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 Amino acids have always played an important
role in the biology of life, in biochemistry and in
(industrial) chemistry.
 amino acids are the building blocks of proteins
and they play an essential role in the reguiation
of the metabolism of living organisms.
 Large scale chemical and microbial production
processes have been commercialised for a
number of essential amino acids.
 current interest in developing peptide-derived
chemotherapeutics has heightened the
importance of rare and non-proteinogenic pure
amino acids.
 amino acids are versatile chiral (optically active)
building blocks for a whole range of fine chemicals.
 Amino acids are, therefore, important as nutrients
(food and feed), as seasoning, flavourings and
starting material for pharmaceuticals, cosmetics and
other chemicals.
 Amino acid can be produced by :
 Chemical synthesis
 Isolation from natural materials
 Fermentation
 Chemo-enzyme methods
 Batch Fermentation
 Fed-batch Fermentation
 Continuous Fermentation
 Enzymatic Method
 Widely use in the production of amino acid
 Fermentation is a closed culture system which contains
an initial, limited amount of nutrient.
 A short adaptation time is usually necessary (lag phase)
before cells enter the logarithmic growth phase
(exponential phase).
 Nutrients soon become limited and they enter the
stationary phase in which growth has (almost) ceased.
 In amino acid fermentations, production of the amino
acid normally starts in the early logarithmic phase and
continues through the stationary phase.
 For economical reasons the fermentation time should
be as short as possible with a high yield of the amino
acid at the end.
 A second reason not to continue the fermentation in
the late stationary phase is the appearance of
contaminant-products
 The lag phase can be shortened by using a higher
concentration of seed inoculum.
 The seed is produced by growing the production
strain in flasks and smaller fermenters.
 Batch fermentations which are fed continuously, or
intermittently, with medium without the removal of
fluid.
 In this way the volume of the culture increases with
time.
 The residual substrate concentration may be
maintained at a very low level.
 This may result in a removal of catabolite repressive
effects and avoidance of toxic effects of medium
components
 Oxygen balance.
 The feed rate of the carbon source (mostly glucose)
can be used to regulate cell growth rate and oxygen
limitation,especially when oxygen demand is high in
the exponential growth phase.
 In continuous fermentation, an open system is
set up.
 Sterile nutrient solution is added to the
bioreactor continuously and an equivalent
amount of converted nutrient solution with
microorganisms is simultaneously removed from
the system.
 Two basic types of continuous fermentations can
be distinguished:
 Homogeneously Mixed Bioreactor
 Plug Flow Reactor
 Advantages :
 higher productivity, operation for a very long
period of time, and lower installation and
maintenance costs
 Disadvantages :
 chance of contamination by other microorganisms
during the long fermentation runs (sometimes
several weeks).
 occurrence of variants of the parent
production strain by back mutation or loss of
genetic elements (plasmids)
 An amino acid precursor is converted to the
target amino acid using 1 or 2 enzymes.
 Allows the conversion to a specific amino acid
without microbial growth, thus eliminating the
long process from glucose.
 Raw materials for the enzymatic step are
supplied by chemical synthesis
 The enzyme itself is either in isolated or whole
cell form which is prepared by microbial
fermentation.
 Bioprocess keys : enzymatic production of amino
acid
Bioreactor :
1) low unit cost of substrate
2) High substrate yields
3) High rate of product production
Biocatalyst Preparation :
1. Low fermentation medium cost
2. Short fermentation time
3. High enzyme recovery yield
 Amino acid fermentation is closely connected
with screening or selection of suitable putative
production organisms.
 The selection of organism based on :
 Non-pathogenicity
 Wide spectrum of assimilable carbon source
 Rapid growth on cheap carbon and nitrogen sources
 High ability to metabolize carbon sources
 Resistance to bacteriophage attack
 Production strains can be divided into 3 type of
strains :
 Wild type strain
 Mutant strain
 Genetically modified strain
Wild type strain
 Capable to produce specific amino acid under defined
conditions
Mutant Strain
 Feedback regulations are bypassed by partially starving
them of their requirements or by genetic removal of
metabolic control
Genetically modified Strain
 Biosynthetic capacity of cells making specific amino acids
is improve by amplifying genes coding for rate-limiting
enzymes
 Improvement involve strains capable to produce
amino acid at higher yields
 They also produce lower by-product because they
dominate costs for downstream procesing
 Specific method is require to separate the amino
acid produced from its contaminant products
 There are 8 methods :
 Centrifugation
 Filtration
 Crystallisation
 Ion exchange
 Electrodialysis
 Solvent extraction
 Decolorisation
 Evaporation
 Common method used in industry
 Can be operate semi-continuous or continuous
basis
 Large scale tests have to performed to choose a
suitable centrifuge
 Poor centrifugation can be improved by adding
flocculation agent
 This agent will neutralize the anionic charges on
the surface of microbial cells.
 Also widely use in industrial
 Based on a few factors :
 Properties of the filtrate
 Nature of the solid particles
 Adequate pressure to obtain adequate flow rate
 Negative effects of antifoaming agents on filtration
 Filtration can be improved by using filteraids
 Filteraids improved the porosity of a resulting
filter cake leading to a faster flow rates.
 Method to recover amino acid
 Because of the amphoteric character of amino acid,
their solubility are greatly influenced by the pH of a
solution
 Temperature also influence the solubility of amino
acid and their salts
 Thus, lowering the temperature can be used to
obtain the required product
 Precipitation of amino acid with salts are commonly
used
 Used for the extraction and purification of amino
acids form the fermentation broth
 Strongly affected by pH of the solutions and the
present of contaminant ions
 There are two types of ion exchange resins
 Cation exchange resins
 Anion exchange resins
 Cation exchange resins
 Bind with positively charged amino acids
 Anion exchange resins
 Bind with negatively charged amino acid
 Anion exchange resins are generally lower in their
exchange capacity and durability than cation
exchange resins
 ion exchange as a tool for separation is only used
when other steps fail, because of its tedious
operation, small capacity and high costs.
 Based on the principle that charged particles
move towards the electrodes in the electric
field.
 A mixture of the required amino acid and
contaminant salts can be separated at a pH
where the amino acid has a net zero charge (at
the IEP).
 The salt ions are captured by the ion exchange
membranes that are present.
 The applications are limited to desalting amino
acid solutions.
 has only limited applications.
 The distribution coefficients of amino acids
between organic solvent and water phases are
generally small.
 Some possibilities based on alteration of amino
acid
 cyclisation of L-glutamic acid and extraction with alkyl
and aromatic alcohols
 conversion of contaminant organic acids (like acetic
acid) to the ester form and extraction of the ester
 extraction of basic amino acids (like L-lysine) from
aqueous solution with water immiscible solvents
containing higher fatty acids;
 performed to get rid of the coloured impurities
in the fermentation broth.
 based on the fact that amino acids (especially
the non-aromatic amino acids) do not adsorb
onto activated charcoal.
 Although the treatment is very effective, some
of the amino acid is lost during this step.
 Alternative ways :
 addition of cationic surfactants, high molecular
synthetic coagulants or some phenolic compounds
 washing of crystals with weakly alkaline water as in the
case of glutamic acid.
 Evaporation of the amino acid containing
solution is a quick but commercially unattractive
way (high energy costs) to obtain amino acids
from solution.
 used when the total amount of contaminant
products is very low, since these compounds are
not removed and appear in a concentrated form
in the product.
 Use natural product such as sugar cane
 Then, the sugar cane is squeezed to make
molasses
 The glutamic acid is produced through the
fermentation process
 The heat sterilize raw material and other
nutrient are put in the tank.
 The microorganism producing glutamic acid is
added to the fermentation broth
 The microorganism reacts with sugar to produce
glutamic acid.
 Then, the fermentation broth is acidified and
the glutamic acid is crystallized.
 The glutamic acid crystal cake is then separated
from the acidified fermentation broth.
 The glutamic acid crystal cake is added to the
sodium hydroxide solution and converted into
monosodium glutamate.
 The monosodium glutamate is more soluble in water,
less likely absorb moisture and has strong umami
taste.
 The monosodium glutamate is cleaned by using
active carbon.
 Active carbon has many micro holes on their surface.
The impurities is absorb onto the surface of active
carbon.
 The clean monosodium glutamate solution is
concentrated by heating and the monosodium
glutamate crystal is formed.
 The crystal produce are dried with a hot air in a
closed system.
 Then, the crystal is packed in the packaging and
ready to be sold.
 The amino acid produces many products.
 For example :
 Lysine HCl
 Threonine
 Aspartate
 Lysine application
 Food & dietary supplement
 Medicine, cosmetics, chemicals
 Feed : essential aminoacid for most mammals
Glucose
Oxygen
Ammonia
Minerals &
Vitamins
Lysine
 The pathway leading to lysine (also threonine,
isoleucine, methione) biosynthesis is initiated with
the conversion of aspartate to aspartyl-P via the
enzyme aspartokinase (AK).
 The phosphorylated aspartate is then converted to
aspartyl-semialdehyde (ASA) that can converted to
homoserine by homoserine dehydrogenase (HSD) or
to diaminopimelic acid (DAP) by a series of five
enzymatic conversions, and hence to lysine.
 Application of theronine
 Vitamins
 supplements
 The regulation of threonine biosynthesis in E. coli is
more complex than that in C. glutamicum.
 Corynebacterium, E. coli has three aspartate
kinases, AKI, AKII and AKIII.
 Two (AKI and AKII) are multidomain proteins that
also have homoserine dehydrogenase activity
responsible for the third step of the pathway.
 AKI is feedback inhibited by threonine and its
synthesis is repressed by a combination of threonine
and isoleucine.
 The synthesis of AKII is repressed by methionine.
 AKIII is feedback inhibited and repressed by lysine.
 The second step of the pathway is catalyzed by
aspartate semialdehyde dehydrogenase (ASD).
 The last two enzymes, homoserine kinase (HK; thrB)
and threonine synthase (TS; thrC) are coexpressed
along with AKI (thrA) as part of the thrABC operon.
 This operon is controlled by transcriptional
attenuation.
 Aspartate is a vitamin-like substance called an
amino acid.
 Aspartates are used to increase absorption of the
minerals.
 reduce brain damage caused by cirrhosis of
the liver.
 Aspartic acid is made by the enzyme aspartate
ammonia lyase (aspartase) that carries out the
following reaction in presence of ammonium
fumarate
 -OOCCH=CHCOO- + NH4 + -OOCCH2CH(NH3+)COOO
 Once immobilized, the cells are quite stable
retaining aspartase activity for well over 600 days
even at 37°C.
 The process is carried out at pH 8.5 with ammonium
fumarate as the substrate.
 Immobilized Pseudomonas dacunhae cells can
convert aspartate to alanine using the
pyridoxalphosphate dependent aspartate β-
carboxylase.
 contamination of the culture by other
microorganisms during fermentation.
 bad fermentation reproducibility due to
differences in raw material.
 back mutation or loss of genetic material of the
production strain.
 infection of the culture by bacterial viruses
(phages)
 make use of fresh starting material
(inoculum) for each run.
 adsorption onto the bacterial cell followed
by introduction of genetic material into the
bacterium.
 isolation of phage resistant strains.
 construction of a strain in such a way that it
is energetically advantageous to overproduce
the required amino acid, thus keeping the
construct in the cell.
 normally the production strain is constructed in
such a way that overproduction of the desired
amino acid is obtained and no, or only minor
concentrations of, unwanted contaminants
appear.
 optical resolution steps are not necessary (as in
the case of most chemical-processes) since only
the L-form is synthesised.
 the required amino acid can be relatively easily
separated from cells and protein impurities.
Industrial processing of amino acid slide

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Industrial processing of amino acid slide

  • 1.  Amino acids have always played an important role in the biology of life, in biochemistry and in (industrial) chemistry.  amino acids are the building blocks of proteins and they play an essential role in the reguiation of the metabolism of living organisms.  Large scale chemical and microbial production processes have been commercialised for a number of essential amino acids.  current interest in developing peptide-derived chemotherapeutics has heightened the importance of rare and non-proteinogenic pure amino acids.
  • 2.  amino acids are versatile chiral (optically active) building blocks for a whole range of fine chemicals.  Amino acids are, therefore, important as nutrients (food and feed), as seasoning, flavourings and starting material for pharmaceuticals, cosmetics and other chemicals.  Amino acid can be produced by :  Chemical synthesis  Isolation from natural materials  Fermentation  Chemo-enzyme methods
  • 3.  Batch Fermentation  Fed-batch Fermentation  Continuous Fermentation  Enzymatic Method
  • 4.  Widely use in the production of amino acid  Fermentation is a closed culture system which contains an initial, limited amount of nutrient.  A short adaptation time is usually necessary (lag phase) before cells enter the logarithmic growth phase (exponential phase).  Nutrients soon become limited and they enter the stationary phase in which growth has (almost) ceased.  In amino acid fermentations, production of the amino acid normally starts in the early logarithmic phase and continues through the stationary phase.
  • 5.  For economical reasons the fermentation time should be as short as possible with a high yield of the amino acid at the end.  A second reason not to continue the fermentation in the late stationary phase is the appearance of contaminant-products  The lag phase can be shortened by using a higher concentration of seed inoculum.  The seed is produced by growing the production strain in flasks and smaller fermenters.
  • 6.
  • 7.  Batch fermentations which are fed continuously, or intermittently, with medium without the removal of fluid.  In this way the volume of the culture increases with time.  The residual substrate concentration may be maintained at a very low level.  This may result in a removal of catabolite repressive effects and avoidance of toxic effects of medium components  Oxygen balance.  The feed rate of the carbon source (mostly glucose) can be used to regulate cell growth rate and oxygen limitation,especially when oxygen demand is high in the exponential growth phase.
  • 8.
  • 9.  In continuous fermentation, an open system is set up.  Sterile nutrient solution is added to the bioreactor continuously and an equivalent amount of converted nutrient solution with microorganisms is simultaneously removed from the system.  Two basic types of continuous fermentations can be distinguished:  Homogeneously Mixed Bioreactor  Plug Flow Reactor
  • 10.  Advantages :  higher productivity, operation for a very long period of time, and lower installation and maintenance costs  Disadvantages :  chance of contamination by other microorganisms during the long fermentation runs (sometimes several weeks).  occurrence of variants of the parent production strain by back mutation or loss of genetic elements (plasmids)
  • 11.
  • 12.
  • 13.  An amino acid precursor is converted to the target amino acid using 1 or 2 enzymes.  Allows the conversion to a specific amino acid without microbial growth, thus eliminating the long process from glucose.  Raw materials for the enzymatic step are supplied by chemical synthesis  The enzyme itself is either in isolated or whole cell form which is prepared by microbial fermentation.
  • 14.  Bioprocess keys : enzymatic production of amino acid Bioreactor : 1) low unit cost of substrate 2) High substrate yields 3) High rate of product production Biocatalyst Preparation : 1. Low fermentation medium cost 2. Short fermentation time 3. High enzyme recovery yield
  • 15.  Amino acid fermentation is closely connected with screening or selection of suitable putative production organisms.  The selection of organism based on :  Non-pathogenicity  Wide spectrum of assimilable carbon source  Rapid growth on cheap carbon and nitrogen sources  High ability to metabolize carbon sources  Resistance to bacteriophage attack
  • 16.  Production strains can be divided into 3 type of strains :  Wild type strain  Mutant strain  Genetically modified strain Wild type strain  Capable to produce specific amino acid under defined conditions Mutant Strain  Feedback regulations are bypassed by partially starving them of their requirements or by genetic removal of metabolic control
  • 17. Genetically modified Strain  Biosynthetic capacity of cells making specific amino acids is improve by amplifying genes coding for rate-limiting enzymes  Improvement involve strains capable to produce amino acid at higher yields  They also produce lower by-product because they dominate costs for downstream procesing
  • 18.  Specific method is require to separate the amino acid produced from its contaminant products  There are 8 methods :  Centrifugation  Filtration  Crystallisation  Ion exchange  Electrodialysis  Solvent extraction  Decolorisation  Evaporation
  • 19.  Common method used in industry  Can be operate semi-continuous or continuous basis  Large scale tests have to performed to choose a suitable centrifuge  Poor centrifugation can be improved by adding flocculation agent  This agent will neutralize the anionic charges on the surface of microbial cells.
  • 20.  Also widely use in industrial  Based on a few factors :  Properties of the filtrate  Nature of the solid particles  Adequate pressure to obtain adequate flow rate  Negative effects of antifoaming agents on filtration  Filtration can be improved by using filteraids  Filteraids improved the porosity of a resulting filter cake leading to a faster flow rates.
  • 21.  Method to recover amino acid  Because of the amphoteric character of amino acid, their solubility are greatly influenced by the pH of a solution  Temperature also influence the solubility of amino acid and their salts  Thus, lowering the temperature can be used to obtain the required product  Precipitation of amino acid with salts are commonly used
  • 22.  Used for the extraction and purification of amino acids form the fermentation broth  Strongly affected by pH of the solutions and the present of contaminant ions  There are two types of ion exchange resins  Cation exchange resins  Anion exchange resins  Cation exchange resins  Bind with positively charged amino acids
  • 23.  Anion exchange resins  Bind with negatively charged amino acid  Anion exchange resins are generally lower in their exchange capacity and durability than cation exchange resins  ion exchange as a tool for separation is only used when other steps fail, because of its tedious operation, small capacity and high costs.
  • 24.  Based on the principle that charged particles move towards the electrodes in the electric field.  A mixture of the required amino acid and contaminant salts can be separated at a pH where the amino acid has a net zero charge (at the IEP).  The salt ions are captured by the ion exchange membranes that are present.  The applications are limited to desalting amino acid solutions.
  • 25.
  • 26.  has only limited applications.  The distribution coefficients of amino acids between organic solvent and water phases are generally small.  Some possibilities based on alteration of amino acid  cyclisation of L-glutamic acid and extraction with alkyl and aromatic alcohols  conversion of contaminant organic acids (like acetic acid) to the ester form and extraction of the ester  extraction of basic amino acids (like L-lysine) from aqueous solution with water immiscible solvents containing higher fatty acids;
  • 27.  performed to get rid of the coloured impurities in the fermentation broth.  based on the fact that amino acids (especially the non-aromatic amino acids) do not adsorb onto activated charcoal.  Although the treatment is very effective, some of the amino acid is lost during this step.  Alternative ways :  addition of cationic surfactants, high molecular synthetic coagulants or some phenolic compounds  washing of crystals with weakly alkaline water as in the case of glutamic acid.
  • 28.
  • 29.  Evaporation of the amino acid containing solution is a quick but commercially unattractive way (high energy costs) to obtain amino acids from solution.  used when the total amount of contaminant products is very low, since these compounds are not removed and appear in a concentrated form in the product.
  • 30.  Use natural product such as sugar cane  Then, the sugar cane is squeezed to make molasses  The glutamic acid is produced through the fermentation process
  • 31.  The heat sterilize raw material and other nutrient are put in the tank.  The microorganism producing glutamic acid is added to the fermentation broth  The microorganism reacts with sugar to produce glutamic acid.  Then, the fermentation broth is acidified and the glutamic acid is crystallized.
  • 32.  The glutamic acid crystal cake is then separated from the acidified fermentation broth.  The glutamic acid crystal cake is added to the sodium hydroxide solution and converted into monosodium glutamate.  The monosodium glutamate is more soluble in water, less likely absorb moisture and has strong umami taste.  The monosodium glutamate is cleaned by using active carbon.  Active carbon has many micro holes on their surface. The impurities is absorb onto the surface of active carbon.
  • 33.  The clean monosodium glutamate solution is concentrated by heating and the monosodium glutamate crystal is formed.  The crystal produce are dried with a hot air in a closed system.  Then, the crystal is packed in the packaging and ready to be sold.
  • 34.  The amino acid produces many products.  For example :  Lysine HCl  Threonine  Aspartate
  • 35.  Lysine application  Food & dietary supplement  Medicine, cosmetics, chemicals  Feed : essential aminoacid for most mammals
  • 37.
  • 38.  The pathway leading to lysine (also threonine, isoleucine, methione) biosynthesis is initiated with the conversion of aspartate to aspartyl-P via the enzyme aspartokinase (AK).  The phosphorylated aspartate is then converted to aspartyl-semialdehyde (ASA) that can converted to homoserine by homoserine dehydrogenase (HSD) or to diaminopimelic acid (DAP) by a series of five enzymatic conversions, and hence to lysine.
  • 39.
  • 40.
  • 41.  Application of theronine  Vitamins  supplements
  • 42.
  • 43.  The regulation of threonine biosynthesis in E. coli is more complex than that in C. glutamicum.  Corynebacterium, E. coli has three aspartate kinases, AKI, AKII and AKIII.  Two (AKI and AKII) are multidomain proteins that also have homoserine dehydrogenase activity responsible for the third step of the pathway.  AKI is feedback inhibited by threonine and its synthesis is repressed by a combination of threonine and isoleucine.  The synthesis of AKII is repressed by methionine.  AKIII is feedback inhibited and repressed by lysine.
  • 44.  The second step of the pathway is catalyzed by aspartate semialdehyde dehydrogenase (ASD).  The last two enzymes, homoserine kinase (HK; thrB) and threonine synthase (TS; thrC) are coexpressed along with AKI (thrA) as part of the thrABC operon.  This operon is controlled by transcriptional attenuation.
  • 45.  Aspartate is a vitamin-like substance called an amino acid.  Aspartates are used to increase absorption of the minerals.  reduce brain damage caused by cirrhosis of the liver.
  • 46.
  • 47.  Aspartic acid is made by the enzyme aspartate ammonia lyase (aspartase) that carries out the following reaction in presence of ammonium fumarate  -OOCCH=CHCOO- + NH4 + -OOCCH2CH(NH3+)COOO  Once immobilized, the cells are quite stable retaining aspartase activity for well over 600 days even at 37°C.  The process is carried out at pH 8.5 with ammonium fumarate as the substrate.  Immobilized Pseudomonas dacunhae cells can convert aspartate to alanine using the pyridoxalphosphate dependent aspartate β- carboxylase.
  • 48.  contamination of the culture by other microorganisms during fermentation.  bad fermentation reproducibility due to differences in raw material.  back mutation or loss of genetic material of the production strain.  infection of the culture by bacterial viruses (phages)
  • 49.  make use of fresh starting material (inoculum) for each run.  adsorption onto the bacterial cell followed by introduction of genetic material into the bacterium.  isolation of phage resistant strains.  construction of a strain in such a way that it is energetically advantageous to overproduce the required amino acid, thus keeping the construct in the cell.
  • 50.  normally the production strain is constructed in such a way that overproduction of the desired amino acid is obtained and no, or only minor concentrations of, unwanted contaminants appear.  optical resolution steps are not necessary (as in the case of most chemical-processes) since only the L-form is synthesised.  the required amino acid can be relatively easily separated from cells and protein impurities.