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Enhancement of isobutanol production in engineered Saccharomyces cerevisiae by optimizing cytosolic valine biosynthesis : 세포질 내 발린 생합성 경로 최적화를 통한 재조합 효모의 아이소부탄올 생산성 향상에 관한 연구

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dc.contributor.advisor서진호-
dc.contributor.author박경혜-
dc.date.accessioned2017-07-14T06:46:36Z-
dc.date.available2018-03-30-
dc.date.issued2016-02-
dc.identifier.other000000133764-
dc.identifier.urihttps://hdl.handle.net/10371/125949-
dc.description학위논문 (석사)-- 서울대학교 대학원 : 농생명공학부 농생명공학전공, 2016. 2. 서진호.-
dc.description.abstractGlobal environmental problems due to fossil fuel and its depletion have promoted the development of microorganisms for synthesizing alternative liquid biofuels. Compared to ethanol, a traditional biofuel, biobutanol has significant advantages such as higher energy density, lower hygroscopicity and compatibility with existing transportation infrastructures. Especially, isobutanol has a higher octane number, a standard measure of the performance of gasoline. Also, it has been applied in various industrial fields and used as an important platform chemical.
In this study, Saccharomyces cerevisiae which has been traditionally used for industrial ethanol production was engineered to produce isobutanol. Naturally S. cerevisiae produces isobutanol at low concentrations by the valine biosynthesis pathway and the Ehrlich pathway. However, there are some problems because of different location of the valine biosynthesis pathway and the Ehrlich pathway. Therefore, this thesis was focused on optimizing the cytosolic valine biosynthesis pathway for improving isobutanol production.
First, investigations of various genes from bacteria involved in the valine biosynthesis pathway were conducted. The alsS gene from Bacillus subtilis which has high specificity to pyruvate was selected for expression of acetolactate synthase (ALS). The genes coding for ketolacid reductoisomerase (KARI) and dihydroxyacid dehydratase (DHAD) from Escherichia coli and Corynebacterium glutamicum were cloned and introduced to the D452-2 strain with keto acid decarboxylase (KDC) of Lactococcus lactis. All of genes which have the mitochondria targeting sequences were modified. The yeast strain containing the endogenous genes of ALS, KARI and DHAD was used as the control strain. Flask fermentations with 40 g/L glucose was carried out under micro-aerobic conditions. As a result, the isobutanol titer and yield of the strain expressing alsS from B. subtilis, ilvC and ilvD from C. glutamicum and kivD from L. lactis were the highest among engineered strains used in this study.
Second, to improve the activity of DHAD, engineering of the Fe-S cluster was conducted. The Grx3 protein controls iron sensing. Cfd1 is an important factor of the cytosolic Fe-S cluster assembly. The CRISPR/Cas9 system was used to replace the GRX3 gene in the chromosome of S. cerevisiae with the CFD1 gene to construct the D_FeS strain. The D_FeS-SK_CCMDC strain was constructed by introducing alsS from B. subtilis, ilvC and ilvD from C. glutamicum and kivD from L. lactis. Compared to the D-SK_CCMDC, the strain D_FeS-SK_CCMDC produced isobutanol titer more than 60%.
Finally, the D_FeS-SK_CCMDC was cultivated in a reactor with gas trapping and the fermentation condition was controlled by altering agitation speed and aeration. The final concentration of isobutanol of the D_FeS-SK_CCMDC was 246 mg/L with isobutanol yield (6.15 mg isobutanol/g glucose), corresponding to a 25% increase in titer and a 32% increase in yield than those obtained in flask fermentation.
These results suggested that modulation of the cytosolic valine biosynthetic pathway in combination with optimization of a fermentation process can be a successful strategy for producing isobutanol in S. cerevisiae.
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dc.description.tableofcontentsI. INTRODUCTION 1
1. Isobutanol 1
1.1. Advanced biofuel 1
1.2. Building block chemical 4
2. Microbial production of isobutanol 6
3. Isobutanol biosynthesis pathway 9
3.1. The valine biosynthesis pathway 9
3.2. The Ehrlich pathway 11
4. Cytosolic localization of the valine biosynthesis of S. cerevisiae 13
5. Cytosolic Fe-S cluster related to activity of dihydroxyacid dehydratase 19
6. Gas trapping based in situ removal system 25
7. Research objectives 26

II. MATERIALS AND METHODS 27
1. Reagents 27
2. Strains and plasmids 28
2.1. Strains 28
2.2. Plasmids 32
3. DNA manipulation and transformation 37
3.1. Enzymes 37
3.2. Polymerase chain reaction (PCR) 37
3.3. Isolation of DNA fragments and DNA sequencing 37
3.4. Transformation of E. coli 38
3.5. Preparation of plasmid DNA and bacteria genomic DNA 39
3.6. Yeast transformation 39
4. Media and culture conditions 40
4.1. Media 40
4.2. Cultivations in flasks 40
4.3. Cultivations in bioreactor with gas trapping 41
5. Analysis 43
5.1 Dry cell weight 43
5.2 Metabolite detection 43
5.3 Isobutanol detection 44

III. RESULTS AND DISCUSSIONS 46
1. Construction of the efficient isobutanol biosynthesis system 46
1.1. Comparison of acetolactate synthases from S. cerevisiae and B. subtilis 46
1.2. Evaluation of ketolacid reductoisomerase and dihydroxyacid dehydratase from various microorganisms 50
2. Engineering Fe homeostasis and Fe-S cluster synthesis 54
2.1. Construction of engineered strain by using CRISPR/Cas9 system 54
2.2. Production of isobutanol from the strain engineered for Fe-S cluster 57
3. Isobutanol production in bioreactor with gas trapping 60
3.1. Confirmation of effect of gas trapping in different conditions 60
3.2. Optimization of fermentation condition 63

IV. CONCLUSIONS 67

V. REFERENCES 68

국 문 초 록 79
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dc.formatapplication/pdf-
dc.format.extent2184812 bytes-
dc.format.mediumapplication/pdf-
dc.language.isoen-
dc.publisher서울대학교 대학원-
dc.subjectbiofuels-
dc.subjectisobutanol-
dc.subjectS. cerevisiae-
dc.subjectvaline biosynthesis pathway-
dc.subjectFe-S cluster-
dc.subjectgas trapping-
dc.subjectin situ removal system-
dc.subject.ddc630-
dc.titleEnhancement of isobutanol production in engineered Saccharomyces cerevisiae by optimizing cytosolic valine biosynthesis-
dc.title.alternative세포질 내 발린 생합성 경로 최적화를 통한 재조합 효모의 아이소부탄올 생산성 향상에 관한 연구-
dc.typeThesis-
dc.contributor.AlternativeAuthorKyung-Hye Park-
dc.description.degreeMaster-
dc.citation.pages82-
dc.contributor.affiliation농업생명과학대학 농생명공학부-
dc.date.awarded2016-02-
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