WO1992019738A1 - Microbial degradation of trichloroethylene, dichloroethylenes and aromatic pollutants - Google Patents

Microbial degradation of trichloroethylene, dichloroethylenes and aromatic pollutants Download PDF

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Publication number
WO1992019738A1
WO1992019738A1 PCT/US1992/003515 US9203515W WO9219738A1 WO 1992019738 A1 WO1992019738 A1 WO 1992019738A1 US 9203515 W US9203515 W US 9203515W WO 9219738 A1 WO9219738 A1 WO 9219738A1
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hazardous chemicals
chemicals
group
cepacia
degrading
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PCT/US1992/003515
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French (fr)
Inventor
Malcolm S. Shields
Peter J. Chapman
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Sbp Technologies, Inc.
United States Environmental Protection Agency
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Publication of WO1992019738A1 publication Critical patent/WO1992019738A1/en

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    • CCHEMISTRY; METALLURGY
    • C02TREATMENT OF WATER, WASTE WATER, SEWAGE, OR SLUDGE
    • C02FTREATMENT OF WATER, WASTE WATER, SEWAGE, OR SLUDGE
    • C02F3/00Biological treatment of water, waste water, or sewage
    • C02F3/02Aerobic processes
    • C02F3/12Activated sludge processes
    • C02F3/1205Particular type of activated sludge processes
    • C02F3/1231Treatments of toxic sewage
    • CCHEMISTRY; METALLURGY
    • C02TREATMENT OF WATER, WASTE WATER, SEWAGE, OR SLUDGE
    • C02FTREATMENT OF WATER, WASTE WATER, SEWAGE, OR SLUDGE
    • C02F3/00Biological treatment of water, waste water, or sewage
    • C02F3/34Biological treatment of water, waste water, or sewage characterised by the microorganisms used
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N1/00Microorganisms, e.g. protozoa; Compositions thereof; Processes of propagating, maintaining or preserving microorganisms or compositions thereof; Processes of preparing or isolating a composition containing a microorganism; Culture media therefor
    • C12N1/20Bacteria; Culture media therefor
    • C12N1/205Bacterial isolates
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    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N15/00Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
    • C12N15/09Recombinant DNA-technology
    • C12N15/11DNA or RNA fragments; Modified forms thereof; Non-coding nucleic acids having a biological activity
    • C12N15/52Genes encoding for enzymes or proenzymes
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    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N9/00Enzymes; Proenzymes; Compositions thereof; Processes for preparing, activating, inhibiting, separating or purifying enzymes
    • C12N9/0004Oxidoreductases (1.)
    • C12N9/0069Oxidoreductases (1.) acting on single donors with incorporation of molecular oxygen, i.e. oxygenases (1.13)
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12RINDEXING SCHEME ASSOCIATED WITH SUBCLASSES C12C - C12Q, RELATING TO MICROORGANISMS
    • C12R2001/00Microorganisms ; Processes using microorganisms
    • C12R2001/01Bacteria or Actinomycetales ; using bacteria or Actinomycetales
    • C12R2001/38Pseudomonas
    • YGENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
    • Y02TECHNOLOGIES OR APPLICATIONS FOR MITIGATION OR ADAPTATION AGAINST CLIMATE CHANGE
    • Y02WCLIMATE CHANGE MITIGATION TECHNOLOGIES RELATED TO WASTEWATER TREATMENT OR WASTE MANAGEMENT
    • Y02W10/00Technologies for wastewater treatment
    • Y02W10/10Biological treatment of water, waste water, or sewage

Definitions

  • TCE trichloroethylene
  • TCE transformation by anaerobic bacteria indicate a very slow process.
  • the rapid mineralization of TCE by aerobic bacteria has been demonstrated for several microbial isolates. All require the addition of exogenous chemicals to induce production of the requisite TCE degrading enzymes.
  • Toluene serves to induce oxygenase enzymes of Pseudomonas putida
  • cepacia G4 has been shown to proceed via a monooxygenation pathway that results first in an ortho- hydroxylation of toluene (catalyzed by _-toluene monooxygenase) and subsequently a second hydroxylation ortho to the first hydroxyl to form 3- methylcatechol (Shields, M.S., S.O. Montgomery, P . Chapman, S.M. Cuskey, and P.H. Pritchard. 1989. Appl. Environ. Microbiol. 55:1624-1629).
  • U.S. 4,749,491 concerns a method for stimulating indigenous bacteria to degrade chlorinated hydrocarbons through the addition of oxygen and propane or methane.
  • U.S. 4,664,805 concerns a method for degradation of halogenated organic pollutants through the addition of non-toxic chemical analogs with or without non-indigenous microorganisms.
  • U.S. 4,452,894 concerns a pure culture of a Pseudomonas spp. that can utilize a variety of chlorinated aromatic chemicals as sole sources of carbon.
  • U.S. 4,477,570 concerns the isolation of bacterial strains, specifically Pseudomonas cepacia var. niagarous, that degrade aromatic and halogenated aromatic chemicals.
  • U.S. 4,954,258 concerns the additiona of alkanes or lower alkanols to methanotrophic bacteria for the degradation of TCE.
  • U.S. 4,925,802 concerns a method for stimulating biodegradation of halogenated aliphatic hydrocarbons.
  • the method uses microbes and an inducer. Specifically exemplified is the non-constitutive microbe, Pseudomonas cepacia strain G4, which is the parent of the constitutive microbe strain of the subject invention.
  • TCE is necessarily linked to the production of an enzyme that can accept TCE as a surrogate substrate, the native substrate being that which is used to induce the enzyme's synthesis. Due to this co-metabolic relationship, TCE cannot be degraded in the environment without the addition of an exogenous inducing substrate, because TCE does not itself induce the enzymes required for its own degradation. As a result, these prior art organisms are faced with the additional limitation of degrading TCE in the presence of the required co- substrate that competes for the same active site on the induced enzyme. In addition, this also means that the organisms are not active beyond the environmental zone that can be controlled through the addition of effective concentrations of inducer. The active bacteria are effectively "tethered" to the inducing substrate. Both of these limitations have serious implications to the design of both environmental and bioreactor applications. In addition, the application of native inducing substrates such as toluene or phenol is not possible in the environment as they are themselves pollutants.
  • the use of the microbe of the subject invention advantageously, does not have the problems associated with the use of prior art microbes to remediate sites contaminated with hazardous chemicals.
  • the microbe of the invention P. cepacia strain G45223 Phe (1), is a natural bacterial isolate that can function over a wide range of environmental conditions without the need for an added chemical inducer; it has a very high likelihood of competitive maintenance among native bacteria over the course of a given treatment; and it has evolved to utilize and grow on many organic pollutants likely to be found at waste treatment sites.
  • the subject invention concerns the use of a novel bacterial strain to degrade TCE over a wide range of environmental parameters without the requirement for added chemical inducers.
  • the subject invention concerns the use of the novel strain designated Pseudomonas cepacia strain G4 5223 Phe (1) to degrade hazardous chemicals, for example, trichloroethylene (TCE), cis-1,2- dichloroethylene, trans-l,2-dichloroethylene, 1,1-dichloroethylene, and aromatic chemicals, for example benzene, phenol, toluene, o-xylene, m-xylene, o-cresol, and m-cresol.
  • TCE trichloroethylene
  • trans-l,2-dichloroethylene 1,1-dichloroethylene
  • aromatic chemicals for example benzene, phenol, toluene, o-xylene, m-xylene, o-cresol, and m-cresol.
  • the novel bacterium is fully capable of the complete removal of the aforementioned pollutants under a variety of conditions, without the need to artificially or externally influence existing
  • this novel bacterium is an attractive biodegradative agent for remediation of TCE pollution for two reasons. First, and most importantly, the organism is free of the requirement of inducer and capable of functioning under a diverse set of conditions. Second, this constitutive degrader does not require an inducer that is a co-substrate for the same enzyme required to degrade TCE; in effect, it is not subject to competitive inhibition. As such, it can be used in both in situ environmental and bioreactor remediation processes.
  • the subject invention also includes the genes(s) harbored by the novel bacterium which gene(s) encode enzyme(s) capable of degrading the hazardous chemicals.
  • gene(s) can be isolated from the parent bacterium by using well-known cloning techniques.
  • the isolated gene(s) can be used to transform other microbes by use of well-known transfer and expression vectors.
  • the transformed host can be used in the same manner as the parent microbe to degrade hazardous chemical compounds.
  • the enzyme(s) responsible for the degradation of the hazardous chemical compounds can be recovered from the extracts of cultures of the novel bacterium and used to degrade hazardous chemical compounds by procedures well known in the art.
  • Figure 1 Illustrates the first two oxidations performed on toluene by P. cepacia G4.
  • Figure 2 A presentation of the probable route of oxidation of the m- cresol analog: 3-trifluoromethylphenol (TFMP) to the yellow ring-cleavage product.
  • TFMP 3-trifluoromethylphenol
  • FIG 3 A portrayal of the known catabolic transformations associated with the initial enzymes of toluene catabolism in P. cepacia G4.
  • FIG. 4 The effects of several environmental variables on the initial (i.e., over the first 1-2 hr) rate of TCE degradation by P. cepacia G4 5223 are shown.
  • accession number is as follows:
  • the taxonomy of Pseudomonas cepacia strain G4 5223 Phe(l) is as follows:
  • Pseudomonas cepacia G4 5223 Phe(l) is an oxidase-positive and catalase-positive gram-negative obligately aerobic rod. It reduces nitrate to nitrite, is incapable of denitrification, and is unable to ferment glucose or hydrolyze esculin. Tests for urease, gelatinase, and arginine dihydrolase activity were negative.
  • Beta-galactosidase activity is present and substrate utilization tests showed growth on D-glucose, D-arabinose, D-mannose, mannitol, N- acetyl-D-glucosamine, maltose, gluconate, caprate, adipate, citrate, and phenylacetate. L-malate is not utilized. Neither pyocyanin or fluorescein pigments are formed on selective media (King, E.O., M.K. Ward, and D.E. Raney. 1954. J. Lab. Clin. Med. 44:301). Pseudomonas cepacia G4 5223 Phe(l) is resistant to kanamycin sulfate (50 ⁇ g/ml) in basal salts medium
  • the procedure of application of P. cepacia G4 5223 Phe(l) to the remediation of TCE-contaminated materials may be carried out through the use of various known procedures.
  • the organism may be used in a bioreatcor (fixed film, fluidized bed, etc.) as well as in situ by methods generally such as those disclosed in U.S. Patent Nos. 4,749,491 and 4,588,506.
  • Enzyme(s) produced by the novel microbe of the invention can be recovered from the cultured cells of the microbe.
  • the recovery process can be one in which the microbial cells at harvest are extracted and the enzyme(s) recovered by standard procedures.
  • the resulting enzyme preparation can be used to degrade hazardous chemicals, as disclosed herein.
  • the treatment of hazaradous chemicals with an enzyme preparation can be by use of columns and other means well known in the enzyme art.
  • the enzyme preparation so used can be in either a crude or essentially pure form.
  • Novel recombinant microbes can be made by isolating the gene(s) from
  • the gene(s) encode enzymes which are capable of degrading hazardous chemical compounds.
  • a wide variety of ways are available for introducing a gene into a microorganism host under conditions which allow for stable maintenance and expression of the gene.
  • Various manipulations may be employed for enhancing the expression of the messenger RNA, particularly by using an active promoter, as well as by employing sequences, which enhance the stability of the messenger RNA.
  • the transcriptional and translational termination region will involve stop codon(s), a terminator region, and optionally, a polyadenylation signal.
  • the construct will involve the transcriptional regulatory region, if any, and the promoter, where the regulatory region may be either 5' or 3' of the promoter, the ribosomal binding site, the initiation codon, the structural gene having an open reading frame in phase with the initiation codon, the stop codon(s), the polyadenylation signal sequence, if any, and the terminator region.
  • This sequence as a double strand may be used by itself for transformation of a microorganism host, but will usually be included with a DNA sequence involving a marker, where the second DNA sequence may be joined to the expression construct during introduction of the DNA into the host.
  • a marker structural gene is used to provide for the selection of the host microbe which has acquired the desired nucleotide sequence. (via, for example, transformation, electroporation, conjugation, or phage mediated).
  • the marker will normally provide for selective advantage, for example, providing for biocide resistance, e.g., resistance to antibiotics or heavy metals; complementation, so as to provide, prototrophy to an auxotrophic host, or the like.
  • complementation is employed, so that the modified host may not only be selected, but may also be competitive in the field.
  • One or more markers may be employed in the development of the constructs, as well as for modifying the host.
  • the organisms may be further modified by providing for a competitive advantage against other wild-type microorganisms in the field.
  • genes expressing metal chelating agents may be introduced into the host along with the structural gene.
  • the enhanced expression of a siderophore may provide for a competitive advantage for the host, so that it may effectively compete with wild-type microorganisms.
  • the construct will also include a sequence of at least 50 basepairs (bp), preferably at least about 100 bp, and usually not more than about 1000 bp of a sequence homologous with a sequence in the host.
  • bp basepairs
  • the gene will be in close proximity to the gene providing for complementation as well as the gene providing for the competitive advantage. Therefore, in the event that a gene is lost, the resulting organism will be likely to also lose the complementing gene and/or the gene providing for the competitive advantage, so that it will be unable to compete in the environment with the organism retaining the intact construct.
  • transcriptional regulatory regions are available from a wide variety of microorganism hosts, such as bacteria, bacteriophage, cyanobacteria, algae, fungi, and the like.
  • Various transcriptional regulatory regions include the regions associated with the trp gene, lac gene, gal gene, the lambda left and right promoters, the Tac promoter, the naturally-occurring promoters associated with the gene, where functional in the host.
  • the termination region may be the termination region normally associated with the transcriptional termination region or a different transcriptional termination region, so long as the two regions are compatible and functional in the host. Where stable episomal maintenance or integration is desired, a plasmid will be employed which has a replication system which is functional in the host.
  • the replication system may be derived from the chromosome, an episomal element normally present in the host or a different host, or a replication system from a virus which is stable in the host.
  • the gene can be introduced between the transcriptional and translational initiation region and the transcriptional and translational termination region, so as to be under the regulatory control of the initiation region.
  • This construct will be included in a plasmid, which will include at least one replication system, but may include more than one, where one replication system is employed for cloning during the development of the plasmid and the second replication system is necessary for functioning in the ultimate host.
  • one or more markers may be present, which have been described previously.
  • the plasmid will desirably include a sequence homologous with the host genome.
  • the transformants can be isolated in accordance with conventional ways, usually employing a selection technique, which allows for selection of the desired organism as against unmodified organisms or transferring organisms, when present. The transformants then can be tested for degrading hazardous chemical compounds.
  • Suitable host cells can be Gram-negative bacteria, including Enterobacteriaceae, such as Escherichia. and other Pseudomonadaceae.
  • the recombinant cellular host containing the gene(s) may be grown in any convenient nutrient medium, where the DNA construct provides a selective advantage, providing for a selective medium so that substantially all or all of the cells retain the gene. These cells may then be harvested in accordance with conventional ways.
  • Mutants of this pathway were detectable in the presence of the fluorinated analog of m-cresol; m-trifluoromethylphenol (TFMP) (Aldrich Chemical Co., Milwaukee, WI). Wild type cells were capable of the oxidation of TFMP to a bright yellow transformation product presumed to be 7,7,7- trifluoro-2-hydroxy-6-oxo-2,4-heptadienoic acid (Engesser, K.H., R.B. Cain, and HJ. Knackmuss. 1988. Arch. Microbiol. 149:188-197). Due to anticipated structural similarities between TFMP oxidation products and intermediates of the toluene pathway, it was predicted that mutants failing to produce yellow color with TFMP would lack either the cresol monooxidation or catechol dioxygenation functions. See Figure 2.
  • Mutants were characterized according to their ability to grow with different aromatic substances and their reaction with TFMP as shown in Table 1. Table 1. Mutant Phenotypes
  • Enzyme activities were derived from lactate grown cells following 6 hours exposure to air-entrained toluene vapor. Cell free extracts were analyzed for catechol-2,3-dioxygenase (Gibson, D.T. 1971. pg. 462-478. In D.J.R. Norris and D.W. Ribbons. Methods in Microbiology, 1971 Academic Press, New York), hydroxymuconic semialdehyde (Hms) hydrolase and Hms dehydrogenase activities (Bayly, R.C., and G.J. Wigmore. 1973. J. Bacteriol. 113:1112-1120).
  • TCE Cells representative of the different mutant classes were induced using toluene and analyzed for their ability to degrade TCE. Washed cells were resuspended in basal salts medium containing 20 ⁇ M TCE to a cell density that yielded an absorbance at 600 nm of 0.2. These samples were sealed in 10ml glass vials with Teflon-lined rubber septa and crimp rings. These vials were incubated inverted at 24 degrees C overnight with rotary shaking (180 rpm). TCE was extracted by injection of two ml pentane (HPLC grade, Aldrich Chemical Co.) with rotary shaking in an upright position at 180 rpm, 24 degrees C for 30 minutes.
  • the pentane phase was transferred to GC vials with Teflon liners and analyzed on an HP 5790 gas chromatograph equipped with an autosampler and electron capture detector. Separation was achieved with a Vocol capillary column, 30 m, 0.53 mm ID, fused silica, 3.0 ⁇ m film thickness (Supelco, Inc., Bellefonte, PA #2-5320) at 50 degrees C.
  • strain G4 100R1 fully regained both its ability to express the toluene o-monooxygenase as well as degrade TCE.
  • Example 3 Isolation of a Tn5 Induced Toluene Monooxygenase Mutant of P. Cepacia G4
  • Transposon mutagenesis was carried by a triparental mating: E. coli JM109 (pRZ102) (Jorgensen, R.A., S.J. Rothstein, and W.S. Reznikoff. 1979. Molec. Genet. 177:65-72) X E. coli JM109 (pRK2013) (Figurski, D.H., and D.R. Helinski. 1979. Proc. Natl. Acad. Sci. USA. 76:1648-1652) X P. cepacia G4. Selection for P.
  • cepacia G4 containing a transposed copy of Tn5 was accomplished by growth of the mating mixture on basal salts medium containing 20 mM sodium lactate and 50 ⁇ g/ml kanamycin sulfate. Exposure to toluene vapor induced the requisite enzymes for toluene catabolism. Colonies were transferred from the surface of the plate to nitrocellulose filters (0.45 ⁇ pore size, Schliecher and Schuell, Keene, NH) previously soaked in an aqueous solution of 5mM TFMP and air dried. Mutants tomA and tomB (i.e.
  • Transposon (Tn5) mutants of tomA were inoculated by patching to basal salts plates containing 2 mM phenol as the sole carbon source. Rare colonies arising were picked to basal salts medium containing 20mM sodium lactate as the sole carbon source. These colonies were in turn pulled to nitrocellulose discs impregnated with TFMP (Example 3) and compared to wild type P. cepacia G4 similarly grown on this non-inducing medium. Colonies that became yellow were picked as potentially constitutive for tomA and tomB gene products. In this way P. cepacia strain G4 5223 Phe(l) was isolated. Table 4: TCE degradation without inducer
  • the genetic stability of the invention strain was assessed by growing the cells under non-selective (i.e. basal salts medium with sodium lactate at 20 mM as the sole carbon source) and under selective conditions (i.e. the same medium containing in addition 50 ⁇ g kanamycin sulphate/ml) through serially diluted batch cultures, allowing 10 generations per transfer. Following the accumulation of ca. 100 generations, the resulting population of cells was tested for kanamycin resistance (in the non-selective group) and the ability to constitutively transform TFMP to a yellow product (both groups):
  • Lactate-grown colonies were picked to lactate plates containing 50 ⁇ g/ml kanamycin. Those from 100 generations without selection exhibited 100% kanamycin resistance (150/150) as did those taken from kanamycin growth selection (75/75).
  • Example 6 Contitutive Degradation of 1.1-Dichloroethylene. cis-1.2- Dichloroethylene. and trans-1.2-Dichloroethylene
  • the range of chlorinated aliphatic substrates acted upon by P. cepacia G4 5223 Phe(l) was determined by the ability of cells to degrade 10 ⁇ M TCE, 1,1-Dichloroethylene, cis-l,2-Dichloroethylene, trans-L2-Dichloroethylene and tetrachloroethylene in 2 ml of basal salts medium without additional carbon sources in 10 ml Teflon lined vessels during an overnight incubation at 24 degrees C. Triplicate samples were analyzed by gas chromatography for appearance of detectable products as well as disappearance of parent compounds: Table 7: Chloroaliphatic substrates of P. cepacia G4 5223 Phef 1.
  • a Percent substrate remaining as compared to uninoculated controls abbreviations: 1,1-DCE, 1,1-Dichloroethylene; cis-l,2-DCE, cis-1,2- Dichloroethylene; trans.-l,2-DCE, trans-l,2-Dichloroethylene; TCE, Trichloroethylene; PCE, Perchloroethylene; ND, Not Detectable. Starting concentration was 10 ⁇ M for all substrates. M indicates that a metabolite was detected using gas chromatography.

Abstract

A novel bacterium named Pseudomonas cepacia G4 5223 Phe(1) has the desirable property of constitutively degrading hazardous chemicals, for example trichloroethylene, 1,1-dichloroethylene, cis-1,2 dichloroethylene, trans-1,2-dichloroethylene, toluene, phenol, o-cresol, m-cresol, o-xylene, and benzene, to harmless chemical entities. This microbe, and mutants thereof which retain the constitutive degradation property of the parent, can be used in bioreactor and in situ processes for degrading hazardous chemical compounds.

Description

DESCRIPTION
MICROBIAL DEGRADATION OF TRICHLOROETHYLENE. DICHLOROETHYLENES AND AROMATIC POLLUTANTS
Background of the Invention Groundwater contamination by organic pollutants is a subject of major concern in the United States and, increasingly, the rest of the industrialized world. The sources of pollution are almost as numerous as the types of pollutants found. Sources range from agricultural uses, injection wells, underground storage tanks and hazardous waste sites, to illegal dumping in localities with no prior history of toxic chemical exposure. In monitoring chemical waste disposal sites within the United States, pollutants have been categorized according to the frequency of detection of certain chemical classes and specific chemicals within that class. The priority pollutants are divided into volatiles, acid extractables, pesticides and base/neutrals. Volatiles are the most frequently detected group, owing largely to their widespread use as solvents. The most often encountered components of these volatile chemical pollutants in 1986 were, in order of frequency, tri-chloroethylene, tetrachloroethylene, trans-1, 2-dichloroethylene, 1,1-dichloroethylene, (ranked first, second, third and fifth respectively of all volatiles detected (Rajagopal, R. 1986. Environ. Prof. 8:244-264). The most prevalent of these, trichloroethylene (TCE), has been in use since the 1940's, and the subject of environmental and human health concerns since its discovery in a contaminated aquifer in 1979 (Muntner, J.E., and S.P. Devries, 1987. Toxics Law Reporter, Jan. 14:874).
All reports of TCE transformation by anaerobic bacteria indicate a very slow process. The rapid mineralization of TCE by aerobic bacteria has been demonstrated for several microbial isolates. All require the addition of exogenous chemicals to induce production of the requisite TCE degrading enzymes. Toluene serves to induce oxygenase enzymes of Pseudomonas putida
Fl (Nelson, M.J.K., S.O. Montgomery, and P.H. Pritchard. 1988. App. Environ. Microbiol. 54:604-606) and P. cepacia G4 (Nelson, M.J.K., S.O. Montgomery, E. J. O'Neill, and P.H. Pritchard. 1986. Appl. Environ. Microbiol. 42:383-384). These enzymes are in turn responsible for TCE degradation by these bacteria. The route of toluene catabolism by P. cepacia G4 has been shown to proceed via a monooxygenation pathway that results first in an ortho- hydroxylation of toluene (catalyzed by _-toluene monooxygenase) and subsequently a second hydroxylation ortho to the first hydroxyl to form 3- methylcatechol (Shields, M.S., S.O. Montgomery, P . Chapman, S.M. Cuskey, and P.H. Pritchard. 1989. Appl. Environ. Microbiol. 55:1624-1629).
U.S. Patents concerning bioremediation are as follow: 4,749,491; 4,452,894; 4,664,805; 4,477,570; 4,925,802; 4,954,258.
U.S. 4,749,491 concerns a method for stimulating indigenous bacteria to degrade chlorinated hydrocarbons through the addition of oxygen and propane or methane.
U.S. 4,664,805 concerns a method for degradation of halogenated organic pollutants through the addition of non-toxic chemical analogs with or without non-indigenous microorganisms.
U.S. 4,452,894 concerns a pure culture of a Pseudomonas spp. that can utilize a variety of chlorinated aromatic chemicals as sole sources of carbon. U.S. 4,477,570 concerns the isolation of bacterial strains, specifically Pseudomonas cepacia var. niagarous, that degrade aromatic and halogenated aromatic chemicals.
U.S. 4,954,258 concerns the additiona of alkanes or lower alkanols to methanotrophic bacteria for the degradation of TCE.
U.S. 4,925,802 concerns a method for stimulating biodegradation of halogenated aliphatic hydrocarbons. The method uses microbes and an inducer. Specifically exemplified is the non-constitutive microbe, Pseudomonas cepacia strain G4, which is the parent of the constitutive microbe strain of the subject invention.
Current technology for the treatment of TCE-contaminated soil and water has relied primarily upon pump-and-treat systems whereby TCE is distilled away from the water under vacuum, or alternatively is air-stripped and transferred onto an adsorbent such as charcoal. Recent reviews of this subject strongly question whether this technology alone will ever be effective in the remediation of hazardous wastes like TCE, since even long term treatments have had only modest effects on pollutant concentrations (Travis, C.C., and C.B. Doty. 1990. Environ. Sci. Technol. 24:1464-1466). In either event, the result of such treatment is simply the transfer of the pollutant to an adsorbent or to the atmosphere. The capability to destroy the contaminant at the site would represent significant environmental and economic benefits. If realized, efficient bioremediation technologies would fill this need. Major limitations to the bacterial systems described in the prior art for the bioremediation of TCE is that they all degrade TCE fortuitously. That is to say their ability to alter
TCE is necessarily linked to the production of an enzyme that can accept TCE as a surrogate substrate, the native substrate being that which is used to induce the enzyme's synthesis. Due to this co-metabolic relationship, TCE cannot be degraded in the environment without the addition of an exogenous inducing substrate, because TCE does not itself induce the enzymes required for its own degradation. As a result, these prior art organisms are faced with the additional limitation of degrading TCE in the presence of the required co- substrate that competes for the same active site on the induced enzyme. In addition, this also means that the organisms are not active beyond the environmental zone that can be controlled through the addition of effective concentrations of inducer. The active bacteria are effectively "tethered" to the inducing substrate. Both of these limitations have serious implications to the design of both environmental and bioreactor applications. In addition, the application of native inducing substrates such as toluene or phenol is not possible in the environment as they are themselves pollutants.
The use of the microbe of the subject invention, advantageously, does not have the problems associated with the use of prior art microbes to remediate sites contaminated with hazardous chemicals. Briefly, the microbe of the invention, P. cepacia strain G45223 Phe (1), is a natural bacterial isolate that can function over a wide range of environmental conditions without the need for an added chemical inducer; it has a very high likelihood of competitive maintenance among native bacteria over the course of a given treatment; and it has evolved to utilize and grow on many organic pollutants likely to be found at waste treatment sites.
Brief Summary of the Invention The subject invention concerns the use of a novel bacterial strain to degrade TCE over a wide range of environmental parameters without the requirement for added chemical inducers.
More specifically, the subject invention concerns the use of the novel strain designated Pseudomonas cepacia strain G4 5223 Phe (1) to degrade hazardous chemicals, for example, trichloroethylene (TCE), cis-1,2- dichloroethylene, trans-l,2-dichloroethylene, 1,1-dichloroethylene, and aromatic chemicals, for example benzene, phenol, toluene, o-xylene, m-xylene, o-cresol, and m-cresol. The novel bacterium is fully capable of the complete removal of the aforementioned pollutants under a variety of conditions, without the need to artificially or externally influence existing conditions (i.e. induce the requisite enzymes). Without the need for exogenous chemical inducers, this novel bacterium is an attractive biodegradative agent for remediation of TCE pollution for two reasons. First, and most importantly, the organism is free of the requirement of inducer and capable of functioning under a diverse set of conditions. Second, this constitutive degrader does not require an inducer that is a co-substrate for the same enzyme required to degrade TCE; in effect, it is not subject to competitive inhibition. As such, it can be used in both in situ environmental and bioreactor remediation processes.
The subject invention also includes the genes(s) harbored by the novel bacterium which gene(s) encode enzyme(s) capable of degrading the hazardous chemicals. These gene(s) can be isolated from the parent bacterium by using well-known cloning techniques. The isolated gene(s) can be used to transform other microbes by use of well-known transfer and expression vectors. The transformed host can be used in the same manner as the parent microbe to degrade hazardous chemical compounds. Further, the enzyme(s) responsible for the degradation of the hazardous chemical compounds can be recovered from the extracts of cultures of the novel bacterium and used to degrade hazardous chemical compounds by procedures well known in the art.
Brief Description of the Drawings Figure 1 Illustrates the first two oxidations performed on toluene by P. cepacia G4.
Figure 2 A presentation of the probable route of oxidation of the m- cresol analog: 3-trifluoromethylphenol (TFMP) to the yellow ring-cleavage product.
Figure 3 A portrayal of the known catabolic transformations associated with the initial enzymes of toluene catabolism in P. cepacia G4.
Figure 4 The effects of several environmental variables on the initial (i.e., over the first 1-2 hr) rate of TCE degradation by P. cepacia G4 5223 are shown.
Detailed Disclosure of the Invention Upon contact with a culture of Pseudomonas cepacia strain G4 5223
Phe(l), or a mutant thereof which retains substantially the degradative capability of the parent bacterium, with a hazardous chemical, as defined herein, the hazardous chemical is degraded to a non-hazardous entity.
A subculture of P. cepacia strain G4 5223 Phe(l) has been deposited in the permanent collection of the Agricultural Research Service Culture
Collection, Peoria, Illinois. The accession number is as follows:
Pseudomonas cepacia strain G4 5223 Phe(l) NRRLB-18811
The taxonomy of Pseudomonas cepacia strain G4 5223 Phe(l) is as follows:
Pseudomonas cepacia G4 5223 Phe(l) is an oxidase-positive and catalase-positive gram-negative obligately aerobic rod. It reduces nitrate to nitrite, is incapable of denitrification, and is unable to ferment glucose or hydrolyze esculin. Tests for urease, gelatinase, and arginine dihydrolase activity were negative. Beta-galactosidase activity is present and substrate utilization tests showed growth on D-glucose, D-arabinose, D-mannose, mannitol, N- acetyl-D-glucosamine, maltose, gluconate, caprate, adipate, citrate, and phenylacetate. L-malate is not utilized. Neither pyocyanin or fluorescein pigments are formed on selective media (King, E.O., M.K. Ward, and D.E. Raney. 1954. J. Lab. Clin. Med. 44:301). Pseudomonas cepacia G4 5223 Phe(l) is resistant to kanamycin sulfate (50μg/ml) in basal salts medium
(Hareland, W., R.L. Crawford, PJ. Chapman, and S. Dagley. 1975. J. Bacteriol 121:272-285) containing 20mM sodium lactate as the sole carbon source and is also capable of growth with penicillin G (5mg/ml) as the sole carbon source. In addition, its demonstrated ability to store excess carbon as a microbial polyhydroxyalkanoate polyester may offer an excellent method to prolong degradative functions under the most extreme conditions.
The procedure of application of P. cepacia G4 5223 Phe(l) to the remediation of TCE-contaminated materials may be carried out through the use of various known procedures. For example the organism may be used in a bioreatcor (fixed film, fluidized bed, etc.) as well as in situ by methods generally such as those disclosed in U.S. Patent Nos. 4,749,491 and 4,588,506. Enzyme(s) produced by the novel microbe of the invention can be recovered from the cultured cells of the microbe. The recovery process can be one in which the microbial cells at harvest are extracted and the enzyme(s) recovered by standard procedures. The resulting enzyme preparation can be used to degrade hazardous chemicals, as disclosed herein. The treatment of hazaradous chemicals with an enzyme preparation, as disclosed above, can be by use of columns and other means well known in the enzyme art. The enzyme preparation so used can be in either a crude or essentially pure form. Novel recombinant microbes can be made by isolating the gene(s) from
P. cepacia strain G4 5223 Phe(l) and transforming suitable hosts with the gene(s). The gene(s) encode enzymes which are capable of degrading hazardous chemical compounds.
A wide variety of ways are available for introducing a gene into a microorganism host under conditions which allow for stable maintenance and expression of the gene. One can provide for DNA constructs which include the transcriptional and translational regulatory signals for expression of the gene, the gene under their regulatory control and a DNA sequence homologous with a sequence in the host organism, whereby integration will occur, and/or a replication system which is functional in the host, whereby integration or stable maintenance will occur. Various manipulations may be employed for enhancing the expression of the messenger RNA, particularly by using an active promoter, as well as by employing sequences, which enhance the stability of the messenger RNA. The transcriptional and translational termination region will involve stop codon(s), a terminator region, and optionally, a polyadenylation signal. In the direction of transcription, namely in the 5' to 3' direction of the coding or sense sequence, the construct will involve the transcriptional regulatory region, if any, and the promoter, where the regulatory region may be either 5' or 3' of the promoter, the ribosomal binding site, the initiation codon, the structural gene having an open reading frame in phase with the initiation codon, the stop codon(s), the polyadenylation signal sequence, if any, and the terminator region. This sequence as a double strand may be used by itself for transformation of a microorganism host, but will usually be included with a DNA sequence involving a marker, where the second DNA sequence may be joined to the expression construct during introduction of the DNA into the host.
A marker structural gene is used to provide for the selection of the host microbe which has acquired the desired nucleotide sequence. (via, for example, transformation, electroporation, conjugation, or phage mediated). The marker will normally provide for selective advantage, for example, providing for biocide resistance, e.g., resistance to antibiotics or heavy metals; complementation, so as to provide, prototrophy to an auxotrophic host, or the like. Preferably, complementation is employed, so that the modified host may not only be selected, but may also be competitive in the field. One or more markers may be employed in the development of the constructs, as well as for modifying the host. The organisms may be further modified by providing for a competitive advantage against other wild-type microorganisms in the field. For example, genes expressing metal chelating agents, e.g., siderophores, may be introduced into the host along with the structural gene. In this manner, the enhanced expression of a siderophore may provide for a competitive advantage for the host, so that it may effectively compete with wild-type microorganisms.
Where no functional replication system is present, the construct will also include a sequence of at least 50 basepairs (bp), preferably at least about 100 bp, and usually not more than about 1000 bp of a sequence homologous with a sequence in the host. In this way, the probability of legitimate recombination is enhanced, so that the gene will be integrated into the host and stably maintained by the host. Desirably, the gene will be in close proximity to the gene providing for complementation as well as the gene providing for the competitive advantage. Therefore, in the event that a gene is lost, the resulting organism will be likely to also lose the complementing gene and/or the gene providing for the competitive advantage, so that it will be unable to compete in the environment with the organism retaining the intact construct. A large number of transcriptional regulatory regions are available from a wide variety of microorganism hosts, such as bacteria, bacteriophage, cyanobacteria, algae, fungi, and the like. Various transcriptional regulatory regions include the regions associated with the trp gene, lac gene, gal gene, the lambda left and right promoters, the Tac promoter, the naturally-occurring promoters associated with the gene, where functional in the host. The termination region may be the termination region normally associated with the transcriptional termination region or a different transcriptional termination region, so long as the two regions are compatible and functional in the host. Where stable episomal maintenance or integration is desired, a plasmid will be employed which has a replication system which is functional in the host.
The replication system may be derived from the chromosome, an episomal element normally present in the host or a different host, or a replication system from a virus which is stable in the host.
The gene can be introduced between the transcriptional and translational initiation region and the transcriptional and translational termination region, so as to be under the regulatory control of the initiation region. This construct will be included in a plasmid, which will include at least one replication system, but may include more than one, where one replication system is employed for cloning during the development of the plasmid and the second replication system is necessary for functioning in the ultimate host. In addition, one or more markers may be present, which have been described previously. Where integration is desired, the plasmid will desirably include a sequence homologous with the host genome.
The transformants can be isolated in accordance with conventional ways, usually employing a selection technique, which allows for selection of the desired organism as against unmodified organisms or transferring organisms, when present. The transformants then can be tested for degrading hazardous chemical compounds.
Suitable host cells can be Gram-negative bacteria, including Enterobacteriaceae, such as Escherichia. and other Pseudomonadaceae.
The recombinant cellular host containing the gene(s) may be grown in any convenient nutrient medium, where the DNA construct provides a selective advantage, providing for a selective medium so that substantially all or all of the cells retain the gene. These cells may then be harvested in accordance with conventional ways.
Following are examples which illustrate procedures, including the best mode, for practicing the invention. These examples should not be construed as limiting. All percentages are by weight and all solvent mixture proportions are by volume unless otherwise noted.
Example 1: Aromatic degradative pathway of P. cepacia G4
The toluene catabolic pathway of P. cepacia G4 was established using mutants induced with nitrosoguanidine and heavy oxygen isotope incorporation into the catabolic products (Shields, M.S., S.O. Montgomery, PJ. Chapman,
S.M. Cuskey, and P.H. Pritchard. 1989. Appl. Environ. Microbiol. 55:1624- 1629). See Figure 1.
Mutants of this pathway were detectable in the presence of the fluorinated analog of m-cresol; m-trifluoromethylphenol (TFMP) (Aldrich Chemical Co., Milwaukee, WI). Wild type cells were capable of the oxidation of TFMP to a bright yellow transformation product presumed to be 7,7,7- trifluoro-2-hydroxy-6-oxo-2,4-heptadienoic acid (Engesser, K.H., R.B. Cain, and HJ. Knackmuss. 1988. Arch. Microbiol. 149:188-197). Due to anticipated structural similarities between TFMP oxidation products and intermediates of the toluene pathway, it was predicted that mutants failing to produce yellow color with TFMP would lack either the cresol monooxidation or catechol dioxygenation functions. See Figure 2.
Mutants were characterized according to their ability to grow with different aromatic substances and their reaction with TFMP as shown in Table 1. Table 1. Mutant Phenotypes
Figure imgf000012_0001
product is indicated by "+". "Toluene (Tol), phenol(Phe), o-cresol (o-Cre) and m-cresol (m-Cre). TFMP conversion was not detectable in colonies due to accumulation of either brown (Br) or yellow (Ye) colored products formed in the presence of inducer. dVery slow growth (5-7 days for recognizable colonies). These classes of mutants were further characterized and confirmed by examination of the effects of mutation on whole cell oxygen uptake in the presence of different substrates and by measurement of the specific activities of enzymes in cell free extracts as shown in Table 2. Table 2. Cell Free Enzyme Activities
Figure imgf000013_0001
cell- free extracts obtained from cells induced with toluene. bAbbreviations: C230, catechol-2,3-dioxygenase, Cat, catechol; 3mCat, 3- methylcatechol; Hms, hydroxymuconic semialdehyde; Hod, 2-hydroxy-6- ketohepta- 2,4-dienoate.
Enzyme activities were derived from lactate grown cells following 6 hours exposure to air-entrained toluene vapor. Cell free extracts were analyzed for catechol-2,3-dioxygenase (Gibson, D.T. 1971. pg. 462-478. In D.J.R. Norris and D.W. Ribbons. Methods in Microbiology, 1971 Academic Press, New York), hydroxymuconic semialdehyde (Hms) hydrolase and Hms dehydrogenase activities (Bayly, R.C., and G.J. Wigmore. 1973. J. Bacteriol. 113:1112-1120).
This allowed the summation of data into the form of this comprehensive aromatic pathway cluster of P. cepacia G4 as shown in Figure 3. Example 2: Toluene o-Monooxygenase of P. cepacia G4 is Required for TCE Degradation
Cells representative of the different mutant classes were induced using toluene and analyzed for their ability to degrade TCE. Washed cells were resuspended in basal salts medium containing 20 μM TCE to a cell density that yielded an absorbance at 600 nm of 0.2. These samples were sealed in 10ml glass vials with Teflon-lined rubber septa and crimp rings. These vials were incubated inverted at 24 degrees C overnight with rotary shaking (180 rpm). TCE was extracted by injection of two ml pentane (HPLC grade, Aldrich Chemical Co.) with rotary shaking in an upright position at 180 rpm, 24 degrees C for 30 minutes. The pentane phase was transferred to GC vials with Teflon liners and analyzed on an HP 5790 gas chromatograph equipped with an autosampler and electron capture detector. Separation was achieved with a Vocol capillary column, 30 m, 0.53 mm ID, fused silica, 3.0 μm film thickness (Supelco, Inc., Bellefonte, PA #2-5320) at 50 degrees C.
Only the mutant impaired in its toluene monooxygenase activity, (tomA)-, failed to degrade TCE. The spontaneous revertant of this mutant: strain G4 100R1 fully regained both its ability to express the toluene o-monooxygenase as well as degrade TCE.
Table 3: TCE degradation by cells induced with Phenol or Toluene
Figure imgf000015_0001
aMeans of triplicate TCE determinations (± standard deviation) after 24 h, using either toluene- (Tol) or phenol- (Phe) induced cultures. bPhenol or toluene induction of G4 was accomplished by exposing an overnight 20 mM lactate culture to 2 mM phenol or toluene. Two hr later the cells were harvested by centrifugation, washed and exposed to TCE in sealed vials with air headspaces.
Example 3: Isolation of a Tn5 Induced Toluene Monooxygenase Mutant of P. Cepacia G4
A method was developed for the isolation of transposon induced tomA mutants: Transposon mutagenesis was carried by a triparental mating: E. coli JM109 (pRZ102) (Jorgensen, R.A., S.J. Rothstein, and W.S. Reznikoff. 1979. Molec. Genet. 177:65-72) X E. coli JM109 (pRK2013) (Figurski, D.H., and D.R. Helinski. 1979. Proc. Natl. Acad. Sci. USA. 76:1648-1652) X P. cepacia G4. Selection for P. cepacia G4 containing a transposed copy of Tn5 was accomplished by growth of the mating mixture on basal salts medium containing 20 mM sodium lactate and 50 μg/ml kanamycin sulfate. Exposure to toluene vapor induced the requisite enzymes for toluene catabolism. Colonies were transferred from the surface of the plate to nitrocellulose filters (0.45 μ pore size, Schliecher and Schuell, Keene, NH) previously soaked in an aqueous solution of 5mM TFMP and air dried. Mutants tomA and tomB (i.e. those lacking the toluene monooxygenase and catechol dioxygenase respectively) are easily differentiated as colorless colonies among a background of yellow wild type colonies. The two mutant types are readily distinguishable from one another as the catechol-2,3-dioxygenase mutant (tomB) turns brown in (>12Hr) basal salts media containing 20 mM sodium lactate and 2mM phenol (due to the accumulation and subsequent auto- oxidation of catechol). Mutants lacking toluene monoxygenase (tomA) do not.
Incorporation of TFMP in solid media was not sufficient to determine a single colony response as the color development required several minutes over which time the yellow product diffused throughout the plate. The nitrocellulose membrane lift technique was developed in response to this limitation. Colonies transferred to its surface immediately begin desiccation.
Any water soluble yellow product produced by that colony does not diffuse away. The result is a distinct yellow coloration of all colonies capable of transforming TFMP to the yellow product.
Using this technique the transposon mutant, P. cepacia G4 5223 was isolated. This mutant class (typified by G4100) lacked the ability to transform
TFMP and to degrade TCE.
Example 4: Procedure for Isolation of a Constitutive TCE Degrader
Transposon (Tn5) mutants of tomA were inoculated by patching to basal salts plates containing 2 mM phenol as the sole carbon source. Rare colonies arising were picked to basal salts medium containing 20mM sodium lactate as the sole carbon source. These colonies were in turn pulled to nitrocellulose discs impregnated with TFMP (Example 3) and compared to wild type P. cepacia G4 similarly grown on this non-inducing medium. Colonies that became yellow were picked as potentially constitutive for tomA and tomB gene products. In this way P. cepacia strain G4 5223 Phe(l) was isolated. Table 4: TCE degradation without inducer
Figure imgf000017_0001
aMean TCE concentration of triplicate samples ± standard deviation after overnight incubation with the indicated strains (at a cell density equivalent to an A ,,,, = 0.2).
Table 5: Enzyme induction vs. constitutivity
Figure imgf000017_0002
semialdehyde; Cat, catechol; 3mCat, 3-methylcatechol; Hod, 2-hydroxy-6- oxohepta-2,4-dienoate.
The genetic stability of the invention strain was assessed by growing the cells under non-selective (i.e. basal salts medium with sodium lactate at 20 mM as the sole carbon source) and under selective conditions (i.e. the same medium containing in addition 50 μg kanamycin sulphate/ml) through serially diluted batch cultures, allowing 10 generations per transfer. Following the accumulation of ca. 100 generations, the resulting population of cells was tested for kanamycin resistance (in the non-selective group) and the ability to constitutively transform TFMP to a yellow product (both groups):
Table 6: Genetic Stability
Figure imgf000018_0001
Lactate-grown colonies were picked to lactate plates containing 50μg/ml kanamycin. Those from 100 generations without selection exhibited 100% kanamycin resistance (150/150) as did those taken from kanamycin growth selection (75/75).
All colonies maintained tomA constitutivity under either growth condition (as demonstrated by pulling colonies to TFMP -impregnated nitrocellulose).
Example 5: TCE Degradation Under Ranges of Physical Conditions
In order to assess the capacity for P. cepacia G45223 Phe(l) to degrade TCE under anticipated ranges of environmental conditions the effects of oxygen concentration, pH, temperature and salinity were determined using a no air headspace TCE degradation assay (Folsom, B.R., P . Chapman, and P.H. Pritchard. 1990. Appl. Environ. Microbiol. 56:1279-1285) that mimicked a contaminated aquifer in that no gas headspaces were present. Unless otherwise noted in the salinity effect determinations, the liquid medium was the basal salts medium buffered with Tris-HCl rather than phosphate. The results are shown in Figures 4a, 4b, 4c and 4d.
Example 6: Contitutive Degradation of 1.1-Dichloroethylene. cis-1.2- Dichloroethylene. and trans-1.2-Dichloroethylene
The range of chlorinated aliphatic substrates acted upon by P. cepacia G4 5223 Phe(l) was determined by the ability of cells to degrade 10μM TCE, 1,1-Dichloroethylene, cis-l,2-Dichloroethylene, trans-L2-Dichloroethylene and tetrachloroethylene in 2 ml of basal salts medium without additional carbon sources in 10 ml Teflon lined vessels during an overnight incubation at 24 degrees C. Triplicate samples were analyzed by gas chromatography for appearance of detectable products as well as disappearance of parent compounds: Table 7: Chloroaliphatic substrates of P. cepacia G4 5223 Phef 1.
Figure imgf000019_0001
aPercent substrate remaining as compared to uninoculated controls, abbreviations: 1,1-DCE, 1,1-Dichloroethylene; cis-l,2-DCE, cis-1,2- Dichloroethylene; trans.-l,2-DCE, trans-l,2-Dichloroethylene; TCE, Trichloroethylene; PCE, Perchloroethylene; ND, Not Detectable. Starting concentration was 10 μM for all substrates. Mindicates that a metabolite was detected using gas chromatography.

Claims

Claims
A process for degrading hazardous chemicals selected from the group consisting of chloroaliphatic and aromatic chemicals which comprises contacting said hazardous chemicals with an effective degrading amount of the bacterium Pseudomonas cepacia G4 5223 Phe(l), or mutants thereof which retain the parental property of being constitutive for the degradation of said hazardous chemicals.
2. The process, according to claim 1, wherein said hazardous chemicals are selected from the group consisting of trichloroethylene, 1,1- dichloroethylene, cis-1,2 dichloroethylene, trans-l,2-dichloroethylene, vinyl chloride, toluene, phenol, o-cresol, m-cresol, o-xylene, and benzene.
3. The process, according to claim 1, wherein said hazardous chemicals are degraded in situ or in a bioreactor.
4. The process, according to claim 3, wherein said m situ degradation is selected from the group consisting of contaminated aquifers, landfills, industrial sites contaminated with hazardous chemicals, and hazardous chemicals waste collection areas.
5. Pseudomonas cepacia G4 5223 Phe(l), a microbe which has the property of being constitutive for the degradation of hazardous chemicals selected from the group consisting of chloroaliphatic and aromatic chemicals.
6. Enzyme(s) obtainable from extracts of the microbe defined in claim 5, wherein said enzyme(s) has the property of degrading hazardous chemicals selected from the group consisting of chloroaliphatic and aromatic chemicals.
7. Gene(s) obtainable from the microbe defined in claim 5, wherein said gene(s) encode enzyme(s) having the property of degrading hazardous chemicals selected from the group consisting of chloroaliphatic and aromatic chemicals.
8. A process for degrading hazardous chemicals in situ or in a bioreactor, wherein said hazardous chemicals are selected from the group consisting of chloroaliphatic and aromatic chemicals, which comprises contacting said hazardous chemicals with an effective degrading amount of a recombinant microbe comprising a gene(s) obtainable from the microbe defined in claim 5, wherein said gene(s) encodes enzyme(s) having the property of degrading hazardous chemicals selected from the group consisting of chloroaliphatic and aromatic chemicals.
9. The process, according to claim 8, wherein said hazardous chemicals are selected from the group consisting of trichloroethylene, 1, 1- dichloroethylene, cis-1,2 dichloroethylene, trans-l,2-dichloroethylene, vinyl chloride, toluene, phenol, o-cresol, m-cresol, o-xylene, and benzene.
10. The process, according to claim 8, wherein said hazardous chemicals are degraded in situ or in a bioreactor.
11. The process, according to claim 10, wherein said in situ degradation is selected from the group consisting of contaminated aquifers, landfills, industrial sites contaminated with hazardous chemicals, and hazardous chemicals waste collection areas.
12. A process for degrading hazardous chemicals in situ or in a bioreactor, wherein said hazardous chemicals are selected from the group consisting of chloroaliphatic and aromatic chemicals, which comprises contacting said hazardous chemicals with an effective degrading amount of an enzyme(s) produced by the microbe defined in claim 5, wherein said enzyme(s) has the property of degrading hazardous chemicals selected from the group consisting of chloroaliphatic and aromatic chemicals.
13. A process for isolating transposon induced tomA mutants of Pseudomonas cepacia G4 which comprises: (a) transposon mutagenesis by a triparental mating comprising E. coli JM109 (pRZ102), E. co]i JM109 (pRZ2013) and P. cepacia: (b) selection for P. cepacia colonies containing a transposed copy of Tn5 by growth of the mating mixture on basal salts medium comprising sodium lactate and kanamycin sulfate; (c) transferring selected P. cepacia colonies of (b) to nitrocellulose filters previously soaked in an aqueous solution of TFMP and air dried; and, (d) isolating P. cepacia G4 5223 which lacks the ability to transform TFMP and to degrade TCE.
14. A process for isolating a constitutive P. cepacia G4 TCE degrader which comprises: (a) inoculating transposon mutants of tomA by patching to basal salts plates comprising phenol as the sole carbon source; (b) picking rare bacterial colonies to basal salts medium containing sodium lactate as the sole carbon source; (c) pulling said rare bacterial colonies to nitrocellulose discs impregnated with TFMP; and, (d) isolating bacterial colonies that turned yellow.
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