CA1094479A - Process for producing xanthomonas hydrophilic colloid for use in displacement of oil from partially depleted reservoirs - Google Patents
Process for producing xanthomonas hydrophilic colloid for use in displacement of oil from partially depleted reservoirsInfo
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- CA1094479A CA1094479A CA284,129A CA284129A CA1094479A CA 1094479 A CA1094479 A CA 1094479A CA 284129 A CA284129 A CA 284129A CA 1094479 A CA1094479 A CA 1094479A
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- colloid
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- C—CHEMISTRY; METALLURGY
- C09—DYES; PAINTS; POLISHES; NATURAL RESINS; ADHESIVES; COMPOSITIONS NOT OTHERWISE PROVIDED FOR; APPLICATIONS OF MATERIALS NOT OTHERWISE PROVIDED FOR
- C09K—MATERIALS FOR MISCELLANEOUS APPLICATIONS, NOT PROVIDED FOR ELSEWHERE
- C09K8/00—Compositions for drilling of boreholes or wells; Compositions for treating boreholes or wells, e.g. for completion or for remedial operations
- C09K8/60—Compositions for stimulating production by acting on the underground formation
- C09K8/84—Compositions based on water or polar solvents
- C09K8/86—Compositions based on water or polar solvents containing organic compounds
- C09K8/88—Compositions based on water or polar solvents containing organic compounds macromolecular compounds
- C09K8/90—Compositions based on water or polar solvents containing organic compounds macromolecular compounds of natural origin, e.g. polysaccharides, cellulose
- C09K8/905—Biopolymers
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12P—FERMENTATION OR ENZYME-USING PROCESSES TO SYNTHESISE A DESIRED CHEMICAL COMPOUND OR COMPOSITION OR TO SEPARATE OPTICAL ISOMERS FROM A RACEMIC MIXTURE
- C12P19/00—Preparation of compounds containing saccharide radicals
- C12P19/04—Polysaccharides, i.e. compounds containing more than five saccharide radicals attached to each other by glycosidic bonds
- C12P19/06—Xanthan, i.e. Xanthomonas-type heteropolysaccharides
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- Genetics & Genomics (AREA)
- Preparation Of Compounds By Using Micro-Organisms (AREA)
- Emulsifying, Dispersing, Foam-Producing Or Wetting Agents (AREA)
- Colloid Chemistry (AREA)
- Micro-Organisms Or Cultivation Processes Thereof (AREA)
- Peptides Or Proteins (AREA)
Abstract
ABSTRACT OF THE DISCLOSURE
A process is described for preparing a Xanthomonas colloid-containing fermentation broth suitable for the pre-paration of mobility control solution used in oil recovery which comprises aerobically fermenting a Xanthomonas organism in an aqueous nutrient medium whose ingredients comprise a carbo-hydrate, a nitrogen source, an assimilable Krebs cycle acid, chelated calcium and trace elements, whereby the whole broth produced provides mobility control solutions of about 100 to 3000 ppm of Xanthomonas colloid which are substantially free of insoluble matter having a particle size greater than about 3 microns.
A process is described for preparing a Xanthomonas colloid-containing fermentation broth suitable for the pre-paration of mobility control solution used in oil recovery which comprises aerobically fermenting a Xanthomonas organism in an aqueous nutrient medium whose ingredients comprise a carbo-hydrate, a nitrogen source, an assimilable Krebs cycle acid, chelated calcium and trace elements, whereby the whole broth produced provides mobility control solutions of about 100 to 3000 ppm of Xanthomonas colloid which are substantially free of insoluble matter having a particle size greater than about 3 microns.
Description
~.0~3 1~9 There are extensive published reports relating to the production of hydrophilic colloids by the aerobic propagation of bacteria of the genus Xanthomonas in aq~eous nutrient media. The earliest work in this field was done at the Northern Rçgional Research Labo~atory of the United States Department of Agriculture at Peoria, Illinois and is described in United States Patent 3,000,790, Modified fermentation processes are described in United States Patents 3,020,206; 3,391,060; 3,427,226; 3,433,708;
3,271,267; 3,251,749; 3,281,329; 3,455,766: 3,565,763; 3,594,280;
and 3,391,061.
~he hydrophilic colloid (xanthan gum) produced by Xanthomonas campestris is a poly~accharide which contains mannose, -glucose, glucuronic acid, O-acetyl radi~als and acetal-linked pyruvic acid in molar ratio o~ 2:2:1:1:0,5, This gum and its lS derivatives have found wide food and industrial applications. Of special interest is the increasing fo~us on tha use of xanthan gum in displacement of oil from partially depleted reservoirs, Typically, oil is recovered from underground reservoirs vla a series of sequential operations. A new well will generally produce a limited amount of oil as a result of release of internal pressure in the well. As this pressure becomes depleted, it is necessary to pump further quantities of oil by mechanical means.
These measures recover only about 25% of the total oil stored in the reservoir. A great doal of oil is still trapped within the pores of the formation. Further enhancement of recovery can then C -2~
109 L~ 479 be effected by secondary recovery. In one method of recovery a waterflood is carried out by pumping water into a well or series of wells, displacing part of the trapped oil from the porous rock and collecting the displaced oil from surrounding wells.
However, waterflooding still leaves about 55-60% of the availab~
oil trapped in the formation. The explanation for this phenomenon is that the water has a very low viscoisty compared to the crude oil and tends to follow the path of least resistance, fingering through the oil and leaving large pockets untouched. In addition, surface forces in the formation tend to bind the oil and prevent its displacement.
A number of processes have been developed in recent years to recover further quantities of oil from these reservoirs by the use of mobility control solutions which enhance oil dis-placement by increasing the viscosity or permeability of thedisplacing fluid. Of interest are those enhanced recovery pro-cesses employing polymer flooding with a polysaccharide or poly-acrylamide to increase the viscosity of the displacing fluid.
Variations of this process include the use of surfactants and co-surfactants to release the oil from the reck formation. Poly-acrylamides have been found to suffer such deficiencies as ~iscosity loss in brines and severe shear sensitivity. Since, as was well documented in the prior art, xanthan gum is in-sensitive to salts (does not precipitate or lose viscosity under normal conditions), is shear stable, thermostable and viscosity stable over a wide pH range, xanthan gum is a good displacing agent. Moreover, the gum is poorly adsorbed on the elements of the porous rock formations and it gives viscosities useful in en-hanced oil recovery (5 to 90 Centipoise units at 1 32 sec. 1 30 shear rate) at low concentrations (100 to 3000 ppm).
. . ~ , .
..
'' .
~09~1i47!~
The use of solutions of xanthan gum or derivatives of xanthan g~m for oil recovery is described in United States Patents 3,243,000; 3,198,268; 3,532,166; 3,305,016; 3,251,417; 3,319,606;
3,319,715; 3,373,810, 3,434,542 and 3,729,460, It is suggested S in United States Patent 3,305,016 that aqueous solution contain-ing the heteropolysaccharide in sufficient ~uantity to increase the viscosity be employed as the thickening agent in preparing viscous waterflooding solutions. The polysaccharide may be pre-pared, separated, purified and then added. Alternatively, accord-ing to this reference, the entire culture, after adding a bacter-icide (e.g., formaldehyde) to kill the bacteria, may be added to the flood water.
United States 3,000,790 describes the culturing of a Xanthomonas bacterium in a well aerated medium containing commer-cial glucoqe, an organic source of nitrogen, dipotassium phosphate and appropriate trace elements. The source of organic nitrogen usually employed is distillers' solubles. The use of this organic nitrogen source contributes a substantial quantity of insolubles to the fermentation broth.
The processes described in United States Patents 3,000,790, 3,391,060 and the other fermentation processes previous-ly listed yield final fermentation broths that contain su~stantial amounts of insoluble matter, even when diluted with water, for injection into oil-bearing subterranean formations to impart the necessary and desired mobility control for oil displacement. The particulate matter and in certain c~ses the Xanthomonas cells in such whole broth would soon plug the oil-bearing formation at the site of injection and thus foul the well and prevent any further oil recovery. Furthermore, the same problem would be encountered with reconstituted xanthan gum precipitated and separated from ~, ~ 3 ~- 4 , , .
, :
:, ~ , ` 1094479 these fermentation broths. The plugging tendencies of these fermentation broths can be obviated by filtration through diatom-aceous earth leaf filters to remove the Xanthomonas cells and particulate and colloidal matter. However~ suah additional filtering steps are expensive and add significantly to the overall cost factors for enhanced oil recovery.
United States 3,853,771 approach~s the plugging pro~lem of whole fermentation broths by claiming a process for dissolving or dispersing cellular microorganisms which comprises contacting said materials with an aqueous solution containing at least one surfactant effective for dispersing outer wall layers of micro-organism cells, at least on~ chelating agent for dispersing the inner wall layers of microorganism cells, and at least one alkali metal hydroxide effective for enhanoing said dispersing actionsO
United States 4,010,071 describes a process for clarify-ing fermentation broths and other aqueous suspensions containing a dissolved xanthan gum and suspended solids resulting from the fermentation by treatment with a minor amount of a pro~ease enzyme. The injectivity of aqueous solutions containing xanthan gum so clarified is improved in oil well flooding operations over solutions not so treated, However, this treatment does not over-come plugging problems due to the presence of insoluble inorganic or non-proteinaceous organic materialæ present in the fermentation medium or producçd during the course of the fermentation.
The object of the process of United States Patent 3,391,060 is to recover a polysaccharide product of substantial purity without the use of extensive separation procedures. A
high quality, high viscosity, iight colored, high purity xanthan gum is recovered from a Xanthomonas fermentation broth. According to this patent, recovery i9 simplified and elaborate purification i `` ` ~5~
. . ~ I ~ : .- ' .
1' . ' . I ' ' ` `
,~ ` `~ ". ` ` ' / . I .; ; ' 109~479 procedures are obviated by the replacement of the organic source of nitrogen in the broth with an inorganic source of nitrogen (i~e., ammonium nitrate). However, the fermentation process de-scribed therein is not economical because of lengthy reaction times required and low yields of biopolymer obtained.
The method of improving the permeability of mobility control solutions by the addition of certain hydroxy substituted carboxylic acids such as malic, tartaric, citric, gluconic, lactic and salicylic is described in United States Patent 2,867,279.
This invention is concerned with an economical process for preparing a Xanthomonas colloid-containing fermentation broth suitable for preparation of mobility control solutions used in oil recovery which comprises aerobically ~ermenting a Xant~Dmonas organism in an aqueous nutrient medium whose ingredients comprise a carbohydrate, a nitrogen source, a Krebs cycle acid, chelated calcium, manganese ions and iron ions. The whole broth produced provides mobility control solutions of about 100 to 3000 ppm Xanthomonas colloid which are substantially free of insoluble ~; matter having a particle size greater than about 3 microns.
According to the present invention there is provided a process for preparing a Xanthomonas colloid-containing ferment-ation broth suitable for the preparation of mobility control solutions used in oil recovery characterized in that a Xanthomonas organism is fermented aerobically in an aqueous nutrient medium whose ingredients comprise a carbohydrate, a nitrogen source, about 0.1 to 10 grams per liter of an assimilable Krebs cycle acid, about 1 to 200 ppm chelated calcium, about 0.25 to 20 ppm iron and trace elements until at least about 100 ppm colloid is present in the broth, whereby the whole broth produced provides mobility control solutions of about 100 to 3000 ppm Xanthomonas C !, -6-.. ,-- . , ~ , . , , .... .. - - ~ :
109~79 colloid content which are substantially free of insoluble matter having a particle size greater than about 3 microns, The present invention now provides for the first time a practical process for prepari~g a Xanthomonas fermentation broth which without treatmant or clarification provides mo~ility control solutions for use in oil recovery ha~ing a use concentra-tion of about 100 to 3000 ppm Xanthomonas colloid which are sub-stantially free of insoluble matter having a particle size greater than about 3 microns. According to this invention, the whole fermentation broth may be used directly as a mobility control solution suoh as where the amount of colloid produaed during fermentation is within the desired range of use concentration.
Alternatively, the broth may be diluted with water or a water 6a-. . ' '' ' ", .
~0~4~79 solution such as ~rine to reduce the level of colloid to the desired range, Additives to modify the properties of the mobility control solutions may be employed in addition to the whole or un-clarified broths of the present invention.
S It has been found that oil in cores from oil fields generally will be effectively recovered by xanthan gum if the poly-saccharide solution at use concentration can be made to pass a Millipore filterability test as described later. Typical pore sizes o~ Millipore filters used for this test are 0.45 to 3.0 m~crons. "Millipore" is a trademark.
In addition to Millipore filterability, core tests are - performed as described by W.B. Gogarty in Mobility Control with Polymer Solutions, Paper ~SPE 1566B) presented at the Society of Engineers 41st Annual Fall Meeting held in Dallas, Texas, lS October 2-5, 1966.
A novel feature of the fermentation broths of the present invention, importantly distinguished from previously reported Xanthomonas fermentation broths and preparations, is the obviated need for expensive and time-consuming filtration or clarification.
Important factors that help make this possible are the following:
1. All nutrient ingredients are essentially water soluble or become essentially water soluble during the course of the fer-~ntation or prior to injection.
3,271,267; 3,251,749; 3,281,329; 3,455,766: 3,565,763; 3,594,280;
and 3,391,061.
~he hydrophilic colloid (xanthan gum) produced by Xanthomonas campestris is a poly~accharide which contains mannose, -glucose, glucuronic acid, O-acetyl radi~als and acetal-linked pyruvic acid in molar ratio o~ 2:2:1:1:0,5, This gum and its lS derivatives have found wide food and industrial applications. Of special interest is the increasing fo~us on tha use of xanthan gum in displacement of oil from partially depleted reservoirs, Typically, oil is recovered from underground reservoirs vla a series of sequential operations. A new well will generally produce a limited amount of oil as a result of release of internal pressure in the well. As this pressure becomes depleted, it is necessary to pump further quantities of oil by mechanical means.
These measures recover only about 25% of the total oil stored in the reservoir. A great doal of oil is still trapped within the pores of the formation. Further enhancement of recovery can then C -2~
109 L~ 479 be effected by secondary recovery. In one method of recovery a waterflood is carried out by pumping water into a well or series of wells, displacing part of the trapped oil from the porous rock and collecting the displaced oil from surrounding wells.
However, waterflooding still leaves about 55-60% of the availab~
oil trapped in the formation. The explanation for this phenomenon is that the water has a very low viscoisty compared to the crude oil and tends to follow the path of least resistance, fingering through the oil and leaving large pockets untouched. In addition, surface forces in the formation tend to bind the oil and prevent its displacement.
A number of processes have been developed in recent years to recover further quantities of oil from these reservoirs by the use of mobility control solutions which enhance oil dis-placement by increasing the viscosity or permeability of thedisplacing fluid. Of interest are those enhanced recovery pro-cesses employing polymer flooding with a polysaccharide or poly-acrylamide to increase the viscosity of the displacing fluid.
Variations of this process include the use of surfactants and co-surfactants to release the oil from the reck formation. Poly-acrylamides have been found to suffer such deficiencies as ~iscosity loss in brines and severe shear sensitivity. Since, as was well documented in the prior art, xanthan gum is in-sensitive to salts (does not precipitate or lose viscosity under normal conditions), is shear stable, thermostable and viscosity stable over a wide pH range, xanthan gum is a good displacing agent. Moreover, the gum is poorly adsorbed on the elements of the porous rock formations and it gives viscosities useful in en-hanced oil recovery (5 to 90 Centipoise units at 1 32 sec. 1 30 shear rate) at low concentrations (100 to 3000 ppm).
. . ~ , .
..
'' .
~09~1i47!~
The use of solutions of xanthan gum or derivatives of xanthan g~m for oil recovery is described in United States Patents 3,243,000; 3,198,268; 3,532,166; 3,305,016; 3,251,417; 3,319,606;
3,319,715; 3,373,810, 3,434,542 and 3,729,460, It is suggested S in United States Patent 3,305,016 that aqueous solution contain-ing the heteropolysaccharide in sufficient ~uantity to increase the viscosity be employed as the thickening agent in preparing viscous waterflooding solutions. The polysaccharide may be pre-pared, separated, purified and then added. Alternatively, accord-ing to this reference, the entire culture, after adding a bacter-icide (e.g., formaldehyde) to kill the bacteria, may be added to the flood water.
United States 3,000,790 describes the culturing of a Xanthomonas bacterium in a well aerated medium containing commer-cial glucoqe, an organic source of nitrogen, dipotassium phosphate and appropriate trace elements. The source of organic nitrogen usually employed is distillers' solubles. The use of this organic nitrogen source contributes a substantial quantity of insolubles to the fermentation broth.
The processes described in United States Patents 3,000,790, 3,391,060 and the other fermentation processes previous-ly listed yield final fermentation broths that contain su~stantial amounts of insoluble matter, even when diluted with water, for injection into oil-bearing subterranean formations to impart the necessary and desired mobility control for oil displacement. The particulate matter and in certain c~ses the Xanthomonas cells in such whole broth would soon plug the oil-bearing formation at the site of injection and thus foul the well and prevent any further oil recovery. Furthermore, the same problem would be encountered with reconstituted xanthan gum precipitated and separated from ~, ~ 3 ~- 4 , , .
, :
:, ~ , ` 1094479 these fermentation broths. The plugging tendencies of these fermentation broths can be obviated by filtration through diatom-aceous earth leaf filters to remove the Xanthomonas cells and particulate and colloidal matter. However~ suah additional filtering steps are expensive and add significantly to the overall cost factors for enhanced oil recovery.
United States 3,853,771 approach~s the plugging pro~lem of whole fermentation broths by claiming a process for dissolving or dispersing cellular microorganisms which comprises contacting said materials with an aqueous solution containing at least one surfactant effective for dispersing outer wall layers of micro-organism cells, at least on~ chelating agent for dispersing the inner wall layers of microorganism cells, and at least one alkali metal hydroxide effective for enhanoing said dispersing actionsO
United States 4,010,071 describes a process for clarify-ing fermentation broths and other aqueous suspensions containing a dissolved xanthan gum and suspended solids resulting from the fermentation by treatment with a minor amount of a pro~ease enzyme. The injectivity of aqueous solutions containing xanthan gum so clarified is improved in oil well flooding operations over solutions not so treated, However, this treatment does not over-come plugging problems due to the presence of insoluble inorganic or non-proteinaceous organic materialæ present in the fermentation medium or producçd during the course of the fermentation.
The object of the process of United States Patent 3,391,060 is to recover a polysaccharide product of substantial purity without the use of extensive separation procedures. A
high quality, high viscosity, iight colored, high purity xanthan gum is recovered from a Xanthomonas fermentation broth. According to this patent, recovery i9 simplified and elaborate purification i `` ` ~5~
. . ~ I ~ : .- ' .
1' . ' . I ' ' ` `
,~ ` `~ ". ` ` ' / . I .; ; ' 109~479 procedures are obviated by the replacement of the organic source of nitrogen in the broth with an inorganic source of nitrogen (i~e., ammonium nitrate). However, the fermentation process de-scribed therein is not economical because of lengthy reaction times required and low yields of biopolymer obtained.
The method of improving the permeability of mobility control solutions by the addition of certain hydroxy substituted carboxylic acids such as malic, tartaric, citric, gluconic, lactic and salicylic is described in United States Patent 2,867,279.
This invention is concerned with an economical process for preparing a Xanthomonas colloid-containing fermentation broth suitable for preparation of mobility control solutions used in oil recovery which comprises aerobically ~ermenting a Xant~Dmonas organism in an aqueous nutrient medium whose ingredients comprise a carbohydrate, a nitrogen source, a Krebs cycle acid, chelated calcium, manganese ions and iron ions. The whole broth produced provides mobility control solutions of about 100 to 3000 ppm Xanthomonas colloid which are substantially free of insoluble ~; matter having a particle size greater than about 3 microns.
According to the present invention there is provided a process for preparing a Xanthomonas colloid-containing ferment-ation broth suitable for the preparation of mobility control solutions used in oil recovery characterized in that a Xanthomonas organism is fermented aerobically in an aqueous nutrient medium whose ingredients comprise a carbohydrate, a nitrogen source, about 0.1 to 10 grams per liter of an assimilable Krebs cycle acid, about 1 to 200 ppm chelated calcium, about 0.25 to 20 ppm iron and trace elements until at least about 100 ppm colloid is present in the broth, whereby the whole broth produced provides mobility control solutions of about 100 to 3000 ppm Xanthomonas C !, -6-.. ,-- . , ~ , . , , .... .. - - ~ :
109~79 colloid content which are substantially free of insoluble matter having a particle size greater than about 3 microns, The present invention now provides for the first time a practical process for prepari~g a Xanthomonas fermentation broth which without treatmant or clarification provides mo~ility control solutions for use in oil recovery ha~ing a use concentra-tion of about 100 to 3000 ppm Xanthomonas colloid which are sub-stantially free of insoluble matter having a particle size greater than about 3 microns. According to this invention, the whole fermentation broth may be used directly as a mobility control solution suoh as where the amount of colloid produaed during fermentation is within the desired range of use concentration.
Alternatively, the broth may be diluted with water or a water 6a-. . ' '' ' ", .
~0~4~79 solution such as ~rine to reduce the level of colloid to the desired range, Additives to modify the properties of the mobility control solutions may be employed in addition to the whole or un-clarified broths of the present invention.
S It has been found that oil in cores from oil fields generally will be effectively recovered by xanthan gum if the poly-saccharide solution at use concentration can be made to pass a Millipore filterability test as described later. Typical pore sizes o~ Millipore filters used for this test are 0.45 to 3.0 m~crons. "Millipore" is a trademark.
In addition to Millipore filterability, core tests are - performed as described by W.B. Gogarty in Mobility Control with Polymer Solutions, Paper ~SPE 1566B) presented at the Society of Engineers 41st Annual Fall Meeting held in Dallas, Texas, lS October 2-5, 1966.
A novel feature of the fermentation broths of the present invention, importantly distinguished from previously reported Xanthomonas fermentation broths and preparations, is the obviated need for expensive and time-consuming filtration or clarification.
Important factors that help make this possible are the following:
1. All nutrient ingredients are essentially water soluble or become essentially water soluble during the course of the fer-~ntation or prior to injection.
2. Absolute asepsis is maintained during the course of the 2S ~ermentation and a bactericide is preferably added at the end of the fermentation.
3. Hard water with high concentrations of calcium ions is ; preferably not used for the make-up of fermentation media. Low levels of calcium ions ~ess than about 100 mg./liter, preferably less than about 60 mg./liter) can be sequestered by the addition B
.i . 10~7g of a chelating agent such as ethylenediaminetetraacetic acid or preferably citric acid.
.i . 10~7g of a chelating agent such as ethylenediaminetetraacetic acid or preferably citric acid.
4. Amounts of manganese ions may be limited to avoid seed crystal formation and precipitation of insoluble calcium and phosphate salts (typically about 0.75 to 60 ppm, preferably 1.5 to 2.4 ppm).
5. Amounts of trace iron are controlled to avoid seed crystal formation and precipitation of insoluble calcium phosphate salts.
Important to the process of the present invention is the incorporation of the following ingredients to promote rapid cell growth and increase xanthan vield while achieving the de-sired mobility control solutions having substantially no insoluble matter with a particle size above about 3.0 microns.
lS 1. Chelated calcium - about 1 to 200 ppm, preferably about 40 to 60 ppm.
2. Trace iron - typically about 0.25 to 20 ppm, preferably 0.5 to 8 ppm.
3. Krebs cycle acid - about 0.1 to 10 grams/li~er, prefer-ably about 1 gram/liter.
Trace amounts of manganese and ferrous ions are added in the form of such salts as MnSO4-H2O, MnC12, FeSO4-7H2O and FeC12.
By Krebs cycle acid is meant an assimilable acid select-ed from the group consisting of citric acid, oxaloacetic acid, l-malic acid, fumaric acid, succinic acid and oxalosuccinic acid.
Cis-aconitic acid is a Krebs cycle acid that is not useful for the process~of this invention. The preferred acid is citric acid be-cause of its added efficiency as a sequestering agent for calcium ions. Citric acid can be incorporated in the fermentation medium at a concentration of about 0.5 to 2 grams/liter, preferably about ~. . . .
~ ......... ' ' ''~. . ` ' . `. `
10~479 l gram/liter.
In the practic~ of this invention, a suitable fermentation medium is inoculated with an organism of the genus Xanthomonas. The inoculum medium may be YM Broth tDifco) or a medium containing crude glucose tcerelose), sodium and potassium phosphates, magnesium sulfate and any of a variety of organic sources of nitrogen such as an en2ymatic di~est of soybean ~Soy Peptone Type T, Humko-Sheffield Chemical Co.) or an enzymatic digest of casein ~NZ-Amine YT, Humko-Sheffield Chemical Co.).
A~ter aerobic propagation for about 30 hours at 28C., an aliquot is transferred to a fermentor for~the second stage inoculum.
A suitable carbohydrate is present in the nutrient medium at a concentration from about 1 to about 5% by weight.
Suitable carbohydrates include, for example, glucose, sucro6e, maltose, fructose, lactose, processed inverted beet molasses, invert sugar, high quality filtered thinned starch~or mixtures of these carbohydrates. The preferred carbohydrates are glucose, maltose, fructose, filtered starchhydrolyzates ~r mixtures thereof.
Inorganic nitrogen is present in the nutrient medlum at a concentration of about 0.02 to about 0.35% by weight, prefer-ably 0.07 to 0.25% by weight. Inorganic nitrate is the preferred nitrogen source; ammonium nitrate at about l gram/liter, sodium nitrate at about 2 gramæ/liter or potassium nitrate at about 2.4 grams/liter may be used. The preferred source of nitrogen in this as well as the production medium is inorganic. However, organic nitrogen sources can also be used although they enhance large Xantho nas cell formation, provided the overall require-ment of substantial freedom from insoluble materials with a particle size above about 3 microns is maintained.
Magnesium in the form of MgSO4.7H2O or epsom salts, 0.1 g_ :`
10~!~479 to 1.0 grams/liter, is added along with trace manganese and iron ions. A chelating agent such as ethylenediaminetetraacetic acid or preferably citric acid which functions as a growth pro-moting Krebs cycle acid and sequestering agent for any calcium present is added.
Sufficient mono- and dipotassium phosphates are added '' to buffer the medium at about pH 5.9 to 8.5, préfera~ly 6.0 to 7.5, After aerobic propagation for about 20-40 hours at 24 to 34C,, preferably 28-30C " an aliquot is transferred to a fermentor containing the production medium.
The production medium i8 similar in composition to that of ~he second stage inoculum medium with the exception that sodium phosphates are preferably used'in place of potassium phosphates because of their lower costs and a small amount of calcium in the form of a salt such as calcium chloride or calcium nitrate or oxide such as lime is added to increase xanthan yield. The amount of calcium added is dependent on the amount of calcium present in the water used for medium make-up, the nitrogen source used and the species and strain of Xanthomonas organism employed. When sodium nitrate or potassium nitrate i8 used in place of ammonium nitrate, less calcium is required (approximately 27 ppm). Deionized water, distilled water or water containing less than about 20 ppm of calcium and other phosphate precipitable cations may also be used for'medium 25 make-up. Calcium ions may be added to a desired concentration. `~
The role of calcium ions in the enhancement of xanthan produc-tion is an important one but critical to the process of the present invention is the prevention of the precipitation of excess calcium cations and other eations as insoluble phosphate salts, This is accomplished, when desired, by the addition of : . ~ . . .. .
.
, . . .
; :
`` lOg4~
a chelating agent such as ethylenediaminetetraacetic acid or other suitable compound known to those skilled in the art a~
a concentration of about 1 to 20 millimolar, preferably 2 to 8 millimolar.
The pH of the fermentation medium is quite important to suitable growth of the Xanthomonas bacteria. The preferred range is about 6.0 to 7.5. Control of the pH within this range can be obtained by the use of a buffer compound such a~ disodium acid phosphate. Ethylenediaminetetraacetic acid or other suit-able chelating agent is also added in the buffer solution used for pH control to prevent the precipitation of calcium ions introduced in the water used for medium make-up as insoluble calci~m salts. The p~ is preferably controlled during the fermçntation cycle by the addition of sodium or potassium hydroxide solution which has the added advantages of decreasing broth viscosity without affec~ing xanthan yield and the elimin-ation of the need for chelation of the buffer solution.
In order to obtain a rapid fermentation, it is essential to have the correct amount of oxygen a~ailable for the growing bacterial culture. The fermentation medium is aerated to provide sufficient oxygen to produce a sulfite oxida-tion value within the range of about 1,5 to about 3.5 millimole~
of oxygen per liter per minute. A description of sulfite oxida-tion value is set forth in Industrial Engineering Chemistry 36, 504 tl936). The sulfite oxidation value is a measure of the rate of oxygen uptake in the fermentor under the agitation and aeration conditions employed.
The fermentation is allowed to proceed at a tempera-ture of about 30C. until the broth has a xanthan concentration of at least about 100 ppm, preferably at least about 1.0% and C : :
~ .
~ 0~4479 more preferably at least about 1.4% (30-96 hours). Viscosities of the broth are typically at least about 4,000 Centipoise units and preferably at about 7,000 Centipoise units.
It is desirable to kill the microbial cells by the addition of a bactericide such as formaldehyde, glutaraldehyde, phenol or substituted phenol such as a cresol or hydroxybenzene or a polyhalogenated phenol such as Corexit ~Exxon Corporation~, or any other preservative well known in the art. The preferred preservative is formaldehyde at a concentration of from about 200 to 10,000 ppm, preferably about lOOO to 3000 ppm, which can be added to the final fermentation broth before or during storage.
The process of this invention works well ~or many of the various species of Xanthomonas bacteria. Illustrative species include Xanthomonas ~haseoli, Xanthomonas malvacear~m, Xanthomonas carotae, Xanthomonas begQniae, Xanthomonas incanae and Xanthomonas vesicatoria. The preferred species is Xanthomonas campestris.
The Millipore filterability test i5 an experimental pro-cedure that measures flow rate through a Millipore filter (0O45 to 3.0 ~ pore size) as a function of volume under a constant ~ "' pressure of 40 psig. The filter ratio is the ratio of the time to collect the fourth 250 ml. of mobility control solution to the time to collect the first 250 ml. of mobility control solu-tion. A filter ratio of 1.0 indicates that the solution has no plugging tendencies. An acceptable mobility control solution has a filter ratio of 1 to 3 (0.45 to 3 ~ Millipore fiter), pre-ferably <1.7.
The desired filter ratio and Millipore filter size for testing of a particular mobility control solution are dependent ~! -12-;;
' .
10~3~479 on the permeability of the subterranean stratum of the oil field for which oil displacement is planned.
Mobility control solutions pr~pared from the whole fermentation broths of the present invention have filter ratios suitable for use in most oil fields. Where subterranean strata are highly impervious, mobility control solutions with low filter ratios must be employed. Under such circumstances, the whole or unclarified broths acco,rding to the present inven-tion preferably have substantially no insoluble matter with a particle size in excess of about 0.65 u. This can be accomplish-ed simply by storage of the final fermentation broth in the presence of about 200 at 10,000 ppm formaldehyde for a period of about 3 to 4 days. This aging process shrinks the Xanthomonas cells so that their minor dimension does not exceed 0,65 ~ in size. Xanthomonas cells are rod-shaped and normally the longer dimension of the cells is greater than 0.65 ~ whereas the shorter dimension of the cells is about 0.4 to 1.0 u. ~he storage temperature is n~tcritical and may range from 0 to 135C., pre-ferably 20 to 45C~ A practical expedient is storage at room temperature for a sufficient period of time so that microscopic examination reveals that the minor dimensions of the Xanthomonas cells are not greater than 0,65 ~ in size ~3-4 days).
The following data show the lnfluence of medium in-gredients on the filter ratios of mobility control solutions pre-pared from aged fermentation broths:
.
:
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n ,~ a~
~r cn er ~ ~ ~ -. ~ ~ ~ u~ o ul r ~ U~
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O ~ I~ t~ OD ~ ~ 00 1 0 ~1 ~ ~1 ~ ~ ~ ~1 ~ ~ ~i ~ O
, I
oc:ooooooooooooooooO~
'C~ ~ ~ 1 0 ~ t O
~n O
:~ ~, X
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~1 ,~ ~ ~ ~ o ~ c~ O ~ O 3 ~ o H H ~ '~ O O O O O O O O O O O O O O O O O O
~3 o~ .u~ a) ~ ,~
r ~ o o L~ O O Q o o u~ o o o o o ~ o o o ~ ~ O
O t~l ~1 ~ + Q
u~ E3 ~
_ :C --O ~~ S~O
U~ -- tJ) P~ U~
.~
, ~ _ ~ Z O
I N
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1 ~ ~L
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o o o o ,, .,, ~ ~ .,.
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CO ~ ~ C~ ~
~ . ~;
Id O ~1 0 0 X O
o ~O O
H
H ;~ O O ,~
;~ h o 1` ~
H H $
H ~ O ::~
'g! 1~ o ~ 1 a~ _ ~ ~i *
O H-- E~
y~
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.
:
1094~79 Alternatively to the aging process, an alkali metal hydroxide such as sodium or potassium hydroxide is added to the final fermenta~ion broth at a concentration of 0.1 to 2.0% w/v, pr~ferably ~.5% w/v, along with an alkali metal salt such as sodium or potassium chloride or sulfate at a concentration of O
to 5% w/v, preferably 1.0% w/v. The preferred salt is sodium chloride. The broth is heated under an oxygen free atmosphere ~e.g., nitrogen~ at a temperature of 55-121C., preferably 85-95C.
The heating time is not crucial and may be extended for several hours. A practical time is 1 to 30 minutes, preferably about 10 minutes. The broth is cooled to room temperature and adjusted to pH 3 to 12, preferably 7, with an acid such as hydrochloric acid.
This alkaline heat treatment hydrolyzes the bacterial cells with-out affecting the xanthan content. Deacetylation of the xanthan occurs during this process and the deacetylated product is quite suitable for use in oil recovery.
The suitably aged or alkaline heat-treated fermentation broth is generally diluted with water or brine to a xanthan con-centration of about 400 to 1000 ppm for use in enhanced oil re-covery. Optionally, a surfactant may be added to enhance the re-covery of oil. Representative surfactants include various petroleum sulfonates well known to those versed in the art of oil recovery.
It i6 understood that there may be conditions and factors that make impractical or expensive the transportation of large volumes of fermentation broth for injection into oil-con-taining reservoirs. For æuch purposes a special composition is provided. To the alkaline heat-treated broth previously described i8 added a water miscible solvent such as methanol, ethanol, acetone, t-butyl alcohol or isopropanol sufficient to precipitate .
.
-` 10~4~79 the xanthan gum which is separated by centrifugation or filtra-tion and dried. The preferred water miscible solvent is isopropanol at a concentration of 20-75% w/w, preferably about 38% w/w. Re-constitution with water or brine to a xanthan concentration of 100 to 3000 ppm provides a composition for enhanced oil recovery that is comparable in performance with that o diluted whole fermenta-tion broth. During the process of re-dissolution, it is important to provide sufficient shear to cause adequate dispersion of the polysaccharide and prevention of clump formation.
TEST PROCEDU~ES
Millipore Filterability Test Prepare 1000 ml. of 750 ppm xanthan solution in 500 ppm salt solution ~10:1 - NaCl:CaC12) as follows:
In a Waring type blender equipped with a rheostat, measure sufficient broth ~ased on xanthan content) to make 0.75 g.
xanthan solids. Dilute 1 to 6 with salt solution. Shear this mix-ture as follows:
40% power/2 minutes 60~ power/2 minutes 80% power/2 minutes Dilute in the blender to 750 ppm of xanthan and shear at 40% power for 2 minutes. ~Solution also used for viscosity determination.) Vse an experimental set-up that allows the flow rate through a Millipore filter disc ~47 mm, 0.45-3.0 y pore size) as a function of volume under a constant pressure of 40 psig. Use a reservoir that will accommodate >1000 ml.
Charge the reservoir with a liter of xanthan solution (750 ppml. Set pressure at 40 psig. Open valve and start record-ing volume filtrate and time ~seconds).
. .. , .. . .. , ~ . ...... . ...
, . ......... .. . ..
:~
. -- ' ;~, ,. ~, .. ..
-: - ~, ~ ' : :
10~4479 . .
Filter Ratio-time to collect the 4th 250 ml, of solution time to collect the 1st 250 ml, of solution Viscosity Determination Measure the viscosity with a Brookfield synchro-lectric viscometer, model LVT, using a UL adapter. Measure at 25C. at
Important to the process of the present invention is the incorporation of the following ingredients to promote rapid cell growth and increase xanthan vield while achieving the de-sired mobility control solutions having substantially no insoluble matter with a particle size above about 3.0 microns.
lS 1. Chelated calcium - about 1 to 200 ppm, preferably about 40 to 60 ppm.
2. Trace iron - typically about 0.25 to 20 ppm, preferably 0.5 to 8 ppm.
3. Krebs cycle acid - about 0.1 to 10 grams/li~er, prefer-ably about 1 gram/liter.
Trace amounts of manganese and ferrous ions are added in the form of such salts as MnSO4-H2O, MnC12, FeSO4-7H2O and FeC12.
By Krebs cycle acid is meant an assimilable acid select-ed from the group consisting of citric acid, oxaloacetic acid, l-malic acid, fumaric acid, succinic acid and oxalosuccinic acid.
Cis-aconitic acid is a Krebs cycle acid that is not useful for the process~of this invention. The preferred acid is citric acid be-cause of its added efficiency as a sequestering agent for calcium ions. Citric acid can be incorporated in the fermentation medium at a concentration of about 0.5 to 2 grams/liter, preferably about ~. . . .
~ ......... ' ' ''~. . ` ' . `. `
10~479 l gram/liter.
In the practic~ of this invention, a suitable fermentation medium is inoculated with an organism of the genus Xanthomonas. The inoculum medium may be YM Broth tDifco) or a medium containing crude glucose tcerelose), sodium and potassium phosphates, magnesium sulfate and any of a variety of organic sources of nitrogen such as an en2ymatic di~est of soybean ~Soy Peptone Type T, Humko-Sheffield Chemical Co.) or an enzymatic digest of casein ~NZ-Amine YT, Humko-Sheffield Chemical Co.).
A~ter aerobic propagation for about 30 hours at 28C., an aliquot is transferred to a fermentor for~the second stage inoculum.
A suitable carbohydrate is present in the nutrient medium at a concentration from about 1 to about 5% by weight.
Suitable carbohydrates include, for example, glucose, sucro6e, maltose, fructose, lactose, processed inverted beet molasses, invert sugar, high quality filtered thinned starch~or mixtures of these carbohydrates. The preferred carbohydrates are glucose, maltose, fructose, filtered starchhydrolyzates ~r mixtures thereof.
Inorganic nitrogen is present in the nutrient medlum at a concentration of about 0.02 to about 0.35% by weight, prefer-ably 0.07 to 0.25% by weight. Inorganic nitrate is the preferred nitrogen source; ammonium nitrate at about l gram/liter, sodium nitrate at about 2 gramæ/liter or potassium nitrate at about 2.4 grams/liter may be used. The preferred source of nitrogen in this as well as the production medium is inorganic. However, organic nitrogen sources can also be used although they enhance large Xantho nas cell formation, provided the overall require-ment of substantial freedom from insoluble materials with a particle size above about 3 microns is maintained.
Magnesium in the form of MgSO4.7H2O or epsom salts, 0.1 g_ :`
10~!~479 to 1.0 grams/liter, is added along with trace manganese and iron ions. A chelating agent such as ethylenediaminetetraacetic acid or preferably citric acid which functions as a growth pro-moting Krebs cycle acid and sequestering agent for any calcium present is added.
Sufficient mono- and dipotassium phosphates are added '' to buffer the medium at about pH 5.9 to 8.5, préfera~ly 6.0 to 7.5, After aerobic propagation for about 20-40 hours at 24 to 34C,, preferably 28-30C " an aliquot is transferred to a fermentor containing the production medium.
The production medium i8 similar in composition to that of ~he second stage inoculum medium with the exception that sodium phosphates are preferably used'in place of potassium phosphates because of their lower costs and a small amount of calcium in the form of a salt such as calcium chloride or calcium nitrate or oxide such as lime is added to increase xanthan yield. The amount of calcium added is dependent on the amount of calcium present in the water used for medium make-up, the nitrogen source used and the species and strain of Xanthomonas organism employed. When sodium nitrate or potassium nitrate i8 used in place of ammonium nitrate, less calcium is required (approximately 27 ppm). Deionized water, distilled water or water containing less than about 20 ppm of calcium and other phosphate precipitable cations may also be used for'medium 25 make-up. Calcium ions may be added to a desired concentration. `~
The role of calcium ions in the enhancement of xanthan produc-tion is an important one but critical to the process of the present invention is the prevention of the precipitation of excess calcium cations and other eations as insoluble phosphate salts, This is accomplished, when desired, by the addition of : . ~ . . .. .
.
, . . .
; :
`` lOg4~
a chelating agent such as ethylenediaminetetraacetic acid or other suitable compound known to those skilled in the art a~
a concentration of about 1 to 20 millimolar, preferably 2 to 8 millimolar.
The pH of the fermentation medium is quite important to suitable growth of the Xanthomonas bacteria. The preferred range is about 6.0 to 7.5. Control of the pH within this range can be obtained by the use of a buffer compound such a~ disodium acid phosphate. Ethylenediaminetetraacetic acid or other suit-able chelating agent is also added in the buffer solution used for pH control to prevent the precipitation of calcium ions introduced in the water used for medium make-up as insoluble calci~m salts. The p~ is preferably controlled during the fermçntation cycle by the addition of sodium or potassium hydroxide solution which has the added advantages of decreasing broth viscosity without affec~ing xanthan yield and the elimin-ation of the need for chelation of the buffer solution.
In order to obtain a rapid fermentation, it is essential to have the correct amount of oxygen a~ailable for the growing bacterial culture. The fermentation medium is aerated to provide sufficient oxygen to produce a sulfite oxida-tion value within the range of about 1,5 to about 3.5 millimole~
of oxygen per liter per minute. A description of sulfite oxida-tion value is set forth in Industrial Engineering Chemistry 36, 504 tl936). The sulfite oxidation value is a measure of the rate of oxygen uptake in the fermentor under the agitation and aeration conditions employed.
The fermentation is allowed to proceed at a tempera-ture of about 30C. until the broth has a xanthan concentration of at least about 100 ppm, preferably at least about 1.0% and C : :
~ .
~ 0~4479 more preferably at least about 1.4% (30-96 hours). Viscosities of the broth are typically at least about 4,000 Centipoise units and preferably at about 7,000 Centipoise units.
It is desirable to kill the microbial cells by the addition of a bactericide such as formaldehyde, glutaraldehyde, phenol or substituted phenol such as a cresol or hydroxybenzene or a polyhalogenated phenol such as Corexit ~Exxon Corporation~, or any other preservative well known in the art. The preferred preservative is formaldehyde at a concentration of from about 200 to 10,000 ppm, preferably about lOOO to 3000 ppm, which can be added to the final fermentation broth before or during storage.
The process of this invention works well ~or many of the various species of Xanthomonas bacteria. Illustrative species include Xanthomonas ~haseoli, Xanthomonas malvacear~m, Xanthomonas carotae, Xanthomonas begQniae, Xanthomonas incanae and Xanthomonas vesicatoria. The preferred species is Xanthomonas campestris.
The Millipore filterability test i5 an experimental pro-cedure that measures flow rate through a Millipore filter (0O45 to 3.0 ~ pore size) as a function of volume under a constant ~ "' pressure of 40 psig. The filter ratio is the ratio of the time to collect the fourth 250 ml. of mobility control solution to the time to collect the first 250 ml. of mobility control solu-tion. A filter ratio of 1.0 indicates that the solution has no plugging tendencies. An acceptable mobility control solution has a filter ratio of 1 to 3 (0.45 to 3 ~ Millipore fiter), pre-ferably <1.7.
The desired filter ratio and Millipore filter size for testing of a particular mobility control solution are dependent ~! -12-;;
' .
10~3~479 on the permeability of the subterranean stratum of the oil field for which oil displacement is planned.
Mobility control solutions pr~pared from the whole fermentation broths of the present invention have filter ratios suitable for use in most oil fields. Where subterranean strata are highly impervious, mobility control solutions with low filter ratios must be employed. Under such circumstances, the whole or unclarified broths acco,rding to the present inven-tion preferably have substantially no insoluble matter with a particle size in excess of about 0.65 u. This can be accomplish-ed simply by storage of the final fermentation broth in the presence of about 200 at 10,000 ppm formaldehyde for a period of about 3 to 4 days. This aging process shrinks the Xanthomonas cells so that their minor dimension does not exceed 0,65 ~ in size. Xanthomonas cells are rod-shaped and normally the longer dimension of the cells is greater than 0.65 ~ whereas the shorter dimension of the cells is about 0.4 to 1.0 u. ~he storage temperature is n~tcritical and may range from 0 to 135C., pre-ferably 20 to 45C~ A practical expedient is storage at room temperature for a sufficient period of time so that microscopic examination reveals that the minor dimensions of the Xanthomonas cells are not greater than 0,65 ~ in size ~3-4 days).
The following data show the lnfluence of medium in-gredients on the filter ratios of mobility control solutions pre-pared from aged fermentation broths:
.
:
~0~ ~79 : ~
n ,~ a~
~r cn er ~ ~ ~ -. ~ ~ ~ u~ o ul r ~ U~
:L ~ A ~ 1 ~ ~ o o:~. 0 : O. ~0 r~
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O ~ I~ t~ OD ~ ~ 00 1 0 ~1 ~ ~1 ~ ~ ~ ~1 ~ ~ ~i ~ O
, I
oc:ooooooooooooooooO~
'C~ ~ ~ 1 0 ~ t O
~n O
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~1 ,~ ~ ~ ~ o ~ c~ O ~ O 3 ~ o H H ~ '~ O O O O O O O O O O O O O O O O O O
~3 o~ .u~ a) ~ ,~
r ~ o o L~ O O Q o o u~ o o o o o ~ o o o ~ ~ O
O t~l ~1 ~ + Q
u~ E3 ~
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I N
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H ;~ O O ,~
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.
:
1094~79 Alternatively to the aging process, an alkali metal hydroxide such as sodium or potassium hydroxide is added to the final fermenta~ion broth at a concentration of 0.1 to 2.0% w/v, pr~ferably ~.5% w/v, along with an alkali metal salt such as sodium or potassium chloride or sulfate at a concentration of O
to 5% w/v, preferably 1.0% w/v. The preferred salt is sodium chloride. The broth is heated under an oxygen free atmosphere ~e.g., nitrogen~ at a temperature of 55-121C., preferably 85-95C.
The heating time is not crucial and may be extended for several hours. A practical time is 1 to 30 minutes, preferably about 10 minutes. The broth is cooled to room temperature and adjusted to pH 3 to 12, preferably 7, with an acid such as hydrochloric acid.
This alkaline heat treatment hydrolyzes the bacterial cells with-out affecting the xanthan content. Deacetylation of the xanthan occurs during this process and the deacetylated product is quite suitable for use in oil recovery.
The suitably aged or alkaline heat-treated fermentation broth is generally diluted with water or brine to a xanthan con-centration of about 400 to 1000 ppm for use in enhanced oil re-covery. Optionally, a surfactant may be added to enhance the re-covery of oil. Representative surfactants include various petroleum sulfonates well known to those versed in the art of oil recovery.
It i6 understood that there may be conditions and factors that make impractical or expensive the transportation of large volumes of fermentation broth for injection into oil-con-taining reservoirs. For æuch purposes a special composition is provided. To the alkaline heat-treated broth previously described i8 added a water miscible solvent such as methanol, ethanol, acetone, t-butyl alcohol or isopropanol sufficient to precipitate .
.
-` 10~4~79 the xanthan gum which is separated by centrifugation or filtra-tion and dried. The preferred water miscible solvent is isopropanol at a concentration of 20-75% w/w, preferably about 38% w/w. Re-constitution with water or brine to a xanthan concentration of 100 to 3000 ppm provides a composition for enhanced oil recovery that is comparable in performance with that o diluted whole fermenta-tion broth. During the process of re-dissolution, it is important to provide sufficient shear to cause adequate dispersion of the polysaccharide and prevention of clump formation.
TEST PROCEDU~ES
Millipore Filterability Test Prepare 1000 ml. of 750 ppm xanthan solution in 500 ppm salt solution ~10:1 - NaCl:CaC12) as follows:
In a Waring type blender equipped with a rheostat, measure sufficient broth ~ased on xanthan content) to make 0.75 g.
xanthan solids. Dilute 1 to 6 with salt solution. Shear this mix-ture as follows:
40% power/2 minutes 60~ power/2 minutes 80% power/2 minutes Dilute in the blender to 750 ppm of xanthan and shear at 40% power for 2 minutes. ~Solution also used for viscosity determination.) Vse an experimental set-up that allows the flow rate through a Millipore filter disc ~47 mm, 0.45-3.0 y pore size) as a function of volume under a constant pressure of 40 psig. Use a reservoir that will accommodate >1000 ml.
Charge the reservoir with a liter of xanthan solution (750 ppml. Set pressure at 40 psig. Open valve and start record-ing volume filtrate and time ~seconds).
. .. , .. . .. , ~ . ...... . ...
, . ......... .. . ..
:~
. -- ' ;~, ,. ~, .. ..
-: - ~, ~ ' : :
10~4479 . .
Filter Ratio-time to collect the 4th 250 ml, of solution time to collect the 1st 250 ml, of solution Viscosity Determination Measure the viscosity with a Brookfield synchro-lectric viscometer, model LVT, using a UL adapter. Measure at 25C. at
6 and 12 RPM. Viscosity is expressed in Centipoise units.
Xanthan Determination Highly purified xanthan contains about 18.4% glucuronic acid. Glucuronic acid in xanthan compositions i8 determined in the absence of formaldehyde and without borate at 100C. by the method of Knutson and Jeanes, Anal. Biochem., 24, 470 (1968);
ibid., 482.
% Glucuronic Acid x 100 % Xanthan = - -18.4 EXAMPLE I
Cells of Xanthomonas campestris from a YM agar slant are transferred to 300 ml. of YM broth contained in a 2.8 liter Fernbach flask and shaken on a rotary shader for about 31 hours at 28C. A 25 ml. aliquot is transferred to a 2.8 liter Fernbach flask containing 500 ml. of a medium of the following composition:
20 Ingredient Grams/liter Glucose-fructose (Isosweet 100, Corn Products)autoclave 10,1 Crude glucose (cerelose) _ separately 25.7 NH4N3 1,0 MgS04-7H20 0,10 MnS04 H20 FeS4'7H2 0,01 Anhydrous citric acid 1.0 K2HP04 4.1 RH2P04 0.69 .t'''.~' ''' ' ~ . '' ' : ' ' '~ , ' : , ;
. ' ' ' ' . ~ , ' . ' ' , ` ' ' . ~' ' ' ' .
, , ' ' ' ' .
10~4~9 The cerelose and Isosweet 100 are dissolved in distilled water and autoclaved. The rest of the ingredients are combined, adjusted to pH 6.4 an~ autoclaved. The separate-ly autoclaved materials are then combined.
After shaking at 28C, for about 33 hours a 200 ml.
portion is transferred to a 4-liter, mechanically agitated fermentor containing 2 liters of medium:
Ingredient Grams/litler Cerelose~ 25.7 autoclave separately 10 Iæosweet 100 ~ 10.1 NH4NO3 1.0 MgS04 ~7H20 0 .10 MnSO4 H2O a .03 FeSO '7H O 0.~1 15 Anhydrous citric acid 1.0 CaC12 2 2 0.20 Na2HPO4 3-34 NaH2PO4 0~70 The sugars dissolved in 300 ml. of water are auto-claved separately. The rest of the ingredients dissolved in 1700 ml. of water are autoclaved, and the two solutions then combined. Aeration is at a rate to provi~e 1.5 to 3.5 milli~
moles of oxygen par liter per minute. The fermentation is conduct-ed at 30C. for 48 hours during which time the pH of the medium is maintained betwee~ 5.9 and 7.5 by the addition of sodium phosphate buffer made up with tap water. Ethylenediaminetetra-acetic acid is also added to ~he sodium phosphate buffer to prevent the precipitation of calcium phosphate salts. At the end of the fermentation, the viscosity of the broth is >7800 Centipoise units (at 6.27 sec. 1 shear rate) and the xanthan : , 10~479 .
yield is >l.5%.
A mobility control solution has a filter ratio of ~1.7 (3.0 ~ Millipore filter). , A mobility control solution prepared from whole fermen-tation broth aged for 4 days has a filter ratio of ~1.7 ~0.65 Millipore filter).
EXAMPLE II
The method of Example I is repeated employing the following fermentation media:
Inoculum Medium (lst Stage~
Ingredient Grams/liter Cerelose lO.0 (NH4)2HPo4 2.0 KH2P4 l.0 MgSO 7H2O 0 5 NZ-Amine Y~ pH - 7.0 ll.0 Inoculum Medium (2nd Sta~e) Ingredient Grams/liter D-Glucose ~ autoclave 27,0 ~r separately 20 D-Fructose 3.0 NH4NO3 1.0 MgSO 7H2O O.lO
MnSO4 2 FeSO 7H O O.Ol 25 Anhydrous citric acid 1.O
K2HPO4 4.l XH2PO4 pH - 6.4 0.69 ,1 ~i -20-~ ' ' , J10~44~9 Production Medium -Ingredient Grams/liter D-Glucose ~ 27.0 ~ autoclave separately 5D-FructoseJ 3.0 Anhydrous citric acid 1.0 NH4NO3 1.0 MgSO4~7H2O 0.10 MnS4~H2 0.03 10 FeS04 ~ 7H20 0 . 01 CaC12~2H2O 0.20 Na2~PO4 3.34 NaH2PO4 0.70 pH - 6.4 The fermentation is conducted as in Example I, with com-parable results, with the exception that pH adjustment is made with sodium hydroxide solution without the concommitant addition of ethylenediaminetetraacetic acid.
EXAMPLE III
A large scale fermentation is conducted in the following manner:
Inoculum M~dium ~lst Stage) Ingredient Grams~liter Cerelose 10.0 25 ~NH4)2HPO4 2.0 KEI2P4 1. 0 MgS~4 ~H20 NZ-Amine YT 11~0 ~ pH - 7O0 1 30 The medium is dispensed in 500 mlO portions into two 2.8liter Fernbach flasks. After autoclaving and cooling, the flasks are inoculated with cells of Xanthomonas campestris. After shaking .~ .
" ~ :
: .' . ~, ~ ' ,' ; .
;' ? ~ ' ~05`~79 for 30 hours at 28C., the two flasks are combined and used to inoculate a 200 gallon fermentor containing the following ingredients in 100 ga~lons of medium:
Inoculum Medium (2nd Stage~
Ingredient A
Cerelose 10~0 ~I4)2HPo4 2.0 KH2P4 1 o O
Epsom salts 0.5 NZ-Amine YT 11.0 pH - 7.0 ~ he fermentation medium is stirred with a mechanical agitator and aerated to provide l.S to 3O5 millimoles of oxygen per liter minute. Sodium hydroxide solution is added at intervals to maintain the pH at 6O0 to 7.5~ Soybean oil is added to control excessive foam. After about 48 hours fermentation, a volume sufficient to provide a 5~ v/v inoculum is transferred to a 2000 gallon fermentor containing 800 gallons of medium of the following composition: `
~
~ Amount . ~
NH4NO3 (50~ solution) 1c33 gallons R2HPO4 27O5 lbs.
KH2PO4 4~75 lbs, Epsom salts 306 grams MnSO4 H2O 94 grams FeSO4~7H2O 30~5 grams Cerelose ~ 175 lbso ~ autoclave separately Isosweet 100~ 70 lbs.
Anhydrous citric acid 6O75 lbs~
pH - 7.0 . !, ' ' 1094~79 After fermentation under the previously described condi-tions for about 31 hours, a sufficient volume to provide a 10% v/v inoculum is transferred to a 2000 gallon fermentor containing 1200 gallons of the following medium:
Production Medium .
I dient Amount nqre - -cerelose-______ 297 lbs, ~ autoclave separately Isosweet lOL~ - 117 lbs.
NH4NO3 ~50% solution~ 2 gallons Hydrated lime 0.73 lbs.
Anhydrous citric acid 10.0 lbs~
Na2HPo4 33~5 lbs~
NaH2P04 7~0 lbs~
Epsom salts ~MgS04~7H20) 454 grams MnSO4 H20 141 grams FeSO4 7H2O 45~ grams pH - 7.0 .~ .
. . .
~ .
.:
: ~,
Xanthan Determination Highly purified xanthan contains about 18.4% glucuronic acid. Glucuronic acid in xanthan compositions i8 determined in the absence of formaldehyde and without borate at 100C. by the method of Knutson and Jeanes, Anal. Biochem., 24, 470 (1968);
ibid., 482.
% Glucuronic Acid x 100 % Xanthan = - -18.4 EXAMPLE I
Cells of Xanthomonas campestris from a YM agar slant are transferred to 300 ml. of YM broth contained in a 2.8 liter Fernbach flask and shaken on a rotary shader for about 31 hours at 28C. A 25 ml. aliquot is transferred to a 2.8 liter Fernbach flask containing 500 ml. of a medium of the following composition:
20 Ingredient Grams/liter Glucose-fructose (Isosweet 100, Corn Products)autoclave 10,1 Crude glucose (cerelose) _ separately 25.7 NH4N3 1,0 MgS04-7H20 0,10 MnS04 H20 FeS4'7H2 0,01 Anhydrous citric acid 1.0 K2HP04 4.1 RH2P04 0.69 .t'''.~' ''' ' ~ . '' ' : ' ' '~ , ' : , ;
. ' ' ' ' . ~ , ' . ' ' , ` ' ' . ~' ' ' ' .
, , ' ' ' ' .
10~4~9 The cerelose and Isosweet 100 are dissolved in distilled water and autoclaved. The rest of the ingredients are combined, adjusted to pH 6.4 an~ autoclaved. The separate-ly autoclaved materials are then combined.
After shaking at 28C, for about 33 hours a 200 ml.
portion is transferred to a 4-liter, mechanically agitated fermentor containing 2 liters of medium:
Ingredient Grams/litler Cerelose~ 25.7 autoclave separately 10 Iæosweet 100 ~ 10.1 NH4NO3 1.0 MgS04 ~7H20 0 .10 MnSO4 H2O a .03 FeSO '7H O 0.~1 15 Anhydrous citric acid 1.0 CaC12 2 2 0.20 Na2HPO4 3-34 NaH2PO4 0~70 The sugars dissolved in 300 ml. of water are auto-claved separately. The rest of the ingredients dissolved in 1700 ml. of water are autoclaved, and the two solutions then combined. Aeration is at a rate to provi~e 1.5 to 3.5 milli~
moles of oxygen par liter per minute. The fermentation is conduct-ed at 30C. for 48 hours during which time the pH of the medium is maintained betwee~ 5.9 and 7.5 by the addition of sodium phosphate buffer made up with tap water. Ethylenediaminetetra-acetic acid is also added to ~he sodium phosphate buffer to prevent the precipitation of calcium phosphate salts. At the end of the fermentation, the viscosity of the broth is >7800 Centipoise units (at 6.27 sec. 1 shear rate) and the xanthan : , 10~479 .
yield is >l.5%.
A mobility control solution has a filter ratio of ~1.7 (3.0 ~ Millipore filter). , A mobility control solution prepared from whole fermen-tation broth aged for 4 days has a filter ratio of ~1.7 ~0.65 Millipore filter).
EXAMPLE II
The method of Example I is repeated employing the following fermentation media:
Inoculum Medium (lst Stage~
Ingredient Grams/liter Cerelose lO.0 (NH4)2HPo4 2.0 KH2P4 l.0 MgSO 7H2O 0 5 NZ-Amine Y~ pH - 7.0 ll.0 Inoculum Medium (2nd Sta~e) Ingredient Grams/liter D-Glucose ~ autoclave 27,0 ~r separately 20 D-Fructose 3.0 NH4NO3 1.0 MgSO 7H2O O.lO
MnSO4 2 FeSO 7H O O.Ol 25 Anhydrous citric acid 1.O
K2HPO4 4.l XH2PO4 pH - 6.4 0.69 ,1 ~i -20-~ ' ' , J10~44~9 Production Medium -Ingredient Grams/liter D-Glucose ~ 27.0 ~ autoclave separately 5D-FructoseJ 3.0 Anhydrous citric acid 1.0 NH4NO3 1.0 MgSO4~7H2O 0.10 MnS4~H2 0.03 10 FeS04 ~ 7H20 0 . 01 CaC12~2H2O 0.20 Na2~PO4 3.34 NaH2PO4 0.70 pH - 6.4 The fermentation is conducted as in Example I, with com-parable results, with the exception that pH adjustment is made with sodium hydroxide solution without the concommitant addition of ethylenediaminetetraacetic acid.
EXAMPLE III
A large scale fermentation is conducted in the following manner:
Inoculum M~dium ~lst Stage) Ingredient Grams~liter Cerelose 10.0 25 ~NH4)2HPO4 2.0 KEI2P4 1. 0 MgS~4 ~H20 NZ-Amine YT 11~0 ~ pH - 7O0 1 30 The medium is dispensed in 500 mlO portions into two 2.8liter Fernbach flasks. After autoclaving and cooling, the flasks are inoculated with cells of Xanthomonas campestris. After shaking .~ .
" ~ :
: .' . ~, ~ ' ,' ; .
;' ? ~ ' ~05`~79 for 30 hours at 28C., the two flasks are combined and used to inoculate a 200 gallon fermentor containing the following ingredients in 100 ga~lons of medium:
Inoculum Medium (2nd Stage~
Ingredient A
Cerelose 10~0 ~I4)2HPo4 2.0 KH2P4 1 o O
Epsom salts 0.5 NZ-Amine YT 11.0 pH - 7.0 ~ he fermentation medium is stirred with a mechanical agitator and aerated to provide l.S to 3O5 millimoles of oxygen per liter minute. Sodium hydroxide solution is added at intervals to maintain the pH at 6O0 to 7.5~ Soybean oil is added to control excessive foam. After about 48 hours fermentation, a volume sufficient to provide a 5~ v/v inoculum is transferred to a 2000 gallon fermentor containing 800 gallons of medium of the following composition: `
~
~ Amount . ~
NH4NO3 (50~ solution) 1c33 gallons R2HPO4 27O5 lbs.
KH2PO4 4~75 lbs, Epsom salts 306 grams MnSO4 H2O 94 grams FeSO4~7H2O 30~5 grams Cerelose ~ 175 lbso ~ autoclave separately Isosweet 100~ 70 lbs.
Anhydrous citric acid 6O75 lbs~
pH - 7.0 . !, ' ' 1094~79 After fermentation under the previously described condi-tions for about 31 hours, a sufficient volume to provide a 10% v/v inoculum is transferred to a 2000 gallon fermentor containing 1200 gallons of the following medium:
Production Medium .
I dient Amount nqre - -cerelose-______ 297 lbs, ~ autoclave separately Isosweet lOL~ - 117 lbs.
NH4NO3 ~50% solution~ 2 gallons Hydrated lime 0.73 lbs.
Anhydrous citric acid 10.0 lbs~
Na2HPo4 33~5 lbs~
NaH2P04 7~0 lbs~
Epsom salts ~MgS04~7H20) 454 grams MnSO4 H20 141 grams FeSO4 7H2O 45~ grams pH - 7.0 .~ .
. . .
~ .
.:
: ~,
Claims (16)
1. A process for preparing a Xanthomonas colloid-containing fermentation broth suitable for the preparation of mobility control solutions used in oil recovery characterized in that a Xanthomonas organism is fermented aerobically in an aqueous nutrient medium whose ingredients comprise a carbohydrate, a nitrogen source, about 0.1 to 10 grams per liter of an assimilable Krebs cycle acid, about 1 to 200 ppm chelated calcium, about 0.25 to 20 ppm iron and trace elements until at least about 100 ppm colloid is present in the broth, whereby the whole broth produced provides mobility control solutions of about 100 to 3000 ppm Xanthomonas colloid content which are substantially free of insoluble matter having a particle size greater than about 3 microns.
2. The process of claim 1, characterized in that a chelating agent is added during the fermentation in an amount of from about 2 to 20 millimolar and said chelating agent is ethylenediaminetetraacetic acid.
3. The process of either of claims 1 and 2, characterized in that said Krebs cycle acid is citric acid and the concentration of said citric acid in the nutrient medium is about 0.5 to 2 grams per liter.
4. The process of either of claims 1 and 2, characterized in that a preservative is added to the broth after fermentation in an amount of from about 200 to 10,000 ppm and said preservative is formaldehyde.
5. A process according to either of claims 1 and 2, wherein said Krebs cycle acid is citric acid which is present in a concentration in said nutrient medium of about 0.5 to 2 grams per liter and wherein a preservat-ive is added to the broth after fermentation in an amount of from about 200 to 10,000 ppm, said preservative being formaldehyde.
6. The process of either of claims 1 and 2, characterized in that said source of nitrogen is selected from the group consisting of ammonium nitrate, sodium nitrate and potassium nitrate.
7. The process of either of claims 1 and 2, characterized in that said aqueous nutrient medium is prepared employing water containing less than 20 ppm of calcium and other phosphate precipitable cations.
8. A process according to either of claims 1 and 2, wherein said Krebs cycle acid is citric acid which is present in a concentration in said nutrient medium of about 0.5 to 2 grams per liter and wherein a preservative is added to the broth after fermentation in an amount of from about 200 to 10,000 ppm, said pre-servative being formaldehyde and further the nutrient medium is prepared containing less than 70 ppm of calcium and other phosphate precipitable cations.
9. A hydrophilic colloid-containing fermentation broth whenever obtained by the process of either of claims 1 and 2.
10. A process for preparing a Xanthomonas colloid-containing fermentation broth suitable for the preparation of mobility control solutions used in oil recovery characterized in that it comprises a) aerobically fermenting a Xanthomonas organism in an aqueous nutrient medium whose ingredients comprise a carbohydrate, a nitrogen source, about 0.1 to 10 grams per liter of an assimilable Krebs cycle acid, about 1 to 200 ppm chelated calcium, about 0.25 to 20 ppm iron and trace elements until at least 100 ppm colloid is present in the broth, and b) storing the broth for 3 to 4 days whereby a hydrophilic colloid-containing fermentation broth substantially free of insoluble matter whose particle size is larger than 0.65µ is obtained,
11. A hydrophilic colloid-containing fermentation broth obtained by the process of claim 10.
12. A process for the recovery of crude oil from an oil-bearing subterranean formation wherein a hydro-philic colloid-containing mobility control solution is injected into said formation, characterized in that there is injected into said formation a mobility control solution containing a fermentation broth obtained by the process of either of claims 1 and 10.
13. A process for preparing a hydrophilic colloid-containing fermentation broth suitable for use in the recovery of oil from an oil-bearing subterranean formation by injecting a mobility control solution containing said broth into said formation characterized in that it comprises a) fermenting by aerobic propagation a Xanthomonas organism in an aqueous nutrient medium whose ingredients comprise a carbohydrate, a nitrogen source, about 0.1 to 10 grams per liter of a Krebs cycle acid, about 1 to 200 ppm chelated calcium, about 0,25 to 20 ppm iron and trace elements until at least 100 ppm colloid is present in the broth, and b) contacting the broth with from 0.1 to 2.04 w/v concentration of an alkali metal hydroxide and an alk-ali metal salt at a concentration of from 0 to 5% w/v, heating for 1 to 30 minutes at about 55 to 121°C under a substantially oxygen free atmosphere and optionally neutralizing.
14. A hydrophilic colloid-containing fermentation broth obtained by the process of claim 13.
15, A process for preparing a hydrophilic colloid suitable for use in the recovery of oil from an oil-bearing subterranean formation by injecting a mobility control solution containing said hydrophilic colloid into said formation characterized in that it comprises a) fermenting by aerobic propagation a Xanthomonas organism in an aqueous nutrient medium whose ingredients comprise a carbohydrate, a nitrogen source, about 0.1 to 10 grams per liter of a Krebs cycle acid, about 1 to 200 ppm chelated calcium, about 0.25 to 20 ppm iron and trace elements until at least 100 ppm colloid is present in the broth, and b) contacting the broth with from 0.1 to 2.0%
w/v concentration of an alkali metal hydroxide and an alkali metal salt at a concentration of from 0 to 5% w/v, heating for 1 to 30 minutes at about 55 to 121°C under a substantially oxygen free atmosphere and optionally neutralizing, and c) adding sufficient water miscible solvent to cause precipitation of said hydrophilic colloid and separating said precipitated hydrophilic colloid therefrom.
w/v concentration of an alkali metal hydroxide and an alkali metal salt at a concentration of from 0 to 5% w/v, heating for 1 to 30 minutes at about 55 to 121°C under a substantially oxygen free atmosphere and optionally neutralizing, and c) adding sufficient water miscible solvent to cause precipitation of said hydrophilic colloid and separating said precipitated hydrophilic colloid therefrom.
16. A hydrophilic colloid composition obtained by the process of claim 15.
Applications Claiming Priority (4)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US71184376A | 1976-08-05 | 1976-08-05 | |
| US711,843 | 1976-08-05 | ||
| US05/793,274 US4119546A (en) | 1976-08-05 | 1977-05-03 | Process for producing Xanthomonas hydrophilic colloid, product resulting therefrom, and use thereof in displacement of oil from partially depleted reservoirs |
| US793,274 | 1977-05-03 |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CA1094479A true CA1094479A (en) | 1981-01-27 |
Family
ID=27108715
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA284,129A Expired CA1094479A (en) | 1976-08-05 | 1977-08-04 | Process for producing xanthomonas hydrophilic colloid for use in displacement of oil from partially depleted reservoirs |
Country Status (13)
| Country | Link |
|---|---|
| BR (1) | BR7705160A (en) |
| CA (1) | CA1094479A (en) |
| DE (1) | DE2734364C2 (en) |
| EG (1) | EG12843A (en) |
| ES (1) | ES461344A1 (en) |
| FR (1) | FR2360665A1 (en) |
| GB (1) | GB1531970A (en) |
| IE (1) | IE45543B1 (en) |
| IL (1) | IL52609A (en) |
| IT (1) | IT1080085B (en) |
| NL (1) | NL168554B (en) |
| NO (1) | NO150965C (en) |
| SU (1) | SU959634A3 (en) |
Families Citing this family (7)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| AU525306B2 (en) * | 1978-04-13 | 1982-10-28 | Merck & Co., Inc. | Low calcium xanthan gum |
| US4265673A (en) | 1978-06-23 | 1981-05-05 | Talres Development (N.A.) N.V. | Polymer solutions for use in oil recovery containing a complexing agent for multivalentions |
| NL7907884A (en) * | 1978-11-06 | 1980-05-08 | Pfizer | METHOD FOR PREPARING A MOTION CONTROLLING SOLUTION FOR USE IN OIL EXTRACTION |
| FR2442955A1 (en) | 1978-12-01 | 1980-06-27 | Ceca Sa | IMPROVEMENTS TO ASSISTED OIL RECOVERY |
| US4263399A (en) * | 1979-05-31 | 1981-04-21 | Merck & Co., Inc. | High phosphate process for making low calcium, smooth flow xanthan gum |
| CA1153971A (en) * | 1980-07-14 | 1983-09-20 | Standard Oil Company | Semi-continuous method for production of xanthan gum using xanthomonas campestris atcc 31601 |
| DE19512731C1 (en) * | 1995-04-05 | 1996-07-11 | Preussag En Gmbh | Flooding agent used to recover oil and natural gas from underground deposits |
Family Cites Families (1)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| DD121954A1 (en) * | 1975-09-05 | 1976-09-05 |
-
1977
- 1977-07-26 NO NO772654A patent/NO150965C/en unknown
- 1977-07-27 IL IL52609A patent/IL52609A/en not_active IP Right Cessation
- 1977-07-29 DE DE2734364A patent/DE2734364C2/en not_active Expired
- 1977-08-03 NL NL7708587.A patent/NL168554B/en not_active Application Discontinuation
- 1977-08-04 CA CA284,129A patent/CA1094479A/en not_active Expired
- 1977-08-04 BR BR7705160A patent/BR7705160A/en unknown
- 1977-08-04 SU SU772512150A patent/SU959634A3/en active
- 1977-08-04 IE IE1628/77A patent/IE45543B1/en not_active IP Right Cessation
- 1977-08-04 ES ES461344A patent/ES461344A1/en not_active Expired
- 1977-08-04 IT IT50559/77A patent/IT1080085B/en active
- 1977-08-04 FR FR7724107A patent/FR2360665A1/en active Granted
- 1977-08-05 GB GB33003/77A patent/GB1531970A/en not_active Expired
- 1977-08-06 EG EG465/77A patent/EG12843A/en active
Also Published As
| Publication number | Publication date |
|---|---|
| DE2734364C2 (en) | 1982-12-02 |
| BR7705160A (en) | 1978-04-25 |
| FR2360665A1 (en) | 1978-03-03 |
| ES461344A1 (en) | 1978-12-01 |
| NO150965C (en) | 1985-01-16 |
| IE45543B1 (en) | 1982-09-22 |
| GB1531970A (en) | 1978-11-15 |
| FR2360665B1 (en) | 1982-07-09 |
| DE2734364A1 (en) | 1978-02-09 |
| SU959634A3 (en) | 1982-09-15 |
| IT1080085B (en) | 1985-05-16 |
| IE45543L (en) | 1978-02-05 |
| IL52609A (en) | 1980-06-30 |
| NL7708587A (en) | 1978-02-07 |
| NO150965B (en) | 1984-10-08 |
| IL52609A0 (en) | 1977-10-31 |
| EG12843A (en) | 1980-03-31 |
| NO772654L (en) | 1978-02-07 |
| NL168554B (en) | 1981-11-16 |
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