Method for manufacturing explosive device having self-remediating capacity

Description

BACKGROUND OF THE INVENTION

1. The Field of the Invention

The present invention is directed to systems, apparatus, and methods for remediating explosives. More particularly, the present invention is directed to the remediation of explosives which have not detonated.

2. Background Art

Explosive charges are inherently dangerous in a number of respects.

Inadvertent detonation poses risks of severe personal injury or death, as well as of substantial property destruction and consequential losses. Explosive charges are, in addition, comprised of material substances, which even when not consolidated in a shape capable of performing as a detonatable explosive charge, may be toxic and thus potentially injurious to human health and to complex as well as simple plant and animal life.

Explosive charges that are not securely stored in a supervised manner, or isolated from the environment and from indiscriminate access by human and animal life forms, thus present both safety and environmental hazards.

Such hazards are pointedly apparent where an explosive charge fails to detonate after the explosive charge has been installed for that purpose during activities pertaining to mining, construction, or to seismic surveying. Fortunately, installed explosive charges that do not detonate as planned are usually locatable and often recoverable through the expenditure of reasonable efforts and without safety risks to personnel. On the other hand, there do routinely arise circumstances in which undetonated explosive charges of this type are not recovered or simply cannot be recovered. Then, the risks are present that the undetonated explosive charge could at some subsequent time be detonated inadvertently or become a source of potentially harmful contaminants.

As an example, seismic survey data used to ascertain the nature of subsurface ground structures is routinely obtained by recording and analyzing shock waves that are propagated into the ground and produced by detonating explosive charges. The shock waves are then monitored during transmission through the ground. In this role, such seismic charges are usually utilized in large sets, installed as an array of individual seismic charges at widely disbursed locations. The seismic charges are interconnected with detonation equipment for remote detonation, either simultaneously or in sequence.

Seismic charges for such surveys can be detonated either above or below the surface of the ground. In either case, it is not uncommon that at least one of any set of such seismic charges does not detonate as intended. Such failures may be caused by defects in the explosive charge itself, by damage caused during installation, by faulty detonation equipment, or by the failure of personnel in the field to make effective interconnections between that detonation equipment and each seismic charge in the installed set.

When a seismic charge installed above the ground fails to detonate as intended, it is usually possible to locate and safely recover the undetonated seismic charge. Nonetheless, circumstances do exist where the detonation of a set of seismic charges installed above the ground dislocates one of the undetonated seismic charges in the set, directing that undetonated seismic charge into a terrain in which the charge cannot be located or cannot be recovered easily. Responsible seismic crews naturally are trained to exercise all reasonable efforts to recover undetonated seismic charges that are located on the surface of the ground, but even the most rigorously indoctrinated and enthusiastic seismic personnel cannot guarantee that all undetonated seismic charges installed above the ground are ultimately recovered.

Aside from the human factor involved, the intervention of severe weather conditions, such as sandstorms, blizzards, tornadoes, or hurricanes, can impede efforts to recover undetonated seismic explosives. Some such weather conditions offer the prospect of even altering the terrain, thereby burying the undetonated seismic charge temporarily or for a substantial duration. Floods can cover the seismic survey site, removing or obscuring undetonated seismic charges. In the extreme, geological surface changes, such as mudslides, rockfalls, and fissures caused by earthquakes, by heavy weather, or even by seismic survey activity itself, can preclude the recovery of undetonated seismic charges, and even obscure the understanding that any seismic charge has failed to detonate.

The safety risks and environmental hazards posed by loose, undetonated explosive charges will be present where any undetonated seismic charge remains unrecovered after the detonation of the set of seismic charges of which it was a part.

The likelihood that an undetonated seismic charge will be abandoned is greatest, however, relative to the conduct of seismic survey activity based on the detonation of seismic charges installed below the surface of the ground. In such sub-surface seismic detonation activity, a series of deep boreholes are drilled into the earth or rock at predetermined locations that are intended to maximize the data to be derived from the shock waves promulgated from the detonation of the seismic charges. A seismic charge is placed at the bottom of each borehole and then shut in the borehole in a relatively permanent manner using a concrete or a sealing compound, such as bentonite. The balance of the borehole is then backfilled with loose soil and rock, a process which alone accounts for the majority of failed seismic detonations. Backfill materials have an understandable tendency to break the detonating cord leg wires or non-electric transmission line that interconnects the installed seismic charge at the bottom of the borehole with detonating equipment located above the ground. If a seismic charge installed below the ground fails to detonate, the easy removal of the undetonated seismic charge is seriously impeded by yards of backfill and the cured concrete or sealing compound in which the seismic charge was embedded at the bottom of the original borehole. Removing such an installed seismic charge by reexcavating the original borehole or by digging around the original borehole to avoid the sealing compound is extremely laborious and time consuming, potentially unsafe, and in many circumstances virtually impossible.

Thus, in conducting seismic survey activities, particularly seismic survey activities involving the detonation of seismic charges below the surface of the ground, undetonated seismic charges are regularly abandoned in the field. Frequently, even the precise location of undetonated seismic charges cannot be pinpointed. The risks from undetonated explosive charges installed in the ground endure for a substantial time, usually exceeding the durability of ground surface warning signs, fencing, or the continued possession and control of access to the site by an original owner. Eventually, the pressure of human population growth may render the site attractive for civil or industrial activities that would not be consistent with buried undetonated explosive charges.

The associated dangers include first that of an accidental detonation at some future time. Less dramatic, but certainly of longer duration, are risks presented by the material substance of those undetonated charges. Once released from the confines of the casing of an explosive assembly, the explosive material therein may cease to present any risk of explosion. This type of release of explosive materials can occur through corrosion of the casing through the action of ground water, the fracture of the casing during careless installation, or the shifting of the ground structure at the location at which the undetonated seismic charge was abandoned. In due course, the prolonged effect of these forces in combination with surface erosion or subsurface fluid migration can disburse over a large area the material of a fractured explosive charge. That material may constitute a potentially problematic contaminant. Even if detected, remedial activities may be required to contain and possibly eliminate the contaminant.

Nonetheless, no practical methods exist for reliably remediating the risks posed by undetonated explosive charges, particularly where those undetonated explosive charges are originally installed below the surface of the ground.

SUMMARY OF THE INVENTION

It is thus the broad object of the present invention to protect public health and safety from risks arising from incidents of abandoned undetonated explosive charges.

Accordingly, it is a related object of the present invention to eliminate the possibility of detonation of abandoned explosive charges.

It is a complementary object of the present invention to reduce the likelihood that abandoned undetonated explosive charges will contribute to environmental pollution.

Thus, it is a specific object of the present invention to provide apparatus, systems, and methods for remediating in situ any installed explosive charge that fails to detonate as intended.

It is a particular object of the present invention to provide such apparatus, systems, and methods as are capable of reliably and safely remediating an undetonated explosive charge abandoned in the ground.

Yet a further object of the present invention is to provide such apparatus, systems, and methods as are capable of remediating an undetonated explosive charge, even if the location of the explosive charge cannot be ascertained with any degree of certainty.

These and other objects and features of the present invention will become more fully apparent from the following description and appended claims, or will be appreciated by the practice of the invention.

To achieve the foregoing objects, and in accordance with the invention as embodied and broadly described herein, apparatus, systems, mixtures and methods are provided that remediate in situ an undetonated explosive utilizing the biological activity of microorganisms.

In one form, an apparatus incorporating teachings of the present invention includes a quantity of explosive material and microorganisms that are disposed in sufficient proximity to the quantity of the explosive material that the microorganisms can initiate bioremediation of the explosive material when the microorganisms are mobile. Similarly, an explosive mixture is formed by intermixing the microorganisms. and the explosive material. The explosive apparatus preferably has a shell that enables water to flow through the shell to contact the explosive material. The shell may for example have an open end, have holes or be water permeable.

The apparatus or mixture may also further comprise a mobilization means for mobilizing the microorganism to contact the explosive material. The mobilization means enables the microorganisms to initiate bioremediation of the explosive material or to continue bioremediating the explosive material. The terms “mobile” and “mobility” refer to the ability of the microorganisms to move, to be carried by the movement of a liquid, to be distributed to the explosive material or to be unrestricted in movement by a barrier that previously confined the microorganisms such that after the barrier is removed the microorganisms can contact the explosive material. The term “active” refers to the state of the microorganisms wherein the microorganisms can bioremediate explosives.

An example of a mobilization means that is useful with an explosive apparatus includes a rigid mechanical structure having a barrier to prevent contact of the microorganisms with the explosive material until the barrier is removed and the microorganisms are mobilized to contact the explosive material. The barrier can be removed by a mechanism that is mechanical, electrical and/or chemical. Other examples of mobilization means which can be utilized with an explosive apparatus or an explosive mixture include a mobilizing liquid such as water or a liquid with nutrients, a sufficient degree of porosity in the explosive material or the explosive mixture, and surfactants in the explosive material or mixture.

The microorganisms can be mobile or deactivated. Examples of deactivated microorganisms include microorganisms that have been dehydrated by air drying or by being lyophilized. The microorganisms are preferably freeze dried to increase the survivability of the microorganisms during the forming process wherein the explosive material and microorganisms are combined. More specifically, it is desirable to heat the explosive material to increase the moldability of the explosive material and to enable the microorganisms and explosive material to be easily intermixed; however, the heat can be lethal to the microorganisms as the microorganisms are placed or mixed in the explosive material. Accordingly, the microorganisms have preferably been prepared such that the microorganisms can be characterized in that the microorganisms are sufficiently resistant to heat that a significant portion of the microorganisms survive the intermixing or placement process even when the process occurs at a temperature of about 100° C.

The microorganisms can be disposed in close proximity to the explosive material or dispersed within the explosive material in many different forms. The microorganisms can be in various aggregations such as in pellets or in capsules. The aggregations can also be added without any processing of the microorganisms to form the microorganisms into a particular distinct form. Accordingly, the microorganisms can be present as a flake, granule, clump, powder or shard of a nutrient medium containing microorganisms. Nutrients, in addition to the explosive material, are generally necessary for the microorganisms to survive and grow. Binders are also often necessary and organic binders are preferred. Depending on the binder or nutrient utilized, one chemical can perform the function of both binder and nutrient. The thermal resistance of the microorganisms can also be increased by utilizing various thermal protection additives.

An example of a structure having a barrier to prevent contact of the microorganisms with the explosive material until the barrier is removed is provided by a bioremediation apparatus in combination with an explosive material. The bioremediation apparatus includes a storage means for releasably containing at least one type of microorganism capable of degrading explosive materials. Stored distinctly therefrom in the bioremediation apparatus is a reservoir means for releasably containing a liquid intended to be mixed with the microorganisms. The storage means is positioned proximate the reservoir means, usually in a relationship that is below the reservoir means in the anticipated installed orientation of the inventive apparatus. The bioremediation apparatus further includes a first valve means for delivering the liquid from the reservoir means to the microorganisms in a storage means. Doing so causes mobilization of the microorganisms. This occurs when a first valve means is opened. The first valve means is at least partially disposed within the reservoir means.

Additionally, the bioremediation apparatus of the present invention comprises a second valve means for delivering hydrated microorganisms to an associated, undetonated explosive material. The second valve means is operably linked to the first valve means and is at least partially disposed within the storage means.

The bioremediation apparatus is coupled in one embodiment of the present invention with an explosive apparatus that has an actuation means for opening the first valve means and the second valve means upon being coupled thereto. The actuation means for opening the valves can be achieved by either a mechanical or electrical mechanism. If the explosive material in the explosive apparatus fails to detonate, the explosive material will eventually be remediated by the action of the microorganisms released from the associated storage means.

Ideally, the remediation occurs in two respects. The explosive is disabled from inadvertent detonation. Subsequently, the material composition of the explosive material is rendered relatively nonharmful.

In another embodiment of the invention, microorganisms are releasably contained by gelatin, a substance that is self-effacing when contacted by microorganisms under favorable conditions. For example, gelatin may be used to fabricate the first valve means that retains liquid in the reservoir means of the bioremediation apparatus or the second valve means that retains the microorganisms in the storage means of the bioremediation apparatus.

In yet another embodiment, microorganisms are applied directly to the exterior of the explosive material or to the shell of an explosive apparatus.

BRIEF DESCRIPTION OF THE DRAWINGS

In order that the manner in which the above-recited and other advantages and objects of the invention are obtained, a more particular description of the invention briefly described above will be rendered by reference to specific embodiments thereof, which are illustrated in the appended drawings. Understanding that these drawings depict only typical embodiments of the invention and are not therefore to be considered to be limiting of the scope of the invention, the present invention will be described and explained with additional specificity and detail through the use of the accompanying drawings in which:

FIG. 1

is a perspective view of a first embodiment of a bioremediation apparatus incorporating teachings of the present invention.

FIG. 2

is a perspective view in partial break-away of the bioremediation apparatus of

FIG. 1

in the process of being coupled with an explosive apparatus in accordance with teachings of the present invention.

FIG. 3

is a cross-sectional elevation view of the bioremediation apparatus and the explosive apparatus illustrated in

FIG. 2

taken along section line

3

—

3

shown therein.

FIG. 4

is a perspective view in partial break-away of the bioremediation apparatus and the explosive apparatus of

FIG. 2

immediately upon becoming fully coupled.

FIG. 5

is a cross-sectional elevation view of the bioremediation apparatus and the explosive apparatus illustrated in

FIG. 4

taken along section line

5

—

5

shown therein.

FIG. 6

is a cross-sectional elevation view like that of

FIG. 5

illustrating the bioremediation apparatus and explosive apparatus in

FIG. 4

at a time subsequent to that illustrated in

FIG. 5

at which the explosive material in the explosive apparatus illustrated is contacted by hydrated microorganisms.

FIG. 7

is a partial cross-sectional elevation view like that of

FIG. 4

, but of a second embodiment of a bioremediation apparatus immediately incorporating teachings of the present invention immediately upon becoming fully coupled with an explosive apparatus.

FIG. 8

is a partial cross-sectional elevation view like that of

FIG. 6

, but of the second embodiment of the bioremediation apparatus and the explosive apparatus illustrated in

FIG. 7

at a time subsequent to that illustrated in

FIG. 7

at which the explosive material in the explosive apparatus illustrated is contacted by hydrated microorganisms.

FIG. 9

is a cross-sectional elevation view of a third embodiment of an explosive apparatus that utilizes an electrical mechanism to control the mobilization of the microorganisms.

FIG. 10

is a cross-sectional elevation view of a fourth embodiment of an explosive apparatus comprising a pellet of microorganisms intermixed in the explosive material.

FIG. 11

is a partial cross-sectional elevation view of a fifth embodiment of an explosive apparatus which comprises an encapsulated pellet.

FIG. 12

is a partial cross-sectional elevation view of a sixth embodiment of an explosive apparatus which comprises an encapsulated suspension of microorganisms.

FIG. 13

is a partial cross-sectional elevation view of a seventh embodiment of an explosive apparatus which comprises shards of moist nutrient wafers containing microorganisms.

FIG. 14

is a partial cross-sectional elevation view of an eighth embodiment of an explosive apparatus which comprises a powder of microorganisms dispersed on top of the explosive material.

FIG. 15

is a partial cross-sectional elevation view of a ninth embodiment of an explosive apparatus which depicts a chamber in the explosive material containing a suspension of microorganisms.

FIG. 16

is a partial cross-sectional elevation view of a tenth embodiment of an explosive apparatus which comprises clumps of microorganisms within the shell of the apparatus.

DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENTS

The present invention pertains to systems, apparatus, and methods for the in situ remediating of undetonated explosive charges. The methodology employs at least one type of microorganism that is capable of digesting an explosive material.

According to the teachings of the present invention, an explosive charge to be installed, for example by being buried in the ground, is so housed in a casing with the microorganisms. If the explosive charge fails to detonate, the explosive charge can then reliably be left undisturbed, and the microorganisms will digest or degrade the explosive material involved. Preferably, the explosive will be thereby both disabled from detonation and detoxified.

The terms “remediate” and “remediation” are used in the specification and the appended claims to refer generally to the conversion or transformation of an explosive material which is detonatable by shock or heat into a different chemical material which is less explosive or nonexplosive. The terms “bioremediate” and “bioremediation” are used to refer to remediation effected by the action of microorganisms. The present invention is thus one intended to bioremediate explosive materials.

The present invention has demonstrated an immediate utility relative to highly explosive materials, such as trinitrotoluene (TNT), pentaerythritol tetranitrate (PETN), cyclotrimethylene trinitramine (RDX), and cyclotetramethylene tetranitramine (HMX). These are typically utilized in seismic charges.

The term “bioremediable explosive” is used in the specification and the appended claims to refer to any explosive material which can be converted into a less explosive or nonexplosive material by the action of microorganisms, whether or not such microorganisms are explicitly disclosed herein. The highly explosive materials listed above are thus bioremediable explosives, since it has been demonstrated that at least the examples of microorganisms disclosed herein are capable of converting those high energy explosive materials into less explosive or nonexplosive materials.

Currently, on the basis exclusively of the examples of microorganisms disclosed herein, known bioremediative explosives include at least explosives which are classified as organic nitroaromatics, organic nitramines, or organic nitric esters. Examples of organic nitroaromatics include TNT, hexanitrostilbene (HNS), hexanitroazobenzene (NAB), diaminotrinitrobenzene (DATB), and triaminotrinitrobenzene (TATB). Examples of organic nitramines include RDX, HMX, nitroguanidine (NQ), and 2,4,6-trinitrophenylmethylnitramine (tetryl). Examples of organic nitric esters include PETN, nitroglycerine, and ethylene glycol dinitrate.

In one embodiment of the present invention, highly explosive materials, such as TNT and PETN, are converted through the action of microorganisms into less explosive materials. These intermediate chemicals can then be fully transformed into materials such as biomass and chemicals such as CO

2

and N

2

. Optimally, the highly explosive materials are reduced according to the teachings of the present invention, first into less explosive intermediate chemicals or nonexplosive products. These intermediate chemicals can then be further transformed as needed into constituents which are either less explosive or less harmful as contaminants in the environment to the health of humans, animals or plants than the intermediate chemicals may be. The final product resulting from the metabolizing action of the microorganisms will thus include any number of combinations of elements that originated in the explosive material as constituted before the initiation of the bioremediation process.

The microorganisms comprise at least a first type of microorganism that disables or deactivates the explosive material by degrading the explosive material into less explosive materials or nonexplosive materials. The microorganisms may also further comprise a second type of microorganism that further bioremediates any intermediate chemicals resulting from the bioremediation action of the first type of microorganism to fully bioremediate the explosive material into nonexplosive materials.

Although any type of microorganism capable of converting explosive material into less harmful chemicals is considered to be within the scope of the present invention, examples of microorganisms that have been demonstrated to exhibit that capacity include the group consisting of Pseudomonas spp., Escherichia spp., Morganella spp., Rhodococcus spp., Comamonas spp., and denitrifying microorganisms. It is within the scope of the present invention to use any combination of these particular microorganisms, or of any other microorganisms that are determined to be capable of bioremediating explosive materials. Suitable Pseudomonas spp. microorganisms include microorganisms in the group consisting of aeruginosa, fluorescens, acidovorans, mendocina, cepacia, and an unidentified type.

The present invention thus utilizes any of numerous different selections of microorganisms capable of degrading explosive materials in any of various relative quantities. Each of these various selections of microorganisms will for convenience hereinafter and in the appended claims be referred to as a “microorganism consortium.” In such a microorganism consortium, one type of microorganism can advantageously reduce the explosive material to a particular intermediate chemical, such as azoaromatics, while that type or another type of microorganism may then further reduce the azoaromatics or other intermediate chemicals to carbon chains, CH

4

, NH

3

, and N

2

. In one presently preferred embodiment, such a microorganism consortium utilizes all or some of various of the microorganisms belonging to Pseudomonas spp., Escherichia spp., Morganella spp., Rhodococcus spp., Comamonas spp., and denitrifying microorganisms.

The bioremediation rate is an important variable in designing a system that is impacted by many factors. One factor that is closely related to the bioremediation rate of explosive materials by the microorganisms is the growth rate of the microorganisms. The growth rate of some species of microorganisms disclosed herein are logarithmic while others are only linear. Accordingly, the growth rate of the consortium depends on the type of microorganisms utilized. Additionally, the growth rate of the consortium of microorganisms depends on other factors, such as the availability of nutrients. The growth rate of the consortium of microorganisms can, however, be generally characterized as logarithmic.

A consortium of microorganisms within the scope of the present invention was deposited on May 23, 1996 with the American Type Culture Collection (hereinafter “ATCC”) in accordance with the provisions of the Budapest Treaty on the International Recognition of the Deposit Microorganisms for the Purpose of Patent Procedure. The ATCC is located at 10801 University Boulevard, Manassas, Va. 20110-2209 U.S.A. The deposited consortium of microorganisms was assigned ATCC Designation No. 55784. For purposes of this disclosure, the microorganism consortium deposited with the ATCC and designated ATCC Designation No. 55784 is hereby incorporated by reference.

The microorganism consortium deposited with the ATCC was obtained from Richards Industrial Microbiology Laboratories, Inc. (hereinafter “RIML”) located at 55 East Center, Pleasant Grove, Utah 84062 U.S.A. The microorganism consortium is identified at RIML by Product No. RL-247. Accordingly, microorganisms sold as RL-247 by RIML under the tradename RL-247 and assigned ATCC Designation No. 55784 are considered to be within the scope of the invention disclosed herein, whether or not constituent microorganisms therein are explicitly identified to any degree herein.

The microorganisms of the microorganism consortium are chosen for having a demonstrated ability to metabolize and degrade explosive materials in any way that contributes to the disabling of the explosive material or to the detoxification of the chemical components thereof. If microorganisms are selected that are both aerobic and anaerobic, bioremediation will occur in shallow and exposed surface locations, as well as in deep explosive boreholes. Ideally, the microorganisms selected for the microorganism consortium should be nonpathogenic and surfactant-producing, as this enhances the digestive action of the microorganism colony.

In one embodiment of a microorganism consortium chosen according to the teachings of the present invention, the Pseudomonas spp. are selected from the group consisting of aeruginosa, flourescens, acidovorans, mendocina, and cepacia. Any microorganisms of Pseudomonas spp. other than the microorganisms identified above are considered to be within the scope of the invention disclosed herein, provided that such microorganisms perform any of the functions described above having utility in the remediating of an explosive charge. Correspondingly, any microorganism is considered to be within the scope of the invention disclosed herein, provided the microorganism exhibits any utility relative to. the bioremediating of explosive materials.

Thus, the disclosure and incorporation herein of the microorganism consortium assigned ATCC Designation No. 55784 or the disclosure of the microorganism consortium available from RIML under the tradename RL-247, are but examples of microorganism consortiums within the teachings of the present invention and are not limiting of the microorganisms that may be selected for inclusion in a microorganism consortium according to the teachings of the present invention.

Various embodiments of explosives are set forth hereinbelow which are configured to enable microorganisms to bioremediate a quantity of explosive material. The microorganisms are disposed in sufficient proximity to the explosive material that the microorganisms initiate bioremediation of the explosive material when the microorganisms are mobilized.

The shelf lives of the explosive material and the microorganisms are increased by delaying the bioremediation activity of the microorganisms at least until the explosive is ready to be utilized. Accordingly, the preferred embodiments involve the use of microorganisms that are temporarily immobilized or have been blocked from contact with the explosive material until the explosive is to be positioned in the ground or after the explosive is in the ground. Configurations can also be utilized wherein the microorganisms are initially mobile when positioned relative to the explosive material, thereby enabling the microorganisms to immediately initiate bioremediation.

The embodiments of the invention designed to delay the bioremediation activity of the microorganisms until a set time utilize a mobilization means for mobilizing the microorganisms to contact the explosive material. The mobilization means enables the microorganisms to initiate bioremediation or continue bioremediation of the explosive material. Any mobilizing means can be utilized including mechanisms which are primarily mechanical, electrical, chemical or combinations thereof.

Examples of combinations of mechanical and chemical mechanisms utilized to mobilize the microorganisms are provided by the embodiment in

FIGS. 1-6

and the embodiment in

FIGS. 7-8

. An embodiment is depicted in

FIG. 9

that utilizes electrical, mechanical and chemical mechanisms to mobilize the microorganisms. In these embodiments, a rigid mechanical structure contains the microorganisms in a relatively immobilized condition or at least separate from the explosive material. Bioremediation of the explosive material is initiated when a barrier between the microorganisms and the explosive material is removed and the microorganisms are in an adequate quantity of a liquid to enable the microorganisms to be sufficiently mobile to flow into contact with the explosive materials.

A first embodiment of an apparatus employing principles of the present invention is illustrated in

FIG. 1

as an explosive bioremediation apparatus

10

. Bioremediation apparatus

10

includes a casing

12

having a top end

14

and a bottom end

16

. Casing

12

is preferably formed from a material which is water resistant and is capable of withstanding extremes of temperature.

A cap

18

is inserted into top end

14

of casing

12

. Cap

18

is preferably formed from a durable material that will withstand being driven down a borehole with a tamping pole. Cap

18

includes a cap top

20

and an external cap member

22

integrally extending from cap top

20

and having cap threads

24

. Cap

18

is secured about top end

14

of casing

12

by engaging cap threads

24

with end threads

26

that are formed on the exterior of top end

14

. Cap

18

may include an internal cap member with an O-ring or a foam seal so configured and positioned as to engage top end

14

of casing

12

. This increases the security of the seal produced.

Cap

18

is but one example of a structure capable of functioning as a cap means for sealing the top end of a casing, such as casing

12

. Another example of a structure capable of performing the function of a cap means according to the teachings of the present invention would be a casing without any external cap member, but rather having an internal cap member that is inserted into top end

14

. Alternatively, bioremediation apparatus

10

could be provided with a structure that performs the foundation of such a cap means but is integrally formed with casing

12

. Any such cap structure that is integrally formed with casing

12

from a plastic material should be constructed to withstand the impacts and pressure encountered in being pushed down a borehole.

Bioremediation apparatus

10

is configured at bottom end

16

of casing

12

for coupling with an explosive apparatus shown and discussed subsequently in relation to

FIGS. 2-6

as housing a bioremediatable explosive material. Bioremediation apparatus

10

also has casing threads

28

on casing

12

that cooperatively engage correspondingly configured threads on the explosive apparatus to effect the intended coupling.

According to teachings of the present invention, microorganisms

30

capable of degrading explosive materials are stored in a storage means for releasably containing microorganisms. By way of example and not limitation, such a storage means within the scope of the present invention can take the form of a storage chamber

32

having sidewalls defined by casing

12

. As shown in

FIGS. 1-5

, microorganisms

30

can be positioned on a ring formed from starch and flour, bran, or another similar nutrient material. The microorganisms

30

can be stored in a moist condition in storage chamber

32

or the microorganisms can also be lyophilized or freeze dried. Microorganisms

30

are preferably not mobilized until bioremediation apparatus

10

is actually coupled with an explosive apparatus which is preferably in the field at the time the seismic charge is to be placed in a borehole or at the time of the intended detonation of the charge in that explosive apparatus. In addition to a ring configuration, microorganisms

30

can be positioned in contact with materials such as starch, flour, or bran assuming any other arrangement.

Microorganisms

30

are mobilized by a liquid

34

stored in a reservoir means for releasably containing a liquid. Liquid

34

may be water or a nutrient medium that can feed microorganisms

30

, but liquid

34

is resistant to freezing at ambient temperatures. By way of example and not limitation, a reservoir means within the scope of the present invention can take the form of a reservoir chamber

36

. Reservoir chamber

36

has sidewalls defined by the interior of casing

12

and a top defined by cap

18

. Reservoir chamber

36

also includes a liquid passage

38

defined by the interior of a neck

40

. Neck

40

is an integral portion of casing

12

and has a diameter that tapers radially inwardly from the outer diameter of the sidewalls of reservoir chamber

36

to a smaller diameter, as observed to best advantage in FIG.

3

.

Preferably, storage chamber

32

is positioned below reservoir chamber

36

in the anticipated orientation of bioremediation apparatus

10

when coupled to and installed with explosive apparatus

60

. Storage chamber

32

is capable of communication with reservoir chamber

36

through liquid passage

38

. Storage chamber

32

is provided with a bioremediation outlet

42

that is formed through bottom end

16

of casing

12

and through a sleeve member

44

which protrudes from bottom end

16

of casing

12

. Accordingly, bioremediation outlet

42

is a portal or opening through casing

12

that is in communication with storage chamber

32

.

Microorganisms

30

are mobilized by liquid

34

upon the opening of a first valve means for delivering liquid

34

from reservoir chamber

36

to storage chamber

32

. By way of example and not limitation, a first valve means according to the teachings of the present invention can take the form of a first valve

46

which comprises the interior of neck

40

and a first valve member

48

. A tapered end

50

is formed around the perimeter of first valve member

48

corresponding in dimension to the interior of neck

40

. The cooperation of these structures forms a seal within liquid passage

38

.

When first valve

46

, which is shown in

FIG. 1

, is closed as shown in

FIG. 3

, first valve

46

is at least partially disposed within reservoir chamber

36

. More particularly, when first valve

46

is closed, first valve

46

is positioned between reservoir chamber

36

and storage chamber

32

and within liquid passage

38

with first valve member

48

defining the bottom of reservoir chamber

36

and the top of storage chamber

32

. The seal formed within liquid passage

38

by first valve

46

thereby retains liquid

34

in reservoir chamber

36

until first valve

46

is opened.

Once mobilized or activated, microorganisms

30

flow out of storage chamber

32

upon the opening of a second valve means for delivering mobilized microorganisms to an explosive material in an explosive apparatus. By way of example and not limitation, a second valve means according to the teachings of the present invention can take the form of a second valve

52

which includes a second valve member

54

in combination with sleeve member

44

. Second valve

52

defines the bottom of storage chamber

32

and is the lower end of a valve connector

56

that extends through bioremediation outlet

42

in sleeve member

44

. Valve connector

56

has an upper end that is connected to first valve member

48

.

When second valve

52

is closed as shown in

FIG. 3

, second valve

52

is at least partially disposed within storage chamber

32

. More particularly, when closed, second valve

52

is positioned at the bottom of storage chamber

32

within bioremediation outlet

42

. Second valve member

54

forms a seal with sleeve member

44

in bioremediation outlet

42

, thereby to retain mobilized microorganisms

30

in storage chamber

32

until second valve

52

is opened. The security of the seal is increased by a valve O-ring

58

, which encircles second valve member

54

.

Valve connector

56

can best be seen in

FIG. 3

to connect first valve member

48

and second valve member

54

. The length of valve connector

56

is selected to enable first valve

46

and second valve

52

to open and close according to a predetermined timing relationship. Thus, first valve

46

, second valve

52

, and valve connector

56

can be configured to effect the simultaneous opening or actuation of first valve

46

and second valve

52

. Alternatively, first valve

46

, second valve

52

, and valve connector

56

can be designed to actuate one of the valves in a delayed manner, after the other valve has been actuated. It may be desirable for example, to allow liquid

34

to contact microorganisms

30

by opening first valve

46

, and only thereafter to open second valve

52

.

When microorganisms

30

and liquid

34

are securely sealed in separate spaces as shown in

FIG. 3

, bioremediation apparatus

10

can be shipped and stored for long periods without any significant decrease in the bioremediating effectiveness thereof. The configuration of bioremediation apparatus

10

is designed for easy combination with a conventional explosive, such as a seismic booster.

FIGS. 2 and 3

depict bioremediation apparatus

10

in the process of being coupled with an explosive apparatus

60

.

FIG. 2

is a perspective view, and

FIG. 3

is a cross-sectional view taken along section line

3

—

3

of FIG.

2

. As best illustrated in

FIG. 3

, first valve member

48

and second valve member

54

remain in closed positions when bioremediation apparatus

10

is initially threaded into explosive apparatus

60

.

Explosive apparatus

60

comprises a shell

62

having an open end

64

and an explosive material

66

housed within shell

62

. The interior of shell

62

is provided with shell threads

70

near open end

64

. These cooperate with correspondingly configured casing threads

28

on bioremediation apparatus

10

. Shell

62

can be formed from distinct components or as an integral structure as shown.

The combination of casing threads

28

and shell threads

70

together serve as an example of a coupling means for coupling a bioremediation apparatus according to the teachings of the present invention with an explosive apparatus, such as explosive apparatus

60

. In the embodiment illustrated, the function of such a coupling means is performed by an extension of casing

12

of bioremediation apparatus

10

and an extension of shell

62

of explosive apparatus

60

. Alternatively configured structures can, however, perform the function of such a coupling means.

For example, a wedge fit can be effected between bioremediation apparatus

10

and explosive apparatus

60

using respective angled male and female parts attached, respectively, to each. While the coupling means is primarily a mechanism to join bioremediation apparatus

10

and explosive apparatus

60

, it is within the teachings of the present invention to provide structures that prevent bioremediation apparatus

10

and explosive apparatus

60

from being unintentionally separated, thereby performing the function of a locking means for securing bioremediation apparatus

10

and explosive apparatus

60

against the disengagement of the coupling together thereof.

Explosive apparatus

60

further comprises a capwell

72

positioned in open end

64

to receive detonators

74

. Detonators

74

are in turn electrically connected by wires

76

to the exterior of shell

62

through wire access openings

78

shown in

FIG. 2. A

bioremediation portal

80

formed through capwell

72

communicates with explosive material

66

to afford access by mobilized microorganisms

30

from bioremediation outlet

42

to explosive material

66

. A portal member

82

extends upwardly as shown in

FIG. 3

from the center of capwell

72

, encircling and defining on the interior thereof bioremediation portal

80

. A portal O-ring

84

encircles portal member

82

to provide a fluid seal between sleeve member

44

and portal member

82

when explosive bioremediation apparatus

10

is coupled with explosive apparatus

60

.

FIGS. 4 and 5

depict bioremediation apparatus

10

immediately after becoming completely coupled with explosive apparatus

60

.

FIG. 4

is a perspective view, and

FIG. 5

is a cross-sectional view taken along section line

5

—

5

of FIG.

4

.

FIG. 5

illustrates to best advantage that as a result of the coupling of bioremediation apparatus

10

with explosive apparatus

60

, first valve

46

and second valve

52

have been opened. Liquid

34

is shown being delivered by gravity from reservoir chamber

36

through liquid passage

38

to storage chamber

32

.

As bioremediation apparatus

10

is being coupled with explosive apparatus

60

, sleeve member

44

and portal member

82

advance toward each other until portal member

82

is positioned within sleeve member

44

. A fluid seal is formed between sleeve member

44

and portal member

82

by portal O-ring

84

. The advancement of bioremediation apparatus

10

brings portal member

82

into abutment against second valve member

54

. As valve connector

56

effects a rigid interconnected relationship between second valve member

54

and first valve member

48

, further advancement of bioremediation apparatus

10

into and toward explosive apparatus

60

forces second valve member

54

out of bioremediation outlet

42

and forces first valve member

48

out of liquid passage

38

.

Sleeve member

44

, second valve member

54

, and portal member

82

can have any lengths that enable first valve

46

and second valve

52

to be opened. In the embodiment shown in

FIGS. 5 and 6

, portal member

82

and second valve member

54

each have a length that is less than the length of sleeve member

44

, and the length of portal member

82

is approximately equal to or greater than the length of second valve member

54

.

Forcing second valve member

54

and first valve member

48

upward within casing

12

opens a flow path that permits mobilized microorganisms

30

to contact explosive material

66

through bioremediation portal

80

as shown in FIG.

6

.

First valve member

48

, second valve member

54

, and valve connector

56

form a divider which is preferably formed at least partially from a lightweight material such as polyethylene. The divider in this manner preferably has a lower density than water. This enables the divider to float to the top of the suspension of microorganisms as shown in

FIG. 6

after the liquid has flowed into contact with explosive material

66

.

The divider formed by first valve member

48

, second valve member

54

, and valve connector

56

is an example of a divider means for releasing microorganisms to an explosive material according to the teachings of the present invention. In an alternative embodiment, the divider means can take the form of a valve means for delivering the mobilized microorganisms from a storage means to an explosive material in a storage chamber of an explosive apparatus. The microorganisms are in a moist condition or are in a sufficient quantity of liquid to be characterized as a suspension or dispersion. Such an alternative embodiment accordingly utilizes but a single chamber and a single valve.

Portal member

82

is an example of an actuation means for initiating contact between mobilized microorganisms and an explosive material by opening first valve

46

and second valve

52

. In an alternative embodiment, portal member

82

has a length greater than sleeve member

44

, thereby rendering unnecessary any second valve member extending within sleeve member

44

to align portal member

82

for contact with the second valve member. In an additional alternative embodiment, second valve

52

is configured similarly to first valve

46

. In this additional alternative embodiment, second valve

52

has a valve member within bioremediation outlet

42

that does not extend downward, and there is no sleeve member to provide alignment for portal member

82

in contacting the valve member to actuate second valve

52

. Any structure capable of initiating access by mobilized microorganisms

30

to explosive material

66

is within the scope of the actuation means of the present invention.

The actuation means and the coupling means are taken together exemplary of a contact means for initiating and maintaining contact between mobilized microorganisms and an explosive material.

The coupling of bioremediation apparatus

10

with explosive apparatus

60

forms a system for in situ bioremediating of an explosive material. The system can be lowered into or driven down a borehole by contacting cap

18

with a tamping pole. Additionally, an anchor member

90

shown only in

FIG. 6

can be positioned about casing

12

to maintain the system in the upright position illustrated during installation of the system at the bottom of a borehole. Anchor member

90

is preferably a disc circumferentially encircling casing

12

and extending perpendicularly outwardly therefrom. The longitudinal position of anchor member

90

along the length of casing

12

is maintained as shown in

FIG. 6

by the increase in the outer diameter of casing

12

above anchor member

90

.

The failure of installed explosives to detonate is primarily caused by the forces experienced during positioning of the system in the bottom of a borehole. In the process, wires

76

are often broken or disconnected from detonators

74

, so that detonation cannot occur. When this happens, the digestion of explosive material

66

by microorganisms

30

will proceed in due course. Eventually, explosive material

66

will be reduced to nonexplosive and non-harmful materials that are neither detonatable by any activities in the vicinity, nor are an environmental contaminant.

Over time, by exposing an undetonated charge to the microorganisms, the entirety of the explosive material of the charge is reduced to a substance that cannot be detonated. In the illustrated embodiments of the present invention, the digestive activity of microorganisms

30

disarms explosive material

66

by first attacking the area around the capwell end of the explosive apparatus. This is where detonation is actually initiated. There is, however, no overall detrimental effect on the ability of an explosive charge to be detonated immediately after being initially contacted by bioremediating microorganisms. The initial activity of the microorganisms in the vicinity of the capwell can prevent accidental detonation of the explosive charge which can be caused, for example, by digging in the area of the explosive charge after the explosive charge is positioned in a borehole.

The time period required for the microorganisms to first disable an explosive, and then to fully remediate a given quantity of intermediate chemical materials depends on the amount and type of explosive material used, as well as the composition of microorganism consortium used therewith. Depending on design, relative concentrations of the explosive, the time required can be days, weeks, months, or years.

FIGS. 7 and 8

depict a second embodiment of a system for in situ bioremediating of an explosive according to teachings of the present invention. The system shown there comprises a bioremediation apparatus

100

and an explosive apparatus

110

. Components shown in

FIGS. 7 and 8

that are identical to the components shown in

FIGS. 1-6

are identified with the same reference characters as are the corresponding components in

FIGS. 1-6

.

Bioremediation apparatus

100

has a cap

18

, a spacer

112

, and an anchor member

90

that encircles top end

14

of casing

12

. Cap

18

and a spacer

112

are configured to maintain anchor member

90

on a nib

114

. Cap

18

has cap threads

24

which cooperate with end threads

26

around top end

14

of casing

12

to seal top end

14

of casing

12

. Spacer

112

is positioned between cap

18

and anchor member

90

. Spacer

112

has a bottom portion not shown in the figures that is positioned within the top end of anchor member

90

. When the system of

FIGS. 7 and 8

is pushed down a borehole with a tamping pole, anchor member

90

cannot be dislodged from nib

114

, since anchor member

90

abuts spacer

112

, and cap

18

retains spacer

112

in position.

Liquid

34

is contained in reservoir chamber

36

and is released to contact microorganism

30

in storage chamber

32

when a first valve

116

in liquid passage

38

is opened. First valve

116

comprises the interior of neck

40

and a first valve member

118

. First valve member

118

has a lip end

120

around the perimeter of first valve member

118

. Lip end

120

is tapered to correspond to the dimensions of the interior of neck

40

and is flexible, thereby to form a fluid seal with liquid passage

38

.

A second valve

122

comprises a second valve member

124

and a lip seal member

126

. Second valve member

124

is the tapered bottom end of a valve connector

128

. Lip seal member

126

extends from sleeve member

44

into bioremediation outlet

42

to form a fluid seal with second valve member

124

.

First valve member

118

is integrally formed with valve connector

128

, and valve connector

128

is integral with second valve member

124

. Accordingly, first valve member

118

, valve connector

128

, and second valve member

124

together form an integral divider. In the first embodiment shown in

FIGS. 1-6

, the first valve means is also connected to the second valve means, as first valve member

48

and second valve member

54

are connected by valve connector

56

. Thus, both in the first embodiment of

FIGS. 1-6

and in the second embodiment of

FIGS. 1-8

, at least a portion or a component of each valve means is connected to at least a portion or a component of the other valve means.

The coupling means for coupling a bioremediation apparatus with an explosive apparatus, such as the combination of casing threads

28

and shell threads

70

as shown in

FIGS. 1-8

, may further comprise a means for indicating the position of the valves. In the preferred embodiment, casing

12

preferably has a bump not shown in the figures that causes a clicking noise when portal member

82

contacts the second valve member after casing threads

28

and shell threads

70

are advanced over each other. The clicking noise informs a user that the bioremediation apparatus and the explosive apparatus are coupled.

In yet additional alternative embodiments of an apparatus similar to the apparatus depicted in

FIGS. 1-6

or in

FIGS. 7-8

, the first or second valve means can be electronically controlled to remain closed until electronically activated. For instance, a battery can provide electricity to retain a valve in a closed position such that the valve opens when the battery is dead. Accordingly, the microorganisms are not mobilized until after a time period equal to or exceeding the life span of the battery. In such an embodiment it is unnecessary to couple a bioremediation apparatus and explosive apparatus together to mobilize the microorganisms so the microorganisms and explosives can be contained in a single housing.

An example of an embodiment that utilizes an electrical mechanism is shown in

FIG. 9

which is similar to the embodiment shown in

FIGS. 7-8

. Bioremediation apparatus

140

shown in

FIG. 9

has microorganisms

30

which are not in the doughnut configuration but are added as a block. A flange

142

extends from valve connector

56

and is above a piston

144

. Piston

144

extends within a spring

146

from a solenoid

148

. Solenoid

148

is electrically connected to a battery

150

. Battery

150

applies power to the coil of solenoid

148

which pulls piston

144

into the coil of solenoid

148

and retains piston

144

against the force of spring

146

as long as power is being supplied to the coil of solenoid

148

. When the battery is dead then piston

144

and spring

146

are released and push against flange

142

which causes first valve member

48

and second valve member

54

to be pushed upward, thereby opening first valve

46

and second valve

52

. In this embodiment, it is not necessary for sleeve member

44

, second valve member

124

or portal member

82

to have lengths that enable the valve members to be opened.

Other embodiments utilize mechanisms which are primarily chemical in nature such as a barrier formed from a material, which is water soluble or slowly self-effacing in the presence of water, an aqueous solution or microorganisms. Thus, for example, self effacing barriers which eventually degrade and release the microorganisms can perform the functions of either or both first or second valve means according to the present invention. Examples of materials that can be utilized as self-effacing valve members include gelatin, alginate, starch, and acrylamide. Careful structural and material design of such barriers can produce relatively precisely timed releases. Alternatively, microorganisms encapsulated in a material such as gelatin or alginate may be releasably contained in a storage means of the present invention for eventual contact with an explosive material.

FIGS. 10-16

depict embodiments of the present invention wherein microorganisms are intermixed in the explosive or are disposed against an exterior surface of the explosive material. The microorganisms depicted in

FIGS. 10-16

are disposed in sufficient proximity to said quantity of explosive material that the microorganisms can initiate bioremediation of the explosive material when the microorganisms are mobile. The explosive apparatus shown in

FIGS. 10-16

do not require the coupling of a distinct bioremediation apparatus with a corresponding explosive apparatus.

The microorganisms intermixed in the explosive material are generally in aggregations or clusters such as pellets as shown in

FIG. 10

, capsules as shown in

FIGS. 11-12

, or shards as shown in FIG.

13

. The embodiments depicted in

FIGS. 14-16

provide examples of microorganisms disposed against an exterior surface of the explosive material.

FIG. 14

shows a powder of microorganisms dispersed on the top surface of the explosive material.

FIG. 15

depicts microorganisms poured into a column within the explosive material.

FIG. 16

depicts a cluster of microorganisms positioned within the shell that contains the microorganisms. In addition to the clusters or aggregations disclosed in

FIGS. 10-16

, the microorganisms can be positioned in any form even as individual microorganisms.

FIG. 10

illustrates an explosive apparatus

200

configured with an optional cap

202

and access openings

204

for wires

76

. As in the embodiments depicted in

FIGS. 1-9

, explosive apparatus

200

has a capwell

72

with detonators

74

. Explosive apparatus

200

further comprises a shell

206

containing an explosive material

208

and pellets

210

of microorganisms dispersed throughout explosive material

208

. Shell

206

preferably enables water to flow through shell

206

to contact the explosive material

208

or at least into contact with the microorganisms in pellets

210

at the exterior surfaces of explosive material

208

. Shell

206

may for example have an open end wherein water can flow, have holes or be water permeable to enable water to enter into the pores of explosive material

208

.

Pellets

210

are dispersed as needed. For example, pellets

210

can be randomly dispersed, as shown, or concentrated as needed to deactivate the explosive charge. Pellets

210

are preferably positioned to facilitate desensitization of the explosive apparatus by being concentrated within explosive material

208

around detonators

74

.

Pellets

210

can be positioned within explosive material

208

by any method and in any desired concentration. Control of the concentration and dispersion of pellets

210

in the explosive material

208

is maximized by adding pellets

210

to explosive material

208

when explosive material

208

is in a liquid state. Explosive material

208

is in a liquid state when being formed into a desired configuration by pouring the explosive material into a mold or directly into shell

206

. The forming temperature of the explosive material is around 100° C. which is generally lethal to the microorganisms. Accordingly, the exposure time of microorganisms in pellets

210

to lethal temperatures is preferably minimized by adding pellets

210

to explosive material

208

while explosive material

208

is being formed or cast into a desired shape. Pellets

210

can also be pressed into explosive material

208

when explosive material

208

is solid or semi-solid at the time that the charge is manufactured.

The microorganisms or pellets

210

containing the microorganisms are preferably heat resistant to increase the survivability of the microorganisms when added to explosive material

208

. There are several methods, which can be utilized alone or in combination, for obtaining heat resistant microorganisms or pellets.

One method for obtaining heat resistant microorganisms involves lyophilizing the microorganisms before the microorganisms are added to the hot explosive material. The microorganisms can be dehydrated by allowing the water to evaporate or preferably by freeze drying the microorganisms. Freeze drying the microorganisms dramatically reduces the mortality of the microorganisms due to thermal stress from exposure to the molten explosive material during the pouring process. It is speculated that freeze dried microorganisms are less susceptible to the lethal temperature effects than a microorganisms in a moist environment because the water content in the moist microorganism provides better heat transfer to the vital and temperature sensitive internal structures. The water removed from the freeze dried microorganisms is replaced at a later time in sufficient quantity to activate and mobilize the microorganisms.

The survivability of the microorganisms to thermal stress is also increased by increasing the thickness of the pellets

210

. Increasing the thickness of pellets

210

decreases the rate of heat transfer to the interior of pellets

210

, thereby protecting the microorganisms in the interior to the extent that the residence time of the microorganisms in the hot melt is not excessive. When the exterior microorganisms are destroyed they act as a thermal insulator for the microorganisms within the interior. Suitable pellets generally have an average diameter of about 3 mm.

Another method for reducing the mortality of microorganisms due to thermal stress is achieved by adding the microorganisms and explosive material into a mold in thin layers. By adding the microorganisms and explosive material incrementally in thin layers the layers can quickly cool thereby minimizing the exposure time of the microorganisms to the hot melt.

The heat resistance can also be increased by slowly raising the growth temperature of the microorganisms. By slowly raising the temperature of the environment of the microorganisms over a period of time during their growth, the high temperature tolerance of the microorganisms is significantly increased. Microorganisms can be utilized which have been adaptively developed or which have also been genetically developed. The microorganisms are preferably developed to have a very high survivability rate even when exposed to temperatures as high as about 100° C. Even microorganisms which have not been adequately developed to survive exposure to temperatures as high as about 100° C. are very useful since the temperature decreases as it is transferred into the pellet, yielding a greater interior portion that survive compared to a pellet utilizing unconditioned microorganisms. Accordingly, all microorganisms that have been developed for high temperature tolerance are useful and yield a higher survivability rate.

Additionally, pellets

210

can also be formed from mixtures of microorganisms and thermal protection additives that increase the heat resistance of the microorganisms. Examples of additives which have been found to increase the survivability of microorganisms when thermally stressed include dry milk and bentonite clay. These viability enhancers also can be used as binders as they tend to bind the constituents in the pellet together and can also be a nutrient source for the microorganisms. Insulative aggregates with no binding capability or that are not nutrient sources can also be used to thermally protect the microorganisms.

The pellets can be formed by compressing the microorganisms together along with any other constituent materials such as nutrients, binders and insulative materials. As previously set forth, the same component can act as a nutrient, binder or an insulative material. Nutrients are generally necessary even when the microorganisms are lyophilized since they provide the microorganisms with all of the materials needed for the microorganisms to fully grow and multiply. The explosives generally provide carbon and nitrogen while the nutrients generally provide phosphate and other chemicals. Any suitable nutrient can be utilized; however, depending on the type of nutrient utilized and the availability of the nutrient the growth rate can be influenced. In addition to the nutrients previously discussed such as starch, flour, bran, and milk; other suitable nutrients include milk sugar and minimal medium glycerol. Many of these nutrients can also act as stabilizers, such as starch, flour, bran, milk, glycerol in addition to phosphate buffered saline.

It is not always necessary to add a component that acts only as a binder since many nutrients can be utilized as a binder which are then converted into nutrients when contacted by a sufficient quantity of water to solubilize the binder. In addition to the binders previously mentioned, any suitable binder can be utilized. The binder is preferably an inorganic binder. A product sold as Diatab is a particularly useful binder or tablet base. Other materials that can be utilized as a binder include acrylamide, alginic acid or alginate, ethylcellulose, guar gum and gelatin.

Pellets

210

can also be encapsulated in a capsule

212

as shown in FIG.

11

. The microorganisms in capsule

212

can be freeze dried, then formed into a pellet and encapsulated or the capsule can be formed by encapsulating moist microorganisms or a suspension of microorganism by pouring the suspension into a capsule and then drying or freeze drying the capsule. Any suitable materials for forming capsule

212

can be utilized. Examples of suitable materials include gelatin, starch, alginate and acrylamide.

While it is preferred to form the explosive by placing pellets of dehydrated microorganisms into molten explosive material since the molten explosive material is easily and relatively quickly molded into a desired shape, it can decrease the viability of the microorganisms. Accordingly, it is also desirable to form pellets

210

from moist microorganisms. Depending on the amount of liquid present, it may be necessary to introduce the microorganisms into explosive material

208

as a suspension of microorganisms as shown at

214

in

FIG. 12

that is contained in a capsule

212

. Microorganisms which are merely moist can also be encapsulated or can be introduced as shards

216

of a moist nutrient wafer containing microorganisms as shown in FIG.

13

. Shards

216

, which are fragments or flakes, can also be a nutrient wafer containing lyophilized microorganisms.

Clusters or aggregations of moist microorganisms in configurations such as pellets, capsules, shards, flakes and the like are preferably blended into explosive material

208

and then pressed into a mold. Moist microorganism clusters can also be pressed into explosive material

208

. When the microorganisms are in a moist state but are blocked from contact with the explosive material or are not sufficiently. mobile, nutrients provide a minimal food source until the microorganisms can metabolize the explosive material. After the mixture is shaped into an explosive charge and the microorganisms are sufficiently moist it will bioremediate automatically within a predetermined time following manufacture.

An explosive apparatus is often left underground for periods of time up to six months and even up to a year. Accordingly, an explosive apparatus is preferably explodable for up to about six months and more preferably for up to about a year.

As previously set forth, the microorganisms can be concentrated around detonators

74

to desensitize the explosive since detonators

74

are typically more sensitive to impact and friction than explosive material

208

. The time required to desensitize explosive apparatus

200

by disabling explosive material

208

around detonators

74

is dependent on many variables in addition to the distribution of the microorganisms, the growth rate of the types of microorganisms utilized, the ratio of microorganisms to explosives, the availability of particular nutrients, the types of microorganisms and explosives utilized and other physical condition such as pH, water availability and temperature. These same variables generally determine the time required to reduce explosive material

208

to a residual or negligible amount and the time required to entirely reduce explosive material

208

to a nonhazardous and preferably nonharmful material. Some of these additional variables include the amount of surface area exposed to the microorganisms, the mobility of the microorganisms, and the porosity of the explosive materials. Accordingly, the bioremediation rate can be designed as needed.

The porosity of the explosive materials is an example of a mobilization means for mobilizing the microorganisms to contact explosive material

208

. The porosity of the explosive materials

30

enables the mobilized microorganisms to move within explosive material

208

and continue bioremediating explosive material

208

. The porosity also enables water to enter into the pores and come into contact with the microorganisms and mobilize the microorganisms. A surfactant in explosive material

208

is another example of a mobilization means. Surfactants facilitate wetting of the crystals in explosive material

208

which enhances the mobility of the microorganisms and the accessibility of the crystals to the microorganisms.

Explosive apparatus

200

can be immersed in water before being placed in a borehole to allow water to pass through shell

206

and enter into the pores to mobilize the microorganisms or clusters thereof intermixed in explosive material

208

. Explosive apparatus

200

is preferably exposed to a vacuum before being dipped in water. It is generally not necessary to immerse explosive apparatus

200

in water as groundwater is almost always present in the borehole. Additionally, water can also be poured into the borehole as needed. Water around or in contact with explosive apparatus

200

are additional examples of mobilization means for mobilizing the microorganisms.

Since groundwater is almost always in a borehole, it is generally desirable to design the explosive apparatus to utilize the groundwater. Accordingly, the porosity is preferably conducive to optimal capillary action through a network of microchannels. The network of microchannels or pores is sufficiently interconnected to provide optimal accessibility to the microorganisms by water and to provide optimal mobility to the mobilized microorganisms. The porosity is also designed to provide optimal surface area for the microorganisms to bioremediate. The porosity is balanced against the amount of explosive material that is preferably present and any necessary amount of mechanical strength for withstanding crushing and other forces experienced while being positioned in the borehole. The porosity can also be heterogenous throughout explosive material

208

such that the area around detonators

74

is more porous compared to other sections to expose more surface area.

The embodiments depicted in

FIGS. 10-13

are dependent primarily on the porosity of explosive material

208

to provide access to the microorganisms and to provide mobilization pathways for the mobilized microorganisms.

FIGS. 14-15

depict embodiments of the present invention that do not rely primarily on the porosity of explosive material

208

.

FIG. 14

depicts microorganisms deposited as granules

218

on top of explosive material

208

. Accordingly, as water passes through shell

206

the initial bioremediation activity of all of the microorganisms is concentrated at the portion of explosive material around detonators

74

.

FIG. 15

depicts a chamber

220

centrally and longitudinally located within explosive material

208

that contains a suspension

222

of microorganisms. Microorganisms can also be positioned in chamber

220

which are merely moist or have been lyophilized. This configuration enables the mobilized microorganisms to bioremediate explosive material

208

from within a particular location in explosive material. The position of chamber

220

provides for controlled bioremediation of explosive material

208

around detonators

74

.

FIG. 16

depicts another embodiment wherein shell

62

contains clumps

224

of microorganisms. Shell

62

is preferably formed from a material that is not only water permeable but also sufficiently water soluble to release the microorganisms contained in the shell. Examples of suitable materials include but are not limited to paper and polyvinyl alcohol. The microorganisms can then bioremediate explosive material

208

by beginning at the exterior of explosive material

208

.

Yet another method of bioremediating explosives involves installing an explosive charge in a detonation site, such as a borehole, and then positioning microorganisms around the explosive charge by depositing microorganisms directly on the explosive charge and the detonation site. Similarly, a solution of microorganisms can be deposited at a detonation site. Then the explosive charge is placed in the suspension of microorganisms. Additionally, an explosive apparatus can be sprayed with or soaked in a suspension of microorganisms before being installed at a given detonation site, preferably while being exposed to a vacuum.

Experiments were conducted to study the process of remediating explosive materials according to the teachings of the present invention. To do so, a microorganism consortium was derived from soil and water samples obtained on the property of an established explosive manufacturer located at 8305 South Highway 6, Spanish Fork, Utah 84660 U.S.A. The microorganism consortium in the form of a suspension was combined with various types of explosive materials, either in solid form or in an aqueous suspension, and the results were observed and documented. The results of several of these tests are set forth below as examples.

EXAMPLE 1

Quantities of the explosive materials TNT and PETN in water were combined with the suspension of the microorganism consortium. The resulting mixture initially included 47.23 ppm of PETN and 40.63 PPM of TNT. The mixture was divided among containers that were stored in aerobic conditions at ambient temperature for various time periods. Table 1 below indicates the explosive analysis of these samples after each designated time interval. The explosive materials were substantially degraded after a period of five weeks.

TABLE 1

Aerobic Bioremediation of TNT and PETN

Explosive

Initial

Analysis After

Analysis After

Material

Analysis

3 Days

5 Weeks

PETN

47.23 ppm

40.94 ppm

7.25 ppm

TNT

40.63 ppm

5.32 ppm

0.62 ppm

EXAMPLE 2

The mixture prepared in Example 1 was stored in anaerobic conditions at ambient temperature and observed. The results were determined by HPLC analysis in ppm and averaged. Table 2 below sets forth the results obtained. As can be seen by comparing the results in Table 2 with the results in Table 1, the explosive materials tested remediated more rapidly under anaerobic conditions than under aerobic conditions.

TABLE 2

Anaerobic Bioremediation of PETN and TNT

Explosive

Initial

Analysis after

Analysis

Analysis after

Material

Analysis

3 Days

after 1 Week

5 Weeks

PETN

47.23 ppm

28.31 ppm

24.46 ppm

0.82 ppm

TNT

40.63 ppm

0.31 ppm

0.31 ppm

None

avg.

avg.

EXAMPLE 3

Discs of the explosive material Pentolite having a diameter of a pencil were split in two. When the discs were split each weighed about 0.1 gram. The discs were placed either in water as a control or in 6 ml to 8 ml of a suspension of the microorganism consortium. After a specific amount of time in aerobic conditions, the discs were dried and weighed or analyzed by HPLC. The liquid portions were analyzed by HPLC. The net remediated weight loss in the explosive material was determined by subtracting the control weight loss as a percentage from the weight loss as a percentage in each remediated explosive. The explosive loss by degradation is listed in Table 3 for each of the samples. The samples in B and C were tested for longer periods of time than the sample in A. The results of the testing of samples B and C show that significant bioremediation did not occur beyond the level achieved in sample A. This was most likely due to insufficient quantities of nutrients in samples B and C as the bioremediation activity probably ceased when the nutrients were consumed.

TABLE 3

Aerobic Bioremediation of Pentolite

Final dry

weight plus

weight of

explosive

Net

Sample

Sample

Initial

in liquid

Remediated

No.

or Test

Time

Weight

portion.

Weight Loss

A

Control

22 days

0.1355 g

0.1266 g =

6.97% Net

6.57% loss

Loss

Test

22 days

0.0981 g

0.0848 g =

13.54% loss

B

Control

88 days

0.0578 g

0.0557 g =

5.52% Net

3.63% loss

Explosive

Test

88 days

0.0743 g

0.0675 g =

Loss

9.15% loss

C

Control

173 days

0.1236 g

0.1236 g =

6.78% Net

no loss

Explosive

Test

173 days

0.0737 g

0.0687 g =

Loss

6.78% loss

EXAMPLE 4

Experiments were conducted to compare remediation rates under aerobic and anaerobic conditions. Separate 5 gram samples of PETN/TNT Pentolite in a ratio of 60:40 were analyzed and placed in 100 ml to 300 ml suspension of a microorganism consortium. One was subjected to aerobic conditions; the other was subjected to anaerobic conditions. After various periods of time the samples were removed, air dried, and weighed to determine the amount of explosive material that had not degraded. The weight of the remaining explosive material was subtracted from the original weight to determine the weight of the explosive material lost due to bioremediation. The results are listed in Table 4 below. The results indicate that an insufficient amount of microorganisms were utilized or that the amount of nutrient was insufficient particularly in light of the results obtained in the other examples.

TABLE 4

Aerobic and Anaerobic Bioremediation of

Pentolite

Percent

Percent

Condition:

Wt Loss

Wt Loss

Aerobic or

Original

at Time

at Time

Anaerobic

Weight

Time

listed

Time

Listed

Aerobic

5.015 g

66 days

3.21%

163 days

5.43%

Anaerobic

6.9027 g

—

—

179 days

3.10%

EXAMPLE 5

Also investigated was the remediation according to the present invention of low levels of explosive materials in water. The explosive materials RDX and PETN were mixed with the water, combined with a suspension of a microorganism consortium, and then stored. The samples were tested by HPLC for explosive content initially and after 2 weeks. As shown in Table 5 below the bioremediation was nearly complete after two weeks.

TABLE 5

Bioremediation of Suspension of RDX and PETN

Explosive

Initial

Analysis

Material

Analysis

after 2 weeks

RDX

6.6 ppm

Not detected

PETN

25.0 ppm

Less than 0.5 ppm

EXAMPLE 6

The remediation according to the present invention of soil contaminated with an explosive material was also investigated. Soil contaminated with the explosive material PETN was mixed with a suspension of a microorganism consortium and stored at ambient temperature. Samples were analyzed initially, after 44 days, and finally after 125 days. The PETN content in the soil dropped from 1659 ppm to 551 ppm. The results are set forth in Table 6 below.

TABLE 6

Bioremediation of Soil Contaminated with PETN

Analysis

Analysis

Initial

after

after

Analysis

44 Days

125 Days

1659.2 ppm

1193.2 ppm

551.8 ppm

EXAMPLE 7

In order to determine the effect of temperature on the growth of microorganism samples, the natural high temperature tolerances of the microorganism consortium were evaluated. The microorganism cultures were adapted to higher temperatures by slowly raising the growth temperature. By raising the temperature, the upper and lower limits of growth were both shifted upwards.

Two separate microbial growth stages were evaluated: the log phase, wherein the microorganisms experience logarithmic growth, and the stationary phase, wherein the microorganisms reach maximum growth. Microorganism cultures that enter the stationary phase late in their growth cycle induce the expression of genes which protect the microorganisms from various environmental stresses.

Four separate microorganism cultures were established. One culture, referred to as “30° C./Log Phase Culture”, was comprised of new inocula, experiencing logarithmic growth, in fresh minimal medium, with TNT extract as the sole nitrogen source, and grown at 30° C. for three days. A second culture, referred to as “30° C./Stationary Phase Culture”, was comprised of microorganisms that had reached maximum growth, in minimal medium, with TNT extract as the sole nitrogen source, previously grown at room temperature for several weeks, and additionally grown at 30° C. for three days. The third culture, referred to as “37° C./Log Phase Culture”, was comprised of new inocula, experiencing logarithmic growth, in fresh minimal medium, with TNT extract as the sole nitrogen source, and grown at 37° C. for three days. The final culture, referred to as “37° C./Stationary Phase Culture”, was comprised of microorganisms that had reached maximum growth, in minimal medium, with TNT extract as the sole nitrogen source, previously grown at room temperature for several weeks, and additionally grown at 37° C. for three days.

Samples of the four different microorganism cultures were subjected to temperatures ranging from 30° C. to 97° C. for twenty minutes. A small sample of each heated culture and a non-heated control culture were spread-plated on both nutrient agar plates, and minimal medium with 10% glycerol plates. The plates were incubated overnight at 30° C.

The microbial growth was evaluated according to the number of colony forming units of the plate or the visualization of distinct colonies. The results of this evaluation are illustrated in Table 7, below. Microbial growth covering the entire plate with few, if any, single colonies, was referred to as “total”. Microbial growth greater than 1000 clearly defined colonies per plate, or too numerous to count, was referred to as “>1000”. If the density of the sample was only slightly less than the density of the previous sample, an asterisk “*” appears after the notation. At the lower density levels, the colonies were distinguishable as comprising at least bacteria, “B” or fungus/filamentous bacteria, “F”. The number preceding “B” or “F” corresponds to the number of distinct colonies.

TABLE 7

Temperature tolerance of microorganism

consortium.

30° C./

37° C./

30° C./Log

Stationary

37° C./

Stationary

Temp.

Phase

Phase

Log Phase

Phase

° C.

Culture

Culture

Culture

Culture

Control

Total

>1000

Total

>1000

30° C.

Total

>1000

Total

>1000

37° C.

Total

>1000

Total

>1000

42° C.

Total

>1000*

Total

>1000

47° C.

Total*

>1000*

Total*

>1000

52° C.

130 B

180 F

Total*

7 F

57° C.

0 colonies

0 colonies

0 colonies

0 colonies

62° C.

0 colonies

0 colonies

0 colonies

0 colonies

67° C.

0 colonies

0 colonies

2 colonies

0 colonies

Control

Total

>1000

Total

>1000

72° C.

0 colonies

0 colonies

0 colonies

0 colonies

77° C.

0 colonies

0 colonies

0 colonies

0 colonies

82° C.

2 colonies

0 colonies

1 colony

0 colonies

87° C.

0 colonies

0 colonies

0 colonies

0 colonies

92° C.

0 colonies

0 colonies

0 colonies

0 colonies

97° C.

0 colonies

0 colonies

0 colonies

0 colonies

Control

Total

>1000

Total

>1000

The log phase cultures appeared predominantly to contain a single colony type of microorganism. The stationary phase cultures contained a single microorganism colony type and an organism that appeared to be a fungus or a filamentous bacterium.

None of the heated culture samples exhibited significant growth beyond 57° C. The difference in the growth phase of the cultures, i.e., log phase versus stationary phase, did not result in a significant difference in growth. However, the 37° C./Log Phase Culture did appear to exhibit some growth advantage. Note that at 52°, the 37° C./Log Phase Culture still had microbial growth covering the entire plate, whereas the growth of the other samples had been reduced to countable quantities.

In addition, the 37° C./Stationary Phase Culture and 37° C./Log Phase Culture samples exhibited a growth advantage over the 30° C./Stationary Phase Culture and 30° C./Log Phase Culture which is commensurate with the differential initial growth temperature of these samples. That is, because microorganism cultures can be adapted to higher temperatures within limits by slowly raising or lowering the growth temperature, by raising the temperature, the upper and lower limits of growth are both shifted upwards. Thus the 37° samples were amenable to more substantial growth at higher temperatures than the 30° samples.

Along these lines, a new culture of the 37° C./Log Phase Culture was established using minimal medium with TNT. A sample of this culture was placed in a water bath wherein the temperature was raised 1° C. every two days. Significant growth was exhibited as high as 41° C.

EXAMPLE 8

In order to assess the survival characteristics of the microorganism culture during cooling of the explosive charge, the following simulated casting experiment was performed using the 37° C./Log Phase Culture. Small samples of this culture were placed in tubes in water baths at 95° C. and 80° C. These water baths were programmed to drop 1° C. every minute based on a reasonable approximation of the rate of cooling experienced by the charge. At five minute intervals, small samples were removed from the tubes in the water baths and plated on nutrient agar plates. These plates were incubated at 30° C. overnight and checked at 12 and 36 hours for microorganism colonies. After 36 hours the growth on the plates was evaluated. A non-heated sample was included as the control. The results of this study are illustrated in Table 8 below.

The results of this study indicate that the samples from the 80° C. water bath had a better survival rate than the samples from the 95° C. water bath.

TABLE 8

Temperature tolerance of microorganism

consortium in simulated casting.

Temperature

Time

95° C. Bath

80° C. Bath

Control

0 min

Total

Total

90° C.

5 min

0 colonies

NA

85° C.

10 min

1 colony

NA

80° C.

15 min

0 colonies

NA

75° C.

20 min/5 min

0 colonies

1 colony

70° C.

25 min/10 min

1 colony

2 colonies

65° C.

30 min/15 min

1 colony

1 colony

60° C.

35 min/20 min

1 colony

3 colonies

55° C.

40 min/25 min

0 colonies

1 colony

50° C.

45 min/30 min

0 colonies

4 colonies

45° C.

NA/35 min

NA

3 colonies

40° C.

NA/40 min

NA

1 colony

35° C.

NA/45 min

NA

5 colonies

EXAMPLE 9

The purpose of the following evaluation was to demonstrate that any growth on TNT was greater than that which might be expected from low level contamination by nitrogen from other sources. In order to evaluate the growth characteristics of the microorganism culture with respect to the nitrogen supply, the following experiment was performed under aerobic conditions.

A sample of the 37° C./Log Phase Culture was placed in each of three fresh media formulations. The first contained mineral salts defined medium (MMO) and ammonia as the nitrogen source. The second contained MMO and TNT as the nitrogen source. The third contained only MMO and no added nitrogen. The cultures were then grown and shaken in an incubator at 37° C.

Growth was measured by evaluating the optical density of the culture. Samples removed from each culture were placed in a spectrophotometer and the optical density was measured at a wavelength of 425 nanometers, a wavelength not normally absorbed by molecules produced by the microorganisms. The optical density of the culture samples represents dispersion of the incident beam by the particulate microorganism. The higher the optical density value, the greater the amount of microbial growth. The optical density results are illustrated in Table 9, below.

TABLE 9

Effect of Nitrogen upon growth of

microorganism consortium under aerobic

conditions.

Optical

Density of

Optical

Optical Density

Culture in

Density of

of Culture

Ammonia

Culture with

Absent Addition

Time

Medium

TNT

of Nitrogen

0 hours

0.006

0.166

0.005

20 hours

0.008

0.152

0.018

48 Hours

0.010

0.144

0.023

146 Hours

1.520

0.432

0.073

Difference

1.514

0.266

0.068

Over

NA

3.99

NA

Background

The TNT and No Nitrogen cultures were significantly less productive than the ammonia supplemented cultures. Still the TNT supplemented culture values were consistently higher than the No Nitrogen values. This indicates that the cultures were using TNT as the nitrogen source in the TNT supplemented culture.

EXAMPLE 10

Another study, similar to Example 9, above, was performed under anaerobic conditions. A sample of the 37° C./Log Phase Culture was placed in each of three fresh media formulations. The first contained mineral salts defined medium (MMO) and ammonia as the nitrogen source. The second contained MMO and TNT as the nitrogen source. The third contained only MMO and no added nitrogen. The cultures were placed in sealed serum bottles and the atmosphere was replaced with pure Nitrogen. Cultures were incubated without shaking in an incubator at 37° C. The results of this study are illustrated in Table 10, below.

TABLE 10

Effect of Nitrogen upon growth of

microorganism consortium under anaerobic

conditions.

Optical

Density of

Optical

Optical Density

Culture in

Density of

of Culture

Ammonia

Culture with

Absent Additional

Time

Medium

TNT

Nitrogen

0 hours

0.008

0.204

0.005

20 hours

0.012

0.218

0.009

48 Hours

0.017

0.268

0.007

146 Hours

0.482

0.272

0.019

Difference

0.474

0.068

0.014

Over

NA

4.88

NA

Background

Once again, the TNT and No Nitrogen cultures were significantly less productive than the ammonia supplemented cultures. Still the TNT supplemented culture values were consistently higher than the No Nitrogen values. This indicates that the cultures were using TNT as the nitrogen source in the TNT supplemented culture. Overall, the anaerobic conditions showed less growth than the aerobic cultures.

EXAMPLE 11

In order to evaluate the thermal resistance of the microorganism consortium in a system which will adequately mimic those of a pentolite pour, fresh samples of a TNT grown consortium and a control absent TNT were freeze dried and tested directly for temperature sensitivity. The freeze dried samples were placed into aluminum foil packets. Aluminum foil was used because its heat transference properties ensured that the temperature experienced by the freezed dried powder approximated that produced by the oven. The foil packets were placed in an oven at a starting temperature of either 100° C. or 80° C. The initial 100° C. and 80° C. temperatures were maintained for 2 minutes. Each temperature was then incrementally decreased at the rate of 1° C. per minute to 35° C. The packets remained at 35° C. for 10 minutes and were then removed from the oven. The contents of the packets were placed in MMO with TNT and glycerol, and then placed in a shaking incubator at 37° C.

The negative controls were void of any color which indicates complete absence of nitrogen degradation. All other samples were in various stages of TNT degradation as indicated by the color reduction in the samples from colorless to light orange to deep red or violet. The samples that started at 80° C. exhibited more advanced TNT degradation than those that started at 100° C.

These results were in accordance with the results of Example, 8, above. To reiterate, in that study the samples from the 80° C. water bath had a more optimal survival rate that the samples from the 95° C. water bath. Therefore, although the consortium did respond after experiencing temperatures as high as 100° C., a maximum of 80° C. represented the more optimal initial temperature.

The lyophilized microorganisms still produced significant bioremediation results even after being exposed to temperatures corresponding to that of a hot melt of explosive material. Accordingly, it can be concluded that lyophilization of microorganisms dramatically improves the thermal resistance of the microorganisms.

EXAMPLE 12

In order to further evaluate the thermal tolerance and protection of the microorganism consortium, freeze drying was compared with microencapsulation. The microencapsulation procedure required maintaining a substantial amount of fresh cell culture. The cells were divided into 4 samples and resuspended in phosphate buffered saline (PBS); PBS and 3% dried milk; PBS and 3% bentonite clay; and minimal medium with glycerol. Samples of the four suspensions were prepared by freeze drying 2 ml portions. The remainder of the suspensions was divided into 2 samples for encapsulation into alginate and polyacrylamide. Encapsulation into alginate was accomplished by adding sodium alginate to the suspension sample and then adding the mixture dropwise into a Calcium Chloride solution, with a molarity of 0.1. Encapsulation into polyacrylamide was accomplished by combining a biacrylamide mixture with a catalyst, such as a product sold as Temed, and beta-mercaptoethanol. As the mixture polymerized, the microorganism suspension was trapped in a gel matrix. Half of each sample selected for encapsulation (alginate or polyacrylamide), was freeze dried and the other half was air dried.

All samples, (freeze dried, encapsulated and freeze dried, encapsulated and air dried), were exposed to the temperature curve of Example 8, above. The samples were then added to low temperature agar and overlaid on total nutrient agar. Outgrowth and survival of the samples was evaluated. Additional portions of each sample were then added back to minimal medium with glycerol and TNT to assess the survival of the TNT-critical portions of the consortium.

The encapsulated samples did not result in a significant difference in growth as compared with the freezed dried samples. Thus encapsulation did not offer any distinct advantage over freeze drying with respect to temperature tolerance and subsequent survivability of the microorganism consortium.

The present invention may be embodied in other specific forms without departing from its spirit or essential characteristics. The described embodiments are to be considered in all respects only as illustrated and not restrictive. The scope of the invention is, therefore, indicated by the appended claims rather than by the foregoing description. All changes which come within the meaning and range of equivalency of the claims are to be embraced within their scope.

Claims

1. A method for manufacturing an explosive device capable of self-remediation, if the explosive device fails to detonate as intended, said method comprising the steps:(a) forming a quantity of an explosive material into an explosive device; (b) identifying microorganisms capable of bioremediating said explosive material; and (c) positioning a quantity of said microorganisms in such proximity to said quantity of said explosive material in said explosive device that, when said quantity of microorganisms is mobilized, said microorganisms in said quantity thereof are capable of bioremediating said quantity of said explosive material in said explosive device, whereby if said explosive device is installed at a detonation site and fails to detonate as intended, when said quantity of microorganisms is mobilized, said microorganisms in said quantity thereof deactivate said explosive device by bioremediating said quantity of said explosive material in situ at the detonation site.
2. A method as recited in claim 1, wherein said microorganisms are selected from a group of microorganisms consisting of Pseudomonas spp., Escherichia spp., Morganella spp., Rhodococcus spp., Comamonas spp., and denitrifying microorganisms.
3. A method as recited in claim 1, wherein said microorganisms are selected from a group of microorganisms in Pseudomonas spp. consisting of aeruginosa, fluorescens, acidovorans, mendocina, and cepacia.
4. A method for manufacturing an explosive device capable of self-remediation, if the explosive device fails to detonate as intended, said method comprising the steps:(a) forming a quantity of an explosive material into an explosive device; (b) identifying microorganisms capable of bioremediating said explosive material, said microorganisms being among a microorganism consortium identified at the American Type Culture Collection by ATCC Designation No. 55784; and (c) positioning a quantity of said microorganisms in such proximity to said quantity of said explosive material in said explosive device that, when said quantity of microorganisms is mobilized, said microorganisms in said quantity thereof are capable of bioremediating said quantity of said explosive material in said explosive device, and if said explosive device is installed at a detonation site and fails to detonate as intended, said microorganisms in said quantity thereof deactivate said explosive device by bioremediating said quantity of said explosive material in situ at said detonation site.
5. A method as recited in claim 1, wherein said explosive material is selected from a group of explosive materials consisting of organic nitroaromatic explosives, organic nitramine explosives, and organic nitric ester explosives.
6. A method as recited in claim 1, wherein said explosive material is selected from a group of explosive materials consisting of trinitrotoluene, hexanitrostilbene, hexanitroazobenzene, diaminotrinitrobenzene and triaminotrinitrobenzene, cyclotrimethylene trinitramine, cyclotetramethylene tetranitramine, nitroguanidine, 2,4,6-trinitrophenylmethylnitramine, pentaerythritol tetranitrate, nitroglycerine, and ethylene glycol dinitrate.
7. A method as recited in claim 1, wherein said microorganisms are sufficiently mobile to commence bioremediation of said explosive material.
8. A method as recited in claim 1, further comprising the step of providing mobilization means for mobilizing said microorganisms to contact said quantity of said explosive material.
9. A method for manufacturing an explosive device capable of self-remediation, if the explosive device fails to detonate as intended, said method comprising the steps:(a) forming a quantity of an explosive material into an explosive device; (b) identifying microorganisms capable of bioremediating said explosive material; and (c) positioning a quantity of said microorganisms in such proximity to said quantity of said explosive material in said explosive device that, when said quantity of microorganisms is mobilized, said microorganisms in said quantity thereof are capable of bioremediating said quantity of said explosive material in said explosive device, whereby if said explosive device is installed at a detonation site and fails to detonate as intended when said quantity of microorganisms is mobilized, said microorganisms in said quantity thereof deactivate said explosive device by bioremediating said quantity of said explosive material in situ at the detonation site, wherein said step of positioning comprises depositing said microorganisms in a structure having a removable barrier between said microorganisms and said quantity of said explosive material.
10. A method as recited in claim 9, wherein said barrier is removable mechanically.
11. method as recited in claim 9, wherein said barrier is removable electrically.
12. A method as recited in claim 9, wherein said barrier is removable chemically.
13. A method as recited in claim 1, wherein said step of positioning comprises the step of dispersing said microorganisms in said quantity of said explosive material.
14. A method as recited in claim 1, wherein said microorganisms are in an aggregation, and said method further comprises the step of shaping said aggregation into a form selected from the group consisting of a pellet, a capsule, a shard, a flake, a granule, a powder, and a clump.
15. A method as recited in claim 1, wherein said microorganisms are dehydrated.
16. A method as recited in claim 1, wherein said microorganisms are freeze dried.
17. A method as recited in claim 1, wherein said microorganisms are sufficiently resistant to heat that a significant portion of said microorganisms survive when said step of positioning occurs at a temperature of about 100° C.
18. A method as recited in claim 14, wherein said aggregation further comprises thermal protection additives.
19. A method as recited in claim 1, wherein said quantity of said explosive material is porous.
20. A method for manufacturing an explosive device capable of self-remediation, if the explosive device fails to detonate as intended, said method comprising the steps:(a) forming a quantity of an explosive material into an explosive device; (b) disposing said quantity of said explosive material in a shell, said shell enabling water from the exterior of said shell to flow through said shell into contact with said quantity of said explosive material; (c) identifying microorganisms capable of bioremediating said explosive material; and (d) positioning a quantity of said microorganisms in such proximity to said quantity of said explosive material in said explosive device that, when said quantity of microorganisms is mobilized, said microorganisms in said quantity thereof are capable of bioremediating said quantity of said explosive material in said explosive device, whereby if said explosive device is installed at a detonation site and fails to detonate as intended, when said quantity of microorganisms is mobilized, said microorganisms in said quantity thereof deactivate said explosive device by bioremediating said quantity of said explosive material in situ at the detonation site.
21. A method for manufacturing an explosive device capable of self-remediation, if the explosive device fails to detonate as intended, said method comprising the steps:(a) forming a quantity of an explosive material into an explosive device; (b) identifying microorganisms capable of bioremediating said explosive material; (c) shaping said microorganisms into aggregations having a form selected from the group consisting of a pellet, a capsule, a shard, a flake, a granule, a powder, and a clump; and (d) positioning said aggregations in such proximity to said quantity of said explosive material in said explosive device that, when said microorganisms in said aggregations are activated, said microorganisms in said aggregations are capable of bioremediating said quantity of said explosive material in said explosive device, whereby if said explosive device is installed at a detonation site and fails to detonate as intended, when said quantity of microorganisms is mobilized, said microorganisms in said quantity thereof deactivate said explosive device by bioremediating said quantity of said explosive material in situ at the detonation site.
22. A method as recited in claim 21, wherein said step of forming occurs before said step of positioning.
23. A method as recited in claim 22, wherein said step of positioning comprises the step of depositing said aggregations on an exposed surface of said explosive material in said explosive device.
24. A method for manufacturing an explosive device capable of self-remediation, if the explosive device fails to detonate as intended, said method comprising the steps:(a) forming a quantity of an explosive material into an explosive device, wherein said step of forming comprises disposing said quantity of said explosive material in a shell, and said shell enables water from the exterior of said shell to flow through said shell into contact with said quantity of said explosive material; (b) identifying microorganisms capable of bioremediating said explosive material; (c) shaping said microorganisms into aggregations having a form selected from the group consisting of a pellet, a capsule, a shard, a flake, a granule, a powder, and a clump; and (d) after said step of forming, positioning said aggregations in such proximity to said quantity of said explosive material in said explosive device that, when said microorganisms in said aggregations are activated, said microorganisms in said aggregations are capable of bioremediating said quantity of said explosive material in said explosive device, whereby if said explosive device is installed at a detonation site and fails to detonate as intended, when said quantity of microorganisms is mobilized, said microorganisms in said quantity thereof deactivate said explosive device by bioremediating said quantity of said explosive material in situ at the detonation site.
25. A method as recited in claim 24, wherein said step of positioning comprises the step of depositing said aggregations on a surface of said quantity of said explosive material in said shell.
26. A method as recited in claim 21, wherein said shell is porous, and said step of positioning comprises the step of embedding said aggregations in said shell.
27. A method as recited in claim 24, wherein said step of positioning comprises the step of inserting into said quantity of said explosive material in said shell a longitudinal core of said aggregations.
28. A method as recited in claim 21, wherein said explosive material in said explosive apparatus is porous.
29. A method as recited in claim 21, wherein a surfactant is mixed with said explosive material.
30. A method as recited in claim 21, wherein said step of positioning occurs before said step of forming.
31. A method as recited in claim 30, wherein said step of positioning comprises the step of dispersing said aggregations in said quantity of said explosive material.
32. A method as recited in claim 30, further comprising the step of introducing thermal protective additives into said aggregations.
33. A method for manufacturing an explosive device capable of self-remediation, if the explosive device fails to detonate as intended, said method comprising the steps:(a) forming a quantity of an explosive material into an explosive device; (b) disposing said quantity of said explosive material of said explosive device in a shell, said shell enabling water from the exterior of said shell to flow through said shell into contact with said quantity of said explosive material therein; (c) identifying microorganisms capable of bioremediating said explosive material; (d) housing.a quantity of said microorganisms in a bioremediation apparatus; and (e) coupling said bioremediation apparatus to said shell with said quantity of explosive material of said explosive device disposed therein, thereby positioning said quantity of microorganisms in such proximity to said quantity of said explosive material in said shell that, whereby when said quantity of microorganisms is mobilized, said microorganisms in said quantity thereof are capable of bioremediating said quantity of said explosive material in said explosive device, and if said explosive device is installed at a detonation site and fails to detonate as intended, said microorganisms in said quantity thereof deactivate said explosive device by bioremediating said quantity of said explosive material in situ at said detonation site.
34. A method as recited in claim 33, wherein said shell has an open end, a capwell positioned at said open end, and a bioremediation portal formed through said capwell communicating with said explosive material in said shell.
35. A method as recited in claim 33, wherein said bioremediation apparatus comprises:(a) storage means for releasably containing said microorganisms; and (b) divider means for selectively releasing said microorganisms from said storage means into contact with said explosive material in said explosive device.
36. A method as recited in claim 35, wherein said divider means comprises a removable barrier between said microorganisms and said quantity of said explosive material when said bioremediation apparatus is coupled to said explosive device.
37. A method as recited in claim 36, wherein said barrier is removable mechanically.
38. A method as recited in claim 36, wherein said barrier is removable electrically.
39. A method as recited in claim 36, wherein said barrier is removable chemically.
40. A method as recited in claim 35, wherein said bioremediation apparatus further comprises:(a) reservoir means for releasably containing a liquid capable of mobilizing said microorganisms; and (b) separation means for selectively releasing said liquid from said reservoir means into said storage means.
41. A method as recited in claim 33, wherein said bioremediation apparatus comprises:(a) reservoir means for releasably containing a liquid capable of mobilizing said microorganisms; (b) storage means for releasably containing said microorganisms, said storage means being in selective communication with said reservoir means; (c) first valve means for releasing said liquid from said reservoir means into said storage means in the open condition of said first valve means; and (d) second valve means for releasing said microorganisms and said liquid into contact with said explosive material in said explosive apparatus when said explosive apparatus is coupled to said explosive device.
42. A method as recited in claim 41, wherein said first valve means and said second valve means are operably interconnected.
43. A method for manufacturing an explosive device capable of self-remediation, if the explosive device fails to detonate as intended, said method comprising the steps:(a) selecting an explosive material from which to form an explosive device; (b) identifying microorganisms capable of bioremediating said explosive material; (c) dispersing a quantity of said microorganisms in a quantity of said explosive material, thereby forming an explosive mixture with bioremediating capacity; and (d) forming a quantity of said explosive mixture into an explosive device, whereby when said quantity of said microorganisms in said explosive mixture is mobilized, said microorganisms in said quantity thereof are capable of bioremediating said quantity of said explosive material in said explosive device, whereby if said explosive device is installed at a detonation site and fails to detonate as intended, when said quantity of microorganisms is mobilized, said microorganisms in said quantity thereof deactivate said explosive device by bioremediating said quantity of said explosive material in situ at the detonation site.
44. A method as recited in claim 43, further comprising the step of shaping said microorganisms into aggregations having a form selected from the group consisting of a pellet, a capsule, a shard, a flake, a granule, a powder, and a clump.
45. A method as recited in claim 44, wherein said microorganisms are dehydrated.
46. A method as recited in claim 44, wherein said microorganisms are freeze dried.
47. A method as recited in claim 44, wherein said aggregations further comprise a thermal protection additive.
48. A method as recited in claim 43, wherein said explosive material in said explosive apparatus is porous.
49. A method for manufacturing an explosive device capable of self-remediation, if the explosive device fails to detonate as intended, said method comprising the steps:(a) selecting an explosive material from which to form an explosive device; (b) identifying microorganisms capable of bioremediating said explosive material; (c) dispersing a quantity of said microorganisms in a quantity of said explosive material, thereby forming an explosive mixture with bioremediating capacity; (d) forming a quantity of said explosive mixture with bioremediating capacity into an explosive device; and (e) disposing said quantity of said explosive mixture of said explosive device in a shell, said shell enabling water from the exterior of said shell to flow through said shell into contact with said quantity of said explosive mixture with bioremediating capacity, thereby mobilizing said microorganisms therein, whereby when said quantity of microorganisms in said explosive mixture is mobilized, said microorganisms in said quantity thereof are capable of bioremediating said quantity of said explosive material in said explosive device, and if said explosive device is installed at a detonation site and fails to detonate as intended, said microorganisms in said quantity thereof deactivate said explosive device by bioremediating said quantity of said explosive material in situ at said detonation site.
50. A method as recited in claim 44, wherein said shell is porous.
51. A method for manufacturing an explosive device capable of self-remediation, if the explosive device fails to detonate as intended, said method comprising the steps:(a) selecting an explosive material from which to form an explosive device; (b) identifying microorganisms capable of bioremediating said explosive material, said microorganisms being among a microorganism consortium identified at the American Type Culture Collection by ATCC Designation No. 55784; (c) dispersing a quantity of said microorganisms in a quantity of said explosive material, thereby forming an explosive mixture with bioremediating capacity; and d) forming a quantity of said explosive mixture with bioremediating capacity into an explosive device, whereby when said quantity of microorganisms in said explosive mixture is mobilized, said microorganisms in said quantity thereof are capable of bioremediating said quantity of said explosive material in said explosive device, and if said explosive device is installed at a detonation site and fails to detonate as intended, said microorganisms in said quantity thereof deactivate said explosive device by bioremediating said quantity of said explosive material in situ at said detonation site.
52. A method as recited in claim 44, further comprising the step of providing mobilization means for mobilizing said microorganisms to contact said quantity of said explosive material.
53. A method as recited in claim 4, wherein said step of positioning comprises the step of dispersing said microorganisms in said quantity of said explosive material.
54. A method as recited in claim 4, wherein said microorganisms are in an aggregation, and said method further comprises the step of shaping said aggregation into a form selected from the group consisting of a pellet, a capsule, a shard, a flake, a granule, a powder, and a clump.
55. A method as recited in claim 4, wherein said microorganisms are dehydrated.
56. A method as recited in claim 4, wherein said microorganisms are freeze dried.
57. A method as recited in claim 4, wherein said microorganisms are sufficiently resistant to heat that a significant portion of said microorganisms survive when said step of positioning occurs at a temperature of about 100° C.
58. A method as recited in claim 54, wherein said aggregation further comprises thermal protection additives.
59. A method as recited in claim 4, wherein said quantity of said explosive material is porous.
60. A method as recited in claim 20, wherein said shell has an open end, a capwell positioned at said open end, and a bioremediation portal formed through said capwell communicating with said explosive material in said shell.
61. A method as recited in claim 20, wherein said shell is porous.
62. A method as recited in claim 20, wherein said microorganisms are selected from a group of microorganisms consisting of Pseudomonas spp., Escherichia spp., Morganella spp., Rhodococcus spp., Comamonas spp., and denitrifying microorganisms.
63. A method as recited in claim 20, wherein said microorganisms are selected from a group of microorganisms in Pseudomonas spp. consisting of aeruginosa, fluorescens, acidovorans, mendocina, and cepacia.
64. A method as recited in claim 20, wherein said microorganisms are among a microorganism consortium identified at the American Type Culture Collection by ATCC Designation No. 55784.
65. A method as recited in claim 20, further comprising the step of providing mobilization means for mobilizing said microorganisms to contact said quantity of said explosive material.
66. A method as recited in claim 20, wherein said step of positioning comprises the step of dispersing said microorganisms in said quantity of said explosive material.
67. A method as recited in claim 20, wherein said microorganisms are in an aggregation, and said method further comprises the step of shaping said aggregation into a form selected from the group consisting of a pellet, a capsule, a shard, a flake, a granule, a powder, and a clump.
68. A method for manufacturing an explosive device capable of self-remediation, if the explosive device fails to detonate as intended, said method comprising the steps:(a) forming a quantity of an explosive material into an explosive device; (b) disposing said quantity of said explosive material in a shell, said shell enabling water from the exterior of said shell to flow through said shell into contact with said quantity of said explosive material; (c) identifying microorganisms capable of bioremediating said explosive material; and (d) positioning a quantity of said microorganisms in such proximity to said quantity of said explosive material in said explosive device that, when said quantity of microorganisms is mobilized, said microorganisms in said quantity thereof are capable of bioremediating said quantity of said explosive material in said explosive device, whereby if said explosive device is installed at a detonation site and fails to detonate as intended, when said quantity of microorganisms is mobilized, said microorganisms in said quantity thereof deactivate said explosive device by bioremediating said quantity of said explosive material in situ at the detonation site, said microorganisms in said quantity thereof being dehydrated.
69. A method as recited in claim 68, wherein said microorganisms in said quantity thereof are freeze dried.
70. A method as recited in claim 20, wherein said microorganisms are sufficiently resistant to heat that a significant portion of said microorganisms survive when said step of positioning occurs at a temperature of about 100° C.
71. A method as recited in claim 67, wherein said aggregation further comprises thermal protection additives.
72. A method as recited in claim 20, wherein said quantity of said explosive material is porous.
73. A method as recited in claim 49, wherein said shell has an open end, a capwell positioned at said open end, and a bioremediation portal formed through said capwell communicating with said explosive material in said shell.
74. A method as recited in claim 49, wherein said microorganisms are selected from a group of microorganisms consisting of Pseudomonas spp., Escherichia spp., Morganella spp., Rhodococcus spp., Comamonas spp., and denitrifying microorganisms.
75. A method as recited in claim 49, wherein said microorganisms are selected from a group of microorganisms in Pseudomonas spp. consisting of aeruginosa, fluorescens, acidovorans, mendocina, and cepacia.
76. A method as recited in claim 49, wherein said microorganisms are among a microorganism consortium identified at the American Type Culture Collection by ATCC Designation No. 55784.
77. A method as recited in claim 49, further comprising the step of providing mobilization means for mobilizing said microorganisms to contact said quantity of said explosive material.
78. A method as recited in claim 49, wherein said microorganisms are in an aggregation, and said method further comprises the step of shaping said aggregation into a form selected from the group consisting of a pellet, a capsule, a shard, a flake, a granule, a powder, and a clump.
79. A method as recited in claim 49, wherein said microorganisms are dehydrated.
80. A method as recited in claim 49, wherein said microorganisms are freeze dried.
81. A method as recited in claim 49, wherein said microorganisms are sufficiently resistant to heat that a significant portion of said microorganisms survive when said step of positioning occurs at a temperature of about 100° C.
82. A method as recited in claim 78, wherein said aggregation further comprises thermal protection additives.
83. A method as recited in claim 49, wherein said quantity of said explosive material is porous.
84. A method as recited in claim 51, further comprising the step of providing mobilization means for mobilizing said microorganisms to contact said quantity of said explosive material.
85. A method as recited in claim 51, wherein said microorganisms are in an aggregation, and said method further comprises the step of shaping said aggregation into a form selected from the group consisting of a pellet, a capsule, a shard, a flake, a granule, a powder, and a clump.
86. A method as recited in claim 21, wherein said microorganisms are among a microorganism consortium identified at the American Type Culture Collection by ATCC Designation No. 55784.
87. A method as recited in claim 51, wherein said microorganisms are dehydrated.
88. A method as recited in claim 51, wherein said microorganisms are freeze dried.
89. A method as recited in claim 51, wherein said microorganisms are sufficiently resistant to heat that a significant portion of said microorganisms survive when said step of positioning occurs at a temperature of about 100° C.
90. A method as recited in claim 85, wherein said aggregation further comprises thermal protection additives.
91. A method as recited in claim 51, wherein said quantity of said explosive material is porous.

RELATED APPLICATIONS

This application, is a divisional application of U.S. patent application Ser. No. 08/743,460 that was filed on Oct. 18, 1996 (hereinafter “the Parent Application”), and that issued as U.S. Pat. No. 6,120,627 on Sep. 19, 2000. The Parent Application; is a continuation-in-part application of both U.S. patent application Ser. No. 08/658,104 that was filed on Jun. 4, 1996, now abandoned, which is a continuation-in-part of U.S. patent application Ser. No. 08/560,074 that was filed on Nov. 17, 1995, now abandoned and U.S. patent application Ser. No. 08/687,092 that was filed Jun. 4, 1996, now abandoned which is a continuation-in-part application of U.S. patent application Ser. No. 08/560,102 that was filed on Nov. 17, 1995, now abandoned. This application discloses subject matter related to that disclosed in U.S. Pat. No. 5,736,669 that issued on Apr. 7, 1998, from U.S. patent application Ser. No. 658,995 filed on Jun. 4, 1996, and which is a continuation-in-part of U.S. patent application Ser. No. 560,527 that was filed on Nov. 17, 1995, and subject matter related to that disclosed in U.S. Pat. No. 5,763,815 that issued on Apr. 7, 1998, from, and U.S. patent application Ser. No. 658,142 that was filed Jun. 4, 1996, and which is a continuation-in-part of U.S. patent application Ser. No. 560,074, filed on Nov. 17, 1995. This application is also related to a U.S. patent application that is being filed contemporaneously herewith and that is related to the same applications and in the same manner as those set forth above for this application.

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Continuation in Parts (4)

	Number	Date	Country
Parent	08/658104	Jun 1996	US
Child	08/743460		US
Parent	08/687092	Jun 1996	US
Child	08/658104		US
Parent	08/560102	Nov 1995	US
Child	08/687092		US
Parent	08/560074	Nov 1995	US
Child	08/658104		US

Method for manufacturing explosive device having self-remediating capacity

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