WO2010151706A1 - Integrated system and process for bioproduct production - Google Patents

Integrated system and process for bioproduct production Download PDF

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Publication number
WO2010151706A1
WO2010151706A1 PCT/US2010/039873 US2010039873W WO2010151706A1 WO 2010151706 A1 WO2010151706 A1 WO 2010151706A1 US 2010039873 W US2010039873 W US 2010039873W WO 2010151706 A1 WO2010151706 A1 WO 2010151706A1
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Prior art keywords
hydrolysis
feedstock
bioreactor
stage
fermentation
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PCT/US2010/039873
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English (en)
French (fr)
Inventor
David C. Walther
Hendrik J. Meerman
Stacy M. Burns-Guydish
Richard W. Wilson
Eamon T. Hogg
Gregory W. Luli
Robert Eckert
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Cobalt Technologies, Inc.
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Priority to EP10792688.3A priority Critical patent/EP2446044A4/en
Priority to IN685DEN2012 priority patent/IN2012DN00685A/en
Priority to CA2804912A priority patent/CA2804912A1/en
Priority to AU2010266035A priority patent/AU2010266035B2/en
Priority to RU2011153546/10A priority patent/RU2011153546A/ru
Priority to CN2010800377718A priority patent/CN102482690A/zh
Priority to BRPI1010056A priority patent/BRPI1010056A2/pt
Priority to MX2011013974A priority patent/MX2011013974A/es
Publication of WO2010151706A1 publication Critical patent/WO2010151706A1/en

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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12MAPPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
    • C12M21/00Bioreactors or fermenters specially adapted for specific uses
    • C12M21/12Bioreactors or fermenters specially adapted for specific uses for producing fuels or solvents
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12MAPPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
    • C12M23/00Constructional details, e.g. recesses, hinges
    • C12M23/58Reaction vessels connected in series or in parallel
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12MAPPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
    • C12M25/00Means for supporting, enclosing or fixing the microorganisms, e.g. immunocoatings
    • C12M25/16Particles; Beads; Granular material; Encapsulation
    • C12M25/18Fixed or packed bed
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12MAPPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
    • C12M25/00Means for supporting, enclosing or fixing the microorganisms, e.g. immunocoatings
    • C12M25/16Particles; Beads; Granular material; Encapsulation
    • C12M25/20Fluidized bed
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12MAPPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
    • C12M43/00Combinations of bioreactors or fermenters with other apparatus
    • C12M43/02Bioreactors or fermenters combined with devices for liquid fuel extraction; Biorefineries
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12MAPPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
    • C12M45/00Means for pre-treatment of biological substances
    • C12M45/06Means for pre-treatment of biological substances by chemical means or hydrolysis
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12MAPPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
    • C12M47/00Means for after-treatment of the produced biomass or of the fermentation or metabolic products, e.g. storage of biomass
    • C12M47/10Separation or concentration of fermentation products
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12PFERMENTATION OR ENZYME-USING PROCESSES TO SYNTHESISE A DESIRED CHEMICAL COMPOUND OR COMPOSITION OR TO SEPARATE OPTICAL ISOMERS FROM A RACEMIC MIXTURE
    • C12P7/00Preparation of oxygen-containing organic compounds
    • C12P7/02Preparation of oxygen-containing organic compounds containing a hydroxy group
    • C12P7/04Preparation of oxygen-containing organic compounds containing a hydroxy group acyclic
    • C12P7/06Ethanol, i.e. non-beverage
    • C12P7/065Ethanol, i.e. non-beverage with microorganisms other than yeasts
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12PFERMENTATION OR ENZYME-USING PROCESSES TO SYNTHESISE A DESIRED CHEMICAL COMPOUND OR COMPOSITION OR TO SEPARATE OPTICAL ISOMERS FROM A RACEMIC MIXTURE
    • C12P7/00Preparation of oxygen-containing organic compounds
    • C12P7/02Preparation of oxygen-containing organic compounds containing a hydroxy group
    • C12P7/04Preparation of oxygen-containing organic compounds containing a hydroxy group acyclic
    • C12P7/16Butanols
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12PFERMENTATION OR ENZYME-USING PROCESSES TO SYNTHESISE A DESIRED CHEMICAL COMPOUND OR COMPOSITION OR TO SEPARATE OPTICAL ISOMERS FROM A RACEMIC MIXTURE
    • C12P7/00Preparation of oxygen-containing organic compounds
    • C12P7/24Preparation of oxygen-containing organic compounds containing a carbonyl group
    • C12P7/26Ketones
    • C12P7/28Acetone-containing products
    • YGENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
    • Y02TECHNOLOGIES OR APPLICATIONS FOR MITIGATION OR ADAPTATION AGAINST CLIMATE CHANGE
    • Y02EREDUCTION OF GREENHOUSE GAS [GHG] EMISSIONS, RELATED TO ENERGY GENERATION, TRANSMISSION OR DISTRIBUTION
    • Y02E50/00Technologies for the production of fuel of non-fossil origin
    • Y02E50/10Biofuels, e.g. bio-diesel
    • YGENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
    • Y02TECHNOLOGIES OR APPLICATIONS FOR MITIGATION OR ADAPTATION AGAINST CLIMATE CHANGE
    • Y02PCLIMATE CHANGE MITIGATION TECHNOLOGIES IN THE PRODUCTION OR PROCESSING OF GOODS
    • Y02P20/00Technologies relating to chemical industry
    • Y02P20/50Improvements relating to the production of bulk chemicals
    • Y02P20/582Recycling of unreacted starting or intermediate materials

Definitions

  • TWs application claims the benefit of U.S. provisional application nos. 61/221,007, filed June 26, 2009, 61/221,474, filed June 29, 2009, and 61/278,932, filed October 13, 2009, all of which are incorporated herein by reference in their entireties.
  • the invention relates to production of a bioproduct, such as biobutanol, in a continuous microbial fermentation process.
  • Butanol is a high quality fuel and fuel additive. Butanol can be mixed, stored and transported together with gasoline. It has more energy per gallon than ethanol, which translates into better fuel economy for consumers using butanol blends, and has lower vapor pressure than ethanol, which translates into less ground level pollution. Butanol's low vapor pressure makes it an attractive low volatility, oxygenated, blend component for refiners to use in complying with stringent vapor pressure specifications. Butanol can provide the oxygenate benefits of ethanol but without undue evaporative emissions, which are a significant source of air pollution, and at a potentially lower cost. Butanol is also more hydrophobic than ethanol, i. e.
  • butanol should be a highly desired component of Reformulated Gasoline Blendstock for Oxygenate Blending (RBOB) and California (CARBOB) fuel blendstock. Butanol is also expected to have a reduced life cycle emission of CO 2 . Butanol blends should have no detrimental effects on modern fuel system elastomers, and corrosion and electrical conductivity are expected to be similar to gasoline. [04] Butanol can also be blended in concentrations in excess of 20% with diesel fuel. The benefits of addition of oxygenates to diesel fuel include the reduction in soot formation, CO, and unburned hydrocarbon emissions.
  • butanol is also widely used as an industrial chemical. It is used in the production of paints, plasticizers, and pesticides, as an ingredient in contact lens cleansers, cement, and textiles, and also as a flavoring in candy and ice cream.
  • the global market for n-butanol was approximately 1 billion gallons in 2006, the U S market was approximately 300 million gallons, and is expected to grow approximately 2% per year
  • Butanol is currently made from petroleum Production costs are high and margins are low, and price trends generally track the price of oil and are heavily influenced by global economic growth
  • a process for producing a bioproduct including continuously fermenting a microorganism in the presence of hydrolyzed feedstock of a carbohydrate-containing material
  • the microorganism is immobilized on a support m
  • Hydrolyzed feedstock is produced by hydrolysis of the feedstock, which produces carbohydrate molecules that serve as a carbon source for the microbial fermentation
  • the microorganism contmuously converts the hydrolyzed feedstock mto a bioproduct
  • the feedstock is hydrolyzed continuously upstream from the bioreactor and the resultmg hydrolyzed feedstock is fed continuously to the bioreactor for the duration of the fermentation
  • the bioproduct is a biofuel (e g , butanol, acetone, ethanol)
  • the bioproduct is a biochemical or a biochemical feedstock, i e , a biochemical that may be de ⁇ va
  • the hydrolyzed feedstock is fed continuously mto multiple bioreactors arranged in parallel and/or m se ⁇ es, the fermentation occurs continuously m the multiple bioreactors, and the multiple bioreactors contain the same or different microorganism(s)
  • the hydrolyzed feedstock is fed continuously mto multiple bioreactors arranged m parallel, the fermentation occurs continuously m the multiple bioreactors, and the multiple bioreactors contain the same or different microorganism(s)
  • the fermentation occurs continuously in multiple bioreactors that are arranged m se ⁇ es, the hydrolyzed feedstock is fed continuously into the first bioreactor in the se ⁇ es, and effluent from each bioreactor is fed to the next bioreactor downstream in the series
  • evolved gas may be removed between senes nodes during operation of the bioreactors
  • bioreactors are arranged in parallel trains in a hybrid series/parallel arrangement
  • fermentation may proceed in multiple bioreactors that are arranged in a combination to optimize productivity, such as a primary reactor arranged in senes with a tram of parallel reactors, with hydrolyzed feedstock fed continuously into the first bioreactor in the senes and effluent from each bioreactor fed to the next bioreactor downstream in the senes
  • the duration of the fermentation is at least about 300 hours
  • the duration of the fermentation is at least about 1000 hours
  • the feedstock is a cellulosic material, for example, a lignocellulosic material
  • the feedstock contains cellulose and hemicellulose, e g , lignocellulosic material or wood pulp
  • the feedstock is wood selected from softwood, hardwood, or a combination thereof
  • the feedstock is a lignocellulos
  • the acid includes nitric acid, formic acid, acetic acid, phosphoric acid, hydrochloric acid, or sulfuric acid, or a combination thereof.
  • the hydrolysis is performed with nitric acid.
  • the hydrolysis is performed with a combination of nitric acid and acetic acid, hi some embodiments, the feedstock contains acetyl groups and releases acetic acid, resulting in autohydrolysis of hemicellulose, which may then release more acetic acid. This autohydrolysis may be supplemented by addition of a mineral acid, or the amount of mineral acid required for hydrolysis of the feedstock may be reduced by "leveraging" the natural acetyl content in the feedstock..
  • hydrolysis of a lignocellulosic feedstock is performed with nitric acid in a process including a first stage and a second stage, with the second stage hydrolysis performed at a higher temperature than the first stage, hi some embodiments, performing hydrolysis at a higher temperature in the second stage decreases or prevents degradation of a desired intermediate product (e.g., monomeric sugar molecules).
  • the conditions in the first stage are chosen to achieve hydrolysis of at least about 70% of the hemicellulose in the feedstock, and the conditions in the second stage are chosen to achieve hydrolysis of at least about 40% of the cellulose in the feedstock.
  • the feedstock is a hardwood, the first stage hydrolysate comprises at least about 60% 5-carbon sugar and at least about 25% 6-carbon sugar, and the second stage hydrolysate comprises at least about 80% 6-carbon sugar.
  • the feedstock is a softwood, the first stage hydrolysate comprises at least about 20% 5-carbon sugar and at least about 70% 6-carbon sugar, and the second stage hydrolysate comprises at least about 90% 6-carbon sugar.
  • lignin is recovered in the residue of the terminal stage, e.g. , second stage, of hydrolysis of lignocellulosic feedstock.
  • the lignin-containing residue is dried to a liquid content of about 15% or less, hi some embodiments, the lignin-containing residue is dried to a liquid content of about 35% to about 15%, e.g., any of about 35%, 30%, 25%, 20%, or 15%, or about 35% to about 30%, about 30% to about 25%, about 25% to about 20%, or about 20% to about 15%.
  • the lignin-containing residue is used as an energy source for said process.
  • the lignin-containing residue is used as a fuel source for electricity generation.
  • the lignin-containing residue is used as a chemical precursor for production of useful products, such as phenolic resins.
  • the lignin-containing residue is used as a feed to an anaerobic digestor for production of useful gaseous products, such as methane or syngas (CO + CH 4) .
  • the lignin-containing residue is used as a soil enhancer.
  • hydrolysis of a feedstock, e g , lignocellulosic feedstock is performed with an acid, e g , nitric acid, in multiple stages including a first and a second stage, and the multiple, e g , first and second, stage hydrolysates are combmed prior to mtroduction into the bioreactor
  • multiple, e g , first and second, stage hydrolysates are introduced as separate hydrolyzed feedstock streams into separate bioreactors
  • the first stage hydrolysate is introduced mto a first bioreactor and the second stage hydrolysate is introduced into a second bioreactor, where the first and second bioreactors contain the same or different microorganism(s)
  • the first bioreactor comprises a first microorganism and the second bioreactor comprises a second microorganism, the first and second microorganisms are different, the first microorganism is optimized for growth and/
  • hydrolysis of a feedstock, e g , lignocellulosic feedstock is performed with an acid, e g , nitric acid, in multiple stages including a first stage and a second stage, the first stage hydrolysis occurs m a first hydrolysis module and the second stage hydrolysis occurs m a second hydrolysis module, the resulting second stage hydrolysate is re-introduced into the first hydrolysis module to produce a third hydrolysate, and the amount of soluble sugar molecules m the third hydrolysate is greater than the amount of soluble sugar molecules m the second stage hydrolysate
  • hydrolysis of a feedstock, e g , lignocellulosic feedstock is performed with an acid, e g , nitric acid, in multiple stages including a first stage and a second stage, flash steam is generated in the first stage hydrolysis, and the flash steam is used to deconstruct the feedstock prior to hydrolysis
  • flash steam is generated in the second stage hydrolysis, and the flash steam is used to deconstruct said feedstock prior to hydrolysis and/or to provide energy for the first stage hydrolysis
  • flash steam is generated in the second stage hydrolysis, the flash steam is recompressed, and the recompressed steam is used to provide energy for the first stage hydrolysis and/or other applications such as, for example, a downstream distillation process for product purification, such as steam stripping distillation
  • flash steam is generated in the second stage hydrolysis, the flash steam is used to provide energy for a third stage hydrolysis, the temperature of the third stage hydrolysis is lower than the temperature
  • removal of inhibitors is performed by contact of hydrolyzed feedstock with an ion exchange resin under conditions such that the inhibitors are retained on the resin.
  • the ion exchange resin is an anion exchange resin.
  • removal of inhibitors is performed by precipitation with a metal salt, such as an aluminum or iron salt, for example, aluminum sulfate or ferric chloride.
  • the inhibitors include organic acids, furans, phenols, soluble lignocellulosic materials, extractives , and/or ketones.
  • fermentation of the immobilized microorganism is conducted under anaerobic conditions.
  • the microorganism is a Clostridium strain
  • the Clostridium strain is derived from a species selected from Clostridium saccharobutylicum, Clostridium saccharoperbutylacetonicum, Clostridium acetobutylicum, and Clostridium beijerinckii.
  • the Clostridium strain is an environmental isolate or is derived from an environmental isolate.
  • the Clostridium strain possesses one or more phenotypic characteristics selected from butanol tolerance, tolerance to inhibitors of fermentation, low acid accumulation, stability in continuous fermentation, high butanol titer, production of biofuel with high butanol to acetone ratio, increased yield of butanol per unit of feedstock, increased yield of butanol per unit of cellular biomass, increased oxygen tolerance, increased ability to adhere to a solid support, and decreased ability to sporulate, relative to a wild- type or parent strain from which the Clostridium strain is derived, or Clostridium saccharobutylicum B643, Clostridium saccharobutylicum P262, Clostridium sacchroperbutylacetonicum Nl -4, Clostridium acetobutylicum 824, or Clostridium beijerinckii 8524, grown under identical conditions.
  • phenotypic characteristics selected from butanol tolerance, tolerance to inhibitors of fermentation, low acid accumulation, stability in continuous fermentation, high butano
  • the support material on which the microorganism is immobilized is selected from bone char, polypropylene, steel, diatomaceous earth, zeolite, ceramic, engineered thermal plastic, clay brick, concrete, lava rock, wood chips, polyester fiber, glass beads, Teflon, polyetheretherketone, and polyethylene.
  • the immobilized microorganism includes a biofilm.
  • the bioreactor in which the immobilized microorganism is grown is in the form of a packed bed, an expanded bed, or a fluidized bed.
  • the bioproduct produced in the process includes a biofuel, such as butanol, acetone, ethanol, or a combination thereof hi one embodiment, the biofuel includes butanol In one embodiment, butanol is produced by a Clostridium strain
  • the process further includes recovery of the bioproduct, e g , biofuel, from the fermentation medium hi some embodiments, the recovery process operates continuously for the duration of the fermentation In some embodiments, the recovery process includes concentration of the bioproduct In one embodiment, concentration of the bioproduct includes mechanical vapor recompression
  • the process further includes distillation to separate the bioproduct, e g , a biofuel, such as butanol, from other components of the fermentation medium
  • flash steam generated during hydrolysis of the feedstock provides energy for the distillation hi one embodiment
  • butyric acid is recovered m the distillation
  • the butyric acid is added to the fermentation medium in the bioreactor
  • the microorganisms m the bioreactor convert the butyric acid to butanol hi one embodiment
  • the bioproduct is butanol
  • butyric acid is recovered m the distillation
  • the butyric acid is recycled back to the fermentation medium in the bioreactor
  • the microorganisms in the bioreactor convert the butyric acid to butanol
  • hydrolysis of a feedstock, e g , hgnocellulosic feedstock is performed with an acid, e g , nitric acid, in multiple stages including a first stage and a second stage, the second
  • a system for production of a bioproduct includes a feedstock hydrolysis unit and a bioreactor A carbon-containing feedstock is hydrolyzed in the hydrolysis unit The hydrolyzed feedstock is continuously fed to a microbial growth medium m the bioreactor, which contains a fermenting microorganism immobilized on a support hi some embodiments, the feedstock hydrolysis unit and the bioreactor are in fluid communication, the hydrolysis unit is upstream from the bioreactor, and the feedstock is continuously hydrolyzed and continuously fed to the bioreactor for the duration of the fermentation Hydrolysis of the feedstock produces carbohydrate molecules that serve as a carbon source for the fermentation, and the microorganism continuously converts the hydrolyzed feedstock into a bioproduct hi one embodiment, the bioproduct is a biofuel (e g , butanol, acetone, ethanol) In other embodiments, the bioproduct is a biochemical or a biochemical feedstock, i e , a biochemical
  • the system contains multiple bioreactors arranged m parallel, the multiple bioreactors are in fluid communication with the hydrolysis unit, the hydrolyzed feedstock is fed continuously into the bioreactors, the fermentation of the microorganism occurs continuously m the bioreactors, and the multiple bioreactors contain the same or different microorganism(s) [32]
  • the system contains multiple bioreactors arranged m series, the first bioreactor in the series is in fluid communication with the hydrolysis unit and with a downstream bioreactor, each subsequent bioreactor m the series downstream from the first bioreactor is in fluid communication with the previous upstream bioreactor in the series, the hydrolyzed feedstock is fed contmuously into the first bioreactor in the series, and effluent from each bioreactor is fed to the next bioreactor downstream in the series
  • evolved gas may be removed between series nodes during operation of the bioreactors
  • bioreactors are arranged in parallel trains in a hybrid series/parallel arrangement
  • fermentation may proceed m multiple bioreactors that are arranged in a combination to optimize productivity, such as a primary reactor arranged in series with a train of parallel reactors with hydrolyzed feedstock fed continuously mto the first bioreactor m the series and effluent from each bioreactor fed to the next bioreactor downstream in the se ⁇ es
  • continuous hydrolysis and fermentation, and optionally conditioning and/or product recovery operate continuously in the system for at least about 300 hours
  • continuous hydrolysis and fermentation operate continuously in the system for at least about 1000 hours
  • the feedstock is a cellulosic matenal, for example, a lignocellulosic material
  • the feedstock is wood selected from softwood, hardwood, or a combmation thereof
  • the feedstock is a lignocellulosic material in the form of wood chips, sawdust, saw mill residue, or a combination thereof
  • the lignocellulosic material (e g , wood chips sawdust, saw mill residue, or a combination thereof) is from a feedstock source that has been subjected to some form of disease in the growth and/or harvest production pe ⁇ od
  • the feedstock source is mountain pine beetle infested pine
  • the feedstock source is sudden oak death syndrome infested oak, e g , coastal live oak, tanoak, etc
  • the feedstock source is Dutch elm disease infested elm
  • the feedstock is a cellulosic matenal, for example, a lignocellulos
  • lignocellulosic feedstock material is deconstructed prior to hydrolysis
  • Deconstruction may include one or more process selected from presteaming, mechanical grinding, and mechanical explosion
  • the feedstock material is deconstructed p ⁇ or to harvest by a natural or non-natural environmental condition, for example, drought, infestation, fire, and/or herbicide exposure
  • the feedstock material may be deconstructed by a disease organism, for example, mountain pine beetle deconstruction of pine
  • lignocellulosic feedstock material is pretreated to remove extractives
  • the extractive removal pretreatment may include compression, water extraction, solvent extraction, alkaline extraction, enzymatic treatment, fungal treatment, oxygen treatment, or air drying
  • the pretreatment to remove extractives may occur prior to or in conjunction with deconstruction
  • hydrolysis of a feedstock is performed by treatment with an acid
  • the acid includes nitric acid, formic acid, acetic acid, phosphoric acid, hydrochloric acid, or sulfuric acid, or a combination thereof
  • the hydrolysis is performed with nitric acid hi another embodiment, the hydrolysis is performed with a combination of nitric acid and acetic acid
  • the hydrolysis is performed with nitric acid
  • the hydrolysis reactor contains stainless steel
  • the hydrolysis reactor contains hastelloy or zirconium
  • hydrolysis is performed in multiple stages in the same or different hydrolysis reactor module(s)
  • the hydrolysis unit contains a first hydrolysis module and a second hydrolysis module, acid, e g , nitric acid, hydrolysis of a feedstock, e g , lignocellulosic feedstock, is performed in multiple stages, including a first stage in the first hydrolysis module and a second stage in the second hydrolysis module, and the temperature of the nitric acid in the first hydrolysis module is higher than the temperature of the nitric acid m the second hydrolysis module
  • the hydrolysis product stream from the second hydrolysis module is re-introduced into the first hydrolysis module to produce a third hydrolysate, and the amount of soluble sugar molecules produced in the third hydrolysate is greater than the amount of soluble sugar molecules m the second stage hydrolysate
  • the hydrolysis product streams from multiple, e g , first and second, hydrolysis modules are combmed prior to introduction into the bioreactor
  • the hydrolysis product streams from multiple, e g , first and second, hydrolysis modules are introduced as separate hydrolyzed feedstock streams mto separate bioreactors.
  • the first stage hydrolysate is introduced into a first bioreactor and the second stage hydrolysate is introduced into a second bioreactor, and the first and second bioreactors contain the same or different microorganism(s).
  • the first bioreactor contains a first microorganism and the second bioreactor contains a second microorganism, the first and second microorganisms are different, and the first microorganism is optimized for growth on the first stage hydrolysate and the second microorganism is optimized for growth on the second stage hydrolysate.
  • the system contains multiple first bioreactors in series and/or multiple second bioreactors in series.
  • hydrolysis of a feedstock, e g , lignocellulosic feedstock is performed with an acid, e g , nitric acid, in multiple stages including a first stage and a second stage, flash steam is generated in the first stage hydrolysis, and the flash steam provided to the feedstock for deconstruction of the feedstock prior to hydrolysis.
  • flash steam is generated in the second stage hydrolysis, and the flash steam is provided to the feedstock for deconstruction of the feedstock prior to hydrolysis and/or to the first hydrolysis module to provide energy for the first stage hydrolysis.
  • flash steam is generated in the second stage hydrolysis, the flash steam is recompressed, and the recompressed steam is provided to the first hydrolysis module to provide energy for the first stage hydrolysis and/or other applications such as, for example, steam stripping distillation, hi some embodiments, flash steam is generated in the second stage hydrolysis, the flash steam is provided to a third hydrolysis module to provide energy for a third stage hydrolysis, the temperature in the third hydrolysis module is lower than the temperature in the second hydrolysis module, and the lower temperature permits hydrolysis of remaining oligomeric sugar molecules with less degradation than hydrolysis performed at a higher temperature.
  • the system further includes a conditioning unit that is in fluid communication with both the hydrolysis unit and the bioreactor, downstream from the hydrolysis unit and upstream from the bioreactor.
  • hydrolysis and conditioning processes occur continuously for the duration of the fermentation
  • hydrolyzed feedstock is conditioned in the conditioning unit to remove inhibitors of microbial growth and/or production of bioproduct,, e g , biofuel, such as butanol, prior to introduction of the hydrolyzed feedstock into the bioreactor, and the conditioning process occurs continuously for the duration of the fermentation.
  • removal of inhibitors includes one or more process(as) selected from overliming, adsorption, precipitation, and ion exchange.
  • the conditioning unit includes an ion exchange resin, and removal of inhibitors is performed by contact of hydrolyzed feedstock with the ion exchange resin under conditions in which the inhibitors are retained on the resin.
  • the ion exchange resin is an anion exchange resin.
  • removal of inhibitors is performed by precipitation with a metal salt, such as an aluminum or iron salt, for example, aluminum sulfate or ferric chloride.
  • the inhibitors include organic acids, furans, phenols, soluble lignocellulosic materials, extractives , and/or ketones.
  • fermentation is conducted under anaerobic conditions.
  • the microorganism is a Clostridium strain.
  • the support material on which the microorganism is immobilized is selected from bone char, polypropylene, steel, diatomaceous earth, zeolite, ceramic, engineered thermal plastic, clay brick, concrete, lava rock, wood chips, polyester fiber, glass beads, Teflon, polyetheretherketone, and polyethylene.
  • the immobilized microorganism includes a biofilm.
  • the bioreactor in which the immobilized microorganism is grown is in the form of a packed bed, an expanded bed, or a fluidized bed.
  • the bioproduct is a biofuel which includes butanol, acetone, ethanol, or a combination thereof.
  • the biofuel includes butanol.
  • the system further includes a recovery unit for recovery of the bioproduct from the fermentation medium.
  • the recovery unit is in fluid communication with and downstream from the bioreactor, and the recovery process operates continuously for the duration of the fermentation.
  • the recovery unit includes a concentration module for concentration of the bioproduct.
  • concentration of the bioproduct includes mechanical vapor recompression.
  • the recovery unit includes a distillation module to separate the bioproduct from other components of the fermentation medium, in fluid communication with and downstream from the concentration module.
  • flash steam generated during hydrolysis of the feedstock provides energy for the distillation.
  • the bioproduct is butanol
  • the system contains a recovery unit for recovery of butanol from the fermentation medium. Recovery of butanol may include distillation to separate butanol from other components of the fermentation medium.
  • butyric acid is recovered in the distillation, butyric acid is recycled back to the bioreactor and is added to the fermentation medium in the bioreactor, and the microorganism in the bioreactor converts butyric acid to butanol.
  • the distillation module includes a first distillation column in fluid communication with and downstream from the concentration module, the distillate exiting the top of the first distillation column contains acetone and ethanol, and the distillate from the bottom of the first distillation column contains butanol
  • the distillation module further includes a decanter in fluid communication with and downstream from the first distillation column, the decanter comprises a top phase and a bottom phase, and butanol and water from the top phase in the decanter are fed into a second distillation column in fluid communication with and downstream from the decanter, and the distillate from the bottom of the second distillation column contains butanol.
  • the distillation module further contains a third distillation column in fluid communication with and downstream from the first distillation column, distillate exiting the top of the third distillation column contains acetone and distillate exiting the bottom of the column comprises ethanol, and the temperature of the third distillation column is lower than the temperature of the first distillation column.
  • the distillate from the bottom of the second distillation column contains both butanol and butyric acid
  • the distillation module further includes a distillation column for separation of butanol and butyric acid in fluid communication with and downstream from the second distillation column, distillate exiting the top of the column for separation of butanol and butyric acid contains butanol and distillate exiting the bottom of the column contains butyric acid, butyric acid is recovered in the distillation, the butyric acid is provided to the fermentation medium in the bioreactor, and the microorganism converts said butyric acid to butanol.
  • lignin is recovered in the residue of the terminal stage, e.g., second stage, of hydrolysis of lignocellulosic feedstock.
  • the lignm-containing residue is dried to a liquid content of about 35% to about 15%, e g , any of about 35%, 30%, 25%, 20%, or 15%, or about 35% to about 30%, about 30% to about 25%, about 25% to about 20%, or about 20% to about 15% or less.
  • the lignin-containing residue is used as an energy source for said process.
  • the lignin-containing residue is used as a fuel source for electricity generation.
  • the lignin-containing residue is used as a chemical precursor for production of useful products, such as phenolic resins. In some embodiments, the lignin-containing residue is used as a feed to an anaerobic digestor for production of useful gaseous products, such as methane or syngas. In some embodiments, the lignin-containing residue is used as a soil enhancer.
  • hydrolysis of a feedstock is performed with an acid, e.g., nitric acid, in multiple stages including a first stage and a second stage
  • the hydrolysis unit includes a first hydrolysis module and a second hydrolysis module
  • nitric acid hydrolysis comp ⁇ ses a first stage in the first hydrolysis module and a second stage in the second hydrolysis module
  • the temperature of the nitric acid in the first hydrolysis module is higher than the temperature of the nitnc acid in the second hydrolysis module
  • flash steam is generated in the second stage hydrolysis
  • the flash steam is recompressed
  • the recompressed steam is used to provide energy for said distillation
  • flash steam is generated in the second stage hydrolysis, optionally recompressed, and used to provide energy for preheating a feed stream to said distillation
  • flash steam is generated in the second stage hydrolysis, the flash steam is recompressed, and the
  • an extractives stream removed before or during feedstock hydrolysis and/or flash steam generated during feedstock hydrolysis is in fluid communication with the product recovery system in order to recover additional products of value, such as terpenes, sterols, sterol esters, resin acids, fatty acids, wax esters, diglycendes, triglycerides, and/or methanol
  • flash steam generated during feedstock hydrolysis is in fluid communication with the product recovery system for use as a distillation aid, for preheating the feed mixture and/or for use in steam stripping distillation
  • material recovered from a primary product recovery column from which a bioproduct, e g , a solvent, has been removed, is reintroduced into the bioproduct production system
  • the material may used as primary dilution water or rinse water (for example, to rmse sugars from biomass), or other water addition stream
  • fermentation nutrients may be reintroduced to the process, reducing cost and/or increasing performance
  • sugars may be reintroduced to the process, improving process yield, and/or water may be reused
  • the bioreactor(s) operated under pressure to compress gas in the bioreactor(s), for example, CO 2 generated by the microorganisms during fermentation
  • FIG. 1 shows a schematic diagram of an embodiment of an integrated biofuel plant in which biobutanol production processes and systems desc ⁇ bed herein may be utilized
  • FIG. 2 shows a schematic diagram of an embodiment of an integrated biofuel plant in which biobutanol production processes and systems described herein
  • Figure 3 shows a process flow diagram for an embodiment of an integrated biofuel plant in which biofuel production processes and systems desc ⁇ bed herein may be utilized
  • Figure 4 shows a schematic diagram of an embodiment of a two-stage feedstock hydrolysis process.
  • Figure 5 shows the results of HPLC analysis of effluent from microbial fermentation on conditioned and unconditioned hydrolyzed feedstock, as described in Example 4.
  • Figure 6 shows the results of continuous culture of immobilized Clostridium, in run no.
  • Figure 7 shows the results of continuous culture of immobilized Clostridium, in run no.
  • Figure 8 shows the results of continuous culture of immobilized Clostridium, in run no.
  • Figure 9 shows the results of continuous culture of immobilized Clostridium, in run no.
  • Figure 10 shows the results of continuous culture of immobilized Clostridium, in run no.
  • Figure 11 shows the results of continuous culture of immobilized Clostridium, in run no.
  • Figure 12 shows the results of continuous culture of immobilized Clostridium, in run no.
  • Figure 13 shows the residual material remaining after performing the hemicellulose extraction procedure described in Example 7 with acid (right hand panel) or water (left hand panel).
  • the invention provides processes and systems for continuous bioproduct, e.g., biofuel, production via microbial fermentation.
  • microbial fermentation is utilized to convert sugars extracted from a carbohydrate-containing feedstock to produce a bioproduct, such as a biofuel, for example, biobutanol and optionally other co-products.
  • a bioproduct such as a biofuel, for example, biobutanol and optionally other co-products.
  • all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which this invention belongs. Singleton, et al., Dictionary of Microbiology and Molecular Biology, second ed., John Wiley and Sons, New York (1994), and Hale & Markham, The Harper Collins Dictionary of Biology.
  • Bioproduct refers to any substance of interest produced biologically, i e , via a metabolic pathway, by a microorganism, e g , in a microbial fermentation process.
  • Bioproducts include, but are not limited to biofuels (e g , butanol, acetone, ethanol), solvents, biomolecules (e g , proteins
  • lipids e g., enzymes, polysaccharides), organic acids (e g, formate, acetate, butyrate, propionate, succinate, lactate, adipic acid, amino acids), alcohols (e g , methanol, propanol, isopropanol, pentanol, hexanol, 2-butanol, isobutanol, glycerol), fatty acids, aldehydes (e g , acetaldehyde, butyraldehyde), ketones (e g , butanone), lipids, long chain organic molecules (for example, for use in surfactant production), vitamins, and sugar alcohols (e g , xylitol).
  • aldehydes e g , acetaldehyde, butyraldehyde
  • ketones e g , butanone
  • lipids long chain organic molecules (for example, for use in surfactant production
  • Biofuel refers to fuel molecules (e.g , butanol, acetone, and/or ethanol) produced biologically by a microorganism, e g , in a microbial fermentation process.
  • fuel molecules e.g , butanol, acetone, and/or ethanol
  • Biobutanol refers to butanol (i e , «-butanol) produced biologically by a microorganism, e g , in a microbial fermentation process.
  • “Byproduct” refers to a substance that is produced and/or purified and/or isolated during any of the processes described herein, which may have economic or environmental value, but that is not the primary process objective.
  • Nonlimiting examples of byproducts of the processes described herein include lignin compounds and derivatives, carbohydrates and carbohydrate degradation products (e g , furfural, hydroxymethyl furfural, formic acid), and extractives (described infra).
  • Feestock refers to a substance that can serve as a source of sugar molecules to support microbial growth in a fermentation process.
  • the feedstock must be pretreated to release the sugar molecules.
  • the feedstock, which contains carbohydrate polymers is hydrolyzed to release 5 and/or 6 carbon containing carbohydrate molecules in monomelic and/or soluble oligomeric forms.
  • Deconstruction refers to mechanical, chemical, and/or biological degradation of biomass into to render individual components (e g , cellulose, hemicellulose) more accessible to further pretreatment processes, for example, a process to release monome ⁇ c and oligomeric sugar molecules, such as acid hydrolysis.
  • “Conditioning” refers to removal of inhibitors of microbial growth and/or bioproduct, e g , biofuel, production from a feedstock or pretreated feedstock (e g , a hydrolysate produced by hydrolysis of a feedstock) and/or adjustments to physical properties of the feedstock or pretreated feedstock to improve conditions that support microbial growth and product production
  • "Titer” refers to amount of a substance produced by a microorganism per unit volume in a microbial fermentation process. For example, biobutanol titer may be expressed as grams of butanol produced per liter of solution.
  • Yield refers to amount of a product produced from a feed material (for example, sugar) relative to the total amount that of the substance that would be produced if all of the feed substance were converted to product.
  • biobutanol yield may be expressed as % of biobutanol produced relative to a theoretical yield if 100% of the feed substance (for example, sugar) were converted to biobutanol.
  • Processivity refers to the amount of a substance produced by a microorganism per unit volume per unit time in a microbial fermentation process. For example, biobutanol productivity may be expressed as grams of butanol produced per liter of solution per hour.
  • Wild-type refers to a microorganism as it occurs in nature.
  • Biomass refers to cellulose- and/or starch-containing raw materials, including but not limited to wood chips, corn stover, rice, grasses, forages, perrie-grass, potatoes, tubers, roots, whole ground corn, grape pomace, cobs, grains, wheat, barley, rye, milo, brans, cereals, sugar-containing raw materials (e.g., molasses, fruit materials, sugar cane, or sugar beets), wood, and plant residues.
  • sugar-containing raw materials e.g., molasses, fruit materials, sugar cane, or sugar beets
  • Starch refers to any starch-containing materials.
  • the term refers to various plant-based materials, including but not limited to wheat, barley, potato, sweet potato, tapioca, corn, maize, cassava, milo, rye, and brans.
  • the term refers to any material comprised of the complex polysaccharide carbohydrates of plants, comprised of amylose, and amylopectin, with the formula wherein "x" can be any number.
  • ABE fermentation refers to production of acetone, butanol, and/or ethanol by a fermenting microorganism.
  • Advanced biofuels are high-energy liquid transportation fuels derived from low nutrient input/high per acre yield crops, agricultural or forestry waste, or other sustainable biomass feedstocks including algae.
  • “Lignocellulosic” biomass refers to plant biomass that contains cellulose, hemicelluloses, and lignin.
  • the carbohydrate polymers cellulose and hemicelluloses) are tightly bound to lignin.
  • n-Butanol (1 -butanol) is also referred to as “butanol” herein.
  • ATCC refers to the American Type Culture Collection, P.O. Box 1549, Manassas, VA
  • a feedstock is a substance that provides the base material from which sugar molecules are generated for inclusion in a microbial growth medium, to support the growth of the microorganism
  • the feedstock is cellulosic biomass
  • the feedstock contains cellulose and hemicellulose, for example, lignocellulosic biomass or wood pulp
  • the feedstock is a polysaccharide from which soluble sugar molecules may be produced that can support growth of a microorganism, for example, a polysaccharide waste product such as crab, shrimp, or lobster shells, chitin, chitosan, pectm, or sucrose
  • the feedstock is woody biomass
  • the feedstock is softwood, for example, pine, e g , Lodgepole or Loblolly pine hi one embodiment, the feedstock contains mountain pine beetle infested pine, for example, dying ("red stage") or dead ("grey" stage)
  • the feedstock is hardwood, for example, maple, birch, or ash
  • the feedstock is mixed hardwood and softwood
  • the feedstock is mixed hardwood
  • the woody biomass is in the form of wood chips, sawdust, saw mill residue, wood fines, or a combination thereof
  • the feedstock is obtained as a process stream from a biomass processing facility, for example, a pulp mill hi vanous embodiments of pulp mill process streams, the process stream may include reject pulp, wood knots or shives, pulp screening room rejects (e g , essentially cellulose in water), prehydrolysis extraction stream, and/or black liquor hi other embodiments, the feedstock
  • Lignocellulose contains a mixture of carbohydrate polymers and non-carbohydrate compounds
  • the carbohydrate polymers contain cellulose and hemicellulose, and the non- carbohydrate portion contains hgnin
  • the non-carbohydrate portion may also contain ash, extractives, and/or other components
  • the specific amounts of cellulose, hemicelluloses, and lignin depends on the source of the biomass For example, municipal solid waste may contain primarily cellulose, and extract streams from a paper and pulp plant may contain primarily hemicelluloses
  • the remaining composition of lignocellulose may also contain other compounds such as protems
  • Cellulose which is a ⁇ -glucan built up of D-glucose units linked by ⁇ (l,4)-glycosidic bonds, is the mam structural component of plant cell walls and typically constitutes about 35-60% by weight (%w/w) of lignocellulosic materials
  • Hemicellulose refers to non-cellulosic polysaccharides associated with cellulose in plant tissues Hemicellulose frequently constitutes about 20-35% w/w of lignocellulosic materials, and the majority of hemicelluloses consist of polymers based on pentose (five-carbon) sugar units, such as D-xylose and D-arabinose units, hexose (six-carbon) sugar units, such as D-glucose and D- mannose units, and uremic acids such as D-glucuronic acid.
  • Lignin which is a complex, cross-linked polymer based on variously substituted p- hydroxyphenylpropane units, typically constitutes about 10-30% w/w of lignocellulosic materials.
  • Any material containing cellulose and/or hemicellulose or cellulose and/or hemicellulose oligomeric and/or monomelic compounds e.g. , sugar monomers, dimers ⁇ e.g. , cellobiose), trimers (e.g., cellotriose)
  • the material may contain cellulose and/or hemicellulose without lignin.
  • Lignocellulosic biomass may be derived from a fibrous biological material such as wood or fibrous plants.
  • suitable types of wood include, but are not limited to, spruce, pine, hemlock, fir, birch, aspen, maple, poplar, alder, salix, cottonwood, rubber tree, marantii, eucalyptus, sugi, and acase.
  • suitable fibrous plants include, but are not limited to, corn stover and fiber, flax, hemp, cannabis, sisal hemp, bagasse, straw, cereal straws, reed, bamboo, mischantus, kenaf, canary reed, Phalaris arundinacea, and grasses.
  • lignocellulosic materials may be used such as herbaceous material, agricultural crop or plant residue, forestry residue, municipal solid waste, pulp or paper mill residue, waste paper, recycling paper, or construction debris.
  • suitable plant residues include, but are not limited to, stems, leaves, hulls, husks, cobs, branches, bagasse, wood chips, wood pulp, wood pulp, and sawdust.
  • suitable waste paper include, but are not limited to, discarded paper of any type (e.g., photocopy paper, computer printer paper, notebook paper, notepad paper, typewriter paper), newspaper, magazines, cardboard, and paper-based packaging material. Materials with high mineral content may potentially require additional pH adjustment (e.g., additional amounts of chemicals for pH adjustment) for effective processing.
  • the bioproduct e.g., biofuel
  • production plant can include a facility to unload, wash and screen incoming wood chips to remove any dirt and debris.
  • the chips can be ground to the optimum size for hydrolysis and conveyed to the feed hopper for introduction into the hydrolysis unit.
  • Data can be collected from a feedstock provider and used to size and specify the wood handling equipment for a given plant.
  • feedstocks that may be used in the bioproduct (e.g., biofuel, for example, biobutanol) production processes described herein include hemicellulose extract from wood, beet extract, beet molasses, sorghum syrup, barley hulls, potato processing waste, and brewers mash.
  • a feedstock mix containing about 40% logging residues, about 20% sustainable roundwood, about 20% woody energy crops, and about 20% herbaceous energy crops may be used This blend can account for regional variation and provide significant flexibility in selecting locations for facilities and in procuring feedstock supply contracts [108]
  • Feedstock flexibility may permit utilization of combinations of feedstocks in geographic locations where the available supply of feedstocks taken individually are not sufficient to justify a commercial scale bioproduct, e g , biobutanol, production plant, or where synergistic value can be realized from combining feedstocks that allow for better practices to be implemented with regard to the underlying land (e g, improved crop rotations) or in terms of more economic harvest, handling and storage logistics
  • Feedstock flexibility may also provide opportunities to locate plants in niche sites where end use markets are m close proximity to otherwise non-utihzable feedstocks
  • diverse feedstocks may be utilized by versatile strains which are capable of converting both 5 -carbon and 6-carbon sugar molecules (including multimeric forms
  • Feedstocks such as those described herein can be pretreated using a variety of methods and systems p ⁇ or to bioconversion
  • Preparation of the feedstock can mclude chemical or physical modification of the feedstock
  • the feedstock can be shredded, sliced, chipped, chopped, heated, burned, dried, separated, extracted, hydrolyzed, and/or degraded
  • These modifications can be performed by biological, non-biological, chemical, or non-chemical processes
  • processes may be used to break down cellulose and/or hemicellulose mto sugar molecules that may be more easily processed by a microorganism
  • Processes that may be used mclude acid hydrolysis, enzymatic hydrolysis, gasification, pyrolysis, and cellulose degradation by a microorganism
  • the feedstock such as hgnocellulosic feedstock, for example, wood chips, sawdust, and/or sawdust residue
  • a downstream pretreatment process such as hydrolysis
  • Deconstruction may include, but is not limited to, presteaming to swell and loosen material, mechanical grinding, mechanical explosion (e g , steam or other chemical treatment followed by rapid decompression), vacuum treatment, acid-feedstock contact (diffusion of acid into feedstock), or a combination thereof
  • deconstruction renders cellulose and/or hemicellulose in the feedstock more accessible for hydrolysis
  • the feedstock such as lignocellulosic feedstock, for example, wood chips, sawdust, and/or sawdust residue
  • Extractives are material that is extracted from the feedstock by a process such as compression, water or solvent extraction, or air drying
  • Non-limiting examples of extractives include terpenes, resm acids, fatty acids, sterols, phenolic compounds, and triglycerides
  • Extractives may include, but are not limited to, p-couma ⁇ c acid, ferulic acid, 4-hydroxybenzoic acid, vanillic acid, sy ⁇ ngaldehyde, vanillin, furfural, hydroxymethylfurfural, and glucuronic acid Extractives may be removed for other uses, such as production of sterols, or burned to provide energy for a bioproduct, e g , biofuel, production process as descnbed herein
  • extractives are removed prior to or in conjunction with deconstruction of the feedstock
  • a feedstock contains sugar molecules m an oligomeric form, e g , a polymeric form, and must be hydrolyzed to extract and release soluble monomenc and/or multimenc sugar molecules, which are converted to bioproduct, e g , biofuel, in a microbial fermentation as described herein
  • the sugar molecules are present m the feedstock in cellulose and/or hemicellulose
  • the feedstock is lignocellulosic biomass and the sugar molecules are present in the feedstock in cellulose and hemicellulose
  • the feedstock is pretreated with an acid hydrolysis process
  • Acids that may be used for hydrolysis include, but are not limited to, nitric acid, formic acid, acetic acid, phosphoric acid, hydrochloric acid, and sulfuric acid, or a combination thereof
  • acid hydrolysis is performed m a single stage
  • acid hydrolysis is performed in two or more stages, under different conditions in each stage to hydrolyze different components of the feedstock in each stage
  • Acid hydrolysis performed m multiple stages may serve to limit the impact of kinetically controlled carbohydrate degradation mechanisms
  • An acid hydrolysis system may be designed to submerge and flood the feedstock with the acid solution in the hydrolysis reactor, e.g.
  • a multiple-stage dilute nitric acid hydrolysis process is used.
  • a two-stage dilute nitric acid process is used, m one embodiment, conditions in the first stage are chosen to achieve hydrolysis of about 70% to about 90% of the hemicellulose in the feedstock and conditions in the second stage are chosen to achieve hydrolysis of about 40% to about 70% of the cellulose in the feedstock.
  • the first stage mainly targets the hydrolysis of the hemicellulose, yielding a mannose and/or xylose rich hydrolysate, whereas the second stage uses the solids remaining from the first stage and targets the cellulose, yielding a glucose rich hydrolysate.
  • first stage hydrolysate liquors contain a mix of 5-carbon and 6-carbon sugars, e.g., extracted primarily from hemicellulose and non-recalcitrant cellulose biomass components
  • second stage hydrolysate contains primarily 6-carbon sugars, e.g., extracted from cellulose fibers, in both cases as soluble monomelic and/or multimeric forms.
  • 6-carbon monosaccharides may include, but are not limited to, glucose, mannose, and galactose.
  • 6-carbon disaccharides may include, but are not limited to, cellobiose, mannobiose, glucomannose, and galactomannose.
  • 5-carbon monosaccharides may include, but are not limited to xylose and arabinose.
  • 5-carbon disaccharides and other multimeric forms may include, but are not limited to, xylobiose, xylotriose, and arabinoxylose.
  • the first stage hydrolysate contains about 60% to about 75% 5-carbon sugar by weight and about 25% to about 40% 6-carbon sugar by weight, and the second stage hydrolysate contains about 80% to about 95% 6-carbon sugar by weight.
  • the first stage hydrolysate contains about 20% to about 30% 5-carbon sugar by weight and about 70% to about
  • the second stage hydrolysate contains about 90% to about 100% 6-carbon sugar by weight, wherein the second stage is performed at a higher temperature than the first stage.
  • a first stage hydrolysis module may be coupled to a second stage hydrolysis module, with solid residue separated from liquid hydrolysate generated in the first stage hydrolysis serving as substrate for the second hydrolysis process.
  • the residual solids may be rinsed/washed in order to increase the separation and recovery yield of soluble sugars separated from the biomass.
  • the second stage hydrolysis is performed at a higher temperature than the first stage hydrolysis.
  • hydrolysis is performed at a nitric acid concentration of about 0.05 to about 0.1%, about 0.1% to about 0.5%, about 0.5% to about 1%, about 1% to about 4%, about 1.3% to about 3.5%, or about 1.3% (w/w of dry feedstock) for both hydrolysis stages, at a temperature of about 170° to about 175°C in the first stage and a temperature of about 210° to about 230°C in the second stage, and at the saturation pressure for steam at the reactor temperature for each hydrolysis stage.
  • the liquid (acid) to solid (feedstock) ratio for hydrolysis is about 10:1 to about 5:1 or about 7.5:1 to about 5:1.
  • the ratio of liquid to solid may be about 5:1 to about 3:1 or about 3.5:1 to about 3:1.
  • the ratio of liquid to solid may be about 4: 1 to about 0.5:1.
  • the soluble sugar extraction yield from the feedstock in the first stage hydrolysis as about or at least about 6, 10, 15, 20, 30, 34, 40, 50, or 60% from cellulose and about or at least about 1, 3, 6, 10, 20, 40, 60, 70, 75, 80, 85, 90, 95, or 99% from hemicellulose.
  • the soluble sugar extraction yield from solid residue remaining after the first stage hydrolysate in the second stage hydrolysis is about or at least about 25, 35, 45, 55, 65, 75, 85, or 95% from cellulose and about or at least about 1, 3, 6, or 10% from hemicellulose.
  • conditions are chosen such that short residence times may be utilized, providing high productivity (smaller reactors) and minimal sugar degradation products.
  • residence time in the hydrolysis reactor for first stage nitric acid hydrolysis with 1 A inch wood chips may be about 5 to about 8 minutes, with longer residence time of about 3 to about 15, or up to about 30 minutes for larger feed material, and residence time for 1 A inch wood chips for second stage nitric acid hydrolysis may be about 3 to about 6 minutes, or about 3 to about 20 minutes, with longer residence time for larger feed material.
  • the residence times may be affected by the degree of material deconstruction and/or the applied acid conditions.
  • nitric acid at lignocellulosic pretreatment conditions permit the use of stainless steel, rather than the more exotic and expensive materials required for other pretreatment processes, such as dilute sulfuric acid treatment. This confers a substantial capital cost advantage.
  • hydrolysis and neutralization process is rich in nitrogen that can be utilized in fermentation.
  • hydrolysate streams are neutralized with ammonia to produce ammonium nitrate.
  • Ammonium nitrate is a nutrient for microorganisms in the downstream fermentation process.
  • hydrolysis reactors for each stage may be the same or different.
  • a second stage reactor may have a higher or lower capacity than a first stage reactor.
  • a hydrolysis reactor may have an internal volume of about or at least about 1, 2, 5, 10, 20, 50, 100, 200, 500, 1000, 2500, 5000, 10,000, 50,000, 100,000, 150,000, or 200,000 gallons.
  • a nitric acid hydrolysis reactor may be smaller than a comparable capacity sulfuric acid hydrolysis reactor.
  • one or more processing operations can be used between stages, such as between first and second nitric acid hydrolysis stages, including mechanical degradation, drying, shaking, mixing, chipping, straining, solid-liquid, liquid-liquid, or gas-liquid separation phase separation, decanting, and shearing. Such operations may be used for separation, degradation, attrition, or shearing of an input material.
  • a hydrolysis system can include a steam compressor to compress low pressure flash steam.
  • low pressure flash steam from the first and/or second stage of a nitric acid hydrolysis process may be compressed. By raising the pressure, the low pressure flash steam can be re-used in downstream product concentration and/or product distillation operations and significantly reduce the energy requirements of the overall process.
  • flash steam may be used productively in steam stripping distillation, permitting recovery of useful products contained in the flash stream.
  • a hydrolysis system for use in the processes described herein can be optimized to produce the greatest yield of products per amount of feedstock, energy required, greenhouse gas emitted, or any combination thereof. Optimization parameters include the type of separations or reactions performed outside of the hydrolysis reactors, and the conditions of the hydrolysis reactors. In some embodiments, degradation and/or hydrolysis of the feedstock material may be reduced or increased due to impact on energy consumption or product yield.
  • a feedstock hydrolysis process as described herein and a fermentation process are coupled to process feedstock in a continuous manner.
  • the continuous operation may be designed such that accumulation of materials between the hydrolysis unit and fermentor is avoided.
  • a hydrolysis unit may be operated continuously for about or at least about 50, 100, 200, 300, 400, 600, 800, 1000, 1350, 1600, 2000, 2500, 3000, 4000, 5000, 6000, or 8500 hours.
  • Lignin-containing residue remaining after hydrolysis of a lignocellulosic feedstock may be used as an energy source for the bioproduct, e.g , biofuel, production process described herein and/or as a fuel source for electricity generation.
  • lignin-containing residue is dried to a liquid content of about 35% to about 15%, e g., any of about 35%, 30%, 25%, 20%, or 15%, or about 35% to about 30%, about 30% to about 25%, about 25% to about 20%, or about 20% to about 15% or less and the dried residue may be burned as a fuel source for energy or electricity generation, gasified for subsequent combustion or conversion to other chemical products, or converted to other chemical products.
  • a method for deconstructing biomass that contains cellulose and hemicellulose for the extraction of sugar molecules from the biomass includes: (a) mechanically disintegrating the biomass in the presence of water and under pressure, thereby producing liquid and/or vapor and solid disintegrated biomass; (b) separating liquid and/or vapor from the biomass, wherein step (b) may be performed after or in conjunction with step (a); (c) contacting the disintegrated biomass with acid in an amount sufficient to depolymerize a polymeric carbohydrate component of the biomass, thereby producing acid impregnated disintegrated biomass;
  • the acid is nitric acid at a concentration of about 0.1% (w/w) to about 0.5% (w/w).
  • the digestor is operated at a pressure of about 90 to about 110 psig, a temperature of about 167°C to about 176°C and a residence time of about 3 to about 20, about 8 to about 20, or about 5 to about 10 minutes, hi some embodiments, the biomass is contacted with steam prior to acid impregnation, which may aid with disintegration of the biomass and extractives removal.
  • the residual solids are further hydrolyzed, for example, by acid hydrolysis, to release soluble sugar molecules from the cellulose fiber, thereby producing a further hydrolysate that may be used to support microbial fermentation in the processes and systems described herein.
  • the method described above for deconstructing biomass that contains cellulose and hemicellulose for the extraction of sugar molecules from the biomass is performed with an acid concentration in step (c), a residence time in step (d), and a temperature in step (d) sufficient to produce a hydrolysate that contains hemicellulose sugars and residual solids that contain cellulosic fiber that is less than about 0.35, 0.30, or 0.28 mm in length.
  • the residual solids do not contain visible cellulosic fiber.
  • the acid concentration in step (c) is about 1% (w/w) to about 1.5% (w/w)
  • the residence time in step (d) is about 5 minutes to about 10 minutes
  • the temperature in step (d) is about 160°C to about 180°C.
  • the acid is nitric acid at a concentration of about 0.05% (w/w) to about 4% (w/w).
  • the digestor is operated at a pressure of about 90 to about 110 psig, a temperature of about 160 0 C to about 180°C, and a residence time of about 4 to about 15 min.
  • the biomass is contacted with steam prior to acid impregnation, which may aid with disintegration of the biomass and extractives removal.
  • the residual solids are further hydrolyzed, for example by acid or enzymatic hydrolysis, thereby producing a further hydrolysate that may be used to support microbial fermentation in the processes and systems described herein.
  • a method for deconstructing biomass that contains cellulose and hemicellulose for the extraction of sugar molecules from the biomass including: (a) contacting the biomass with acid in an amount sufficient to depolymerize a polymeric carbohydrate component of the biomass, thereby producing acid impregnated disintegrated biomass; (b) feeding the acid impregnated disintegrated biomass into a digestor through a pressure changing device, wherein the acid impregnated disintegrated biomass is heated in said digestor at a temperature and for an amount of time sufficient to permit the depolymerization reaction to occur; and (c) separating solids from liquids to produce a liquid hydrolysate and residual solids, wherein the hydrolysate comprises hemicellulose sugar molecules and the residual solids contain fiber that is less than about 0.35, 0.30, or 0.28 mm in length.
  • the residual solids do not contain visible cellulosic fiber.
  • the acid is nitric acid at a concentration in step (a) is about 0.1% (w/w) to about 5% (w/w), or about 1% (w/w) to about 3% (w/w), the residence time in step
  • step (b) is about 8 to about 20 minutes, and the temperature in step (b) is about 160 0 C to about 18O 0 C.
  • the biomass is contacted with steam prior to acid impregnation, which may aid with disintegration of the biomass and extractives removal
  • the residual solids are further hydrolyzed, for example by acid or enzymatic hydrolysis, thereby producing a further hydrolysate that may be used to support microbial fermentation in the processes and systems described herem
  • hydrolyzed feedstock is "conditioned" to remove inhibitors of microbial growth and/or bioproduct, e g, biofuel, production, prior to addition of the hydrolyzed feedstock to microbial growth medium
  • inhibitors may include, but are not limited to, organic acids, furans, phenols, soluble lignocellulosic matenals, extractives, and ketones
  • Inhibitors present in wood hydroly sates may include, but are not limited to, 5-hydroxyy-methyl furfural (HMF), furfural, aliphatic acids, levulinic acid, acetic acid, formic acid, phenolic compounds, vanillin, dihydroconiferylalcohol, comferyl aldehyde, vanillic acid, hydroquinone, catechol, acetoguaiacone, homovanillic acid, 4-hydroxy-benzoic acid, Hibbert's ketones , ammonium nitrate and/or other salts, p-cous, 5-hydroxyy
  • Nonhmiting examples of conditioning processes include vacuum or thermal evaporation, overhming, precipitation, adsorption, enzymatic conditioning (e g , peroxidase, laccase), chemical conversion, distillation, and ion exchange
  • conditioning includes contact of hydrolyzed feedstock with an ion exchange resm, such as an anion or cation exchange resm Inhibitors may be retained on the resin
  • the ion exchange resin is an anion exchange resin
  • Ion exchange resins may be regenerated with caustic, some solvents, potentially including those generated m the bioproduct, e g biofuel, production processes described herein, or other known industrial materials
  • inhibitors may be precipitated by a metal salt (for example, a trivalent metal salt, for example, an aluminum or iron salt, such as aluminum sulfate or ferric chloride), and/or a flocculant such as polyethylene oxide or other low density, high molecular weight polymers
  • hydrolysate is conditioned on ion exchange resin, such as an anion exchange resm, e g , Duolite A7, at acidic pH, for example, pH about 2 5 to about 5 5, about 3 5 to about 4 5, or about 2 5, 3, 3 5, 4, 4 5, 5, or 5 5
  • ion exchange resin such as an anion exchange resm, e g , Duolite A7
  • acidic pH for example, pH about 2 5 to about 5 5, about 3 5 to about 4 5, or about 2 5, 3, 3 5, 4, 4 5, 5, or 5 5
  • hydrolysate is conditioned with a metal salt, for example, a trivalent metal salt, such as an aluminum or iron salt, e g , aluminum sulfate or ferric chloride
  • a metal salt for example, a trivalent metal salt, such as an aluminum or iron salt, e g , aluminum sulfate or ferric chloride
  • the metal salt is added at a concentration of about 1 g/L to about 6 g/L, or about 3 g/L to about 5 g/L.
  • the pH is adjusted with a base to a basic pH, such as about
  • microbial growth and/or bioproduct e.g., biofuel, titer, yield, and/or productivity is increased when conditioned hydrolyzed feedstock is used, in comparison to identical hydrolyzed feedstock which has not been subjected to the conditioning process.
  • a microorganism that is tolerant to inhibitors in hydrolyzed feedstock is used, or the microorganism used for bioproduct production develops increased tolerance to inhibitors over time, e.g., by repeated passaging, rendering the conditioning step unnecessary or uneconomical.
  • an extractive removal process is used instead of a conditioning process to improved microbial growth and/or bioproduct, e.g., biofuel, titer, yield, and/or productivity.
  • an extractive removal process is used in addition to a conditioning process to improve microbial growth and/or bioproduct, e.g., biofuel, titer, yield, and/or productivity.
  • An extractive removal process may also be used in some embodiments to generate an additional stream to provide products with commercial value ⁇ e.g.
  • sterols and/or to improve operational parameters (e.g., less resin and regenerant to regenerate the resin (e.g,, caustic) required for removal of fermentation and/or bioproduct, e.g., biofuel, production inhibitors.
  • operational parameters e.g., less resin and regenerant to regenerate the resin (e.g,, caustic) required for removal of fermentation and/or bioproduct, e.g., biofuel, production inhibitors.
  • the bioproduct production process herein includes fermentation of a microorganism that produces a bioproduct, e. g. , a biofuel, in an immobilized cell bioreactor (i. e., a bioreactor containing cells that are immobilized on a support, e.g., a solid support), hi some embodiments, an immobilized cell bioreactor provides higher productivity due to the accumulation of increased productive cell mass within the bioreactor compared with a stirred tank (suspended cell) bioreactor.
  • the microbial cells form a biofilm on the support and/or between support particles in the growth medium.
  • the bioproduct, e.g.,_biofuel, production process herein includes continuous fermentation of a microorganism (continuous addition of feedstock (e.g., hydrolyzed feedstock) and withdrawal of product stream). Continuous fermentation minimizes the unproductive portions of the fermentation cycle, such as lag, growth, and turnaround time, thereby reducing capital cost, and reduces the number of inoculation events, thus minimizing operational costs and risk associated with human and process error.
  • Fermentation may be aerobic or anaerobic, depending on the requirements of the bioproduct- producing microorganism.
  • an immobilized butanol-producing Clostridium strain is fermented anaerobically in a continuous process as described herein, hi one embodiment, the support is bone char. In another embodiment, the support is lava rock. In another embodiment, the support is a ceramic/steel support material. In some embodiments, the Clostridium strain has an increased tolerance to butanol and/or an increased ability to grow on the support, in comparison to a corresponding parent or wild-type strain, and/or in comparison to Clostridium saccharobutylicum
  • reactor support materials and implementation thereof are designed so as to maximize reactor productivity. This may include such features as maximizing fermentation gas removal efficiency, liquid-microorganism contact time, minimization of pressure drop, or optimization for cleaning in place.
  • bacterial strains such as Clostridium strains, are substituted or rotated periodically to prevent or reduce the occurrence of phage infections.
  • One or more bioreactors may be used in the bioproduct, e.g., biofuel, systems and processes described herein. When multiple bioreactors are used they can be arranged in series and/or in parallel. The advantages of multiple bioreactors over one large bioreactor include lower fabrication and installation costs, ease of scale-up production, greater ability to control the reaction, and greater production flexibility. For example individual bioreactors may be taken off-line for maintenance, cleaning, sterilization, and the like without appreciably impacting the overall plant production schedule. In embodiments in which multiple bioreactors are used, the bioreactors may be run under the same or different conditions.
  • hydrolyzed feedstock is fed into multiple bioreactors, and effluent from the bioreactors is removed.
  • the effluent may be combined from multiple bioreactors for recovery of the bioproduct, e.g , biofuel, or the effluent from each bioreactor may be collected separately and used for recovery of the bioproduct.
  • the effluent from the final bioreactor in the series is collected and may be used for recovery of the bioproduct, e.g., biofuel.
  • the effluent may be treated between stages (e.g., primary to secondary bioreactor) to increase the overall productivity of the system.
  • stages e.g., primary to secondary bioreactor
  • processes for such treatment include removal of non-condensable gases and pervaporation for the removal of solvents.
  • Each bioreactor in a multiple bioreactor arrangement can have the same species, strain, or mix of species or strains of microorganisms or a different species, strain, or mix of species or strains of microorganisms compared to other bioreactors in the series.
  • the fermentation effluent is then removed and sent to separation and recovery.
  • feedstock is hydrolyzed in a multi-stage process as described herein, and hydrolysate from each stage is fed to a separate bioreactor.
  • the bioreactors to which the different hydrolysates are fed may contain the same or different microbial species or strains.
  • the bioreactors to which the different hydrolysates are fed contain different microbial species or strains that have each been optimized for growth on the particular hydrolysate being fed to that bioreactor.
  • different sets of multiple bioreactors in series are fed hydrolysate from different stages of hydrolysis of the feedstock.
  • effluent can be recycled after the harvesting of bioproduct, e.g., biofuel, and used to make the initial fermentation media or a feed stream for future fermentations, thereby allowing maximum utilization of unassimilated and recovered nutrients and minerals.
  • product is isolated from the effluent and the product reduced effluent is then used as a feedstock for the next bioreactor in the series.
  • the order of bioreactors in a series can be adjusted to prevent or remove blockage due to excessive microbial growth. For example, when the first fermentor in a series reaches a high level of cell mass, it can be placed second in the series to instead now receive effluent with high product concentration or reduced nutrient levels that may inhibit further cell growth. The timely shifting of the order of fermentors may prevent cell overgrowth and blockage of the bioreactor, which may increase overall productivity of the system and/or reduce operational costs and burdens. [154] In a continuous process, it is possible to obtain a higher productivity than in batch or fed- batch processes since the cell concentration and the effluent flow rate can be varied independently of each other.
  • volumetric productivity is calculated by multiplying the product concentration (herein, interchangeably called the "titer") times the nutrient dilution rate (i. e. , the rate of changeover of the volume of the bioreactor, or the inverse of the bioreactor residence time).
  • the maximum achievable dilution rate is determined by the concentration of cell mass that one can stably maintain in the bioreactor.
  • a constant dilution rate i. e. , nutrient consumption rate
  • the productivity is proportionately increased.
  • Immobilized cell bioreactors allow higher concentrations of productive cell mass to accumulate and therefore, the bioreactors can be run at high dilution rates, resulting in a significant improvement in volumetric productivity relative to cultures of suspended cells Since a high density, steady state culture can be maintained through continuous cultu ⁇ ng, with the attendant removal of product containing fermentation broth, smaller capacity bioreactors can be used
  • Bioreactors for use in the bioproduct, e g , biofuel, production processes and systems herein are designed for continuous operation for at least about 100, 250, 300, 500, 750, 1,000, 1250, 1,500,
  • Bioreactor capacities contemplated for use in the bioproduct, e g , biofuel, production systems herein have a capacity (total nominal volume) of about or at least about 10OL, 100OL, 6,000
  • support material may be added to the reactor through bottom, top, or side loading to replemsh support material that becomes degraded or lost from the bioreactor
  • Mixing of the bioreactor contents can be achieved through the sparging of sterile gas, e g , carbon dioxide or N 2 , which may also serve to prevent contamination of the culture through the maintenance of positive pressure within the fermentor
  • sterile gas e g , carbon dioxide or N 2
  • the evolved gas (CO 2 , H 2 ) from the fermentation may also be recovered and compressed for utilization in a gas lift or other type reactor to maintain anaerobic, pressurized, well mixed conditions
  • immobilized microorganisms are cultured in packed bed bioreactors, also known as plug- flow bioreactors.
  • the microorganisms are cultured in expanded bed bioreactors.
  • the microorganisms are cultured in fluidized bed bioreactors.
  • the microorganisms are cultured in bioreactors that are designed to operate in "dual mode," i.e., the bioreactors are capable of operating in either packed bed or expanded/fluidized bed mode, e.g., during the same period of operations to increase overall productivity ⁇ e.g., removal of detritus, removal of "underperforming" cells).
  • Immobilized cell bioreactors use relatively small sized solid or semi-solid supports that provide a large surface area relative to the volume of the particles, allowing for the microorganisms immobilized on the particles to process large volumes of fluid.
  • cells are immobilized on or in structured packing ⁇ e.g., Rashig rings, steel/ceramic wool) or semi-solid or solid particles that because of particle size, mechanical restraint and/or low fluid flow rates do not cause or allow for appreciable axial movement of the supporting material.
  • structured packing e.g., Rashig rings, steel/ceramic wool
  • fluidized and expanded bed reactors use semi-solid or solid support that is not substantially restrained mechanically so that with sufficient fluid flow, usually an upward-flowing stream, the particles become suspended in the stream or "fluidized," i.e., act as if they are part of the fluid stream.
  • the initial seed support particles may become covered by a biofilm over time and can become fully encapsulated by the biofilm. In some cases, agglomeration of cellular mass may lead to suspended biofilm particles in which there is no "seed" purposefully introduced. Fluid drag on the particles is the primary suspension mechanism, but buoyancy forces can also contribute to the suspension of the particles.
  • the bioreactors use vertical fluid motion to suspend the particles, but other fluid motion is possible including fluid flow at a direction perpendicular to the vertical axis of the bioreactor.
  • the fluid velocity should be sufficient to suspend the particles, but not large enough to carry them out of the vessel.
  • the fluidization of the bed allows the solid particles to move around the bioreactor, causing the fluid within the bioreactor to thoroughly mix. The magnitude of mixing depends on the extent of particle fluidization achieved in the bioreactor.
  • Fluidized and expanded bed bioreactors require relatively larger amounts of energy to operate compared to packed beds because of the volume of fluid that must be circulated to keep the particles suspended.
  • a "fluidized bed” bioreactor contains support particles with immobilized microorganisms fluidized throughout the full volume of the bioreactor. Particles exit the bioreactor through the outflow and have to be separated from the effluent liquid and returned to the bioreactor. Support material can be removed, optionally cleaned, and recovered from the effluent stream through the use of settling tanks, dissolved air flotation (DAF) systems, centrifuges, hydrocyclones, filters (e.g., rotary drum), filter aids, dryers, or distillation apparatus.
  • DAF dissolved air flotation
  • An "expanded bed” bioreactor contains support particles with immobilized microorganisms fluidized in the bioreactor, but the bioreactor is designed such that the particles are retained in the bioreactor and do not exit through the outflow.
  • An expanded bed bioreactor contains a particle disengagement zone for separating the fluidized particles from the fluid, thereby retaining the particles within the bioreactor.
  • separation of the particles from the fluid includes slowing the velocity of the fluid, hi some embodiments, this is accomplished by increasing the cross sectional area of the bioreactor. As the fluid velocity slows, the particles start to settle out of the fluid.
  • the top section of the particle disengagement zone is free of particles. An outlet can be located at this top portion to remove effluent.
  • particles are retained by including filters or screens within the bioreactor.
  • a dual mode, packed bed-fluidized or expanded bed bioreactor allows for the option of conducting fermentations in either mode for the course of a whole fermentation run. Alternately, the fermentation can alternate between modes during the course of a single fermentation. Dual mode bioreactors can have reduced energy usage compared to conventional fluidized or expanded bed bioreactors because fluidization with its requisite increased energy requirement need only be performed, for example, at relatively high cell densities, high product concentrations, or when pH or nutrient inhomogeneities develop that can be corrected through increased mixing of the bioreactor contents.
  • a bioreactor may be configured in a vertical, horizontal, or inclined configuration, to maximize gas/liquid separation and/or to improve elution of evolved fermentation gas to improve overall operation and metrics for the production process, e.g. , titer, productivity, and/or yield of bioproduct, e.g., biofuel, production.
  • a bioreactor may be configured as a "trickle bed reactor," in which the material to be reacted is fed into the bed by a slow flow.
  • the amount of a bioproduct such as a biofuel, e.g.
  • biobutanol, produced per amount of sugar fed to a bioreactor may be about or at least about 0.1, 0.15, 0.2 0.25, 0.3, 0.33, 0.35, 0.4, 0.45, or 0.5 grams per gram sugar converted, subject to the particular reaction stoichiometry.
  • the fermentation may utilize about or at least about 40, 50, 60, 65, 70, 75, 80, 85, 90, 95, 96, 97, 98, or 99% of the available sugar.
  • biofuel e.g., biobutanol
  • about or at least about 20, 30, 40, 50, 60, 70, 80, 90, or 95 gallons of biofuel, e.g., biobutanol, is produced per tonne of feedstock, or an amount that approaches the theoretical limit, depending on the feedstock that is used.
  • a bioproduct such as a biofuel, e.g. , biobutanol
  • a productivity of about or at least about 1, 2, 3, 5, 6, 7, 8, 9, 10, 12, 15, 20, 25, 30, 35, 40, 45, or 50 g/L/h.
  • bioreactor volumetric productivity and bioproduct may be improved by reducing the particle size of the immobilized support, which can increase available surface area for cell growth, resulting in higher bioreactor productivity.
  • biofuel for example, butanol
  • titer may be improved by reducing the particle size of the immobilized support, which can increase available surface area for cell growth, resulting in higher bioreactor productivity.
  • Clostridium strains convert sugars into butanol, acetone, and ethanol in a 6:3:1 mass ratio.
  • strains used in the systems and processes described herein produce a larger proportion of butanol relative to acetone - for example, approximately 75%- 25% - with very little ethanol (about 2%).
  • the ratio of butanol to acetone to ethanol can be about or at least about 58:12:1. In some embodiments, the ratio of butanol to acetone to ethanol is greater than about 58:12:1.
  • the distribution of products produced by the Clostridium strain can be such that the amount of butanol is at least about 70%, the amount of acetone is at least about 25%, and the amount of ethanol is less than about 5%.
  • This higher butanol selectivity results in a higher yield of butanol per unit weight of feedstock.
  • selecting strains having a higher butanol tolerance and higher butanol selectivity in an immobilized environment can result in a higher concentration of butanol in the fermentation broth leaving the reactor, thereby requiring less energy in the product separation phase, and reducing operating costs, cooling water use, and lifecycle GHG emissions.
  • Fermentation media for the production of bioproduct, e.g. , biofuel, products contain feedstock, e.g., a hydrolyzed feedstock, as described herein, as a source of fermentable carbohydrate molecules.
  • feedstock e.g., a hydrolyzed feedstock, as described herein, as a source of fermentable carbohydrate molecules.
  • fermentation media in addition to an appropriate carbon source, fermentation media must contain suitable nitrogen source(s), mineral salts, cofactors, buffers, and other components suitable for the growth of the cultures and promotion of the enzymatic pathway necessary for the production of the desired target (e g , biofuel, such as butanol)
  • salts and/or vitamin B 12 or precursors thereof are mcluded in the fermentation media
  • hydrolyzed feedstock may contain some or all of the nutrients required for growth, minimizing or obviatmg the need for additional supplemental material
  • the nitrogen source may be any suitable nitrogen source, including but not limited to, ammonium salts, yeast extract, corn steep liquor (CSL), and other protein sources including, but not limited to, denatured proteins recovered from distillation of fermentation broth or extracts derived from the residual separated microbial cell mass recovered after fermentation ⁇ Clostridium extract)
  • Phosphorus may be present in the medium in the form of phosphate salts, such as sodium, potassium, or ammonium phosphates
  • Sulfur may be present in the medium in the form of sulfate salts, such as sodium or ammonium sulfates
  • Additional salts include, but are not limited to, magnesium sulfate, manganese sulfate, U ⁇ sulfate, magnesium chlo ⁇ de, calcium chloride, manganese chlonde, ferric chlo ⁇ de, ferrous chlo ⁇ de, zinc chlo ⁇ de, cup ⁇ c chloride, cobalt chlo ⁇ de, and sodium moly
  • the culture conditions may be anaerobic, microaerotolerant, or aerobic Aerobic conditions are those that contain oxygen dissolved in the media such that an aerobic culture would not be able to discern a difference in oxygen transfer with the additional dissolved oxygen, and microaerotolerant conditions are those where some dissolved oxygen is present at a level below that found m air or air saturated solutions and frequently below the detection limit of standard dissolved oxygen probes, e g , less than 1 ppm
  • the cultures can be agitated or left undisturbed
  • the pH of the media changes over time as the microorganisms grow in number, consume feedstock and excrete organic acids
  • the solubility of CO 2 produced du ⁇ ng fermentation or present m the media, can also affect pH
  • the pH of the media can be modulated by the addition of buffering compounds to the initial fermentation media in the bioreactor or by the active addition of acid or base to the growing culture to keep the pH in a desired range
  • the temperature is about 25° C to about 35° C.
  • Useful pH ranges for the conversion medium include about 4.0 to about 6.0, about 4.5 to about 6.0, and about 5.5 to about 5.8.
  • the culture is grown under anaerobic conditions without agitation.
  • Clostridium fermentations are generally conducted under anaerobic conditions.
  • ABE fermentations by C. acetobutylicum are typically conducted under anaerobic conditions at a temperature in the range of about 25° C to about 40° C.
  • suspension cultures did not use agitators, but relied on evolved or sparged gas to mix the contents of the bioreactors. Cultures, however, can be agitated to ensure more uniform mixing of the contents of the bioreactor.
  • a bioreactor may be run without agitation in a fixed bed (plug flow) or fluidized/expanded bed (well-mixed) mode.
  • Thermophilic bacterial fermentations can reach temperatures in the range of about 50° C to about 80 0 C. In some embodiments, the temperature range is about 55° to about 70° C. In some embodiments, the temperature range is about 60°C to about 65° C.
  • Clostridium species such as C. thermocellum or C. thermohydrosulfiiricum may be grown at about 60°C to about 65°C.
  • the pH of the Clostridium growth medium can be modulated by the addition of buffering compounds to the initial fermentation media in the bioreactor or by the active addition of acid or base to the growing culture to keep the pH in a desired range. For example, a pH in the range of about 3.5 to about 7.5, or about 5 to about 7, may be maintained in the medium for growth of Clostridium.
  • Immobilization of the microorganism, from spores or vegetative cells can be by any known method.
  • entrapment or inclusion in the support is achieved by polymerizing or solidifying a spore or vegetative cell containing solution.
  • Useful polymerizable or solidifiable solutions include, but are not limited to, alginate, ⁇ -carrageenan, chitosan, polyacrylamide, polyacrylamide-hydrazide, agarose, polypropylene, polyethylene glycol, dimethyl acrylate, polystyrene divinyl benzene, polyvinyl benzene, polyvinyl alcohol, epoxy carrier, cellulose, cellulose acetate, photocrosslinkable resin, prepolymers, urethane, and gelatin.
  • the microorganisms are incubated in growth medium with a support.
  • Useful supports include, but are not limited to, bone char, cork, clay, resin, sand, porous alumina beads, porous brick, porous silica, celite (diatomaceous earth), polypropylene, polyester fiber, ceramic, (e.g. , porous ceramic, such as porous silica/alumina composite), lava rock, vermiculite, ion exchange resin, coke, natural porous stone, macroporous sintered glass, steel, zeolite, engineered thermal plastic, concrete, glass beads, Teflon, polyetheretherketone, polyethylene, wood chips, sawdust, cellulose fiber (pulp), or other natural, engineered, or manufactured products.
  • ceramic e.g. , porous ceramic, such as porous silica/alumina composite
  • lava rock e.g., vermiculite, ion exchange resin, coke, natural porous stone, macroporous sintered glass, steel, zeolite, engineered thermal plastic, concrete, glass beads, Te
  • microorganisms may adhere to the support and form an aggregate, e.g., a biofilm.
  • the microorganism is covalently coupled to a support using chemical agents like glutaraldehyde, o-dianisidine (U.S. Pat. No. 3,983,000), polymeric isocyanates (U.S. Pat. No. 4,071,409), silanes (U.S. Pat. Nos. 3,519,538 and 3,652,761), hydroxyethyl acrylate, transition metal-activated supports, cyanuric chloride, sodium periodate, toluene, or the like. See also U.S. Pat. Nos. 3,930,951 and 3,933,589.
  • immobilized spores such as those of Clostridium, e.g., C. ⁇ cetobutylicum, are activated by thermal shock and then incubated under appropriate conditions in a growth medium whereby vegetative growth ensues. These cells remain enclosed in or on the solid support. After the microorganisms reach a suitable density and physiological state, culture conditions can be changed for bioproduct, e.g. , biofuel, production. If the immobilized cells lose bioproduct, e.g. , biofuel, production, they can be reactivated by first allowing the cells to sporulate before repeating the thermal shock and culture sequence.
  • bioproduct e.g. , biofuel, production
  • Vegetative cells can be immobilized in different phases of their growth.
  • cells can be immobilized after they enter the desired culture phase in order to maximize production of the desired products, where in the case of C. ⁇ cetobutylicum it is the organic acids acetic acid and butyric acid in the acidogenic phase and the solvents acetone, butanol and ethanol in the solventogenic phase.
  • biphasic cells can be immobilized in the acidogenic phase and then adapted for solvent production.
  • microorganisms to be immobilized in a bioreactor are introduced by way of a cell suspension. Generally, these microorganisms are dispersed in the media as single cells or small aggregates of cells.
  • the microorganisms are introduced into the bioreactor through the use of suspended particles that are colonized by the microorganisms. These suspended particles can be absorbed onto the solid support and frequently are of sufficiently small size that they can enter and become immobilized in the pore structures of the solid support. Typically, regardless of the suspended particle size, microorganisms can be transferred by contact with the solid support. A biofilm on the introduced particles can transfer to and colonize these new surfaces.
  • the desired characteristics of the microorganisms can only be maintained by culturing on a solid support, thereby necessitating the use of small colonized particle suspensions for seeding a solid support in a bioreactor.
  • Support for immobilized microbial growth can only be maintained by culturing on a solid support, thereby necessitating the use of small colonized particle suspensions for seeding a solid support in a bioreactor.
  • a bioproduct e.g. , biofuel, producing microorganism is grown in an immobilized form on a solid or semi-solid support material in a bioreactor as described herein.
  • the support comprises a porous material.
  • suitable support materials include bone char, synthetic polymers, natural polymers, inorganic materials, and organic materials.
  • Natural polymers include organic materials such as cellulose, lignocellulose, hemicellulose, and starch.
  • Organic materials include feedstock such as plant residue and paper.
  • Composites of two or more materials may also be used such as mixtures of synthetic polymer with natural plant polymer.
  • semi-solid media examples include alginate, ⁇ -carrageenan and chitosan, polyacrylamide, polyacrylamide-hydrazide, agarose, polypropylene, polyethylene glycol, dimethyl acrylate, polystyrene divinyl benzene, polyvinyl benzene, polyvinyl alcohol, epoxy carrier, cellulose, cellulose acetate, photocrosslinkable resin, prepolymers, urethane, and gelatin.
  • solid support examples include cork, clay, resin, sand, porous alumina beads, porous brick, porous silica, celite, wood chips or activated charcoal.
  • Suitable inorganic solid support materials include inorganic materials with available surface hydroxy or oxide groups. Such materials can be classified in terms of chemical composition as siliceous or nonsiliceous metal oxides.
  • Siliceous supports include, inter alia, glass, colloidal silica, wollastonite, cordierite, dried silica gel, bentonite, and the like.
  • Representative nonsiliceous metal oxides include alumina, hydroxy apatite, and nickel oxide.
  • the support material is selected from bone char, polypropylene, steel, diataomaceous earth, zeolite, ceramic, (e.g., porous ceramic, such as porous silica/alumina composite), engineered thermal plastic, clay brick, concrete, lava rock, wood chips, polyester fiber, glass beads, Teflon, polyetheretherketone, polyethylene, vermiculite, ion exchange resin, cork, resin, sand, porous alumina beads, coke, natural porous stone, macroporous sintered glass, or a combination thereof.
  • the support material is bone char.
  • Useful support material has a high surface area to volume ratio such that a large amount of active, productive cells can accumulate in the bioreactor.
  • Useful supports may contain one or more macrostructured components containing one or more useful support material(s) that promotes good fluid-mechanical properties, for example, a wire mesh/gauze packing material used for traditional distillation tower packing.
  • the support material comprises a surface area of at least about 100 m 2 /m 3 .
  • the support material comprises a bulk density of at least about 0.15 g/cm 3 .
  • the support material comprises a ball-pan hardness number of at least about 60.
  • the support material comprises a yield strength of at least about 20 MPa.
  • the particle size for the support material will vary depending upon bioreactor configuration and operation parameters.
  • the support material is sized by sieving.
  • the particles are classified by the sieve number of the mesh that they can pass through.
  • the particles are sieved with a mesh that has a U.S. Sieve Number of 3 V 2 , 4, 5, 6, 7, 8, 10, 12, 14, 16, 18, 20, 25, 30, 35, 40, 45, 50, 60, or 70.
  • the particles are sieved at least twice, first using a mesh with larger openings followed by a mesh with smaller openings to yield particles within a defined particle size distribution range.
  • the particles are at least about 100 ⁇ m, 200 ⁇ m, 300 ⁇ m, 400 ⁇ m, 500 ⁇ m, 600 ⁇ m, 700 ⁇ m, 800 ⁇ m, 900 ⁇ m, 1000 ⁇ m, 1,100 ⁇ m, 1,200 ⁇ m, 1,300 ⁇ m, 1,400 ⁇ m, 1,500 ⁇ m, 1,600 ⁇ m, 1,700 ⁇ m, 1,800 ⁇ m, 1,900 ⁇ m, 2,000 ⁇ m, 3,000 ⁇ m, 4,000 ⁇ m, 5,000 ⁇ m, 6,000 ⁇ m, 7,000 ⁇ m, 8000 ⁇ m, 9,000 ⁇ m, 10,000 ⁇ m, 12,500 ⁇ m, 15,000 ⁇ m, 17,500 ⁇ m, 20,000 ⁇ m, 22,500 ⁇ m, or 25,000 ⁇ m in diameter.
  • the particles are less than about 100 ⁇ m, 200 ⁇ m, 300 ⁇ m, 400 ⁇ m, 500 ⁇ m, 600 ⁇ m, 700 ⁇ m, 800 ⁇ m, 900 ⁇ m, 1000 ⁇ m, 1,100 ⁇ m, 1,200 ⁇ m, 1,300 ⁇ m, 1,400 ⁇ m, 1,500 ⁇ m, 1,600 ⁇ m, 1,700 ⁇ m, 1,800 ⁇ m, 1,900 ⁇ m, 2,000 ⁇ m in diameter.
  • At least about 80%, 85%, 90%, 95%, or 100% of the particle have diameters that are in the range of about 100-400 ⁇ m, 100-600 ⁇ m, 100-800 ⁇ m, 200-500 ⁇ m, 200-800 ⁇ m, 200-1000 ⁇ m, 400-800 ⁇ m, 400-1000 ⁇ m, 500-1000 ⁇ m, 600-1,200 ⁇ m, 800-1,400, ⁇ m 1,000- 1,500, ⁇ m 1,000-2000 ⁇ m, 2,000-4,000 ⁇ m, 4,000-6,000 ⁇ m, 5,000-12,000 ⁇ m, 3,000-15,000 ⁇ m, or 6,000-25,000 ⁇ m.
  • the particle diameters are the equivalent diameters, a parameter that takes into account the irregular shapes of the individual particles.
  • the semi-solid or solid support material should have a high surface area. This can be achieved through the use of small sized particles, particles with high porosity, or a combination thereof.
  • the surface area of the particles is at least about 0.003 m 2 /g, 0.01 m 2 /g, 0.02 m 2 /g, 0,05 m 2 /g, 0.1 m 2 /g, 0.5 m 2 /g, 1 m 2 /g, 5 m 2 /g, 10 m 2 /g, 25 m 2 /g, 50 m 2 /g, 75 m 2 /g, 100 m 2 /g, 125 m 2 /g, 150 m 2 /g, 175 m 2 /g, 200 m 2 /g, 225 m 2 /g, 250 m 2 /g, 275 m 2 /g, 300 m 2 /g, 325 m 2 /g, 350 m 2 /g, 375 m 2 /g, 400 m 2 /g, 425 m 2 /g, 450 m 2 /g, 500 m 2 /g, 600
  • the bulk density of the support is at least about 0.1 g/cm 3 , 0.2 g/cm 3 , O.3g/cm 3 , 0.4 g/cm 3 , 0.5 g/cm 3 , 0.6 g/cm 3 , 0.7 g/cm 3 , 0.8 g/cm 3 , 0.9 g/cm 3 , 1.0 g/cm 3 , 1.1 g/cm 3 , 1.2 g/cm 3 , or 1.3 g/cm 3 .
  • the support material should have sufficient hardness to resist abrasion and thereby avoid appreciable dust formation when the support particles touch or collide with each other.
  • the support has aball-pan hardness number of at least about 20, 40, 60, 80, 100, 120, 140, 160 or 200.
  • the support material should also have sufficient tensile strength to resist shattering due to internal stresses, which may be caused by the growth of biofilms inside support material pores.
  • the support has a yield strength of at least about 20 MPa, 40 MPa, 60 MPa, 80 MPa, 100 MPa, 120 MPa, 140 MPa, 160 MPa, 180 MPa, 200 MPa, 300 MPa, or 400 MPa.
  • the support material should also have the ability to resist being crushed by the accumulated weight of material above it.
  • Crush strength is another measurement of the mechanical strength of the support and is typically a function of the composition, shape, size, and porosity of the material (increase in port volume may negatively impact particle strength). In some embodiments, the crush strength is at least about 8 kg.
  • the support material is chosen to support growth of the fermenting bioproduct, e.g., biofuel, producing microorganism as a biofihn.
  • the biofilm may grow on exterior surfaces of support particles, in the fluid space between support particles, and/or on surfaces in the interior of pores of the support material.
  • the systems and processes described herein include one or more microorganism(s) that is
  • the microorganisms may be the same or different microbial species and/or different strains of the same species.
  • the microorganisms comprise bacteria or fungi. In some embodiments, the microorganisms comprise a single species. In some embodiments, the microorganisms comprise a mixed culture of strains from the same species, hi some embodiments, the microorganism comprises a mixed culture of different species. In some embodiments, the microorganism comprises an environmental isolate or strain derived therefrom.
  • a fungal microorganism such as a yeast.
  • yeasts include, but are not limited to, Saccharomyces cerevisiae, S bayanus, S carlsbergensis, S Monacensis, S Pastonanus, S uvarum and Kluyveromyces species
  • anaerobic or aerotolerant fungi include, but are not limited to, the genera Neocalhmastix, Caecomyces, Piromyces and other rumen denved anaerobic fungi
  • a bacte ⁇ al microorganism including Gram-negative and Gram-positive bacteria
  • Gram-positive bacteria include bacteria found in the genera of Staphylococcus, Streptococcus, Bacillus, Mycobacterium, Enterococcus, Lactobacillus, Leuconostoc, Pediococcus, and Propionibactenum
  • Non-limiting examples of specific species include Enterococcus faecium and Enterococcus gallinarmm
  • Non-limiting examples of Gram-negative bacteria m clude bacteria found in the genera Pseudomonas, Zymomonas, Spirochaeta, Methylosinus, Pantoea, Acetobacter, Gluconobacter, Escherichia and Erwima
  • the bacteria are Clostridium species, including but not limited to, Clostridium saccharobutylicum, Clostridium acetobutylicum, Clostridium beijennckn, Clostridium puniceum, and environmental isolates of Clostridium
  • Clostridium contemplated for use in this invention can be selected from C aurant ⁇ utyricum, C butyricum, C cellulolyticum C phytofermentans, C saccharolyticum C saccharoperbutylacetomcum, C tetanomorphum C thermobutyricum, C thermocellum, C puniceum, C thermosaccharolyticum, and C pastenanum
  • Other bacteria contemplated for use in the processes and systems herem include Corynebacteria, such as C d ⁇ htheriae, Pneumococci, such as Diplococcus pneumoniae, Streptococci, such as S pyogenes and S salivarus, Staphylococci, such as S aureus and S albus, Myovindae, S ⁇ hoviridae, Aerobic Spore-forming Bacilli, Bacilli, such as B anthracis, B subtihs, B megatermm, B cereus, But
  • the microorganisms comprise Clostridium acetobutyhcum, Clostridium beijerinchi, Clostridium pumceum, Clostridium saccharobutyhcum, Enterococcus faecium, Enterococcus galhnarium, Clostridium aurantibutyricum, Clostridium aurantibutyricum, Clostridium tetanomorphum, or Clostridium thermosaccharolyticum
  • the microorganisms are obligate anaerobes
  • obligate anaerobes include Butyrtvibno fibrosolvens and Clostridium species
  • microorganisms are microaerotolerant and are capable of surviving in the presence of small concentrations of oxygen
  • microaerobic conditions mclude, but are not limited, to fermentation conditions produced by sparging a liquid media with a gas of at least about 0 01% to at least 5% or more O 2 (e g , 0 01%, 0 05%, 0 10%,
  • the microaerobic conditions include, but are not limited to, culture conditions with at least about 0 05ppm dissolved O 2 or more (e g , 005, 0 075, 0 1, 0 15, 0 2, 0 3, 0 4, 0 5, 0 6, 0 8,
  • Microbial strains may be optimized, mutated, or otherwise selected for desirable characteristics
  • parent strains of bacte ⁇ a and fungi may be used for the development of higher product tolerant mutants See, for example, PCT/US09/40050 Sources of such parent strains mclude established culture collections, and researchers in universities, government institutions, or companies
  • parent strains can be isolated from environmental samples such as wastewater sludge from wastewater treatment facilities including municipal facilities and those at chemical or petrochemical plants The latter are especially attractive as the isolated microorganisms can be expected to have evolved over the course of numerous generations in the presence of high product concentrations and thereby have already attained a level of desired product tolerance that may be further improved upon
  • Parent strains may also be isolated from locations of natural degradation of naturally occurring feedstocks and compounds (e g , a woodpile, a saw yard, under fallen trees, landfills)
  • environmental isolates and/or microbial consortiums are used to generate microbial consortiums that have increased product tolerance Isolates, including microbial consortiums can be collected from numerous environmental niches including soil, rivers, lakes, sediments, estuaries, marshes, industrial facilities, etc.
  • the microbial consortiums are strict anaerobes.
  • the microbial consortiums are obligate anaerobes.
  • the microbial consortiums are facultative anaerobes.
  • the microbial consortiums do not contain species of Enterococcus or
  • a selective growth inhibitor for undesired species or genera can be used to prevent or suppress the growth of these undesired microorganisms.
  • cocultures are utilized.
  • one microorganism may secrete enzymes into the media that break down a feedstock into constituent compounds that can be utilized by another microorganism.
  • ethanol may be produced from a coculture of Clostridium thermocellum and C thermohydrosulfuricum (Eng et al. (1981) Applied and Environmental
  • the microorganisms comprise one or more heterologous genes, the expression of which increases the product tolerance of the microorganisms.
  • the one or more heterologous genes are introduced into the microorganism before adaptation on a solid support or selection for product tolerance, while in other embodiments, the one or more heterologous genes are introduced into the microorganisms after adaptation or selection for product tolerance.
  • the microorganisms are engineered to over-express endogenous genes that increase the product tolerance of the microorganisms.
  • the microorganisms comprise additional copy numbers of endogenous genes that increase resistance to products.
  • the product tolerant microorganisms are not E coli and the heterologous or over-expressed genes are not yfdE, yhhL, yhhM, and csrC
  • the microorganisms are not recombinant microorganisms that have increased expression of heat shock proteins.
  • the microorganisms are not recombinant microorganisms that comprise a heterologous gene that encodes a polypeptide that exports butanol out of the microorganism.
  • the microorganism is a Clostridium strain that possesses one or more phenotypic characteristics selected from increased butanol tolerance, increased tolerance to inhibitors of fermentation, low butyric acid and/or acetic acid accumulation, increased stability in continuous fermentation, increased butanol titer, production of biofuel with increased butanol to acetone ratio, increased yield of butanol per unit of feedstock, increased yield of butanol per unit of cellular biomass, increased oxygen tolerance, increased ability to adhere to a solid support, and decreased ability to sporulate, relative to a wild-type or parent Clostridium strain and/or relative to Clostridium saccharobutyhcum B643 (Contag et al (1990) Applied Environmental Microbiology 56 3760-65), Clostridium saccharobutyhcum P262 (ATCC BAA-I l), Clostridium saccharoperbutylacetomcum Nl-4 ATCC 27021, Clostridium aceto
  • the microorganism is a strain, for example, a Clostridium strain, e g , Clostridium acetobutyhcum, Clostridium saccharobutyhcum, Clostridium saccharoperbutylacetomcum, or Clostridium beijerinckn, having tolerance to at least about 2%, 2 5%, 5%, 10%, 12%, or 15% biofuel, m the growth medium by weight, for example, tolerance to at least about 2%, 2 5%, 5%, 10%, 12%, or 15% butanol in the growth medium by weight [217]
  • the microorganism is a mutant strain having at least about 125%, 150%, 200%, 250%, 500%, or 1,000% increased tolerance to a biofuel in the growth medium, for example, at least about 125%, 150%, 200%, 250%, 500%, or 1,000% increased tolerance to butanol in the growth medium, measured by growth of the microorganism in comparison to
  • the fermentation effluent containing the bioproduct may be concentrated and/or purified
  • the product is concentrated prior to further purification using any suitable concentration technique known in the art, including but not limited to distillation, steam stripping distillation, mechanical vapor recompression (MVR) distillation, vacuum distillation, pervaporation, and liquid-liquid extraction
  • the bioproduct is a biofuel, for example, butanol, ethanol, and/or acetone
  • primary components of the fermentation effluent are butanol, acetone, ethanol, butyric acid, and acetic acid, all of which may be recovered and used as starting materials for downstream chemical syntheses to produce derivatives and/or further chemical products
  • Secondary components of the fermentation effluent include, but are not limited to, proteins and other products of metabolic pathways, which may also be used as starting materials for production of derivatives or further chemical products
  • Secondary components include, but are not limited to, solvents, biomolecules (e g , proteins (e g , enzymes), polysaccharides), organic acids (e g formate, acetate, butyrate, propionate, succinate), alcohols (e g , methanol, propanol, isopropanol, hexanol), vitamins, sugar alcohols (e g , xyhtol) Further, chemical
  • fermentation product streams from multiple bioreactors or series of bioreactors are combined prior to further purification
  • fermentation product streams from multiple bioreactors or series of bioreactors are fed to separate purification units
  • a fermentation product stream from a first bioreactor processing C5 sugars can be combined with fermentation products from a second bioreactor processing C5 and C6 sugars
  • the product streams from the first and second bioreactors may be processed separately
  • fermentation broth may be separated from products in situ ( ⁇ e , extractive fermentation) by any of a variety of methods (e g , LLE (liquid-liquid extraction), vacuum distillation, stripping, pervaporation), to mcrease the total productivity of the overall conversion process
  • LLE liquid-liquid extraction
  • MVR distillation is used for concentration of a bioproduct, such as a biofuel, from the microbial fermentation medium.
  • a bioproduct such as a biofuel
  • MVR reduces separation energy requirements by at least about 80% in comparison to conventional distillation.
  • a conventional distillation process is used for the remaining product separation, optionally with thermally cascaded heat integration.
  • separation of biobutanol from fermentation media has been hindered due to the impact of secondary compounds on the separation process. Distillation avoids this issue since surface chemistry is not the basis for the separation.
  • process equipment is selected to optimize energy, water, and/or other metric of interest. In the case of energy use, this may include the addition of heat exchangers to recover stream enthalpy for useful purposes, or to avoid complete condensation or evaporation of feed and/or overhead streams.
  • fermentation broth is passed from a fermentation module to a product recovery module in which solvents ⁇ e.g., butanol, acetone, ethanol) and other volatile compounds are separated from water and less volatile compounds such as biomass residue, carbohydrates and hydrolysis generated sugars. Some water accompanies the solvents and other volatiles in the overhead of the product recovery module.
  • the volatile-water stream may or may not be passed to a decanting operation to increase the effectiveness and efficiency of the remaining product separation.
  • the product recovery overhead stream is passed to a high-low volatile splitter module in which two (or more) streams are generated - a light fraction, a heavy fraction and potentially a mixed solvent side draw.
  • the mixed solvent side draw may contain primarily acetone, ethanol, and water.
  • the light fraction contains primarily acetone, ethanol and water.
  • the light fractions are sent to an acetone column in which acetone is separated from the other components in the feed stream ⁇ e.g. , ethanol and water).
  • the lower volatility stream exiting the high-low volatility splitter (heavy fraction) is passed to a decanter where a phase separation occurs.
  • the upper phase is an organic rich phase which is passed to a butanol column.
  • the upper phase may contain about 80% butanol and about 20% water.
  • the operating temperature and pressure affect the partitioning of compounds in the phases.
  • the phase separation unit may be in fluid contact with a butanol column and a water column.
  • the butanol column separates butanol from an overhead stream primarily comprised of a butanol-water azeotropic stream.
  • the azeotrope stream is returned to the decanter (phase separation operation) for further separation.
  • the aqueous phase of the decanter which may contain nearly or about 9% butanol and about 89% water, is passed to the aqueous column in which water is separated from a mostly butanol-water azeotrope.
  • the butanol-water azeotrope is returned to the decanter for further processing.
  • butyric acid is removed from the butanol product stream formed in the distillation process.
  • butyric acid is adsorbed from the butanol product stream.
  • a tertiary amine ion-exchange resin may be used for adsorption of butyric acid.
  • butanol and butyric acid are separated by distillation.
  • butanol and butyric acid are separated by pervaporation.
  • the butyric acid is removed and may be sold as a chemical product.
  • the butyric acid is returned to the solventogenic portion of the process, and may be added to the fermentation medium in the bioreactor as a feedstock which may be converted to butanol by the fermenting microorganism.
  • furfural is removed from the butanol product stream formed in the distillation process.
  • furfural is adsorbed from the butanol product stream.
  • a tertiary amine ion-exchange resin or activated carbon may be used for adsorption of furfural.
  • butanol and furfural are separated by pervaporation.
  • butanol and furfural are separated from one another through the use of a solvent, such as triocyl-phosphine oxide (TOPO).
  • TOPO triocyl-phosphine oxide
  • the furfural is removed and may be sold as a chemical product.
  • other products are removed from the butanol product stream to remove impurities from the butanol product stream and recovered as useful products, for example, acetic acid, butyric acid, HMF, extractives.
  • Biobutanol produced according to the methods described herein may also serve as a platform molecule for the production of other compounds.
  • butanol may be converted into propylene, from which a wide variety of plastics and other compounds may be produced.
  • a mixture of butanol, dibutyl ether (a derivative of butanol), and plant oil in specified proportions may constitute a full performance diesel fuel.
  • butanol may be converted into full performance jet fuel.
  • Biobutanol produced according to the methods described herein may also be used as an intermediate chemical for producing other chemical products, including but not limited to, butyl aery late, n-butyl acetate, and glycol ethers. It may also be dehydrated to produce 1-butene, which may be oligomerized to produce other products, including but not limited to, jet fuel, diesel fuel, lubricants, or alpha olefins. Butanol may also be used directly to produce butene derivatives Any of these derivatives of butanol may be produced using chemical processes that are well known in the art.
  • a continuous process for bioproduct, e g , biofuel, production is provided
  • a carbohydrate-containing feedstock is continuously pretreated to produce soluble sugar molecules
  • the pretreated feedstock containing soluble sugar molecules is continuously fed to one or more bioreactors for microbial production of the bioproduct, e g , biofuel
  • the bioproduct is continuously produced by immobilized microorganism(s) in the one or more bioreactors
  • bioproduct-contaimng effluent, i e , fermentation broth is continuously withdrawn from the one or more reactors, for the duration of fermentation
  • the feedstock is continuously hydrolyzed to release soluble sugar molecules
  • the feedstock is lignocellulosic feedstock, and is hydrolyzed with nitric acid to release soluble sugar molecules from cellulose and hemicellulose, as described supra
  • the continuous process may also include downstream continuous concentration and/or purification processes for recovery of the bioproduct, e g , biofuel, product, wherein continuously withdrawn effluent is continuously processed in one or more concentration and/or purification processes to produce a bioproduct
  • the process may also include a conditioning process to remove inhibitors of microbial growth or bioproduct, e g , biofuel, production, as described herein
  • the conditioning process may operate continuously downstream from a feedstock hydrolysis process, and upstream from the bioreactor(s), and conditioned hydrolyzed feedstock may be continuously fed to the bioreactor for the duration of fermentation
  • the process may also include deconstruction of the feedstock and/or removal of extractives from the feedstock, as descnbed herein Deconstruction and/or removal of extractives may be continuous or may occur prior to or periodically throughout the continuous process
  • the process operates continuously for at least about 50, 100, 200, 300, 400, 600, 800, 1000, 1350, 1600, 2000, 2500, 3000, 4000, 5000, 6000, 7000, 8000, or 8400 hours
  • a "continuous" process as described herein may include periodic or intermittent partial or complete shutdowns of one or more parts of the bioproduct, e g , biofuel, production system for processes such as maintenance, repair, regeneration of resin, etc
  • Continuous fermentation, with constant feed of hydrolyzed feedstock and withdrawal of product-containing microbial broth can minimize the unproductive portions of a fermentation cycle, such as lag, growth, and turnaround time, thereby reducing the capital cost, and can reduce the number of inoculation events, thus minimizing operational costs and risk associated with human and process error.
  • the continuous methods and systems described herein can utilize one or more, e.g., one, two, or three or more, bioreactors. When multiple (two or more) bioreactors are used, they may be arranged in parallel, series, or a combination thereof.
  • the bioreactors can grow the same or different strains of microorganism(s). The strains can be different based on the type of sugar they metabolize to maximize bioproduct, e.g., biofuel, production.
  • a first bioreactor or multiple bioreactors arranged in parallel, series, or a combination thereof can grow a strain that has been selected to metabolize C5 sugars and a second bioreactor or multiple bioreactors arranged in parallel, series, or a combination thereof can grow another strain that has been selected to metabolize C5 and C6 sugars.
  • the bioreactors are coupled to an upstream feedstock hydrolysis unit, and may also be coupled to a downstream recovery/separation unit.
  • the connection may be interdigitated, such that some product separation may occur between primary and/or secondary and/or further reactors in series.
  • a first bioreactor or multiple bioreactors arranged in parallel, series, or a combination thereof with a strain that metabolizes C5 sugars can be coupled to an upstream first stage hydrolysis module of a nitric acid hydrolysis unit for hydrolysis of lignocellulosic feedstock.
  • a second set of bioreactors or multiple bioreactors arranged in parallel, series, or a combination thereof with a strain that metabolizes C5 and C6 sugars can be coupled to an upstream second stage hydrolysis module of a nitric acid hydrolysis unit for hydrolysis of a lignocellulosic feedstock.
  • the same bioreactor or multiple bioreactors arranged in parallel, series, or a combination thereof may be used for conversion of both C5 and C6 sugars to bioproduct, e.g., biofuel.
  • bioproduct e.g., biofuel.
  • both first and second stage nitric acid hydrolysates of a lignocellulosic feedstock may be added either separately or as a combined mixture to the bioreactor(s).
  • butanol may be produced by a microbial strain, such as a Clostridium strain, at a titer of about or at least about 5, 6, 7, 8, 10, 12, 15, 20, 25, 30, 40, 50, 60, 70, 80, or 90 g butanol per liter, or about 5 to about 90, about 5 to about 10, about 8 to about 20, about 15 to about 30, about 25 to about 50, about 40 to about 80, or about 60 to about 90 g butanol per liter.
  • Titer may be affected by ambient conditions (e.g., pressure/temperature) and composition (acetone, salts, etc.).
  • butanol may be produced by a microbial strain, such as a Clostridium strain, with a yield of about or at least about 30, 35, 40, 50, or 60% or about 30% to about 60%, about 40% to about 60%, or about 50% to about 60%
  • butanol may be produced by a microbial strain, such as a Clostridium strain, with a productivity of about or at least about 1, 3, 5, 10, 15, or 20 g, butanol per liter per hour, or about 1 to about 20, about 3 to about 10, about 5 to about 15, or about 10 to about 20 g butanol per liter per hour
  • water saturated butanol may be skrmmed off the top of the liquid or separated by equipment known in the art for the separation of two liquid phases in the bioreactor, for further processing/product recovery operations
  • the invention provides a system for continuous production of a bioproduct, e g , biofuel, i e , for conducting a continuous bioproduct production process as descnbed herein
  • the system contains a feedstock hydrolysis unit upstream from and m fluid communication with one or more bioreactor(s)
  • a carbon-containing feedstock is continuously hydrolyzed in the hydrolysis unit to produce soluble sugar molecules, and the hydrolysate is continuously fed to the bioreactor(s) as a carbon source to support microbial growth
  • One or more immobilized microorganism(s) m the bioreactor(s) continuously convert the hydrolysate into a bioproduct, e g , biofuel, and bioproduct- containing effluent is continuously withdrawn from the system
  • the system contains multiple bioreactors arranged in parallel, series, or a combination thereof
  • multiple bioreactors in parallel are all in fluid communication with a single hydrolysis unit or multiple bioreactors in parallel are each in fluid communication with a different hydrolysis unit wherein the hydrolysis units are arranged in parallel and each feed a different bioreactor, and hydrolyzed feedstock is fed continuously to each bioreactor, with effluent continuously withdrawn from each bioreactor
  • the system contains multiple bioreactors arranged in senes, the first bioreactor in the series is m fluid communication with the hydrolysis unit, and hydrolyzed feedstock is fed continuously to the first bioreactor in the senes, with effluent continuously withdrawn from each bioreactor and fed to each subsequent downstream bioreactor in the series, and effluent from the last bioreactor in the series continuously withdrawn from the system
  • the system for bioproduct, e g , biofuel, production operates with the bioreactor(s) under pressure to compress gas in the bioreactor(s), including CO 2 generated by the microorganisms during fermentation CO 2 generated during fermentation effectively reduces the liquid volume in the bioreactor, thus decreasing the residence time of the liquid hydrolyzed feedstock Compression of gas in the bioreactor has the effect of increasing residence time of the hydrolyzed feedstock in the reactor, which improves utilization of the sugar molecules in the feedstock and conversion of the sugar to bioproduct, e g , biofuel, for example, butanol Operation under pressure impacts the solubility of gaseous species (CO 2 and H 2 ) and may affect fermentation parameters of interest, such as product yield, selectivity and/or productivity, for example, by affecting the redox potential, pH, or other parameters Hydrolyzed feedstock may be added to the bioreactor continuously under pressure
  • the pressure in the bioreactor may be about 1 to about 30 arm, or about or at least about 1,
  • the system may also include downstream continuous concentration and/or purification modules for recovery of the bioproduct, e g , biofuel, product, for processing of continuously withdrawn effluent to produce a bioproduct
  • the system includes a module for concentration of the bioproduct-contaming effluent, in fluid communication with and downstream from the bioreactor(s) hi one embodiment, concentration mcludes distillation
  • distillation comprises MVR hi a further embodiment
  • the system includes a module for purification of bioproduct, e g , biofuel, from the concentrated bioproduct- contaming effluent, in fluid communication with and downstream from the concentration module hi one embodiment, purification includes distillation
  • the system may also include a conditioning unit for removal of inhibitors of microbial growth or bioproduct, e g , biofuel, production, as described herein
  • the conditioning unit may operate continuously downstream from and m fluid communication with the feedstock hydrolysis process, and upstream and in fluid communication with the bioreactor(s), and conditioned hydrolyzed feedstock may be continuously fed to the bioreactor for the duration of fermentation hi one embodiment, the conditioning unit includes ion exchange resin, and the inhibitors are retained on the resm In another embodiment, the conditioning unit includes a precipitation unit and the inhibitors are removed with the separated precipitate In a further embodiment, inhibitory compounds are separated from the hydrolysate in a steam stripping operation.
  • the system may also include units for deconstruction of the feedstock and/or removal of extractives from the feedstock, as described herein.
  • Deconstruction and/or removal of extractives may operate continuously upstream and in fluid communication with the hydrolysis unit, or may occur prior to or periodically throughout the continuous process.
  • the bioproduct e.g. , biofuel, production processes and systems described herein may include one or more energy integration systems, for capturing and recycling energy generated in one part of the bioproduct production process and using the captured energy to drive another part of the process.
  • the energy integration schemes described herein include integration between process areas and effect a global change to the overall plant energy use.
  • flash steam generated in the first stage and/or second stage hydrolysis process(es) may be captured and used for deconstruction of the feedstock prior to hydrolysis.
  • flash steam generated in the second stage hydrolysis process may be recompressed and the recompressed steam used to provide energy for the first stage hydrolysis.
  • the flash stream is not compressed.
  • flash steam generated as part of the hydrolysis process may be used to provide lie steam for steam stripping operations, to preheat streams, remove inhibitory compounds from hydrolysate, and/or to facilitate product separation and recovery operations.
  • flash steam is generated in the second stage hydrolysis process may be used to provide energy for a third stage hydrolysis, with the temperature of the third stage lower than the temperature of the second stage, and with the temperature and/or residence time of the second stage reduced in comparison to a process without the third stage, thus permitting hydrolysis of remaining oligomeric sugar molecules with less degradation than hydrolysis performed at a higher temperature than the temperature of the third stage.
  • This method could also be extended to four or more stages of hydrolysis with decreasing temperature in a cascade effect.
  • flash steam generated in the second stage is used to provide energy for the first stage
  • flash steam generated in the first stage is used to provide energy for the third stage.
  • flash steam generated in the first and/or second stage hydrolysis process may be recompressed and the recompressed steam is used to provide energy for a distillation process for purification of bioproduct, e.g., biofuel, from bioproduct containing effluent from continuous microbial fermentation, as described supra.
  • bioproduct e.g., biofuel
  • flash steam generated in the first and/or second stage hydrolysis process may be used to provided energy for preheating a feed stream to a distillation process for purification of bioproduct, e.g., biofuel, from bioproduct containing effluent from continuous microbial fermentation, as described supra.
  • bioproduct e.g., biofuel
  • the flash steam may optionally be recompressed prior to use for preheating the feed stream.
  • flash steam generated in the first and/or second stage hydrolysis process may be recompressed and the recompressed steam is used to provide energy for drying and/or dehydration of products separated in a distillation process as described supra.
  • the recompressed steam may be used to provide energy for drying and/or dehydration of biomass from the fermentation process.
  • lignin is recovered in the solids-containing residue remaining after hydrolysis of lignocellulosic feedstock, for example, in the solids-containing residue remaining after the second stage of a two stage nitric acid hydrolysis process, as described supra.
  • the lignin- containing residue may be used as an energy source for the bioproduct, e.g., biofuel, production process, as a fuel source for electricity generation, as a feedstock for chemical production, for example, production of phenolic resins, and/or as a soil enhancer.
  • An integrated plant is provided that can produce a bioproduct, such as a biofuel.
  • a bioproduct such as a biofuel.
  • biobutanol may be produced from a wide variety of feedstocks in a capital and energy efficient process, with low greenhouse gas (GHG) emissions and the potential to make a significant contribution to reducing oil imports, achieving advanced biofuels targets, developing a domestic bioindustry, creating jobs, and promoting economic development
  • GHG greenhouse gas
  • Embodiments of such an integrated biofuel, e g , biobutanol, plant, utilizing processes and systems for continuous biofuel production desc ⁇ bed herein, are schematically depicted in Figures 1-3 [261]
  • a biorefinery as described herein may provide an economic benefit, the production of bioproducts with a reduced carbon intensity (emission, footprint) as compared to petrochemically derived counterparts
  • the primary driver for this reduction in carbon intensity is the relatively rapid utilization of carbon in the feedstock as compared to petroleum based chemical
  • An integrated bioproduct, e g , biofuel, plant can be built to a variety of capacities In some instances, a pilot plant has the capacity to process one to five dry tonne(s) of feedstock per day
  • the feedstock for the plant can be cellulosic biomass, for example, lignocellulosic biomass such as woody biomass, which may be sourced locally and is available in many regions of the country
  • Pretreatment of the biomass can be accomplished an acid hydrolysis process, such as a two stage dilute acid process to extract soluble sugars from the hemicellulose and cellulose
  • these sugars can be fermented to biofuel, e g , biobutanol, using Clostridium strains
  • a Clostridium strain can produce w-butanol from both monomelic and multime ⁇ c forms of both C5 and C6 sugars Fermentation can occur in an immobilized bed bioreactor running a continuous process, which can deliver up to or more than ten times the
  • the integrated bioproduct, e g , biofuel, production plant can be a fully integrated standalone facility In addition to the operations contamed in the integrated plant, the facilities can include feedstock storage and handling, product storage and loadout, and on-site utilities
  • the integrated plant can have one or more streams to recover heat and/or materials For example, recycle streams can be used to improve efficiency of separation processes or bioconversion processes Other streams can be used for heat exchange from one process unit to another, or within a process unit [266]
  • an integrated bioproduct, e g , biofuel, production plant may be co- located to utilize a waste stream, such as hemicellulose from a pulp mill, to achieve economic advantages gained through co-location and co-utilization of utilities, feed handling, feed logistics, off-take, chemical production, etc
  • the bioproduct, e g , biofuel, production plant can utilize one or more hydrolysis stages for feedstock preparation, one or more conditioning processes to prepare hydrolysates for bioconversion, one or more fermentors for growing one or more strains that are capable of producing a bioproduct such as butanol and optionally other products of interest, and one or more separation processes to isolate the desired products
  • the various processing units can be designed and coordinated such that the complete operation of the plant is in a continuous manner Accumulation of products or feed materials between process operations can be avoided Residence time of processed materials prior to being fed to a downstream operation can be reduced to avoid undesirable degradation or modification of materials Rates of processing for upstream processing units can be controlled based on performance of downstream processing units and vice-versa For example, if a reduction in bioconversion by a microbial stram is observed, the rate of hydrolysis of a feedstock can be reduced such that accumulation of products is avoided
  • commercial plant output can mclude butanol as the primary product, acetone, a mixed solvent containing acetone, ethanol and sugar degradation products, and hgnin Per tonne of a particular feedstock, the plant can produce about or at least about 53 5 gallons of butanol, 4 1 gallons of acetone, 0 039 tonnes of mixed solvents and 0419 tonnes of a hgnin
  • the butanol and acetone can be sold into the fuels and chemicals markets, respectively
  • the mixed solvents (which may mclude acetone, ethanol, butanol, degradation products, woody biomass compounds, fermentation byproducts, fermentation generated biomass, and/or water) and most of the hgnin can be used in an onsite co-generation unit to generate all of the steam and electricity required to operate the plant, and the remaining hgnin can be dned to remove water, for example to about 15% moisture content, and sold as boiler fuel
  • An integrated biobutanol plant can produce butanol at a variety of scales.
  • Butanol can be produced at pilot scale at about 13,000 gallons per year, at demonstration scale at about 2 to 2.5 million gallons per year (consuming about 150 tonnes of feedstock per day) and at commercial scale at about 50 million gallons per year.
  • the plant can produce about or at least about 0.08 gallons of acetone and about or at least about 2.7kg of lignin.
  • the estimated feedstock consumption of the commercial plant can be about 2,700 dry tonnes per day (112,500 dry kg/hr), based on a yield of 53 gallons of biobutanol per tonne of feedstock.
  • the amount of butanol that can be produced per tonne of feedstock can be about, up to about or at least about 10, 20, 30, 40, 50, 60, 70, or 80 gallons.
  • a petroleum analysis indicates a displacement of 2.7 million equivalent barrels of oil annually for a 50 million gallon per year facility.
  • the plant can be located in numerous areas in the country where this amount of forest waste, with sufficient surplus to avoid market pressure, is available locally.
  • the plant can include all of the unit operations of the feedstock bioconversion, plus feedstock handling and product distribution and load out operations.
  • the commercial facility can have its own biomass- f ⁇ red power plant on site, which can use lignin in the solids-containing residue remaining after feedstock hydrolysis, the small amount of ethanol and a portion of the acetone produced in the fermentation process recovered in the distillation system, plus furfural and HMF extracted from the feedstock to provide all of the steam and electricity required by the process, with excess lignin sold to offsite power facilities.
  • the facility may require about or at least about 20,000, 30,000, 40,000, 50,000, 60,000, 70,000, 80,000, 90,000, 100,000, 150,000, 200,000, 250,000, 300,000, 350,000, 400,000, 450,000, or 500,000 BTUs of thermal energy per gallon of butanol, about or at least about 1, 1.5, 2, 2.5, 3, 3.5, 4, 5, or 10 kilowatt hours per gallon and about or at least about 1, 2, 3, 4, 5, 6, 7, 8, 10, 20, or 30 gallons of water per gallon of biobutanol produced, depending on the process configuration.
  • These numbers can be reduced, including further reductions in the estimated water usage.
  • air coolers can be used whenever possible to reduce cooling tower evaporative losses and minimize the fresh water footprint.
  • the equipment for an integrated bioproduct production plant as described herein can be purchased from commercial manufacturers of industrial process equipment.
  • the equipment materials can be selected based on corrosion and erosion resistance.
  • the equipment materials can be evaluated for the hydrolysis processes, which may be performed under acidic conditions at elevated temperatures and pressures
  • the equipment design does not require the use of exotic materials or specialized equipment available from a single or limited number of vendors
  • pretreatment vessels can be made of stainless steel (e g , Duplex 2205) rather than the expensive alloys often required in other processes Spare parts can be kept at the plant to ensure continuous processing without a lengthy interruption or turnaround
  • An integrated bioproduct for example, biofuel, e g , biobutanol production plant can include a high degree of instrumentation and control using a supervisory control and data acquisition (SCADA) system and/or distributed control system (DCS) These systems collect real time data on a wide range of performance parameters and the data may be used to optimize process control parameters, setpoints, and conditions
  • SCADA supervisory control and data acquisition
  • DCS distributed control system
  • SCADA supervisory control and data acquisition
  • DCS distributed control system
  • a variety of products can be produced using the systems and methods descnbed herein These products include butanol, acetone, ethanol, green gasoline, and mixed alcohols Other products include lignin, cellulose, hemicellulose, sugars, acids, or any other product described herein Natural products such as xylitol, vitamin B 12, and other compounds may be separated m the production process to improve plant economics Organic products that can be used as a fuel can be blended with each other, or blended with additional materials For example, butanol can be blended with gasolme or any other combustible fuel [276] Butanol produced by the systems and methods described herein, including fermentation and separation, can be at a purity of about or at least about 30, 40, 50, 60, 70, 75, 80, 85, 90, 95, 97, 99, 99.5, 99.8, 99.9, or 99.99%.
  • Acetone produced by the systems and methods described herein, including fermentation and separation can be at a purity of about or at least about 30, 40, 50, 60, 70, 75, 80, 85, 90, 95, 97, 99, 99.5, 99.8, 99.9, or 99.99%.
  • Ethanol produced by the systems and methods described herein, including fermentation and separation can be at a purity of about, up to about, or greater than about 30, 40, 50, 60, 70, 75, 80, 85, 90, 95, 97, 99, 99.5, 99.8, 99.9, or 99.99%.
  • Butanol produced by the systems and methods described herein, after fermentation or separation, can be a blend of butanol, acetone, and ethanol.
  • the blend can be 70 parts butanol to 30 parts acetone. This can be determined on an organic solvent basis, excluding water.
  • the blend can include butanol:acetone:ethanol at a ratio of 33:12:1, 58:12:1, or 90:9:1.
  • Butanol production for a commercial plant can be about 50 million gallons of butanol per year.
  • a plant may be designed to produce less than about 1 million gallons per year of butanol, or about 1 to about 2, about 2 to about 5, about 5 to about 10, about 10 to about 50, about 20 to about 50, about 30 to about 50, about 40 to about 50, or about 45 to about 50 million gallons per year of butanol.
  • Lignin separated in an integrated bioproduct production plant as described herein in the form of lignin-containing residue remaining after hydrolysis of lignocellulosic feedstock, can be stored or processed by a lignin handling and storage unit.
  • this unit operation can process the lignin-containing residual material from the second stage acid hydrolysis of lignocellulosic feedstock, as described supra, including unconverted cellulose and hemicellulose material.
  • the lignin product stream can be dried, for example, using hydrolysis flash steam. At about 35 wt% moisture, the material will have a usable heating value.
  • the material can be further dried to improve the product value, for example, to about 15 wt% moisture, subsequently pelletized, and stored for sale as fuel, for example, for electricity generation or burned as dried to provide thermal energy.
  • Dried, pelletized lignin may also be used to generate high pressure steam to provide energy for use in first and second stage nitric acid hydrolysis processes for hydrolysis of lignocellulosic feedstock, as described supra.
  • biomass can be removed from the fermentation broth during the product separation and distillation phase.
  • the recovered material can be dried and burned for process heat or can be digested to generate methane and remove the cellular mass without release to the environment.
  • the effluent streams from a nitric acid pretreatment process can contain significant levels of nitrogen. Ammonium nitrate created during neutralization of nitric acid can be converted to nitrogen and water Ammonium nitrate containing solutions may also be used as feedstocks for subsequent microbial water treatment ponds.
  • the following examples are intended to illustrate, but not limit, the invention
  • Clostridium strains were grown in 100 mL or 1 L continuous packed bed bioreactors for lengths of time as shown in Table 1
  • Co-7449 is a strain of Clostridium saccharobutylicum that is very stable in continuous culture, possesses increased acid recycle capabilities in comparison to wild-type, and utilizes mixed sugars in a softwood hydrolysate well
  • Co-5673 an environmental isolate of Clostridium, is also stable in continuous culture, and possesses increased tolerance to acids.
  • the microbial cells were grown anaerobically on bone char, using a sugar substrate Butanol titer, yield, and performance are included m Table 1, calculated using the best sustained performance (100 hours or more) for each fermentation. Substrate concentrations in the table are expressed as weight of substrate per volume of liquid Data from representative fermentation runs is presented m Figures 6-12.
  • a continuous biobutanol production and recovery process is described below, with all of the described component processes (e.g., feedstock hydrolysis, fermentation, recovery of product) operating simultaneously and continuously in an integrated biobutanol production plant.
  • component processes e.g., feedstock hydrolysis, fermentation, recovery of product
  • C5 and C6 sugars are produced from hemicelluloses and cellulose components of wood chips in a two-stage dilute nitric acid hydrolysis process.
  • the two-stage approach includes two reaction stages at two different temperatures, minimizes thermal degradation products and maximizes sugar recovery from both the hemicelluloses and cellulose components of the feedstock.
  • Wood chips are mixed with nitric acid and water and pressured into the first stage hydrolysis reactor using a progressive reducing screw auger.
  • the first stage hydrolysis reactor operates at or around 175 0 C using 115 psig steam and is sized to provide a residence time of 5 to 9 minutes.
  • a discharge auger and blow valve deliver reactor effluent to a flash tank where low pressure steam is recovered for re-use in the process.
  • the steam may be augmented by recovered steam from other operations.
  • C5 hydrolysate is separated from the unconverted biomass in a screw press, stripped with nitrogen for oxygen removal, and pumped to the C5 fermentation section of the biobutanol production plant.
  • stage 1 hydrolysate liquor contains nearly all of the C5 sugars, and as a matter of nomenclature has been termed "C5 hdyrolysate” herein.
  • the C5 hydrolysate is brought to about pH 3.5 with ammonium hydroxide and passed through an anion exchange resin bed upstream of fermentation.
  • the screw press may include a solids wash step to maximize recovery of fermentable sugars.
  • Residual uncoverted biomass from the first stage hydrolysis is mixed with nitric acid and water and pressured into the second stage hydrolysis reactor using a progressive reducing screw auger.
  • the second stage hydrolysis utilizes a higher temperature than the first stage hydrolysis to break down the recalcitrant cellulose component.
  • the second stage reactor operates by injecting saturated live steam at 215°C (with the relationship between temperature and pressure well known by those of skill in the art) and is sized to provide a residence time of 3-8 minutes.
  • a discharge auger is used to deliver reactor effluent to a flash tank where additional low pressure steam is recovered.
  • the C6 hydrolysate is separated from solids containing unconverted cellulose and lignin in a screw press, stripped with nitrogen for oxygen removal, evaporated to remove water and some acetic acid, brought to about pH 3.5 with ammonium hydroxide, passed through an anion exchange resin bed (e.g., Duolite A7), and pumped to the C6 fermentation section of the biobutanol production plant.
  • the screw press separation also contains a solids wash step to maximize recovery of fermentable sugars. Residual cellulose/lignin is either neutralized and disposed of or steam dried and utilized as boiler fuel for process steam and/or electricity generation.
  • Neutralized C5 hydrolysate from the first stage hydrolysis unit operation is cooled to fermentation temperature, treated to remove fermentation inhibitors via anion exchange as discussed above, mixed with nutrients and charged to a bioreactor or the first bioreactor in a series of bioreactors.
  • the C5 hydrolysate is fermented into biobutanol in the bioreactor using an immobilized Clostridium strain that has been selected to maximize titer, yield, and butanol selectivity for C5 hydrolysate.
  • the fermentation process also produces fermentation off gas, primarily carbon dioxide and hydrogen, which strips some solvent from the bioreactor. All three reactors operate near atmospheric pressure and include a heating/cooling jacket to maintain temperature at 32°C. Each of the reactors includes a controlled nitrogen purge into the vapor space that is sampled and vented to a vent gas treatment unit operation along with fermentation off gas.
  • the fermentation is carried out in a temperature controlled bioreactor under anaerobic conditions after supplementing the hydrolysate with nutrients for growth of the microorganism. After colonization of the bioreactor by the microorganism is achieved, a continuous feed of supplemented hydrolysate is started together with the simultaneous continuous withdrawal of the same amount of fermentation broth.
  • Neutralized C6 hydrolysate from the second stage hydrolysis unit operation is cooled to fermentation temperature, treated to remove fermentation inhibitors via anion exchange as discussed above, mixed with nutrients and charged to a separate bioreactor or a series of bioreactors.
  • the C6 fermentation unit operation is nearly identical to the C5 fermentation, discussed above, with the exception that the specific strain of Clostridium has been optimized to maximize titer, yield, and butanol selectivity for C6 hydrolysate. Alternatively, the same strain is used for both C5 and C6 fermentations in the same or separate bioreactors.
  • Reactor effluent from the C5 and C6 fermentations is combined into a product recovery feed tank (or “harvest tank") where fermentation continues before being fed to the product recovery distillation column feed tank.
  • Fermentor effluent is pumped from the feed tank to the distillation column where the dilute product stream is concentrated, for example from about 2.5 wt% total organics in the feed to about 50 wt% in the overhead liquid product or from about 1 wt% total organics to about 35 wt% in the overhead liquid product.
  • Overhead vapor from the distillation column is condensed in the overhead condensor.
  • the recovered bottoms stream is passed through a heat exchanger, where energy is exchanged with the column feed stream to recover energy.
  • the overhead stream is pumped to additional separation equipment for further purification of separate biofuel products, for example, acetone, butanol, and ethanol.
  • Organic products are further purified from the concentrate by distillation. For example, high purity butanol and acetone may be produced with some ethanol removed via a side draw.
  • Example 3 Two-stage nitric acid hydrolysis of lignocellulosic feedstock in a batch reactor
  • Nitric acid hydrolysis of a lignocellulosic feedstock was performed in two stages.
  • the feedstock was beetle killed lodgepole pine obtained through Renewable Fiber in Fort Lupton, CO.
  • Three quarter inch wood chips were milled to pass through a 1 A inch screen.
  • Approximately 1.3% nitric acid on a dry wood basis was reacted with feedstock in a 1.9 L reactor. The milled % inch wood chips were loaded into a five gallon bucket and charged with water and nitric acid.
  • the nitric acid concentration was approximately 1.3% on a dry wood basis and water was added to the bucket to completely submerge the wood chips.
  • the total solids loading of the mixture was approximately 12 wt%, which corresponded to a liquids to solids ratio of approximately 7.5.
  • the bucket was then sealed and placed on rollers where the contents of the bucket mixed for approximately 30 minutes. This step was done to impregnate the acid into the wood chips.
  • the contents of the bucket were then transferred to the 1.9 L reactor, where the hydrolysis reaction took place.
  • the reactor was sealed and charged with steam in order to reach a reaction temperature of 175 °C.
  • the time that the contents of the reactants were at this temperature was approximately 7 minutes, after which the contents of the reactor were flashed into a vessel at atmospheric pressure with additional cooling to rapidly cool the material and stop the hydrolysis reaction.
  • the pH of the solution was approximately 2 during the reaction.
  • the reaction mixture was separated using a vacuum filtration unit into first stage hydrolysate and solid residue.
  • the first stage hydrolysate was analyzed for conversion of cellulose and hemicellulose to soluble sugar molecules using high performance liquid chromatography (HPLC).
  • HPLC high performance liquid chromatography
  • the yields of soluble sugars based on cellulose and hemicellulose conversion were calculated by measuring sugars produced from complete hydrolysis of cellulose and hemicellulose concentrations in the starting material. Concentrated acid was used to hydrolyze both the cellulose and hemicellulose fractions of the wood. A theoretical maximum amount of sugar was then calculated based on the conversion of cellulose and hemicellulose to sugars. The yield from the dilute nitric acid hydrolysis was then compared to the theoretical maximum.
  • the solid residue from the first stage hydrolysis was rinsed with water to remove residual soluble sugars from the solids and to minimize the amount of sugar degradation in the second stage hydrolysis reaction.
  • a nitric acid concentration of approximately 1.3 wt% on a dry solids basis was used to for hydrolysis of the solid residue.
  • the residual solids were contacting with acid in a rolling bucket for approximately 30 minutes, as described above.
  • the solids loading was approximately 14 wt%, or a ratio of about 6.5 liquid to solids.
  • the acid impregnated residual material was then transferred to the 1.9 L reactor and injected with steam.
  • the operating temperature of the second stage hydrolysis reaction was approximately 220°C.
  • the contents in the reactor were heated to 220 0 C for approximately 4.5 minutes and then flashed into a flash vessel to rapidly cool the reactants and stop the reaction.
  • the pH of the solution was approximately 2 during the reaction.
  • the reaction mixture was separated into second stage hydrolysate and residual biomass using a vacuum filtration process.
  • the second stage hydrolysate was analyzed for conversion of cellulose and hemicellulose to soluble sugar molecules, as described above. 23% of hydrolyzed cellulose was detected as soluble sugars (glucose and oligomers) and 0% of hydrolyzed hemicellulose was detected as soluble sugars (xylose, mannose, and other oligomers) in the second stage hydrolysis reaction.
  • Example 4
  • Duolite A7 resin was used for conditioning of the first stage hydrolysate.
  • the anion exchange resin was prepared using a 1 M solution of sodium hydroxide and then rinsed with distilled water.
  • Effluents from the fermentations with conditioned and unconditioned hydrolysate were analyzed by HPLC. Based on the HPLC analysis, an increase in an unidentified peak correlates well with the inhibited growth that was observed with the microorganism. Therefore, this peak may have played a role in the toxicity of the hydrolysate. Based on the residence time in the HPLC column, the peak is believed to contain a phenolic compound that is strongly related to toxicity.
  • Duolite A7 is a phenolic based anion exchange resin, so it is possible that the postulated phenolic inhibitor compound was retained on the resin due to hydrophobic interaction with phenolic groups on the resin.
  • Clostridium saccharobutylicum Co-7449 (PCT/US09/40050) was grown anaerobically in a packed bed bioreactor with 110 L nominal volume and 63.7 L working volume. The L/D ratio of the bioreactor was 8.
  • the Clostridium was immobilized on bonechar.
  • the bonechar particles had a size of 3000 to 5000 microns, with a bulk density of about 0.72 /ml. About 100 pounds of bonechar was loaded into the reactor. Immobilization was achieved by first filling the reactor with about 40 L of CP3 media with 4% sucrose and then adding to the reactor 20 L of Clostridium broth that had an OD at 600nm of about 1, and recalculating the contents of the reactor for 24 hours.
  • the growth medium was essentially identical to P2 medium, as described in Jesse et al. (2002) Journal of Industrial Microbiology and Biotechnology 29:117-123, with 4% sucrose as carbohydrate feed.
  • the feed rate for the run was initially 800 g/min, was reduced to 400 g/min at about 60 hours, and was increased to 500 g/min at about 143 hours.
  • the average pH was about 4.95 and the average pressure was about 3.24 psi.
  • N 2 was added at a rate of 0.7 L/min for the duration of the fermentation.
  • the average butanol titer, productivity, and yield were 3.44 g butanol/L, 1.55 g butanol/L/hr, and 0.172 g butanol/g sucrose, respectively.
  • Example 6 Conditioning of hvdrolvzed feedstock with metal salts.
  • a hydrolysate was prepared from beetle killed Lodgepole pine using nitric acid as the catalyst for the hydrolysis reaction. The following conditions were used for hydrolysis: nitric acid concentration 0.4-0.5% on a dry wood basis, pH approximately 1.9 - 2.2, temperature 170 0 C, time 7 minutes, approximately 25-30% solids in the feed.
  • the tubes were then inoculated with a butanol-producing Clostridium strain at a concentration of approximately 5 x 10 7 CFU
  • the conditions used for fermentation were as follows volume 10 ml, pH approximately 6 8 before inoculation, temperature 30 c C
  • Aluminum sulfate and ferric chlo ⁇ de were both successful in transforming an otherwise un- fermentable hydrolysate into a fermentable feedstock that supported microbial growth and production of butanol Under the conditions used for fermentation, aluminum sulfate produced a feedstock that resulted m higher butanol production along with less precipitate in the final product than feme chloride
  • metal salt concentration 3 g/L, pH 9 5, room temperature (about 20°C) The butanol concentrations after microbial fermentation for 72 hours were 8 64 g/L and 7 69 g/L for aluminum sulfate and feme chlo ⁇ de, respectively
  • Example 7 Heiiiicellulose extraction from wood chips with decons traction of residual cellulose.
  • the material was collected in drums, stored at about 10 0 C for processing 12-18 hours later.
  • the temperature of the material at the exit of the disintegrator was 6O 0 C, and cooled about 15-20 0 C in
  • the acid impregnated material was then added to a feed hopper for a digester feeding system.
  • the digestor was a continuous feed, pressure rated, screw conveyor vessel operated nominally at 7.92-6.13 bar (90-110 psig), which corresponds to a steam saturation temperature of
  • Material was fed at an average rate of 11 ODMT/day to the -1000L digestor through a plug screw feeder (PSF) system with a compression ratio of approximately 8:1 or a rotary valve.
  • PSF plug screw feeder
  • the liquids to solids ratio feeding the digestor was 2.1 :1.
  • the residence time within the digestor was 300-480 seconds.
  • the liquid pressate from the PSF was measured at a rate of approximately 2 gallons per minute (gpm) (7.6 liters/minute) and contained free nitric acid (pH 1.3), as well as turpentine/tall oil type components (by smell). In some cases, all of the liquid pressate was added back to the digestor. In other cases, a portion of the liquid pressate was added back to the digestor with the balance of the 2 gallons per minute supplied by city water, hi other cases, the PSF pressate was discarded and 2 gallons per minute of water were added to the digestor.
  • the residual material had very little fiber quality or structure. Microscopic imaging of the residual material showed little distinguishable cellulosic fiber.
  • the fiber had the following characteristics:
  • the hydrolysate liquor contained significant concentrations of primarily hemicellulose sugars ( ⁇ 75g/L) in the ratios typical of softwood dilute acid hydrolysis: mannose, xylose, glucose, arabinose, and galactose.
  • Example 8 Hemicellulose extraction from wood chips.
  • the fiber had the following characteristics:
  • the hydrolysate liquor contained significant concentrations of hemicellulose sugars ( ⁇ 43.5g/L) in the ratios typical of softwood dilute acid hydrolysis: mannose, xylose, glucose, arabinose, and galactose.
  • Example 9 Continuous fermentation of Clostridium immobilized in a 1 liter packed bed bioreactor for 422 hours with conditioned hvdrolvsate.
  • a butanol-producing Clostridium strain was grown anaerobically in a packed bed bioreactor with 1 L nominal volume and 670 mL working volume. The L/D ratio of the bioreactor was 3. [338] The Clostridium was immobilized on bonechar. The bonechar particles had a size of 3000 to 5000 microns, with a bulk density of about 0.72 /ml. About 1.5 pounds of bonechar was loaded into the reactor.
  • Immobilization was achieved by first filling the reactor with about 670 mL of CP3 media with 6% w/v softwood sugars synthetic mix (20.04% w/w D-glucose, 31.32% w/w D-xylose, 12.88% w/w L-arabinose, 35.76% w/w D-mannose) and then adding to the reactor 60 mL of Clostridium broth that had an OD at 600nm of about 0.8, and recirculating the contents of the reactor for 24 hours.
  • the initial growth medium as well as the medium used during the continuous part of the fermentation contained conditioned beetle killed lodgepole pine acid hydrolysate with about 45 g/L sugar, supplemented with P2 medium components and trace elements, except that ammonium was added as ammonium sulfate instead of as ammonium acetate.
  • the hydrolysate was prepared as described in Example 7, and conditioned on Duolite A7 resin at acidic pH.
  • Continuous culture was started around 21 hours after inoculation by pumping the growth media at a constant rate into the bottom of the bioreactor and continuously removing broth from the top of the bioreactor in order to maintain a constant liquid level in the bioreactor. Continuous fermentation continued for 422 hours.
  • the feed rate for the run was 8 g/min and N 2 was added at a rate of 0.1 L/min for the duration of the fermentation. During the fermentation period between 164 and 422 hours the average pH was about 5.1.
  • the average butanol titer, productivity, and yield were 7.6 g butanol/L, 5.5 g butanol/L/hr, and 0.26 g butanol/g carbohydrate, respectively.
  • Example 10 Production of multiple bioproducts in a continuous immobilized microbial fermentation
  • Clostridium was grown anaerobically in a packed bed bioreactor with 111.3 L nominal volume and 65.7 L working volume. The L/D ratio of the bioreactor was 5.7.
  • the Clostridium was immobilized on bonechar initially screened with a 5x8 mesh, with a bulk density of about 45 Ib/ft3 . About 100 pounds of bonechar was loaded into the reactor. Immobilization was achieved by first filling the reactor with about 100 L of fermentation media with 4% by weight softwood hydrolysate, prepared as described in Example 8 and conditioned on Duolite A7 resin at acidic pH, draining approximately 15L of feed media and then adding to the reactor about 15L of Clostridium broth that had A600 absorbance of about 1.
  • the fermentation broth was circulated for approximately 24h prior to setting the reactor into continuous operation.
  • Continuous culture was achieved after the bioreactor had been inoculated by pumping the growth media at a constant rate into the bottom of the bioreactor and continuously removing broth from the top of the bioreactor in order to maintain a constant liquid level in the bioreactor. .
  • the feed rate for the run was about 540 g/min.
  • the average pH was about 5.5 and the average pressure was about 3.4 psi.
  • N 2 was added at a rate of 1.0 L/min for the duration of the fermentation.
  • yield of butanol, acetone, ethanol, acetic acid, and butyric acid were 0.220, 0.050, 0.020, 0.015, and 0.111 g/g sugars converted, respectively.
  • Sugar conversion in the reactor varied throughout the run and was approximately 50- 80%.
  • Example 11 Purification of biobutanol from fermentation broth.
  • Fermentation broth from a continuous culture of immobilized Clostridium, grown in a packed bed bioreactor with 111.3 L nominal volume, 73.4 L working or packed bed volume, and L/D ratio (packed section) 5.7 was collected from the bioreactor and pumped into a 500 gallon harvest tank. The residence time in the harvest tank was about 6Oh, depending on the bioreactor harvest rate. When sufficient material had been collected, a microfiltration step (2" x 3' microfiltration membrane unit, 0.1 urn cutoff) was performed to remove cell mass and other debris. [347] The material was then transferred to a 75 gallon steam heated batch distillation vessel with an insulated, packed overhead 4" column to provide some reflux.
  • the vessel was indirectly heated with steam and the overheads were condensed and collected by a receiver. Vessel pressure was maintained at ambient pressure. Upon discharge from the receiver, the material was decanted and the butanol rich organic phase (60-80% BuOH by weight) was further distilled in a smaller, electrically heated 5-stage Snyder distillation apparatus. The aqueous butanol phase (7-9% BuOH by weight) was discarded rather than subsequently separated. Recovery yield was 12%.

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