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BTE 302: MICROBIAL BIOTECHNOLOGY
Microbial Strain Improvement
1
2
3
4
5
Strain improvement
 Metabolite concentration produced
by wild strains are usually too low for
economic processes. That is why
strain improve is needed.
 Success of strain improvement
depends greatly on the target
product.
6
Strain improvement
 Simply raising the gene dose can
increase the yield from products
involving activity of one or few
genes.
 This is beneficial if the product is cell
biomass or primary metabolites.
7
Mutation
8
Spontaneous mutation
 Rate depends on growth condition of
organisms
 Between 10-10 to 10-5 per generation per
gene
 All mutant types are found although
deletions are frequent
 Not cost effective because of low
frequency of mutation
9
10
11
12
13
14
15
16
17
Induced mutation
 Mutation frequency is significantly
increased
 10-5 to 10-3 for secondary metabolite
producers
 10-2 to 10-1 for auxotrophic mutants
18
 Genome mutation may cause:
 Change in no. of chromosomes
 Chromosome mutation may change:
 Order of genes by
deficiency, deletion, inversion, dup
lication or translocation
 Gene or point mutation
19
Changes due to mutation
 Less lethal and mutagenic effects than short
wavelength UV
 Exposure of cells in the presence of various
dyes causes interaction of DNA with UV with
greater rates which results in increased
frequency of mutation
 Effective activators are psoralen derivatives
(e.g. 8-methoxypsoralen)
 Mechanism of action: Biadduct formation
between complementary strands which
20
Long wavelength UV
21
Optimizing mutagenesis
 Molecular mode of action of some
mutagens is well known but what can
never be predicted is:
 Effect of mutagen on specific gene
 Effect of mutation on a complex
process (e.g. biosynthesis of
secondary metabolite)
 Appearance of mutants depends on
several factors
 Base sequence of gene
22
Mode of action of mutagens
 Base sequence of gene to be
mutated:
 Mutation are not evenly
distributed
 There are areas of high mutation
frequency known as hot spots
 Different mutagens cause hot
spots at different sites in the
23
Factors affecting appearance of
mutants
 Strains with partially defective repair
mechanisms:
 Organisms may be killed without
having induced mutation
 Specific mutagen may be
ineffective
24
Factors affecting appearance of
mutants
 Gene activity:
 Become lost through mutation
 Can be restored through a second
mutation (suppressor mutation)
25
Factors affecting appearance of
mutants
 Act in several different ways
 Occurs in the same gene that already
carries primary mutation (intragenic
suppressors)
 Compensated through exchange of
amino acid or additional insertion or
deletion which corrects primary
mutation
26
Suppressor mutation
 Occurs in another gene (extragenic
suppressor)
 Compensate primary mutation at the
level of translation by formation of
mutant tRNA or ribosome
27
Suppressor mutation
28
Selection of mutants
29
30
31
Isolation of auxotroph
32
 By using certain blocked mutants,
desired products such as amino acids and
nucleotides may be formed via branching
biosynthetic pathways.
The isolation of auxotrophs is done by
plating of the mutagenized population on
a complete agar medium, on which the
biochemically deficient mutants can also
grow.
Isolation of auxotroph
33
 The antibiotic resistance character
can not only be used as a genetic
marker, but mutants isolated may
also have increased cell
permeability or a protein synthesis,
making them useful for industrial
purposes.
34
 By means of Lederberg’s well-known replica
plating technique, the clones are transferred
to minimal medium where the auxotrophic
colonies cannot grow.
These mutants are picked up from the master
plates and their defect is characterized.
35
36
Isolation of auxotroph
 Since in this method a large number havof plates must be
 observed, various procedures e been developed to enrich
for
 auxotrophic mutants by removing or killing prototrophic
 organisms.
37
Isolation of auxotroph
 After mutagenesis the spores of filamentous
organisms (actinomycetes, fungi) are allowed to
develop in a liquid minimal medium.
 The developing micro colonies of prototrophs are
then separated by filtration, leaving behind in the
filtrate spores of auxotrophs, which have been
unable to grow.
 The filtrate is then plated and the resulting colonies
are checked for auxotrophic characteristics.
38
39
Penicillin selection method
 Penicillin kills growing cells but not non-growing
cells. In this procedure, growing cells are selectively
killed by antibiotic treatment, thus enriching for
auxotrophs, which cannot grow on minimal medium.
 Several inhibitors other than penicillin can also be
used in this procedure: dihydrostreptomycin for
Pseudomonas aeruginosa, nalidixic acid for
Salmonella typhimurium.
40
41
42
43
44
45
46
47
48
49
50
51
52
53
54
55
56
 An enrichment procedure with sodium
pentachlorophenolate makes use of the
greater toxicity of this compound against
germinating spores than against
vegetative cells.
 The method has been successfully
applied with Penicillium chrysogenum,
Streptomyces aureofaciens, S. olivaceus,
and Bacillus subtilis.
57
Enrichment method
 By these methods, enrichments for
auxotrophs of 10- to100-fold can be
attained, thus increasing the probability of
obtaining mutants.
 However, it should be remembered that
the types of mutants present in the
original population may be shifted; for
instance, an increased proportion of
proline auxotrophs has been found in E.
58
Enrichment method

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Strain improvt25 (2)

  • 1. BTE 302: MICROBIAL BIOTECHNOLOGY Microbial Strain Improvement 1
  • 2. 2
  • 3. 3
  • 4. 4
  • 5. 5
  • 6. Strain improvement  Metabolite concentration produced by wild strains are usually too low for economic processes. That is why strain improve is needed.  Success of strain improvement depends greatly on the target product. 6
  • 7. Strain improvement  Simply raising the gene dose can increase the yield from products involving activity of one or few genes.  This is beneficial if the product is cell biomass or primary metabolites. 7
  • 9. Spontaneous mutation  Rate depends on growth condition of organisms  Between 10-10 to 10-5 per generation per gene  All mutant types are found although deletions are frequent  Not cost effective because of low frequency of mutation 9
  • 10. 10
  • 11. 11
  • 12. 12
  • 13. 13
  • 14. 14
  • 15. 15
  • 16. 16
  • 17. 17
  • 18. Induced mutation  Mutation frequency is significantly increased  10-5 to 10-3 for secondary metabolite producers  10-2 to 10-1 for auxotrophic mutants 18
  • 19.  Genome mutation may cause:  Change in no. of chromosomes  Chromosome mutation may change:  Order of genes by deficiency, deletion, inversion, dup lication or translocation  Gene or point mutation 19 Changes due to mutation
  • 20.  Less lethal and mutagenic effects than short wavelength UV  Exposure of cells in the presence of various dyes causes interaction of DNA with UV with greater rates which results in increased frequency of mutation  Effective activators are psoralen derivatives (e.g. 8-methoxypsoralen)  Mechanism of action: Biadduct formation between complementary strands which 20 Long wavelength UV
  • 22.  Molecular mode of action of some mutagens is well known but what can never be predicted is:  Effect of mutagen on specific gene  Effect of mutation on a complex process (e.g. biosynthesis of secondary metabolite)  Appearance of mutants depends on several factors  Base sequence of gene 22 Mode of action of mutagens
  • 23.  Base sequence of gene to be mutated:  Mutation are not evenly distributed  There are areas of high mutation frequency known as hot spots  Different mutagens cause hot spots at different sites in the 23 Factors affecting appearance of mutants
  • 24.  Strains with partially defective repair mechanisms:  Organisms may be killed without having induced mutation  Specific mutagen may be ineffective 24 Factors affecting appearance of mutants
  • 25.  Gene activity:  Become lost through mutation  Can be restored through a second mutation (suppressor mutation) 25 Factors affecting appearance of mutants
  • 26.  Act in several different ways  Occurs in the same gene that already carries primary mutation (intragenic suppressors)  Compensated through exchange of amino acid or additional insertion or deletion which corrects primary mutation 26 Suppressor mutation
  • 27.  Occurs in another gene (extragenic suppressor)  Compensate primary mutation at the level of translation by formation of mutant tRNA or ribosome 27 Suppressor mutation
  • 29. 29
  • 30. 30
  • 31. 31
  • 32. Isolation of auxotroph 32  By using certain blocked mutants, desired products such as amino acids and nucleotides may be formed via branching biosynthetic pathways. The isolation of auxotrophs is done by plating of the mutagenized population on a complete agar medium, on which the biochemically deficient mutants can also grow.
  • 33. Isolation of auxotroph 33  The antibiotic resistance character can not only be used as a genetic marker, but mutants isolated may also have increased cell permeability or a protein synthesis, making them useful for industrial purposes.
  • 34. 34
  • 35.  By means of Lederberg’s well-known replica plating technique, the clones are transferred to minimal medium where the auxotrophic colonies cannot grow. These mutants are picked up from the master plates and their defect is characterized. 35
  • 36. 36
  • 37. Isolation of auxotroph  Since in this method a large number havof plates must be  observed, various procedures e been developed to enrich for  auxotrophic mutants by removing or killing prototrophic  organisms. 37
  • 38. Isolation of auxotroph  After mutagenesis the spores of filamentous organisms (actinomycetes, fungi) are allowed to develop in a liquid minimal medium.  The developing micro colonies of prototrophs are then separated by filtration, leaving behind in the filtrate spores of auxotrophs, which have been unable to grow.  The filtrate is then plated and the resulting colonies are checked for auxotrophic characteristics. 38
  • 39. 39
  • 40. Penicillin selection method  Penicillin kills growing cells but not non-growing cells. In this procedure, growing cells are selectively killed by antibiotic treatment, thus enriching for auxotrophs, which cannot grow on minimal medium.  Several inhibitors other than penicillin can also be used in this procedure: dihydrostreptomycin for Pseudomonas aeruginosa, nalidixic acid for Salmonella typhimurium. 40
  • 41. 41
  • 42. 42
  • 43. 43
  • 44. 44
  • 45. 45
  • 46. 46
  • 47. 47
  • 48. 48
  • 49. 49
  • 50. 50
  • 51. 51
  • 52. 52
  • 53. 53
  • 54. 54
  • 55. 55
  • 56. 56
  • 57.  An enrichment procedure with sodium pentachlorophenolate makes use of the greater toxicity of this compound against germinating spores than against vegetative cells.  The method has been successfully applied with Penicillium chrysogenum, Streptomyces aureofaciens, S. olivaceus, and Bacillus subtilis. 57 Enrichment method
  • 58.  By these methods, enrichments for auxotrophs of 10- to100-fold can be attained, thus increasing the probability of obtaining mutants.  However, it should be remembered that the types of mutants present in the original population may be shifted; for instance, an increased proportion of proline auxotrophs has been found in E. 58 Enrichment method