JP4553242B2 - Method for producing carboxylic acid (ammonium) using biocatalyst - Google Patents

Description

The present invention provides a practical industrial method of producing a carboxylic San'a Nmoniu beam using a biocatalyst having nitrilase activity.

The method of synthesizing a target compound using a biocatalyst having enzyme activity can simplify the reaction process because the reaction conditions are mild, or can obtain a high-purity reaction product with few byproducts. Due to its advantages, it has recently been used in the production of various compounds. Also in the production of carboxylic San'a Nmoniu arm, since it was found an enzyme that converts a nitrile compound into a carboxylic San'a Nmoniu arm nitrilase, or a method for manufacturing ammonium carboxylate with a biocatalyst having the nitrilase activity Several methods for producing carboxylic acid by separating and recovering ammonium salt as ammonia by heat-treating the obtained ammonium carboxylate have been studied.

Among these examples, as a method of using a microbial cell and / or its treated product as it is as a biocatalyst having nitrilase activity, a method of producing 2-amino acid using Arthrobacter genus or the like (see Patent Document 1), A method for producing an amino acid using Acinetobacter genus (see Patent Literature 2, Patent Literature 4 to 7, Patent Literature 12, Patent Literature 24, Patent Literature 32) or a method for producing an α-substituted carboxylic acid (see Patent Literature 15) ) Or a method for producing an optically active carboxylic acid (see Patent Literature 17), a method for producing an unsaturated organic acid (see Patent Literature 27), a method for producing ibuprofen (see Non-Patent Literature 10), Arthrobacter genus, etc. A method for producing an α-hydroxy acid (see Patent Document 3), a method for producing 2-hydroxy-4-methylthiobutyric acid using Rhodococcus or the like (see Patent Document 8), or Acrylic San'a Nmoniu method for producing a beam (JP 9-10, JP 13-14, JP 33-34, Patent Document 25, Non-Patent Documents 2 and 7, see Non-Patent Document 9) or nicotine A method for producing an acid (see Non-patent Document 14), a method for producing an α-hydroxy acid using Pseudomonas genus (see Patent Document 16, Patent Document 18, Patent Document 21), Alcaligenes genus and the like A method for producing an optically active α-substituted carboxylic acid (see Patent Documents 19 to 20 and Patent Document 22), a method for producing a monocarboxylic acid (see Patent Documents 26 and 31), nicotine using Agrobacterium genus and the like A method for producing an acid (see Patent Document 23), a method for producing an organic acid using a Corynebacterium genus (see Patent Documents 28 to 29), and a method for producing 5-cyanovaleric acid using a Comamonas genus, etc. (See Non-Patent Documents 5-6. Etc.) are disclosed.

However, the above-mentioned conventional technology does not necessarily have industrially satisfactory nitrilase initial specific activity, and has problems such as a very large reactor size, and further improvement of nitrilase initial specific activity is required. It was done. Furthermore, when manufacturing industrial carboxylic San'a Nmoniu beam, if it is necessary a higher product accumulation concentration for economic reasons, to produce a particular 4 0 wt% or more highly concentrated ammonium carboxylate such as, reaction Despite the high initial nitrilase specific activity, product inhibition and / or deactivation, or substrate inhibition and / or deactivation that becomes significant only at high product accumulation concentrations as the reaction proceeds and the accumulated concentration of reaction products increases. for active, resulting in time-averaged nitrilase specific activity leading at the end of the reaction from the initial stage of the reaction is low, a large amount of carboxylic San'a in achieving high storage density at a practical reaction times and or practical reactor size was not a level can be produced of Nmoniu arm. In addition, as a solution, a method of achieving a high accumulated concentration of the product in a short time using a large amount of biocatalyst can be considered. The catalyst cost is very high, so it was not very practical. In addition, when such a large amount of biocatalyst is used, a great load is imposed on the subsequent purification step, resulting in a decrease in quality or an increase in purification cost, which becomes an industrial disadvantage.

On the other hand, many methods using a nitrilase enzyme-containing solution purified from microbial cells as a biocatalyst have been disclosed, and a method for producing an acidic sugar derivative using a nitrilase derived from the genus Acinetobacter (see Patent Document 11). Alternatively, a method for producing ibuprofen (see Non-patent Document 8), a method for producing a carboxylic acid using a nitrilase derived from the genus Acidovorax (see Patent Document 30), an enantioselective using a nitrilase derived from the genus Pseudomonas, etc. a method for producing hydroxycarboxylic acids and (see non-Patent Document 1), or aliphatic and method for producing an aromatic carboxylic San'a Nmoniu arm (see non-Patent Document 3), using a nitrilase from Rhodococcus sp carboxylic San'a method for producing Nmoniu arm (non-Patent Document 4, non-Patent Document 12), a method using a nitrilase from Alcaligenes sp ( Patent Document 11), a method using a nitrilase derived from Fusarium sp (Non-patent Document 13 reference) are known. Certainly, some of these have a very high initial reaction nitrilase specific activity, but none have a high time-average specific activity when the product is accumulated to a high concentration. There was nothing that could accumulate things to a high concentration.

Further, the present inventors have already when manufacturing the carboxylic San'a Nmoniu beam from a nitrile compound using a biocatalyst having nitrilase activity, high purity carboxylic San'a Nmoniu beam production method capable of reducing the impurities from the biological catalyst As a result, the inventors have found a method of reducing the weight of the dry biocatalyst used to the produced ammonium carboxylate to 1/2000 or less. (See Patent Document 35), however, it was not sufficient for the preparation of large quantities of carboxylic San'a Nmoniu beam in achieving and or practical reactor size of the high storage density at practical reaction times.

That is, it required to have an industrially sufficient productivity can be produced a large quantity of carboxylic San'a Nmoniu beam in a practical high storage density can be achieved at reaction times and or practical reactor size, substantially have no industrial carboxylic San'a Nmoniu beam producing method of using a biocatalyst with high nitrilase specific activity is actual situation.

An object of the present invention, in producing a carboxylic San'a Nmoniu beam from a nitrile compound using a biocatalyst having nitrilase activity, a large amount in achieving and or practical reactor size of the high storage density at practical reaction time to provide a carboxylic San'a Nmoniu preparation of industrially carboxylic San'a Nmoniu beam that can be achieved with catalyst cost and product quality practical level production of beam.

In the production of ammonium carboxylate from a nitrile compound using a biocatalyst having nitrilase activity, the present inventors can achieve a high accumulation concentration with a practical reaction time, and a large amount of carboxylic acid with a practical reactor size. can achieve the production of a Nmoniu arm with catalyst cost and the product quality of practical level, was carried out an extensive study for industrial carboxylic San'a Nmoniu beam production method, the biocatalyst used in the present invention surprisingly found The inventors have found that it is sufficient to satisfy at least one of the following three conditions, and have completed the present invention. That is, the following conditions are satisfied.
(1) Biocatalyst that satisfies the following two conditions (a) and (b)
(a) When acrylonitrile is used as a substrate, the specific activity of nitrilase at the beginning of the reaction is 30 g-
It must be at least ammonium acrylate / g-dry biocatalyst / Hr.
(b) When ammonium acrylate is produced using acrylonitrile and water, the maximum concentration of ammonium acrylate must exceed 30% by weight.
(2) Biocatalyst that satisfies the following two conditions (c) and (d)
(c) When acrylonitrile is used as the substrate, the nitrilase specific activity at the initial stage of the reaction is
It must be at least 30 g-ammonium acrylate / g-dry biocatalyst / Hr.
(d) When ammonium acrylate is produced using acrylonitrile and water, the maximum production per dry biocatalyst weight (= production capacity) is 500 g-ammonium acrylate / g-
Achieving more than a dry biocatalyst.
(3) Biocatalyst that satisfies the following two conditions (e) and (f)
(e) When acrylonitrile is used as a substrate, the specific activity of nitrilase at the beginning of the reaction is 30 g-
It must be at least ammonium acrylate / g-dry biocatalyst / Hr.
(f) When ammonium acrylate is produced using acrylonitrile and water, the time-average nitrilase specific activity until the ammonium acrylate accumulation concentration reaches 40% by weight is 25 g-ammonium acrylate / g-dried biocatalyst / Hr or higher.

  Furthermore, in the present invention, at a stage where the accumulated concentration of ammonium carboxylate is low, for example, when it is less than 30% by weight, the steady concentration of the nitrile compound may be controlled to 2% by weight or less. When the ammonium carboxylate accumulation concentration is increased, for example, 30% by weight or more, when the nitrile compound steady concentration is larger than 1% by weight, the product inhibition and / or deactivation that appears suddenly, or the high product accumulation concentration is the first time. We have discovered the fact that the specific activity of nitrilase decreases rapidly due to significant substrate inhibition and / or inactivation. Further, at this time, the steady feeding of the nitrile compound was stopped, and when the concentration of the nitrile compound decreased to 1% by weight or less, the specific activity of the nitrilase increased again, and the fact that the reaction could be continued was discovered.

That is, when producing a carboxylic acid (ammonium) from a nitrile compound using a biocatalyst having nitrilase activity, while the accumulated concentration of the ammonium carboxylate is low, for example, less than 30% by weight, the steady concentration of the nitrile compound is 2% by weight. %, And when the ammonium carboxylate accumulation concentration increases and the specific activity of nitrilase decreases rapidly, or before or after, for example, ± 10% by weight, preferably ± 5% by weight %, For example, when the ammonium carboxylate accumulation concentration is 30% by weight or more, by reducing the nitrile compound concentration to 1% by weight or less, a high accumulation concentration can be achieved in a practical reaction time. Production of large quantities of carboxylic acids (ammonium) at a reasonable reactor size and product quality at a practical level It discovered that can be formed, which resulted in the completion of the present invention.

That is, the present invention has a configuration as described below.
[1] the genus Acinetobacter and or processed product thereof, using a biocatalyst having immobilized product and or consist of a suspension nitrilase activity, a method for producing a carboxylic San'a Nmoniu beam from a nitrile compound, the biological catalyst there a said carboxylic San'a Nmoniu beam producing method of having the following characteristics, while the carboxylic acid ammonium salt accumulation concentration increases the control the nitrile compound concentration 2 wt% or less, abruptly nitrilase specific activity A method for producing ammonium carboxylate, characterized in that the concentration of the nitrile compound is reduced to 1% by weight or less before or after the decrease.
1) When acrylonitrile is used as a substrate, the specific activity of nitrilase at the beginning of the reaction must be 30 g-ammonium acrylate / g-dry biocatalyst / Hr or more.
2) When ammonium acrylate is produced using acrylonitrile and water, the maximum accumulated concentration of ammonium acrylate must exceed 30% by weight.
[2] of the genus Acinetobacter and or processed product thereof, using a biocatalyst having immobilized product and or consist of a suspension nitrilase activity, a process for producing a carboxylic San'a Nmoniu beam from nitrile compounds, and biological catalyst a the carboxylic San'a Nmoniu beam producing method of having the following characteristics, while the carboxylic acid ammonium salt accumulation concentration increases the control the nitrile compound concentration 2 wt% or less, abruptly nitrilase specific activity A method for producing ammonium carboxylate, characterized in that the concentration of the nitrile compound is reduced to 1% by weight or less before or after the decrease.
1) When acrylonitrile is used as a substrate, the specific activity of nitrilase at the beginning of the reaction must be 30 g-ammonium acrylate / g-dry biocatalyst / Hr or more.
2) When ammonium acrylate is produced using acrylonitrile and water, the maximum production per dry biocatalyst weight (= production capacity) should be 500 g-ammonium acrylate / g-dry biocatalyst or more.
[3] of the genus Acinetobacter and or processed product thereof, using a biocatalyst having immobilized product and or consist of a suspension nitrilase activity, a process for producing a carboxylic San'a Nmoniu beam from nitrile compounds, and biological catalyst a the carboxylic San'a Nmoniu beam producing method of having the following characteristics, while the carboxylic acid ammonium salt accumulation concentration increases the control the nitrile compound concentration 2 wt% or less, abruptly nitrilase specific activity A method for producing ammonium carboxylate, characterized in that the concentration of the nitrile compound is reduced to 1% by weight or less before or after the decrease.
1) When acrylonitrile is used as a substrate, the specific activity of nitrilase at the beginning of the reaction is 30 g-ammonium acrylate / g-dry biocatalyst / Hr or more.
2) When ammonium acrylate is produced using acrylonitrile and water, the time average nitrilase specific activity until the ammonium acrylate accumulation concentration reaches 40% by weight is 25 g-ammonium acrylate / g-dry biocatalyst / Hr or more There is.
[4] Carboxyl according to any one of [1] to [ 3 ], wherein the biocatalyst is an immobilized product and / or suspension of a microbial cell and / or a processed product thereof and / or a nitrilase enzyme thereof. San'a Nmoniu-time method of manufacturing.
[5] biocatalyst is microbial cells and or processed product thereof, characterized in that it is a fixed product and or suspensions [1] to [4] according to any one of the carboxylic San'a Nmoniu arm Production method.
[6] of the biocatalyst Gram-negative bacteria and or processed product thereof, characterized in that it is a fixed product and or suspensions [1] to [5] of the carboxylic San'a Nmoniu beam according to any one Production method.
[7] biocatalyst of Acinetobacter spp and or processed product thereof, the production of carboxylic San'a Nmoniu beam according to [1] to [6] any one, which is a fixed product and or suspensions Method.
[8] The biocatalyst is an immobilized product and / or suspension of at least one microbial cell selected from Acinetobacter sp. AK226 and / or Acinetobacter sp. AK227 and / or its treated product [1] ] - [7] carboxylic San'a Nmoniu beam method according to any one.
[9] the biocatalyst Acinetobacter Sp.AK226 and or processed product thereof, carboxylic San'a Nmoniu beam according to [1] to [8] any one, which is a fixed product and or suspensions the method of production.

The present invention, in producing a carboxylic San'a Nmoniu beam from a nitrile compound using a biocatalyst having nitrilase activity, practical large amount of carboxylic at achieving and or practical reactor size of the high concentration of accumulated reaction time the preparation of San'a Nmoniu beam can provide a method for producing carboxylic San'a Nmoniu beam that can be achieved with catalyst cost and the product quality of practical level.

The biocatalyst having nitrilase activity in the present invention, capable of converting directly the nitrile group to the carboxylic San'a Nmoniu beam group may be of any form as long as catalysts possess nitrilase enzyme derived from a living body . Examples of organisms from which the nitrilase enzyme is derived include microorganisms, animal and plant cells, and the like, but it is preferable to use microbial cells in view of the amount of enzyme expression per weight and ease of handling.

Many microbial species are known, and examples of those having high nitrilase activity include Rhodococcus genus, Acinetobacter genus, Alcaligenes genus, Psudomonas genus, Corynebacterium genus and the like. Among these, the genus Acinetobacter and Alcaligenes, which are Gram-negative bacteria, are particularly preferable in the present invention, and more preferably the genus Acinetobacter.
Specifically, Acinetobacter sp. AK226 (FERM BP-08590) and Acinetobacter sp. AK227 (FERM BP-08591). These strains are described in JP-A No. 2001-299378, JP-A No. 11-180971, JP-A No. 06-303991, JP-A No. 63-209592 and JP-B No. 63-2596.

Further, for example, it may be a microorganism in which a natural or artificially improved nitrilase gene is incorporated by genetic engineering techniques, or a nitrilase enzyme taken out from it. to produce the carboxylic San'a Nmoniu beam with a small amount of conversion microorganism that expressed low nitrilase active to San'a Nmoniu arm is because it takes more reaction time, microorganisms highly expressed nitrilase as possible, and Alternatively, it is desirable to use a microorganism expressing a nitrilase having a high conversion activity, or a nitrilase enzyme extracted therefrom.

  As a form of the biocatalyst, microorganisms / animal / plant cells or the like may be used as they are, or the microorganisms / animal / vegetable cells themselves, or those treated by disruption, or necessary nitrilase enzymes from the microorganisms / animal / plant cells, etc. A product obtained by fixing the product by a general inclusion method, a crosslinking method, a carrier binding method or the like may be used. Examples of the immobilization carrier used for immobilization include, but are not limited to, glass beads, silica gel, polyurethane, polyacrylamide, polyvinyl alcohol, carrageenan, alginic acid, and photocrosslinking resin.

  When microorganisms, animal and plant cells are used as they are, they may be suspended only in water (distilled water and / or ion-exchanged water), but are usually suspended in an inorganic salt buffer solution due to osmotic pressure. . Moreover, also when using what was fix | immobilized, it is normally suspended and used for a buffer solution from the relationship of osmotic pressure. The buffer solution concentration at this time is preferably as low as possible from the viewpoint of reducing impurities in the reaction solution, but from the viewpoint of maintaining the stability and specific activity of the biocatalyst, it is usually less than 0.1M, preferably 0.01. It is -0.08M, More preferably, it is 0.02-0.06M.

  The specific activity of nitrilase at the beginning of the reaction in the present invention is a very important factor for the present invention. Originally, the nitrilase specific activity at the initial stage of the reaction varies greatly depending on the reaction conditions and / or the reaction substrate, etc., but the nitrilase specific activity at the initial stage of the reaction in the present invention uses acrylonitrile as a substrate and a reaction temperature of 30 ° C. The reaction was started by adding acrylonitrile to the biocatalyst suspension under the reaction conditions of pH = 7.0, and the ammonium acrylate production weight in 5 minutes from the start of the reaction was divided by the dry biocatalyst weight used, and It is defined as ammonium acrylate production weight per hour per dry biocatalyst weight obtained by dividing by reaction time (5 minutes = 1/12 hours). In the present invention, it is essential that the initial specific activity is 30 g-ammonium acrylate / g-dry biocatalyst weight / Hr or more, preferably 40 g-ammonium acrylate / g-dry biocatalyst weight / Hr or more. More preferably 50 g-ammonium acrylate / g-dry biocatalyst weight / Hr or more, more preferably 60 g-ammonium acrylate / g-dry biocatalyst weight / Hr or more, most preferably 70 g-ammonium acrylate / g- More than dry biocatalyst weight / Hr.

  Further, the maximum accumulation concentration of ammonium acrylate referred to in the present invention is a very important factor for the present invention. Originally, the maximum accumulated concentration varies greatly depending on reaction conditions. In the present invention, acrylonitrile is used as a substrate, and reaction conditions are 30 ° C. and pH = 7.0. Is continuously or intermittently added to start the reaction, and the steady state concentration of acrylonitrile in the reaction solution during the reaction is controlled to 1% by weight or less. The maximum accumulation concentration here refers to the highest ammonium acrylate weight concentration that can be accumulated by the biocatalyst when the reaction is allowed to proceed under the above-mentioned constant conditions. Alternatively, it is the product accumulation concentration that can be reached while being affected by substrate inhibition and / or deactivation that becomes significant only at the inactivation or high product accumulation concentration. The maximum accumulated concentration must be over 30% by weight, preferably 35% by weight or more, more preferably 40% by weight or more.

  Further, the maximum production amount (= production capacity) per dry biocatalyst weight referred to in the present invention is a very important factor for the present invention. Originally, the production capacity varies greatly depending on reaction conditions. In the present invention, acrylonitrile is used as a substrate, and reaction temperature is 30 ° C. and pH = 7.0. The reaction is started by adding continuously or intermittently, and is performed by controlling the steady concentration of acrylonitrile in the reaction solution during the reaction to 1% by weight or less. The production capacity here refers to product inhibition and / or deactivation that occurs with an increase in product accumulation concentration, or substrate inhibition and / or deactivation that becomes noticeable only at a high product accumulation concentration. The ammonium acrylate production weight per dry biocatalyst weight obtained by dividing the production weight of ammonium acrylate up to the point when the reaction is completely stopped by the dry biocatalyst weight used. It is essential that the production capacity is 500 g-ammonium acrylate / g-dry biocatalyst or more, preferably 1000 g-ammonium acrylate / g-dry biocatalyst or more, more preferably 2000 g-ammonium acrylate / g- More than dry biocatalyst, more preferably 3000 g-ammonium acrylate / g-dry biocatalyst or more, still more preferably 4000 g-ammonium acrylate / g-dry biocatalyst or more, most preferably 5000 g-ammonium acrylate / g-dry Better than biocatalyst.

  In addition, the time-average nitrilase specific activity until the ammonium acrylate accumulation concentration of 40% by weight in the present invention is a very important factor for the present invention. Originally, the time-average nitrilase specific activity varies greatly depending on the reaction conditions. In the present invention, acrylonitrile is used as a substrate, the reaction temperature is 30 ° C., and the reaction condition is pH = 7.0. The reaction is started by continuously or intermittently adding acrylonitrile to the liquid, and the steady state concentration of acrylonitrile in the reaction liquid during the reaction is controlled to 1% by weight or less. The time-average nitrilase specific activity referred to here is a product inhibition and / or inactivation that occurs with an increase in the product accumulation concentration, or a substrate inhibition that becomes noticeable only at a high product accumulation concentration. And / or the amount of ammonium acrylate produced up to the point at which the reaction is completely stopped due to deactivation, divided by the weight of the dry biocatalyst used and further divided by the reaction time, per hour per dry biocatalyst weight It is the production weight of ammonium acrylate. The average nitrilase specific activity for this time must be 25 g-ammonium acrylate / g-dry biocatalyst / Hr or more, preferably 30 g-ammonium acrylate / g-dry biocatalyst / Hr or more, more preferably 40 g-ammonium acrylate / g-dry biocatalyst or more, more preferably 50 g-ammonium acrylate / g-dry biocatalyst or more, more preferably 60 g-ammonium acrylate / g-dry biocatalyst, most preferably 70 g -More than ammonium acrylate / g-dry biocatalyst.

  It is important that the biocatalyst used in the present invention satisfies the requirements for the nitrilase specific activity at the initial stage of the reaction and the requirements for the maximum accumulation concentration of ammonium acrylate. Is more preferable. Further, in addition to these requirements, it is most preferable to satisfy the requirement of the time average nitrinase specific activity at the same time.

  The final concentration of ammonium carboxylate to be produced in the reaction solution is usually 20% by weight or more, but for economic reasons, a higher concentration is better, preferably 30% by weight or more, more preferably 35% by weight or more, More preferably, it is 40% by weight or more.

  The reaction method for producing the carboxylic acid (ammonium) may be any of a fixed bed, a moving bed, a fluidized bed, a stirring tank, etc., and may be a continuous reaction or a semi-batch reaction. When used, a half-batch reaction using a stirring tank is preferable because of the ease of reaction. In that case, it is good to perform appropriate stirring from the viewpoint of reaction efficiency.

  In addition, when a half-batch reaction is performed, the biocatalyst may be disposable for one batch or may be repeatedly performed. However, when the reaction is repeated, the biocatalyst is rapidly changed from a high concentration of ammonium carboxylate to a low concentration, so that the specific activity may be reduced due to the influence of osmotic pressure, etc., so care must be taken.

  The nitrile compound used in the present invention is not particularly limited as long as it is converted into the corresponding carboxylic acid (ammonium) by the catalytic action of nitrilase. For example, saturated aliphatic nitriles such as acetonitrile, propionitrile, succinonitrile and adiponitrile, or unsaturated aliphatic nitriles such as acrylonitrile and methacrylonitrile, or aromatic nitriles such as benzonitrile and phthalodinitrile, Alternatively, heterocyclic nitriles such as 3-cyanopyridine, 2-cyanopyridine, and 4-cyanopyridine, amino nitriles such as glycinonitrile, and hydroxynitriles such as mandelonitrile are included. Among these, representative examples of suitable for the production of carboxylic acid (ammonium) using a biocatalyst from the relative high activity are propionitrile, acrylonitrile, methacrylonitrile, 3-cyanopyridine, glycino. Although it is a nitrile, acrylonitrile and 3-cyanopyridine are particularly preferred.

When the ammonium carboxylate accumulation concentration is less than 30% by weight, the steady concentration of the nitrile compound as the reaction substrate is 2% by weight or less, preferably 0.2 to 1.5% by weight, more preferably 0.5 to 1% by weight, and still more preferably 0.7 to 1%. When the ammonium carboxylate accumulation concentration is 30% by weight or more, the steady concentration of the nitrile compound as the reaction substrate is 1% by weight or less, preferably 0.1 to 0.7% by weight, more preferably 0.2 to 0.5% by weight, More preferably, it is controlled to 0.3 to 0.5% by weight. In particular, when ammonium carboxylate has a high accumulation concentration of 30% by weight or more, if the concentration of the nitrile compound is too high, product inhibition and / or deactivation, or substrate inhibition and / or deactivation that becomes noticeable for the first time at a high product accumulation concentration will be observed. In some cases, the influence of life increases rapidly, and the reaction that has progressed until then stops. However, in that case, if measures such as stopping the addition of the nitrile compound are taken at an early stage when the activity has declined, the activity may be restored again, and the control of the concentration of the nitrile compound will have a very significant effect. This is a good example. On the other hand, if the concentration of the nitrile compound is too low, the reaction rate is lowered, which is disadvantageous because carboxylic acid (ammonium) cannot be efficiently produced. For the above reasons, it is important to control the steady concentration of the nitrile compound during the reaction within an appropriate range at two stages.

  The dry biocatalyst weight used for the ammonium carboxylate produced should be 1/500 or less, preferably 1/600 to 1/5000, more preferably 1/700 to 1/3000, and still more preferably 1/800 to 1 /. 1500, most preferably 1/1000 to 1/1300. If the weight of the dry biocatalyst used relative to the ammonium carboxylate produced is too large, a large amount of impurities derived from the biocatalyst suspension is entrained in the reaction solution, which increases the purification cost and decreases the product quality. Conversely, if the weight of the dry biocatalyst used for the ammonium carboxylate produced is too small, the productivity per reactor volume is reduced, and a large reactor size is required, which is economically disadvantageous.

If the reaction temperature is too low, the reaction activity becomes low, and more reaction time is required to produce a high concentration of ammonium carboxylate. On the other hand, if the reaction temperature is too high, the biocatalyst is deactivated due to heat, and if the target ammonium carboxylate concentration is high, it is difficult to reach that concentration, resulting in the addition of a new biocatalyst, etc. Therefore, the cost of the catalyst becomes high. In the case of using a polymerizable high substrates such as acrylonitrile, reducing the yield of carboxylic San'a Nmoniu Mumo Nomar of interest under the influence of polymerization substrate, or the polymerization of the product unsaturated carboxylic San'a Nmoniu arm This is not preferable. Therefore, the reaction temperature is usually from the freezing point to 40 ° C, preferably from 10 to 40 ° C, more preferably from 20 to 40 ° C, still more preferably from 30 to 35 ° C.

  The reaction charging solution for suspending microorganisms at the initial stage of the reaction is not particularly limited as long as it is an aqueous solution, but water is usually used. Further, a buffer solution may be used from the viewpoint of increasing the stability of the microorganism due to the osmotic pressure.

  The pH of the reaction solution is preferably adjusted to an optimum pH for the nitrilase specific activity of the biocatalyst to be used. Usually, the reaction solution pH is preferably 6 to 13, and more preferably 9 to 11. However, for the convenience of the product to be obtained, this is not limited as long as the required pH is specified, and it can be arbitrarily selected within a range in which the decrease in reaction specific activity does not appear extremely.

  When the substrate has an unsaturated group and is polymerizable, the reaction is usually performed in the presence of a polymerization inhibitor. The type of the polymerization inhibitor used is not particularly limited as long as it can sufficiently suppress the by-product of the oligomer or low molecular weight polymer during the reaction. For example, a normal radical polymerization inhibitor such as hydroquinone or p-methoxyphenol is used. Can be mentioned. Further, the polymerization inhibitor may be added to the reaction system together with the nitrile compound in the form of being added to the raw material nitrile compound, or may be added to the reaction system separately from the raw material. In general, these polymerization inhibitors are generally known to increase the polymerization inhibition effect due to the presence of oxygen, and it is desirable that the reaction system be in the presence of oxygen.

  Hereinafter, the present invention will be described in more detail with reference to examples. In addition, this invention is not necessarily limited by these Examples, A various change and modification are possible unless it exceeds the summary.

  The method for measuring the weight of the dried biocatalyst in the non-immobilized biocatalyst suspension was performed as follows. First, an appropriate amount of a biocatalyst suspension having an appropriate concentration was taken, cooled to −80 ° C., completely dried using a freeze dryer, and the concentration of the biocatalyst suspension was calculated from the weight value. The biocatalyst suspension having a known concentration was diluted to a plurality of appropriate concentrations, the turbidity was measured at room temperature using a turbidimeter, and a calibration curve for the biocatalyst with the turbidity clock was prepared. Thereafter, the dry biocatalyst concentration of any biocatalyst suspension was calculated from the indicated value of the turbid clock.

  In the case of an immobilized biocatalyst, the dry biocatalyst concentration of the biocatalyst suspension before immobilization was measured, and the immobilized carrier in the immobilized catalyst was removed based on the mixing ratio of the immobilized carrier and the biocatalyst. The dry weight of the biocatalyst itself was calculated.

  The reaction solution was analyzed as follows. First, the nitrile compound as a substrate was measured by gas chromatography (Shimadzu GC-14B). The column was a capillary column (Shinwa Kako ULBON HR-20M 0.25 mm ID x 30 m, film thickness 0.25 μm), and the detector was detected by FID. Next, the product carboxylic acid (ammonium) monomer was measured by high performance liquid chromatography. The column was a reverse phase column (Tosoh TSK-GEL ODS-80Ts), the column temperature was 40 ° C., the mobile phase was a 10 mM phosphoric acid aqueous solution, and the detector was UV (Shimadzu SPD-10A, 210 nm).

[Preparation of biocatalyst]
Sodium chloride 0.1 wt%, potassium dihydrogen phosphate 0.1 wt%, magnesium sulfate heptahydrate 0.05 wt%, ferrous sulfate heptahydrate 0.005 wt%, ammonium sulfate 0.1 wt%, potassium nitrate 0.1 wt% manganese sulfate pentahydrate 250 ml of a culture solution containing 0.005% by weight of the Japanese product was charged into an Erlenmeyer flask, adjusted with sodium hydroxide to a pH of 7, sterilized at 121 ° C. for 20 minutes, and then 0.5% by weight of acetonitrile was added. This was inoculated with Acinetobacter sp. AK226 and cultured with shaking at 30 ° C. (preculture). 3 L of the same composition culture solution was charged into a 5 L jar fermenter, sterilized at 121 ° C. for 20 minutes, inoculated with the pre-culture solution, and aerated and stirred at 30 ° C. The acetic acid feed was started 2 hours after the start of the culture. The pH was controlled with phosphoric acid and aqueous ammonia so that the pH was 7, and finally a suspension of about 1% by weight of Acinetobacter sp. AK226 was obtained. Furthermore, it was washed twice with 0.06M phosphate buffer, and finally Acinetobacter sp. AK226 suspension (dry cell concentration 10-15% by weight) suspended in phosphate buffer was obtained.

[Preparation of immobilized bacterial cell catalyst]
Acinetobacter sp.AK226 suspension (dry cell concentration 15% by weight), acrylamide, N, N'-methylenebisacrylamide, 5% by weight N, N, N ', N'-tetramethylethylenediamine aqueous solution, 0.06M phosphoric acid A 2.5 wt% potassium persulfate aqueous solution was mixed with the buffer mixture to obtain a polymer. The final composition is 3% dry cell concentration, 52% 0.06M phosphate buffer (pH = 7), 18% acrylamide, 1% N, N'-methylenebisacrylamide, 5% by weight N, N, N ' , N′-tetramethylethylenediamine aqueous solution 12%, 2.5 wt% potassium persulfate aqueous solution 14% (both wt%). The polymer was cut into approximately 1 × 3 × 3 mm squares to obtain immobilized cells. The immobilized cells were washed with 0.06M phosphate buffer (pH = 7) to obtain an immobilized cell catalyst.

[Example 1]
The hydrolysis reaction of acrylonitrile was performed using Acinetobacter sp. AK226 as a biocatalyst. First, Acinetobacter sp. AK226 (substrate: acrylonitrile, 30 ° C, pH = 7, specific activity is 100 g-ammonium acrylate / g-dried cells / Hr) was suspended in 1525 g of distilled water previously charged in a 2 L SUS reactor so as to have a concentration of 436 ppm by weight. The SUS reactor was equipped with a jacket so that the internal temperature could be controlled, and the internal temperature was controlled at 30 ° C. The reactor was equipped with a stirrer and stirred at a stirring speed of 150 rpm during the reaction. Next, the raw material acrylonitrile (special grade Wako Pure Chemicals, p-methoxyphenol 40 wtppm / acrylonitrile included as a polymerization inhibitor) was fed using a feed pump at a feed rate corresponding to the initial specific activity. Incidentally, the initial specific activity was 100 g-ammonium acrylate / g-dry cells / Hr. Sampling was periodically performed during the reaction, the acrylonitrile concentration was measured by gas chromatography, and the acrylic acid (ammonium) concentration was measured by high performance liquid chromatography. The reaction was continued while controlling the acrylonitrile feed so that the acrylonitrile concentration during the reaction did not exceed 2% by weight from the value of the gas chromatography. Further, the pH of the reaction solution after completion of the reaction was measured and found to be 7.1. The final results of the reaction continued for 22 hours are shown in Table 1.

[Example 2]
The reaction and various analyzes were performed in the same manner as in Example 1 except that the reaction temperature (internal temperature) was controlled at 35 ° C. Incidentally, the initial specific activity was 122 g-ammonium acrylate / g-dry cell / Hr. The pH of the reaction solution after the reaction was 7.0. The final results of the reaction continued for 16 hours are shown in Table 1.

[Comparative Example 1]
Acinetobacter sp. AK226 (substrate: acrylonitrile, 30 ° C, pH = 7, specific activity 18g-ammonium acrylate / g-), entrapped and immobilized in polyacrylamide stored refrigerated in 0.06M phosphate buffer The reaction was carried out in the same manner as in Example 1 except that the dry cell / Hr) was dispersed in 1525 g of distilled water previously charged in a 2 L SUS reactor so that the dry cell concentration was 436 ppm by weight. Various analyzes were performed. The pH of the reaction solution after completion of the reaction was 7.3. Table 1 shows the final results obtained by continuing the reaction for 87 hours.

[Example 3]
Acinetobacter sp. AK226 refrigerated and stored in 0.06M phosphate buffer (Substrate: Acrylonitrile, specific activity 74g-ammonium acrylate / g-dried cells / Hr at 30 ° C, pH = 7) Was suspended in 920 g of distilled water previously charged in a 2 L glass four-necked flask to a concentration of 198 ppm by weight. The four-necked flask was immersed in a constant temperature water bath to control the internal temperature at 30 ° C. The four-necked flask was equipped with a stirrer, and stirred at a stirring speed of 200 rpm during the reaction. Next, the raw material acrylonitrile (special grade Wako Pure Chemicals, p-methoxyphenol 40 wtppm / acrylonitrile included as a polymerization inhibitor) was fed using a feed pump at a feed rate corresponding to the initial specific activity. Incidentally, the initial specific activity was 74 g-ammonium acrylate / g-dry cell / Hr. Sampling was periodically performed during the reaction, the acrylonitrile concentration was measured by gas chromatography, and the acrylic acid (ammonium) concentration was measured by high performance liquid chromatography. The reaction was continued while controlling the acrylonitrile feed so that the acrylonitrile concentration during the reaction did not exceed 2% by weight from the value of the gas chromatography. Since the reaction specific activity dropped sharply after 27 hours from the start of the reaction, the acrylonitrile feed was stopped. After a while, about 30 hours after the start of the reaction, the acrylonitrile concentration dropped to 1% or less, and then the reaction was continued for 38 hours. The results are shown in FIG.

[Comparative Example 2]
The same operation as in Example 3 was performed except that the acrylonitrile feed was not stopped when the specific activity decreased during the reaction, but the ammonium acrylate concentration was stopped at around 35% by weight, and sampling was performed for a while. The analysis was continued, but the activity did not return again as in Example 3 .

According to the present invention method, not only a high initial specific activity, by high carboxylic San'a Nmoniu arm accumulation concentration and time average specific activity until the said accumulation concentration having a high biocatalyst, any nitrile practical reactor size industrially useful carboxylic San'a Nmoniu beam from a compound, the reaction time, can be produced in catalyst costs.

The change of the substrate acrylonitrile density | concentration with respect to reaction time in Example 3 and the ammonium acrylate density | concentration to produce | generate is shown.

Claims (9)

The genus Acinetobacter and or processed product thereof, using a biocatalyst having immobilized product and or consist of a suspension nitrilase activity, a method for producing a carboxylic San'a Nmoniu beam from a nitrile compound, the biological catalyst is less a the carboxylic San'a Nmoniu beam method for manufacturing having the features, time during which the carboxylic acid ammonium salt accumulation concentration increases to control the nitrile compound concentration 2 wt% or less, nitrilase specific activity rapidly decreases Alternatively, before and after that, a method for producing ammonium carboxylate, wherein the concentration of the nitrile compound is reduced to 1% by weight or less.
1) When acrylonitrile is used as a substrate, the specific activity of nitrilase at the beginning of the reaction must be 30 g-ammonium acrylate / g-dry biocatalyst / Hr or more.
2) When ammonium acrylate is produced using acrylonitrile and water, the maximum accumulated concentration of ammonium acrylate must exceed 30% by weight. The genus Acinetobacter and or processed product thereof, using a biocatalyst having immobilized product and or consist of a suspension nitrilase activity, a process for producing a carboxylic San'a Nmoniu beam from nitrile compounds, and biological catalysts or less a the carboxylic San'a Nmoniu beam method for manufacturing having the features of, while the carboxylic acid ammonium salt accumulation concentration increases the control the nitrile compound concentration 2 wt% or less, nitrilase specific activity rapidly decreases A method for producing ammonium carboxylate, characterized in that the concentration of the nitrile compound is reduced to 1% by weight or less at or around that time.
1) When acrylonitrile is used as a substrate, the specific activity of nitrilase at the beginning of the reaction must be 30 g-ammonium acrylate / g-dry biocatalyst / Hr or more.
2) When ammonium acrylate is produced using acrylonitrile and water, the maximum production per dry biocatalyst weight (= production capacity) should be 500 g-ammonium acrylate / g-dry biocatalyst or more. The genus Acinetobacter and or processed product thereof, using a biocatalyst having immobilized product and or consist of a suspension nitrilase activity, a method for producing a carboxylic San'a Nmoniu beam from a nitrile compound, the biological catalyst is less a the carboxylic San'a Nmoniu beam method for manufacturing having the features, and while the carboxylic acid ammonium salt accumulation concentration increases the control the nitrile compound concentration 2 wt% or less, nitrilase specific activity rapidly decreases A method for producing ammonium carboxylate, characterized in that the concentration of the nitrile compound is reduced to 1% by weight or less at or around that time.
1) When acrylonitrile is used as a substrate, the specific activity of nitrilase at the beginning of the reaction is 30 g-ammonium acrylate / g-dry biocatalyst / Hr or more.
2) When ammonium acrylate is produced using acrylonitrile and water, the time average nitrilase specific activity until the ammonium acrylate accumulation concentration reaches 40% by weight is 25 g-ammonium acrylate / g-dry biocatalyst / Hr or more There is. Biocatalyst is microbial cells and or processed product thereof and or nitrilase enzyme, carboxylic San'a Nmoniu beam according to claim 1 to 3 any one, which is a fixed product and or suspensions Production method. The biocatalyst microbial cells and or processed product thereof, according to claim 1-4 or carboxylic San'a Nmoniu beam method according to item 1, which is a fixed product and or suspensions. The biocatalyst Gram-negative bacteria and or processed product thereof, carboxylic San'a Nmoniu beam method according to claims 1 to 5 any one, which is a fixed product and or suspensions. Biocatalyst of Acinetobacter spp and or processed product thereof, a manufacturing method of a carboxylic San'a Nmoniu beam according to any one of claims 1-6, characterized in that the immobilized product and or suspensions. Claim 1-7 which biocatalyst is characterized in that at least one cell and or processed product thereof selected from the group consisting of Acinetobacter Sp.AK226 and or Acinetobacter sp.AK227, an immobilized product and or suspensions carboxylic San'a Nmoniu beam method according to any one. The biocatalyst Acinetobacter Sp.AK226 and or processed product thereof, a manufacturing method of a carboxylic San'a Nmoniu beam according to any one of claims 1-8, characterized in that the immobilized product and or suspensions.

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