g) and 15 g of agar were mixed, adjusted to a pH of 5.4-5.8, and added to 1000 mL of distilled water, thoroughly mixed to make mediums of four different carbon contents (50%, 30%, 10%, or 0%). The medium prepared as above were divided into 250 ml portions and sterilized at 121° C. for 20 min. Before use, the medium was heated to melt, allowed to cool to about 50-56° C., and added with 200 mg of ethylene oxide by a sealed syringe to make four types of culture plates with different amounts of carbon source (50%, 30%, 10%, or 0%) and 800 mg/L of ethylene oxide.
Using the method of plate streaking, the strain with tolerance against high concentration of ethylene oxide obtained from Phase I was inoculated onto the degradation acclimation medium with 800 mg/L ethylene oxide and 50% carbon source, and incubated at a constant temperature of 37° C. for 48 h. Then the single colony with the largest radius was selected and subcultured onto the degradation acclimation medium with 800 mg/L ethylene oxide and 30% carbon source and incubated at 37° C. for 48 h. Again, the single colony with the largest colony radius on the plate was selected and subcultured onto the degradation acclimation medium with 800 mg/L ethylene oxide and 10% carbon source and incubated at a constant temperature of 37° C. for 48 h. The single colony with the largest colony radius on the plate was selected and subcultured onto the degradation acclimation medium with 800 mg/L ethylene oxide and 0% carbon source and incubated at a constant temperature of 37° C. for 48 h. The single colony with the largest colony radius on the plate was selected as a strain with strong tolerance and degradation ability against high concentration of ethylene oxide, which was then designated as the EO-05 strain.
The EO-05 strain was preserved on agar medium slope with corresponding nutrients at −80° C. using the glycerin preservation method (culture medium: 50% glycerol=1:1).
The results of Phase I and Phase II inductive acclimation of the bacteria strains were summarized in Table 1. It shows that the strain EO-05 was obtained with strong tolerance and degradation ability against high concentration of ethylene oxide by gradual control of the cultivation conditions of the dominant strains against ethylene oxide. The EO-05 strain was able to use ethylene oxide as a carbon source and grow normally with ethylene oxide being the sole carbon source in the culture.
The 16s rDNA sequence of the strain EO-05 acclimated in Example 3 was sequenced and the sequencing result is shown in SEQ ID NO: 4.
The Alcaligenes faecalis EO-05 strain was deposited on Aug. 29, 2019 at China General Microbiological Culture Collection Center, with the deposit number being CGMCC No. 18435 and the deposit address being Institute of Microbiology of Chinese Academy of Sciences, NO. 1 West Beichen Road, Beijing 100101, China.
This is an example testing the ability of the EO-05 strain to degrade ethylene oxide.
I. Experimental Method:
1. Culture and activation: the EO-05 strain and the EO-degrading potential bacteria (i.e., the original strain before acclimation) were taken out from −80° C. refrigerator and 10 μL of each was inoculated in 100 mL tryptone soy broth (TSB) medium, respectively, and cultivate for 48 h (37° C., 200 rpm). The number of cells in the culture liquid is 1010-1012 cfu/mL.
2. Nutrient broth liquid culture medium was made as follows: 10 g peptone and 5 g sodium chloride were added to 1000 mL of distilled water, divided into 400 mL portions, sterilized at 121° C. for 20 min, and cool to room temperature for storage. To make liquid medium containing no carbon source but 400 mg/L or 800 mg/L ethylene oxide, 160 mg or 320 mg of ethylene oxide, respectively, were injected to the medium with a closed syringe before use.
3. Comparative Test of Ethylene Oxide Degradation
To conduct a comparative experiment of ethylene oxide degradation, the following treatment and control groups were incubated in a 37° C. incubator for 48 hours.
Treatment Group 1 (EO-05 strain/800 mg/L ethylene oxide): 5 mL of the bacterial culture of the pure cultured strain EO-05 obtained according to Example 3, with a live cell count of 1010-1012 cfu/mL, was inoculated into 400 mL of nutrient broth liquid medium containing no carbon source but 800 mg/L ethylene oxide as the inducer, with a live bacteria cell count in the medium being 108-1010 cfu/mL. The cell culture result after 48 hours is shown in
Treatment Group 2 (original strain before acclimation/800 mg/L ethylene oxide): 5 mL of the bacterial culture of the EO-degrading potential bacteria (i.e., the original strain before acclimation) obtained according to Example 1, with a live cell count of 1010-1012 cfu/mL, was inoculated into 400 mL of nutrient broth liquid medium containing no carbon source but 800 mg/L ethylene oxide as the inducer, with a live bacteria cell count in the medium being 108-1010 cfu/mL. The cell culture result after 48 hours is shown in
Control group 1 (No inoculation/800 mg/L ethylene oxide): Nutrient broth liquid medium containing no carbon source but 800 mg/L ethylene oxide without inoculation of the EO-05 strain or EO-degrading potential bacteria.
Treatment Group 3 (EO-05 strain/400 mg/L ethylene oxide): 5 mL of the bacterial culture of the pure cultured strain EO-05 obtained according to Example 3, with a live cell count of 1010-1012 cfu/mL, was inoculated into 400 mL of nutrient broth liquid medium containing no carbon source but 400 mg/L ethylene oxide as the inducer, with a live bacteria cell count in the medium being 108-1010 cfu/mL;
Treatment Group 4 (original strain before acclimation/400 mg/L ethylene oxide): 5 mL of the bacterial culture of the EO-degrading potential bacteria (i.e., the original strain before acclimation) obtained according to Example 1, with a live cell count of 1010-1012 cfu/mL, was inoculated into 400 mL of nutrient broth liquid medium containing no carbon source but 400 mg/L ethylene oxide as the inducer, with a live bacteria cell count in the medium being 108-1010 cfu/mL; and
Control Group 2 (No inoculation/400 mg/L ethylene oxide): Nutrient broth liquid medium containing no carbon source but 400 mg/L ethylene oxide without inoculation of the EO-05 strain or EO-degrading potential bacteria.
4. Gas Chromatography (GC) Analysis
To calculate the concentrations of residual ethylene oxide and the degradation rates, samples were taken from the above Treatment groups 1-4 and Control groups 1-2 after the comparative test and sent to the Shaanxi Provincial Center for Disease Control and Prevention for gas chromatography analysis according to the methods described in “Sanitary Standards for Disposable Hygiene Products” (GB15979-2002) of China National Standards as follows:
Additionally, the percentage of increase in the ethylene oxide degradation ability of the strain before and after acclimation was calculated according to the following formula:
Percentage of increase in degradation ability (%)=(Degradation Rate (%) of the strain after acclimation−Degradation Rate (%) of the strain before acclimation)/Degradation Rate (%) of the strain before acclimation).
Other details of the experiment include Column: Chromosorb 101HP60-80 mesh, glass column 2 m long, diameter 3 mm Column temperature: 120° C. Detector: 150° C., Gasifier: 150° C.; Carrier gas volume: Nitrogen: 35 ml/min, Hydrogen: 35 ml/min, Air: 350 ml/min, and the pre-column pressure is about 108 Kpaa.
II. Experimental Results
The experimental results are summarized in Table 2 below. As shown in Table 2, the EO-05 strain was capable of degrading ethylene oxide with concentrations as high as 400 mg/L and 800 mg/L with no carbon source, while the degradation rates were greatly improved compared to the original strain without acclimation. Specifically, the degradation rate of EO-05 strain of 400 mg/L ethylene oxide was as high as 92.90%, which was 350.97% higher than that of the original strain without acclimation. For 800 mg/L ethylene oxide, the EO-05 strain demonstrated a degradation rate of 68.65% and an increase of 585.12% compared to the original strain without acclimation.
Alcaligenes faecalis strain before acclimation
Comparative tests may be carried out in other samples containing ethylene oxide, such as sewage, sludge, exhaust gas, or wastewater, such as industrial (including industries related to petroleum and derivative products), medical treatment (such as ethylene oxide sterilant) and other sewage, sludge, exhaust gas, or wastewater.
An Alcaligenes faecalis strain of the invention comprising the 16S rDNA sequence of SEQ ID NO: 4 can also be used in comparative tests.
In general, ethylene oxide sterilization waste gas can be absorbed into water. The water containing the absorbed ethylene oxide can be contacted with an Alcaligenes faecalis strain of the present invention in a method of biodegrading ethylene oxide. The water containing the absorbed ethylene oxide can be discharged or transferred to an anaerobic vessel, such as an anaerobic sewage tank. An Alcaligenes faecalis strain of the present invention can then be added to the tank, thereby biodegrading the ethylene oxide.
In particular, (1) after the ethylene oxide sterilizer has sterilized, the ethylene oxide sterilization exhaust gas generated is fed into a hydration system, which uses the internal circulating water to absorb the incoming ethylene oxide sterilization exhaust gas, and several cycles of absorption produce ethylene oxide wastewater containing about 243.15 mg/L of ethylene oxide.
(2) The ethylene oxide wastewater with the concentration of about 243.15 mg/L of ethylene oxide was passed into an aerobic bio-ethylene oxide treatment cell inoculated with the EO-05 strain, the strain concentration was 1010-1012 cfu/mL, the inoculation amount was 1%-2%, the EO-05 strain used the active sludge in the aerobic bio-ethylene oxide treatment cell as the culture, ethylene oxide was used as the carbon source and energy for metabolism, growth and proliferation, thus achieving the purpose of ethylene oxide treatment.
The mixture in the treatment cell was continuously stirred, the temperature was controlled at 32° C.-42° C. and the treatment was for 48 hours. The results showed that the residual concentration of ethylene oxide in the treated wastewater was 20.96 mg/L with a treatment efficiency of 91.38%.
The above concentrations were detected by gas chromatography in accordance with GB 15979-2002 (Appendix D), which is explained above. The degradation rate was calculated according to the following formula: Degradation rate=(starting concentration−residual concentration)/starting concentration.
As another practical application, activated sludge can be contacted with an Alcaligenes faecalis strain of the present invention, thereby biodegrading ethylene oxide in the activated sludge.
In the above-described tests and applications, the degradation rate is at least 10%, 15%, 20%, 25%, 30%, 35%, 40%, 50%, 60%, 70%, 75%, 80%, 90%, 95%, 100%, 125%, 150%, 200%, or 500% greater relative to the degradation rate of ethylene oxide in the absence of the Alcaligenes faecalis strain EO-05 or Alcaligenes faecalis strain comprising the 16S rDNA sequence of SEQ ID NO: 4.
The detailed embodiments described herein are only for the purpose of illustrating the present disclosure, and are not intended to limit the scope of the present disclosure in any way. It would be understood by a person skilled in the art that various changes and modifications can be made to the embodiments described herein without departing from the scope and spirit of the present disclosure. Such changes and modifications are contemplated by the present disclosure, the scope of which should only be defined by the following claims.
| Number | Date | Country | Kind |
|---|---|---|---|
| 202010064633.4 | Jan 2020 | CN | national |
| 202010064718.2 | Jan 2020 | CN | national |
This application is a Bypass Continuation of PCT/CN2020/101139, filed Jul. 9, 2020, which application claims the benefit of Chinese Patent Application No. 202010064718.2, filed on Jan. 20, 2020 and Chinese Patent Application No. 202010064633.4, filed on Jan. 20, 2020, the entire contents of which are incorporated herein by reference in their entirety for all purposes.
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| Number | Date | Country | |
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| Number | Date | Country | |
|---|---|---|---|
| Parent | PCT/CN2020/101139 | Jul 2020 | US |
| Child | 17012843 | US |
