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    • 专利摘要:
    The present invention relates to a process for recovering fermentative products present in a fermentation broth produced in a bioreactor (9), comprising a step a) in which a gaseous flow (15) is fed to the fermentation broth under pressure so as to entrain at least a portion of the products and produce a gaseous stream (16) enriched in fermentation products. The process comprises a step b) of storage of the fermentation gases and the gas stream that is sent to step a) is constituted by the stored fermentation gases.
    公开号:FR3053357A1
    申请号:FR1656209
    申请日:2016-06-30
    公开日:2018-01-05
    发明作者:Vincent Coupard;Helena GONZALEZ PENAS;Eszter Toth;Mehdi LE MOEL
    申请人:IFP Energies Nouvelles IFPEN;
    IPC主号:
    专利说明:

    (54) METHOD FOR RECOVERING ALCOHOLS FROM
    ©) The present relates to a process for recovering fermentative products present in a fermentation must produced in a bioreactor (9), comprising a step a) in which a gaseous flow (15) under pressure is sent into the fermentation must. entraining at least part of the products and producing a gas flow (16) enriched in fermentation products. The method comprises a step b) of storing the fermentation gases and the gas flow which is sent to step a) consists of the stored fermentation gases.

    The present invention relates to a process for recovering fermentation products from a fermentation juice contained in a fermenter. The process according to the invention is particularly suitable for recovering alcohols, esters, carboxylic acids and ketones, aldehydes produced by fermentation of an aqueous solution of C5 and / or C6 sugars. The recovery process can be applied in particular to a fermentation process of the ABE (Acetone / Butanol / Ethanol) or IBE (Isopropanol / Butanol / Ethanol) type.
    State of the art
    In order to meet the challenges of the energy transition, a great deal of research is being carried out to develop so-called "green" processes, making it possible to access chemical intermediates in an alternative way to petroleum refining and / or petrochemicals.
    Alcohols from fermentation (n-butanol, isopropanol) are the most promising substitutes for petrochemical derivatives. ABE fermentation (Acetone - Butanol - Ethanol) is one of the oldest fermentations to have been industrialized (early 20th century) and has since been widely studied. Mention may also be made of IBE fermentation, producing a mixture of isopropanol, butanol and ethanol. These two types of fermentation are carried out under strict anaerobiosis in the presence of a fermentation microorganism generally of the genus Clostridium.
    One of the obstacles in the development of fermentation processes is the stage of recovery of the products from the highly diluted aqueous medium. This is the determining parameter in terms of the economics of these types of process. In order to make large-scale fermentation production economically viable, it is necessary to maximize the final titer as well as the volume productivity in the bioreactor, these two parameters being greatly limited by the marked inhibition of microorganisms with respect to products of interest. It is indeed known that butanol from a concentration in the fermentation medium has an inhibitory effect on the microorganism, for example in Clostridium. The use of fermentation-separation coupling techniques (liquid extraction, adsorption, stripping ...) allows the recovery of inhibitor products as they are produced. These techniques offer means of crossing the inhibition limit imposed during microbial production, and consequently of reducing the energy demand required for the distillation of an extremely diluted final fermentation juice.
    In situ recovery techniques for butanol have been widely explored in the literature for acetone / butanol / ethanol fermentation.
    The recovery of products from an ABE fermentation by stripping with a gas injected into the bioreactor has been proposed in the literature (Quereshi and Blaschek (Renewable Energy, 22 (4)) or Ezeji et al. (Appl. Microbio. Biotechnol. , 63 (6)). In these schemes, the alcohols are recovered by condensation of the gas from the reactor, which proves to be extremely costly from the energy point of view.
    Kuan-Ming & al. (Journal of the Taiwan Institute of Chemical Engineers, 45 (2014) 21062110) describe an integrated process coupling gas stripping and liquid-liquid extraction with oleyl alcohol in situ, that is to say within the fermenter.
    Document US 8,945,891 is also known, which discloses a scheme for recovering metabolites from ABE fermentation by injecting gas into the bioreactor followed by a step for recovering the metabolite by absorption with a composition comprising isophorone as solvent .
    US 8,460,439 describes a method for recovering the butanol contained in a fermentation juice in which part of the fermentation juice is sent to a stripping step using an inert gas so as to recover a gas enriched in butanol which is then treated in a section absorption in the presence of an organic solvent, for example an alcohol having at least 8 carbon atoms.
    An object of the invention is to provide an alternative process for recovering fermentative products present in a fermentation must of a bioreactor which is efficient, simple to implement and for which the capital expenditure (CAPEX) and operations (OPEX) are optimized.
    Summary of the invention
    The present invention therefore relates to a process for recovering fermentation products present in an aqueous fermentation juice produced in a bioreactor which comprises a step a) in which a gaseous flow under pressure is sent into the aqueous fermentation juice so as to entrain at least part of the alcohols and produce a gas stream enriched in alcohols. The method according to the invention is characterized by the presence of a step b) of prior storage of the fermentation gases produced in the bioreactor which thus constitute the gas flow which is sent to the bioreactor in order to entrain the fermentation products.
    The method according to the invention thus valorizes the gases produced by fermentation, which can be considered as by-products of fermentation, as stripping gas making it possible to extract the products of interest outside the fermentation system. The implementation of the process thus no longer requires the supply of external gas to the process which generates significant transport costs. Finally in terms of investment, the process requires only a storage device (balloon) which is however already necessary in the case where the stripping gas is not produced in situ.
    The method according to the invention also has the advantage of allowing the recovery of at least part of the fermentation products by a method other than distillation, the latter being particularly energy-consuming due to the diluted nature of the products present in the must. fermentation.
    The in situ recovery process for fermentation products also allows better control of their content in the fermentation medium in order to limit this content to a threshold value which remains acceptable for the microorganism. Indeed, it is known that from a certain content in the fermentation medium, fermentation products, and in particular alcohols (e.g. butanol), have an inhibitory effect on the microorganism.
    The process according to the invention can be carried out according to a mode in which a fraction of the fermentation must is withdrawn from the bioreactor, step a) being carried out outside the bioreactor on said fraction and in which at least one is recycled into the bioreactor. part of the fermentation must depleted in fermentation products. Alternatively, step a) is carried out in situ in the bioreactor.
    In order to recover the fermentation products present in the gas flow, the method comprises a step c) in which the gas flow enriched in fermentation products from step a) is sent to an absorption section in which said contact is brought into contact gas flow with an organic solvent so as to recover a gas flow depleted in fermentation products and a solvent enriched in fermentation products. Advantageously, the gas stream depleted in alcohols is at least partially returned to stage b) of storage.
    According to an embodiment in which step a) is carried out directly in the bioreactor, a step cj is implemented in which the gas flow enriched in fermentative products is brought into contact with an organic solvent immiscible with water forming an organic phase supernatant the fermentation must so as to transfer at least part of the fermentation products in said solvent.
    The organic solvent can be chosen from straight or branched chain hydrocarbons, aromatic hydrocarbon compounds, carboxylic acids, alcohols or esters.
    The method according to the invention can comprise a step d) in which the solvent enriched in fermentation products is regenerated so as to separate said fermentation products and produce a regenerated solvent. Preferably, the solvent regenerated in step c) or cj is recycled.
    The process according to the invention advantageously applies to a fermentation must containing fermentation products chosen from esters, ketones, aldehydes, carboxylic acids and alcohols, alone or as a mixture. For example, the fermentation wort contains butanol, optionally mixed with acetone and / or isopropanol and ethanol.
    Preferably the gas flow used as stripping gas in step a) comprises carbon dioxide optionally in mixture with hydrogen. According to the invention, the stripping gas stream constituted by the fermentation gases can be treated before being sent to the bioreactor. The term treated designates a step making it possible to eliminate part of the compounds which constitute said gas flow. In the context of the invention, the stripping gas can include a preliminary treatment step in order to minimize its hydrogen content, for example by oxidation or by combustion of the hydrogen in an oxidizing medium (for example in the presence of air, pure oxygen, oxygen supported on a solid acting as an oxidation catalyst).
    The method according to the invention can be implemented in particular in order to recover alcohols which can be fermentation inhibiting products. For example, butanol from a threshold value of approximately 10 g / L is a fermentation inhibitor in Clostridium. According to one embodiment, step a) is only carried out when the fermentation must has a content of fermentative products which is greater than a threshold value.
    The subject of the invention is also a process for the production of fermentation products, comprising the following steps:
    i. an aqueous solution of C5 and / or C6 sugars is fermented in a bioreactor in the presence of a microorganism so as to produce a fermentation must containing fermentation products and fermentation gases;
    ii. fermentation gas produced in the bioreactor is sent to a storage unit;
    iii. the stored fermentation gases are sent under pressure to the aqueous fermentation juice so as to entrain the fermentation products in the gas flow and produce a gas flow enriched in fermentation products;
    iv. the fermentation products are separated in a gas / liquid absorption section from the gas stream enriched in fermentation products by contacting said flow with an organic solvent so as to produce a solvent enriched in fermentation products;
    v. the organic solvent enriched in fermentation products is regenerated so as to produce a flow enriched in fermentation products and a regenerated solvent.
    Steps iii) and iv) can be carried out in the bioreactor or outside the bioreactor while step v) is carried out outside the bioreactor.
    According to a preferred embodiment, the fermentation must contains butanol, optionally in admixture with acetone and / or isopropanol and ethanol.
    Preferably, the process comprises a step vi) in which a fraction of the fermentation must is sent to a section for recovery and separation of the fermentation products, said section including at least one distillation unit.
    Preferably, the stream enriched in fermentation products obtained in step v) is sent to the recovery and separation section of the fermentation products.
    The process for producing fermentation products can be applied when the microorganisms are immobilized on a support in the bioreactor.
    Detailed description of the invention
    The other characteristics and advantages of the invention will appear on reading the description which follows, given by way of illustration only and not limiting, and with reference:
    • in Figure 1 which is a block diagram of a process for the production of alcohols by fermentation of C5 and / or C6 sugars including a process for the partial recovery of alcohols by the process according to the invention;
    • in Figure 2 which shows a block diagram of a unit for separation of alcohols produced by fermentation in a bioreactor.
    Load
    The method according to the invention makes it possible to treat any fermentation must (or fermentation juice) which comprises an aqueous phase containing fermentative products and microorganisms. For example, the fermentation must may contain a mixture of alcohols having at least two carbon atoms.
    The recovery process is applicable to fermentation juices obtained from an aqueous solution of C5 and / or C6 sugars brought into contact with anaerobic microorganisms capable of converting said sugars into alcohols and / or solvents. Preferably, the process according to the invention is used to treat fermentation musts produced by microorganisms of the genus Clostridium (bacteria of the family of anaerobic gram-positive bacilli). Preferably the fermentative microorganism is chosen from the Clostridium acetobutylicum and Clostridium beijerinckii strains, natural or genetically modified capable of producing solvents of the ABE type (Acetone-Butanol-Ethanol) or of the IBE type (Isopropanol-Butanol-Ethanol).
    For these types of fermentation (ABE or IBE), the process advantageously makes it possible to extract, continuously or discontinuously, part of the alcohols / solvents of interest from the fermentation juice. The process also makes it possible to limit the content of fermentation products in the fermentation medium, the presence of which from a threshold value has the effects of inhibiting fermentation. For example, in the case of butanol, this inhibitory effect in Clostridium is observed from a content greater than 10 g / L.
    The aqueous solution of C5 and / or C6 sugars which is fermented can have different origins. It preferably comes from the treatment of a renewable source. Preferably, this source is of the lignocellulosic biomass type which comprises in particular the woody substrates (hardwoods and conifers), the by-products of agriculture (straw) or those of industries generating lignocellulosic waste (food industries, paper mills). The aqueous sugar solution can also be obtained from sugar plants, such as, for example, sugar beet and sugar cane, or also from starchy plants such as corn or wheat.
    FIG. 1 represents a diagram for the production of solvents (mixture of alcohols) from a substrate of the lignocellulosic biomass type.
    With reference to FIG. 1, a load of biomass is brought into the pretreatment unit 2 via the conduit 1. The load of biomass can be composed of wood, straw or corn cobs, crop products dedicated forests (for example of conifers such as spruces or pines, or deciduous trees such as eucalyptus), plants of dedicated cultures such as miscanthus or switchgrass, residues of alcoholic or sugar plants (for example sugar cane or beet) and cereals (for example maize, wheat, etc.), products and residues from the paper industry and products for processing lignocellulosic materials. The filler can be composed of approximately 35 to 50% by weight of cellulose, from 20 to 30% by weight of hemicellulose and from 15 to 25% by weight of lignin.
    The acidic or basic compound and the water necessary for the pretreatment are brought into the pretreatment unit 2 via conduits (not shown) in order to carry out a hydrolysis reaction therein in acidic or basic medium. In unit 2, the biomass charge is brought into contact and mixed with water and the acid or basic compound in a reactor. The pretreatment unit 2 can also implement a mechanical action, created for example by means of a twin-screw extruder or a defibrator. The acid compound for the pretreatment can be chosen from sulfuric acid, hydrochloric acid, nitric acid, acetic acid or formic acid. As for the basic compound, it can be chosen from potassium hydroxide, sodium hydroxide, ammonia.
    The pretreatment unit can implement an AFEX (Ammonia Fiber Explosion) process which consists in introducing the lignocellulosic substrate into a high pressure cooker in the presence of ammonia, then causing an explosive expansion at the outlet of the reactor and recycling the ammonia then in gaseous form. This type of process is described in particular by Teymouri et al., 2005, Biores. Technol. 96 (2005) p. 2014-2018. This process mainly leads to a destructuring of the biomass matrix but there is no phasic separation of the lignin, hemicellulose and cellulose compounds at the end of the treatment. According to a second embodiment, an acid pretreatment is carried out in unit 2. For example, it is possible to use a pretreatment of the cooking type with dilute acid. In this embodiment, the biomass is brought into contact with a strong acid diluted in water, for example sulfuric acid, using the biomass at low dry matter contents, generally between 5 and 20%. dry matter. The biomass, the acid and the water are brought into contact in a reactor and brought up to temperature, generally between 120 ° C. and 200 ° C. During this process, the hemicellulosic compounds are mainly hydrolyzed into sugars, thus making it possible to destructure the lignocellulosic matrix. At the end of this acid pretreatment, the result is the production of a solid pretreated substrate, enriched in cellulose and in lignin as well as a liquid fraction enriched in sugars.
    According to a third embodiment, it is also possible to implement the process called steam explosion, or SteamEx or Steam Explosion according to English terminology, in unit 2. It is a process in which the lignocellulosic biomass is brought into contact with water in a reactor with a short residence time, generally between 2 and 15 minutes and at moderate temperatures, generally between 120 ° C and 250 ° C and at a pressure between 0.5 and 5 MPa (5 and 50 bars). To the water can be added an acidic compound, for example sulfuric acid, or a basic compound. At the outlet of the reactor, the biomass is expanded, for example at atmospheric pressure, in a gas / solid separator container in order to produce a pretreated biomass with high dry matter, generally between 20 and 70% of dry matter.
    A substrate pretreated through line 3 is removed from the pretreatment unit 2. The pretreated substrate is composed of sugars dissolved in the liquid phase and of solid material composed of lignin, cellulose and hemicellulose which has not been liquefied in pretreatment. The pretreated substrate stream circulating in the conduit 3 preferably contains between 10% by weight and 60% by weight of dry matter and even more preferably between 20% by weight and 55% by weight of dry matter.
    The pretreated substrate is introduced into a reactor 4 to undergo a step called enzymatic hydrolysis. Water and enzymes are respectively added to reactor 4 in order to carry out an enzymatic hydrolysis reaction of the pretreated substrate. The amounts of substrate pretreated with water and of enzyme are adjusted in the hydrolysis reactor so that the reaction medium has a solid content generally between 5% and 40% by weight, preferably between 10% and 25% weight. The enzymatic hydrolysis is preferably carried out at a pH between 4 and 5.5 and at a temperature between 35 ° C and 60 ° C. The enzymes can be produced by a microorganism, for example fungi belonging to the genera Trichoderma, Aspergillus, Penicillium or Schizophyllum, or anaerobic bacteria belonging for example to the genus Clostridium. The enzymes produced by these microorganisms contain in particular cellulases and possibly hemicellulases, adapted to carry out a thorough hydrolysis of cellulose and possibly hemicelluloses. Cellulases and hemicellulases respectively transform cellulose, hemicellulose by hydrolysis, into sugars which can dissolve in the aqueous phase. In the enzymatic hydrolysis unit, the operating conditions, mainly the dry matter content of the mixture to be hydrolyzed and the quantity of enzymes used, are chosen so that a solubilization of the cellulose of between 20% is obtained. and 99% by weight, preferably between 30% and 95% by weight relative to the total weight of cellulose contained in the pretreated substrate. A hydrolyzate is removed from the hydrolysis reactor 4 via line 5. Thus the hydrolyzate 5 comprises sugars dissolved in the aqueous phase and solid matter composed mainly of lignin, and of cellulose and hemicellulose which have not been hydrolyzed.
    The hydrolyzate 5 then undergoes, in unit 6, a separation step between liquid and solid in order to extract the solid material, in particular the lignin. The separation of the solid material can use one of the following techniques: centrifugation, spinning or pressing, filtration, decantation. The unit 6 produces a liquid stream depleted in solid matter discharged through the pipe 7 and a stream enriched in solid matter, in particular lignin, discharged through the pipe 8.
    The aqueous stream depleted in solid and containing sugars C5 and / or C6 is then introduced via line 7 into a fermentation unit 9 to undergo a fermentation step. In unit 9, the aqueous stream is then brought into contact with one or more fermentation microorganisms. The microorganisms can be chosen, for example, from the following elements: yeasts of the genus Saccharomyces, Saccharomyces cerevisiae, Schizosaccharomyces pombe, Saccharomyces uvarum, Saccharomyces diastaticus, Kluyveromyces fragilis, Candida shehatae, Pichia stipitis, Pachysolen tannophilis or bacteria of the genus Zymomonas , Escherichia coli. Fermentable sugars are thus transformed into alcohols and / or solvents by microorganisms. The fermentation step in unit 9 can be carried out at a temperature between 30 ° C and 37 ° C so as to produce a fermentation must (or juice or wine) containing products of the fermentation reaction, for example alcohols and / or organic solvents, which is then evacuated via line 10.
    The fermentation wort is introduced via the conduit 10 into a separation unit 11 making it possible to separate and extract the compounds of interest from the fermentation wort, the latter being evacuated via the conduit 12. The residues of the separation, commonly called vinasses, are discharged from the separation unit 11 through the conduit 13. Vinasses are generally composed of water as well as any liquid or solid product not converted or not extracted during the preceding steps. The separation unit 11 can carry out one or more distillations, and optionally a separation of the suspended matter, for example by centrifugation, decantation, filtration.
    Preferably the fermentation process is a so-called ABE or IBE process making it possible to produce a mixture (Acetone-Butanol-Ethanol) or (Isopropanol-Butanol-Ethanol) respectively.
    In the context of the invention, the fermentation step can be implemented either according to a semi-continuous operating mode (or fed-batch according to English terminology), or according to a so-called continuous operating mode which are well known to those skilled in the art.
    It should be noted that the fermentation step can be carried out after the enzymatic hydrolysis step or even simultaneously with the hydrolysis step (fermentation of the SSF or Simultaneous Saccharification and Fermentation type according to English terminology).
    Finally, it is also possible to use a bioreactor in which the fermentative microorganisms are immobilized on a support.
    According to an alternative embodiment, the bioreactor can comprise an assembly including a first reactor coupled by a first line to a second reactor in which the fermentation microorganisms are immobilized on a support and a second line allowing the recycling of the fermentation must produced in the second reactor in the first reactor. In this embodiment, the stripping with fermentation gas is carried out at the level of the first reactor.
    As indicated in FIG. 1, the process for the production of alcohols furthermore includes a step of partial recovery of the alcohols produced present in the fermentation must (or wine). This alcohol extraction step calls for a first stripping step with a pressurized gas. As indicated in FIG. 1, a pressurized gas stored in a storage device 14 (for example a balloon) is sent by line 15 to the fermenter 9 in order to entrain the alcohols present in the aqueous phase. Generally the gas is sent under pressure to the bioreactor at a volume speed per minute of between 0.5 and 3 L / L / min. According to an important characteristic of the invention, the stripping gas is a gas produced directly by fermentation and which has been previously stored before its implementation. The stripping gas typically comprises carbon dioxide and optionally hydrogen. The recovery stage thus brings into play a gas produced in situ by the fermentation stage and therefore does not require the addition of a gas external to said process consequently limiting the operating costs (OPEX) linked in particular to the purchase and transport of make-up gas. In the context of the invention, the storage of fermentation gases can be done with one (or more) bell gasometer sealed by a water level. It is conceivable to carry out storage under pressure with prior recompression, typically up to 6 MPa (60 bars). The expansion of the gas used after storage advantageously makes it possible to compensate for part of the compression energy. Fermentation gas can also be stored in geological cavities, of the aquifer type when it contains little hydrogen, the latter having been burned, for example.
    This gas stripping step advantageously makes it possible to control during the fermentation the content of alcohols present in the medium in order to limit the phenomena of inhibition of microorganisms which appear when the content of alcohols reaches a critical value. According to the invention, this gas stripping step can either be carried out continuously or discontinuously. The fermentative gas flow rate relative to the fermenter volume is for example between 0.5 and 2.5 l / l / min, preferably between 0.7 and 1.1 l / l / min.
    Advantageously, the bioreactor contains fermentation microorganisms which are immobilized on a support so that during the stripping step, the gases are not able to entrain part of the microorganisms present in the fermentation must.
    With reference to FIG. 1, a gas stream enriched in alcohols is extracted from the fermenter 9 by line 16, then is treated in a separation step in order to recover the alcohols contained in the gas stream 16. To this end, the gas stream is sent to a solvent extraction section using at least one absorption column 17.
    The gas stream 16 is brought into contact with a solvent or a mixture of solvents supplied by the line 18, preferably against the current, so as to produce a purified gas stream with a low alcohol content 19 and a stream of solvent enriched in alcohols and low water content 20. The solvent can also contain several compounds. Preferably, the solvent used in the gas / liquid extraction step has a boiling point at least 50 ° C higher than that of the product to be recovered. The solvent can be chosen from straight or branched chain hydrocarbon compounds, aromatic hydrocarbon compounds, carboxylic acids, alcohols or esters. Among the possible solvents, mention will be made of vegetable oils (liquid from 30 ° C.), alcohols with more than eleven carbon atoms, preferably β-branched, acids with more than eleven carbon atoms, branched or not, preferably comprising one or two hydroxyl functions.
    The gas flow is brought into contact with a solvent supplied by line 18, preferably against the current, so as to produce a purified gas flow with low alcohol content 19 and a solvent flow enriched with alcohol and low content water 20.
    As indicated in FIG. 1, the purified gas stream 19 is pressurized by means of a compressor 21 and sent to the storage device 14 with a view to being again sent to the fermenter 9. As for the stream of enriched solvent in alcohols 20, it is advantageously treated in a solvent regeneration unit 22 so as to separate the alcohols from the organic phase. For example, this regeneration step can be carried out by distillation. The regeneration step produces a stream of alcohol and a stream of regenerated solvent which are discharged from the regeneration unit 22 by lines 23 and 24 respectively. The regenerated solvent is then recycled to the solvent extraction section.
    The concentrated stream of alcohols 23 which is moreover with a lower water content than the fermentation wort (typically of the order of 50% by weight) is advantageously mixed in a mixing zone 25 with the wort 10 withdrawn from the bioreactor 9 Said mixed is then treated in the alcohol separation unit 11. Compared to a conventional scheme in which only the fermentation wort is treated in the alcohol separation unit 11, the step of separating the mixture (must fermentation + concentrated alcohol flow) in the alcohol separation unit 11 requires lower energy consumption at iso-recovery rate of the alcohols produced insofar as the alcohol flow treated by said section contains a higher content low in water.
    According to another embodiment, the recovery process according to the invention can also be implemented so that the gas stripping step is carried out in a bioreactor 9 containing an organic solvent immiscible with water, the solvent forming an organic phase supernatant above the fermentation must. The solvent will also be chosen so as to be biocompatible with the microorganism.
    The stripping gas is thus injected into the fermentation must so as to entrain the alcohols produced in the supernatant organic phase and in such a way that part of the alcohols are transferred to the organic phase when the stripping gas passes through said organic phase. The stripping gas which still contains alcohols is withdrawn from the fermenter 9 and is treated in a solvent absorption unit 17 as described above. When the organic phase contained in the fermenter 9 is saturated with alcohols, it is drawn off and sent to the solvent regeneration unit 22 in order to recover the alcohols and provide a regenerated solvent which is recycled in the fermenter 9. This method of placing therefore does not require a continuous solvent regeneration loop. As regards the organic phase enriched in alcohols 20 from the absorption unit, this is advantageously regenerated in the same solvent regeneration unit 22.
    This operating mode improves the recovery of the alcohols contained in the fermentation must since the products entrained by the stripping gas are immediately brought into contact with the organic phase.
    Furthermore, when the process for recovering fermentation products according to the invention essentially aims at controlling the content of the products in the fermentation medium with a view to limiting the effects of inhibition on the microorganism, this embodiment makes it possible in particular to reduce the total time gas stripping when the amount of solvent and / or the absorption capacity and / or the selectivity of the solvent (or mixture of solvents) introduced into the bioreactor are chosen so that the threshold value of product concentration in the phase aqueous is only reached after the saturation of the organic phase.
    Figure 2 shows a block diagram of a separation unit 11 of the alcohols produced by a fermentation of the IBE type, that is to say an Isopropanol-Butanol-Ethanol mixture with optionally acetone.
    In accordance with a preferred embodiment of the process for the production of fermentation products according to the invention, the aqueous mixture 10 ′ comprising the fermentation must 10 withdrawn from the bioreactor and the stream enriched in alcohols 23 coming from the solvent regeneration unit 22 is treated in the alcohol separation unit 11. With reference to FIG. 2, the mixture 10 ′ is sent to a first distillation column 30, also called a beer column. Column 30 is designed to separate part of the water 31 contained in the mixture which is recovered at the bottom of said column. The composition of this water is such that it can partly be recycled directly upstream of the bioreactor, the other part being sent to water treatment, before it too is recycled upstream of the fermenter. At the top of column 30 is withdrawn an aqueous mixture enriched in alcohols 32 (IBE with optionally acetone). The flow recovered at the head of this first column is more concentrated in alcohols than the feed. It is for example possible to reach a concentration factor in alcohols greater than or equal to 25 (gl · 1 per gl 1 ).
    Preferably as shown in FIG. 2, the column 30 implements a reboiling system 50 by mechanical recompression of the overhead vapors. This system lowers the energy demand of this column by about 30 to 50%.
    The flow recovered at the head of this first column 30 is partly recycled in column 30 as reflux via line 33. The other part of the non-recycled flow 34 is optionally sent to a second distillation column 35. The role of this second column 35 is to separate the acetone from the flow of alcohols, the acetone being extracted at the top of column 35 via line 36, and to produce an aqueous stream concentrated in isopropanol-butanol-ethanol which is drawn off at the bottom by line 37.
    The stream 37 is then sent to a third distillation column 38 designed and operated to separate an overhead mixture 39 containing ethanol / isopropanol / water with an azeotropic composition and an aqueous bottom effluent 40 concentrated in butanol. In order to manage the demixing phenomena which may appear from a certain concentration of butanol, the column 38 is preferably equipped with one or more liquid / liquid / vapor demixing zones comprising specific internals. Alternatively, the column 38 can be operated at a slightly higher pressure in order to eliminate these demixing phenomena.
    Depending on the water content of the treated mixture 10 ′ and the water content of the azeotropic ethanol / isopropanol / water mixture 39 produced at the top of the third column 38, the water content of stream 40 is more or less high. If it is necessary to dry the aqueous stream of butanol 40, it can be treated by a heteroazeotropic distillation system.
    As shown in FIG. 2, the aqueous stream of butanol 40 is sent to a butanol demixing unit in order to recover the butanol. To this end, the aqueous stream of butanol is cooled, for example to a temperature of 60 ° C. in a separator flask 41 in order to demix the mixture into two phases, namely an organic phase containing essentially butanol (for example at least 70% butanol weight) and an aqueous phase.
    The two phases are treated in a heteroazeotropic distillation system which comprises two columns 42, 43 operating in parallel. The organic phase mainly containing butanol is sent via line 44 to the heteroazeotropic distillation column 42 which operates, for example, at a pressure between 0.3 and 10 MPa and at a temperature between 115 and 150 ° C in order to avoid liquid-liquid-vapor demixing problems. An effluent having a mass content of at least 99% butanol at the bottom of said column 42 is drawn off and at the head, via line 46, an aqueous effluent which is returned to the separator flask 41.
    The aqueous phase still containing butanol, which is withdrawn from the biphasic separator flask 41 by line 47 in the heteroazeotropic distillation column 43. From said column 43 is recovered respectively at the bottom a stream rich in water 48 and at the top an effluent containing butanol which is recycled, via line 49, to the two-phase separator flask 41. Column 43 is operated under less severe conditions, for example at a pressure lower than that of column 42.
    Example
    The example below is constructed by simulation using design software and operational process analysis (Simsci Pro / ll) which integrates results from laboratory tests and from the literature concerning fermentation using microorganisms from the genus Clostridium.
    For simulation, it was assumed that the fermentation production unit implements a fermentation unit comprising ten fermenters which processes an aqueous solution of glucose at 50 g / L. The total volume of the fermentation unit is 10 * 500 m 3 and with a total useful volume of 10 * 400 m 3 . Based on the assumption that the total productivity is 0.54 g / l / h of solvent with a weight percentage distribution in Isopropanol / Butanol / Ethanol: 28% / 62% / 10%). The production unit thus produces 17,000 t / year of IBE mixture, or approximately 4,800 t / year of isopropanol, 10,560 t / year of butanol and 1,600 t / year of ethanol.
    The sugar consumption of the plant is about 53,000 t / year of glucose assuming a yield of 0.32 g of IBE / g of sugar
    The fermenters operate at 37 ° C. in a batch mode for 34 hours, then inhibition by butanol is achieved.
    The final composition of the fermentation wort from the fermenters is as follows: 4.8 g / l of isopropanol, 10.5 g / l of butanol and 1.7 g / l of ethanol, or approximately 17 g / l of IBE products in fermentation must.
    On the assumption that the energy required for the separation of the alcohols contained in the fermentation must on the one hand and to separate the butanol from the isopropanol + ethanol mixture (directly recoverable in petrochemicals) on the other hand is approximately 20 MJ / kg of IBE mixture, the steam consumption is estimated to be approximately 150,000 t / year of vapor (ie approximately 8.81 of vapor / t of IBE mixture.
    The natural fermentation process releases 12,000 Nm 3 / h assuming that the gas flow rate (in liters per minute) relative to the volume of the fermenter (in liters) is 0.05 l / l / min of gas which is a mixture essentially comprising CO 2 and H 2 which is not used as a stripping gas.
    Example according to the invention
    The method according to the invention is implemented in the same unit described above which comprises ten IBE fermenters.
    Fermenters are subjected to stripping with fermentation gas when the concentration of inhibitory metabolite of butanol in the fermentation medium is less than 80% of the inhibition threshold (fixed at 10 g / l of butanol). The stripping is carried out with a gas flow rate (in liters per minute) relative to the volume of the fermenter (in liters) of 1 l / l / min, or 240,000 Nm3 / h of fermentation gas. This fermentation gas was previously stored, for example from the start of fermentation in order to have a sufficient volume.
    In order to limit the phenomenon of jerks during the injection of the fermentation gas for stripping, it is preferable to have a reserve of fermentation gas which is equivalent to at least 3 minutes of injection for a given flow rate.
    Fermentation gas continues to be produced at a flow rate of 12,000 Nm3 / h and is stored at the storage unit and optionally purged when the fermentation gas is in excess of the quantity required for stripping. The fermentation stripping gas containing the alcohols is sent to an alcohol separation unit which uses said gas to contact with a liquid vegetable oil at 37 ° C. (for example rapeseed, palm or sunflower). The effluents produced by the alcohol separation stage are a vegetable oil loaded with alcohols and a fermentation gas depleted in alcohols. The latter is advantageously recycled as stripping gas. The vegetable oil containing the alcohols produced is sent to a vacuum distillation column so as not to thermally degrade the oil. At the bottom of this column, the purified oil of the alcohols is recovered and at the head an aqueous mixture of alcohols. This concentrated alcohol flow is ultimately mixed with the must remaining in the fermenters at the end of fermentation.
    The extraction by stripping with the fermentation gas of the most inhibiting product, that is to say in the present case butanol, has several effects:
    1. On productivity
    Given that the most inhibitory metabolite of the fermenting must is eliminated over time, the Clostridium strain increases its overall productivity, which is around 0.94 g of IBE / l / h. It is then possible to produce approximately 30,000 t / year of IBE mixture, ie approximately 7,300 t / year of isopropanol, 20,500 t / year of butanol and 2,200 t / year of ethanol. We increase the production of the unit by about 75%.
    2. On performance
    We need less relative sugar to increase production. The yield is estimated at 0.4 g IBE / g glucose (i.e. a 25% increase in yield), which implies a consumption of 75,000 t / year of glucose.
    3. Separation energy
    The final fermentation must still contains approximately 17 g / l of IBE mixture, with approximately 4 g / L of isopropanol, 11.6 g / l of butanol and 1.4 g / l of ethanol. However, 90% of the alcohols produced are recovered by the stages of stripping, contacting with a solvent and regeneration of the solvent. Sending the alcohols from the regeneration stage into the final must recovered from the fermenters makes it possible to significantly reduce the energy costs associated with the final separation of the butanol. Thus taking into account the energy of distillation of vegetable oil on the one hand (2 MJ / kg of IBE mixture) and the separation of butanol from the isopropanol + ethanol mixture (5 MJ / kg of IBE mixture) on the other hand On the other hand, steam consumption is estimated at around 93,000 t / year of steam, or around 3.1 t steam / t of IBE mixture, resulting in an energy reduction of around 65%.
    4. Extension of cycle time
    Due to the lifting of inhibition by eliminating the butanol from the must, the fermentations can be carried out in fed-batch or continuous mode, which has the advantage of extending the operating time by approximately 500 hours.
    权利要求:
    Claims (17)
    [1" id="c-fr-0001]
    1. Method for recovering fermentative products present in a fermentation must produced in a bioreactor, comprising a step a) in which a gaseous flow under pressure is sent into the fermentation must so as to entrain at least part of the products and produce a gas stream enriched in fermentation products, characterized in that the process comprises a step b) of storing the fermentation gases produced in the bioreactor and in that the gaseous stream which is sent to step a) consists of the gases of stored fermentation.
    [2" id="c-fr-0002]
    2. Method according to claim 1, in which a fraction of the fermentation must is withdrawn from the bioreactor, step a) is carried out outside the bioreactor on said fraction of the fermentation must and in which at least one is recycled into the bioreactor. part of the fermentation must depleted in fermentation products.
    [3" id="c-fr-0003]
    3. Method according to claim 1, wherein step a) is carried out directly in the bioreactor.
    [4" id="c-fr-0004]
    4. Method according to one of the preceding claims, comprising a step c) in which the gas stream enriched in fermentation products from step a) is sent to a gas / liquid absorption section in which said contact is brought into contact gas flow with an organic solvent so as to produce a solvent enriched in fermentation products and a gas flow depleted in fermentation products.
    [5" id="c-fr-0005]
    5. Method according to claim 3, comprising a step cj carried out in the bioreactor, in which the gas stream enriched in fermentation products is brought into contact with an organic solvent immiscible with water forming an organic phase supernatant the fermentation must of so as to transfer at least part of the fermentation products into said solvent.
    [6" id="c-fr-0006]
    6. Method according to claims 4 or 5, comprising a step d) in which the solvent enriched in fermentation products is regenerated so as to separate said fermentation products and produce a regenerated solvent.
    [7" id="c-fr-0007]
    7. Method according to one of the preceding claims, in which the fermentation must contains fermentation products chosen from esters, ketones, aldehydes, carboxylic acids and alcohols, alone or as a mixture.
    [8" id="c-fr-0008]
    8. The method of claim 7, wherein the fermentation must contains butanol, optionally in admixture with acetone and / or isopropanol and ethanol.
    [9" id="c-fr-0009]
    9. Method according to one of the preceding claims, wherein the gas stream comprises carbon dioxide optionally in admixture with hydrogen.
    [10" id="c-fr-0010]
    10. Method according to one of the preceding claims, in which the gas flow is treated before being sent to the bioreactor.
    [11" id="c-fr-0011]
    11. Method according to one of claims 4 to 10, in which the organic solvent is chosen from straight or branched chain hydrocarbons, aromatic hydrocarbon compounds, carboxylic acids, alcohols or esters.
    [12" id="c-fr-0012]
    12. Process for the production of fermentation products, comprising the following steps:
    i. an aqueous solution of C5 and / or C6 sugars is fermented in a bioreactor in the presence of a microorganism so as to produce a fermentation must containing fermentative products and fermentation gases;
    ii. fermentation gas produced in the bioreactor is sent to a storage unit;
    iii. the stored fermentation gases are sent under pressure to the aqueous fermentation juice so as to entrain the fermentation products in the gas flow and produce a gas flow enriched in fermentation products;
    iv. the fermentation products are separated in a gas / liquid absorption section from the gas stream enriched in fermentation products by contacting said flow with an organic solvent so as to produce a solvent enriched in fermentation products;
    v. the organic solvent enriched in fermentation products is regenerated so as to produce a flow enriched in fermentation products and a regenerated solvent.
    [13" id="c-fr-0013]
    13. The method of claim 12, wherein steps iii) and iv) are performed in the bioreactor or outside the bioreactor and wherein step v) is performed outside the bioreactor.
    [14" id="c-fr-0014]
    14. Method according to one of claims 12 to 13, wherein the fermentation must contains butanol, optionally in admixture with acetone and / or isopropanol and ethanol.
    [15" id="c-fr-0015]
    15. Method according to one of claims 12 to 14, further comprising a step vi) in which a fraction of the fermentation must is sent to a section for recovering and separating fermentation products, said section including at least one distillation unit .
    [16" id="c-fr-0016]
    16. The method of claim 15, wherein the stream enriched in fermentative products obtained in step v) is sent as a mixture with the fermentation wort fraction.
    5 in the recovery and separation section of fermentation products.
    [17" id="c-fr-0017]
    17. Method according to one of claims 12 to 16, wherein the microorganisms are immobilized on a support in the bioreactor.
    1/2
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    同族专利:
    公开号 | 公开日
    EP3478815A1|2019-05-08|
    US10961489B2|2021-03-30|
    CA3028837A1|2018-01-04|
    FR3053357B1|2019-07-26|
    CN109477049A|2019-03-15|
    BR112018074955A2|2019-04-16|
    WO2018001628A1|2018-01-04|
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    引用文献:
    公开号 | 申请日 | 公开日 | 申请人 | 专利标题
    FR2974116A1|2011-04-14|2012-10-19|IFP Energies Nouvelles|PROCESS FOR THE PRODUCTION OF ETHANOL AND SOLVENTS FROM LIGNOCELLULOSIC BIOMASS WITH RECYCLING OF BUTYLIC WINE OBTAINED BY FERMENTATION OF PENTOSES|
    FR3023300A1|2014-07-01|2016-01-08|IFP Energies Nouvelles|IBE FERMENTATION PROCESS|
    GB0818093D0|2008-10-02|2008-11-05|Weyland As|Method|
    US20150087040A1|2013-09-26|2015-03-26|E I Du Pont De Nemours And Company|Production of ethanol and recycle water in a cellulosic fermentation process|CN109486868A|2017-09-09|2019-03-19|中国石油化工股份有限公司|A method of isopropanol and butanol are produced by fermenting raw materials of lignocellulosic|
    EP3703952A4|2018-03-09|2021-06-30|Hewlett-Packard Development Company, L.P.|Thermal sense monitors for fluid ejection dies|
    FR3111914A1|2020-06-29|2021-12-31|IFP Energies Nouvelles|IBE FERMENTATION PROCESS OPTIMIZED TO RECOVER ACETONE|
    法律状态:
    2017-06-22| PLFP| Fee payment|Year of fee payment: 2 |
    2018-01-05| PLSC| Publication of the preliminary search report|Effective date: 20180105 |
    2018-06-27| PLFP| Fee payment|Year of fee payment: 3 |
    2020-06-26| PLFP| Fee payment|Year of fee payment: 5 |
    2021-06-25| PLFP| Fee payment|Year of fee payment: 6 |
    优先权:
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    FR1656209A|FR3053357B1|2016-06-30|2016-06-30|PROCESS FOR RECOVERING ALCOHOLS IN A FERMENTER|
    FR1656209|2016-06-30|FR1656209A| FR3053357B1|2016-06-30|2016-06-30|PROCESS FOR RECOVERING ALCOHOLS IN A FERMENTER|
    CA3028837A| CA3028837A1|2016-06-30|2017-05-17|Process for the recovery of alcohols in a fermenter|
    US16/314,209| US10961489B2|2016-06-30|2017-05-17|Process for recovering alcohols in a fermenter|
    BR112018074955-9A| BR112018074955A2|2016-06-30|2017-05-17|alcohol recovery process in a fermenter|
    CN201780040727.4A| CN109477049A|2016-06-30|2017-05-17|The method of alcohol is recycled in the fermenter|
    EP17723132.1A| EP3478815A1|2016-06-30|2017-05-17|Process for the recovery of alcohols in a fermenter|
    PCT/EP2017/061801| WO2018001628A1|2016-06-30|2017-05-17|Process for the recovery of alcohols in a fermenter|
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