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Strain
Improvement/Development
The Science and technology of manipulating and
improving microbial strains, in order to enhance their
metabolic capacities for biotechnological applications,
are referred to as strain improvement/development.
Targets of strain improvement
 Rapid growth
 Genetic stability
 Non-toxicity to humans
 Large cell size, for easy removal from the culture fluid
 Ability to use cheaper substrates
 Elimination of the production of compounds that may interfere with
downstream processing
 Increase productivity.
 To improve the use of carbon and nitrogen sources.
 Reduction of cultivation cost
-lower price in nutrition.
-lower requirement for oxygen.
 Production of
-additional enzymes.
-compounds to inhibit contaminant microorganisms.
Optimization of microbial activity
It can be done by
 Optimizing environmental conditions
 Optimizing nutrition of microorganisms
 Other includes
1. Method not involving foregin DNA—Mutagenesis
2.
Method involving Foreign
DNA(recombination)
Transduction
Conjugation
Transformation
Genetic
engineering
Optimizing environment
conditions
 Modification of physical parameter
(temperature,agitation,etc)
 Modification of chemical parameter (pH,O2
concentration)
 Modification of biological parameter (enzymes )
Optimization of nutrition of microorganisms
 Carbon sources
 Nitrogen sources
 Mineral sources and other sources
 Precursor
 Enzymes
Proper strain used in Industry Genetically Regarded As
Safe (GRAS)
Bacteria – Bacillus subtilis
– Lactobacillus
bulgaricus
– Lactococcus lactis
– Leuconostoc oenos
Yeasts – Candida utilis
– Kluyveromyces
marxianus
– Kluyveromyces lactis
– Saccharomyces
cerevisiae
•Filamentous fungi
– Aspergillus niger
– Aspergillus oryzae
– Mucor javanicus
– Penicillium roqueforti
1. MUTAGENESIS
 Mutagenesis is a process of treatment given to
microorganism which will cause an improvement in their
genotypic and phenotypic performances
.
Mutagenesis
Spontaneous
mutation
Direct mutation
(addition,deletion,
substitution,point)
Induced mutation
Types of mutation
1.Spontaneous mutation:
 A mutation that arises naturally and not as a result of
exposure to mutagens. Also called natural mutation .
2. Induced mutation:
 A mutation that is produced by treatment with a
physical or chemical agent that affects the
deoxyribonucleic acid molecules of a living organism.
 The rate of mutation can be increased by various factors
and agents called mutagens.
 ionizing radiations (e.g. X-rays, gamma rays)
 non-ionizing radiations (e.g. ultraviolet radiations)
 various chemicals (e.g. mustard gas, benzene, ethidium
bromide, Nitroso guanidine-NTG)
3.Direct mutations
2.Transduction-
 Transduction is the transfer of bacterial DNA from one bacterial
cell to another by means of a bacteriophage.
 Two types:
 general transduction and
 specialized transduction.
 In general transduction, host DNA from any part of the host’s
genetic apparatus is integrated into the virus DNA.
 In specialized transduction, which occurs only in some phages,
DNA from a specific region of the host DNA is integrated into the
viral DNA and replaces some of the virus’ genes.
 The method is a well-established research tool in bacteria
including actinomycetes but prospects for its use in fungi appear
limited.
3.Transformation
 When foreign DNA is
absorbed by, and integrates
with the genome of, the donor
cell.
 Cells in which transformation
can occur are ‘competent’
cells.
In some cases competence is artificially induced by
treatment with a calcium salt.
The method has also been used to increase the level of
protease and amylase production in Bacillus spp.
The method therefore has good industrial potential.
4.Conjugation--
 Conjugation involves cell to
cell contact or through sex
pili (singular, pilus) and the
transfer of plasmids.
 The donor strain’s plasmid
must possess a sex factor as a
prerequisite for conjugation;
only donor cells produce pili.
 The sex factor may on
occasion transfer part of the
hosts’ DNA.
 Plasmids play an important
role in the formation of some
industrial products, including
many antibiotics.
5.Genetic Engineering
 Genetic engineering, also known as recombinant DNA technology,
molecular cloning or gene cloning.
 Recombinant DNA Technology enables isolation of genes from an
organism, this gene can be amplified, studied, altered & put into another
organism
 Recombinant DNA procedure:
i. Cutting of donor DNA : Restriction endonucleases cut DNA
molecule at specific sites and desired fragment is isolated by gel
electrophoresis.
ii. Cloning of a gene : DNA fragment, which wanted to be cloned,
is joined to one of vectors (plasmid, phage, cosmid). For this purpose,
vector and donor DNA are first cleaved with the same restriction
endonuclease, or with the ones producing the same ends
 Then by using DNA ligase, DNA fragment and vector DNA is joined. If
fragment has no sticky ends, homopolymer tailing or linker DNA
segments can be applied for this step.
iii. Transformation : Recombinant vector is put into suitable host organism,
like; bacteria, yeast, plant or animal cells, by several physical or
chemical methods.
Insertional inactivation-
Strain development techniques of industrially important microorganisms

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Strain development techniques of industrially important microorganisms

  • 1.
  • 2. Strain Improvement/Development The Science and technology of manipulating and improving microbial strains, in order to enhance their metabolic capacities for biotechnological applications, are referred to as strain improvement/development.
  • 3. Targets of strain improvement  Rapid growth  Genetic stability  Non-toxicity to humans  Large cell size, for easy removal from the culture fluid  Ability to use cheaper substrates  Elimination of the production of compounds that may interfere with downstream processing  Increase productivity.  To improve the use of carbon and nitrogen sources.  Reduction of cultivation cost -lower price in nutrition. -lower requirement for oxygen.  Production of -additional enzymes. -compounds to inhibit contaminant microorganisms.
  • 4. Optimization of microbial activity It can be done by  Optimizing environmental conditions  Optimizing nutrition of microorganisms  Other includes 1. Method not involving foregin DNA—Mutagenesis 2. Method involving Foreign DNA(recombination) Transduction Conjugation Transformation Genetic engineering
  • 5. Optimizing environment conditions  Modification of physical parameter (temperature,agitation,etc)  Modification of chemical parameter (pH,O2 concentration)  Modification of biological parameter (enzymes )
  • 6. Optimization of nutrition of microorganisms  Carbon sources  Nitrogen sources  Mineral sources and other sources  Precursor  Enzymes
  • 7. Proper strain used in Industry Genetically Regarded As Safe (GRAS) Bacteria – Bacillus subtilis – Lactobacillus bulgaricus – Lactococcus lactis – Leuconostoc oenos Yeasts – Candida utilis – Kluyveromyces marxianus – Kluyveromyces lactis – Saccharomyces cerevisiae •Filamentous fungi – Aspergillus niger – Aspergillus oryzae – Mucor javanicus – Penicillium roqueforti
  • 8. 1. MUTAGENESIS  Mutagenesis is a process of treatment given to microorganism which will cause an improvement in their genotypic and phenotypic performances . Mutagenesis Spontaneous mutation Direct mutation (addition,deletion, substitution,point) Induced mutation
  • 9. Types of mutation 1.Spontaneous mutation:  A mutation that arises naturally and not as a result of exposure to mutagens. Also called natural mutation . 2. Induced mutation:  A mutation that is produced by treatment with a physical or chemical agent that affects the deoxyribonucleic acid molecules of a living organism.  The rate of mutation can be increased by various factors and agents called mutagens.  ionizing radiations (e.g. X-rays, gamma rays)  non-ionizing radiations (e.g. ultraviolet radiations)  various chemicals (e.g. mustard gas, benzene, ethidium bromide, Nitroso guanidine-NTG)
  • 11.
  • 12. 2.Transduction-  Transduction is the transfer of bacterial DNA from one bacterial cell to another by means of a bacteriophage.  Two types:  general transduction and  specialized transduction.  In general transduction, host DNA from any part of the host’s genetic apparatus is integrated into the virus DNA.  In specialized transduction, which occurs only in some phages, DNA from a specific region of the host DNA is integrated into the viral DNA and replaces some of the virus’ genes.  The method is a well-established research tool in bacteria including actinomycetes but prospects for its use in fungi appear limited.
  • 13.
  • 14. 3.Transformation  When foreign DNA is absorbed by, and integrates with the genome of, the donor cell.  Cells in which transformation can occur are ‘competent’ cells.
  • 15. In some cases competence is artificially induced by treatment with a calcium salt. The method has also been used to increase the level of protease and amylase production in Bacillus spp. The method therefore has good industrial potential.
  • 16. 4.Conjugation--  Conjugation involves cell to cell contact or through sex pili (singular, pilus) and the transfer of plasmids.  The donor strain’s plasmid must possess a sex factor as a prerequisite for conjugation; only donor cells produce pili.  The sex factor may on occasion transfer part of the hosts’ DNA.  Plasmids play an important role in the formation of some industrial products, including many antibiotics.
  • 17. 5.Genetic Engineering  Genetic engineering, also known as recombinant DNA technology, molecular cloning or gene cloning.  Recombinant DNA Technology enables isolation of genes from an organism, this gene can be amplified, studied, altered & put into another organism  Recombinant DNA procedure: i. Cutting of donor DNA : Restriction endonucleases cut DNA molecule at specific sites and desired fragment is isolated by gel electrophoresis. ii. Cloning of a gene : DNA fragment, which wanted to be cloned, is joined to one of vectors (plasmid, phage, cosmid). For this purpose, vector and donor DNA are first cleaved with the same restriction endonuclease, or with the ones producing the same ends
  • 18.  Then by using DNA ligase, DNA fragment and vector DNA is joined. If fragment has no sticky ends, homopolymer tailing or linker DNA segments can be applied for this step. iii. Transformation : Recombinant vector is put into suitable host organism, like; bacteria, yeast, plant or animal cells, by several physical or chemical methods.