Medium Design of Fermentation
Medium Design of Fermentation
Medium Design of Fermentation
Industrial Fermentation Medium The basic ingredients of media include carbon source nitrogen source inorganic salt growth factor and distilled water etc.
Medium Development
Medium design should be a relatively simple process, but is often complicated by factors such as cost: availability of substrates, reliability of substrate supply, handling, storage, ease of preparation and storage, transportation of components, health and safety considerations, \
It is often easy to forget that the primary consideration is really quite simple: to supply the microorganism or cell line with a source of necessary nutrients in a readily utilisable form. In an ideal world all medium components should readily dissolve in water in order to be available to the cell.
Many media, especially at industrial scale, depart from this ideal, and contain suspended solids and oil phases that add to the complexity of sterilisation and fermenter operation.
Many scientists have applied the technique of response surface methodology in order to optimise medium. Although undoubtedly a useful technique, especially in the very earliest stages of process definition, the same improvements in yields can be obtained simply by applying sound logic to the answers to the above questions.
Select the correct carbon and nitrogen sources, add the required macro and micronutrients and growth factors, and the yield of cells should be very good.
A simple calculation of how muchbiomass is wanted and how much product is required, and applying simple microbial kinetics can determine the optimum levels of the substrates added. The key point here is that ideally, though, understanding of cell physiology, and quantitative approaches to the latter, are probably all that is needed to formulate a suitable medium for
Applying PlackettBurman design to identify significant factors (i.e., identify key nutrients which can be carried out by finding out the elemental composition of the cell line chosen), followed by central composite design (CCD) to determine the optimal level of medium constituents and their interaction
Media Type
Media can be solid, semi-solid or liquid. Most liquid media can, of course, readily be converted to solid media by addition of a suitable gelling agent, such as agar or gellan. Just make sure the gelling agent is fully dissolved and dispersed before attempting to sterilise the medium.
Synthetic Media
Synthetic media are fully chemically defined. All the components are known, as is the specific concentration of each of the components. Such media are usually quite simple, containing a carbon/energy source, nitrogen source, and a range of salt (usually inor-ganic);
Synthetic media are useful in research and laboratory situations where experimental accuracy is paramount and data interpretation needs to be clear. In general, such media are much more costly than other media types, especially if specific components such as vitamins and growth factors are required, as these ingredients tend to be very expensive when supplied in the pure form.
Yields of cells tend to be much lower than those obtained when the same cell line is grown in either semisynthetic or complex media, as the synthetic media often do not match an organisms or cell lines exact requirements. It is, of course, easier to investigate the impact of single nutrients upon cell growth and physiology using these media than the more complex ones
Semi-synthetic Media
Semi-synthetic media are largely chemically defined, as above, but include one or more poorly specified component(s) of variable but controlled composition, for example, yeast extract, which is particularly useful if a cell line requires a range of B vitamins.
Such media are useful in research and laboratory situations where a particular organism has a requirement for a substrate that would be too expensive to supply in the pure form on a routine basis.
Such components are also valuable where the specific nutritional needs are not well known, and a rich source of many nutrients such as yeast extract is used in a shotgun approach to provision of minor nutrients.
Plant, animal, fish and microbial extracts have routinely been used in the past to supply vitamins and essential growth factors for specific organisms. The current trend in medium design is to avoid extracts of animal origin, especially bovine sources, as there are potential health risks associated with these products.
Complex Media
Complex media are largely composed of substances that are usually of plant or animal origin. These materials vary from batch to batch, and composition is influenced by time of year, location of origin, and small changes in production methods.
They are usually relatively cheap, can be supplied in bulk and the source should be reli-able. Substrates such as beet and cane molasses, corn steep liquor, soya bean meals and extracts, whey powders, hydrolysed starches and a range of many different oils all fall into this category.
Medium component
Carbon Nitrogen Other substrates: elements, trace elements, growth factors
Fermentation media
Nutrient Carbon Nitrogen Raw material molasses, starch corn steep liquor, soybean meal, pure ammonia or ammonium salts, urea, nitrate salts, phosphate salts Vitamins biotin, yeast extract, beef and growth extract, corn steep liquor, factors wheat germ meal
Carbon source
A carbon source is necessary to provide the cell with energy as well as the material with which to grow and synthesise arange of primary and secondary metabolites. There is obviously a wide range of carbon sources and the one chosen should be appropriate to the organism but also to the economics of the process
GLucose
Glucose is universally acceptable for growth of most cell lines, be they animal, plant or microbial. Supplied as a powder in the pure form, the substrate is readily available, reliable, easily stored, easily handled and has no signifi cant implications for health and safety. These qualities make glucose a popular choice of carbon source.
Sucrose
Often the sugar of choice in research laboratories, sucrose, is utilised by many but not all cell lines. Commercially available sucrose comes in many forms and grades, from pure granulated forms to complex molasses solutions
Sucrose does not tend to suffer from the same drawbacks as glucose and, although it can be subject to caramelisation when over sterilised, generally it can be autoclaved/sterilised with nitrogen compounds without the same problems as glucose.
LACTOSE
Lactose can only be utilised by a few cell types, e.g. Escherichia coli, and is usually only metabolised very slowly. The sugar is only really useful for some commercial processes that use the complex substrate whey, a byproduct of the dairy industry, which contains both lactose (approximately 50 g lactose per litre of whey and 4%
Other Sugars
Other sugars can be used as substrates but tend to be very specifi c to the cell line chosen, e.g. melobiose is sometimes used for the cultivation of yeast cells. Sugars falling into this category tend to be too expensive to use on a routine basis. If choosing an unusual sugar the questions to be posed are Why is this sugar required? and What
Oils
A number of oils are now routinely used as carbon sources in the bioprocess industries. Rapeseed oil (canola oil in the USA/Canada) and methyl oleate are two popular choices. Representing both a carbon and an energy source, oils are economical and readily avail-able.
(2) Molasses
Byproduct of cane or beet sugar production A dark viscous syrup containing 50% -75% fermentable sugars (mainly sucrose) with 2% nitrogen, vitamins and minerals
Cheaper
NITROGEN SOURCE
The amount of nitrogen in any medium really determines the amount of biomass that will be achieved for the particular cell line, given that plenty of carbon is available and all required nutrients are present in the initial medium. Nitrogen is required for growth and synthesis of, for instance, proteins and nucleic acids.
Trace elements
Trace elements are regarded as micronutrients, being required only in tiny amounts, usually g quantities per litre. The functions of trace elements within the cell are many and varied but are usually associated with enzyme activity, where the trace element forms part of the enzyme or functions as a catalyst for the
where complex or semi-synthetic media are utilised, it may not be necessary to supply these elements separately. Local water supplies may even contain adequate amounts of these elements. If, however, a very pure synthetic medium utilised in the laboratory, or if a cell has an absolute requirement for a particular element or ele-ments, they must be added to the medium.
Growth factors
Small amount of organic compounds necessary for microbial growth. e.g. amino acids, vitamins, biotin Sources: normally organic nitrogen source e.g. corn steep liquor
Corn steep liquor is the water extract byproduct resulting from the steeping of corn during the commercial production of corn starch and other corn products.
Starch found in grains, potatoes, beans, peas, cassava Typically 20-30% amylose, remainder amylopectin
Characteristics of starch
Insoluble in hot water Blue complex compound by reaction with iodine. Insoluble in 30% of ethanol solution or above. Hydrolyzed by acid and enzyme, the ultimate product is glucose.
starch granule
IV.A.ii.-52
Starch: Amylose
CH2 OH O OH OH O OH Dglucose
O .....
[2 ]linkage ,2
reducingend
IV.A.ii.-53
Starch: Amylopectin
.....
O .....
[2 ]linkage ,2 reducingend CH 2 OH O OH OH OH
Dglucose
[1 ]linkage ,1
.....
CH 2 O OH OH
O ...
Starch: Amylopectin
[1,6] branch points result in tree-like structure less extended (more compact) than amylose larger MW
[1,6] linkages
reducinge nd
and decomposition
reaction
starch
acid
Advantage
Simple Time saving
Disadvantage More by-product, DE value only 90 Requiring fine starch Need corrosion resistant materials Need more energy for heating
Extent of hydrolysis measured using dextrose equivalents (DE ) value reducing sugars DE value 100 total solids
The higher the DE, the more sugars and less dextrins are present. The DE value of starch is zero and that of dextrose is 100.
DE
A B C
time
remove after
and
minutes
with
with
2. Enzyme hydrolysis method Which enzyme is used to break down starch into sugar syrup?
Amylase Glucoamylase Also called: double enzyme hydrolysis
Endoenzymes
amylase
Lower MW!
Exoenzymes(non-reducing end)
-amylase
Source
Bacillus subtilis
Action
Only -1,4-oligosaccharide links are cleaved to give dextrins with maltose and up to 50% (w/w) glucose Only -1,4-links are cleaved, from non-reducing ends, to give limit dextrins and maltose -1,4 and -1,6-links are cleaved, from the non-reducing ends to give glucose
-Amylase
Malted barley
Glucoamylase
Aspergillus niger
Pullulanase
There are two basic steps in enzymatic starch conversion: liquefaction and saccharification
1) Liquefaction
Higher temperature hydrolysis of starch involve a starch gelatinization process, dissolution of the nanogram-sized starch granules (swells and bursts)to form a viscous suspension.
Why should be two steps, liquefaction and saccharification? a. Low DE value b. Retrogradation (ageing) c. Substance size
2) Saccharification
Involving the production of glucose and a little maltose by further hydrolysis. Enzyme: glucoamylase End-point : DE is the highest
Advantage
Higher quality Save energy Protect environment
Disadvantage
Complex operation Time consuming
glucoamylase->produces glucose
(saccharification)
1) Acid-enzyme hydrolysis Acid--- liquefaction Glucoamylase----- saccharification Suitable for: starch granule is hard