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Characterization of Fusarium viruses and host factor fghal2 required for host defense against Fusarium graminearum virus 1 infection : 붉은 곰팡이에 감염하는 바이러스의 분자 생물학적 특성 및 방어 반응 관련 기주 요인의 특성 구명

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dc.contributor.advisor김국형-
dc.contributor.author유지숙-
dc.date.accessioned2017-07-13T08:22:05Z-
dc.date.available2017-07-13T08:22:05Z-
dc.date.issued2015-02-
dc.identifier.other000000025373-
dc.identifier.urihttps://hdl.handle.net/10371/119482-
dc.description학위논문 (박사)-- 서울대학교 대학원 : 농생명공학부, 2015. 2. 김국형.-
dc.description.abstractMany mycoviruses have been identified from diverse plant-pathogenic Fusarium species including F. graminearum. Infections with mycoviruses in F. graminearum mostly remain persistently and asymptomatically in their host, however, some mycoviruses causing altered phenotype, such as reduced growth, pigmentation, sporulation or virulence. Among the Fusarium graminearum viruses (FgVs), FgV1 or FgV2 infections caused several phenotypic alterations in F. graminearum. In contrast, FgV3 and FgV4 infections did not cause any phenotypic change. In this study, we determined complete genome sequences of FgV2, FgV3, and FgV4 and analyzed its phylogenetic relationship with other mycoviruses. The three mycoviruses consist of one to five different segments of dsRNA ranging in size from approximately 1.7 to 9.3 kb. FgV2 consist moinocistronic dsRNA segments, denoted as dsRNA-1 to dsRNA-5. The lengths of FgV2 dsRNAs 1–5 ranged from 2414 to 3580 base pairs (bp). The viral genome of FgV3 is 9098 bp long and contains open reading frame (ORF) encoding a putative RNA-dependent RNA polymerase and a protein of unknown function. The FgV4 genome is composed of two dsRNA genome segments of 2383bp and 1739bp. According to phylogenetic analysis, the FgV2, FgV3, and FgV4 is closed to Chrysoviridae, Totiviridae, and Partitiviridae, respectively, but consist a distinct virus clade within the Family.
Transcriptomic and protein expression profiling have shown that many F. graminearum genes are differentially expressed as a consequence of FgVs infection. Of the identified host genes involved in the interaction between mycovirus and fungus host, FgHal2 shows reduced expression in response to FgV1 infection. FgHal2 has a highly conserved 3'-phosphoadenosine 5'-phosphatase (PAP phosphatase-like) domain or inositol monophosphatase (IMPase) superfamily domain. We generated targeted gene deletion and over-expression mutants to clarify the role(s) of FgHal2 in FgV1 infection. The FgHal2 deletion led to decrease in mycelial growth, aerial mycelia formation, and pigmentation whereas over-expression mutants were morphologically similar to the wild type (WT). Furthermore, compared to the WT, the gene deletion mutant produced fewer conidia and these showed abnormal morphology. The FgHal2 expression level was decreased by FgV1 infection at 120 h post-inoculation (hpi) whereas the levels were 9-fold greater for both the virus-free and virus-infected over-expression mutant than for the WT. FgV1 RNA accumulation was decreased in the deletion mutant at 48, 72, and 120 hpi. FgV1 RNA accumulation in the over-expression mutant was reduced relative to the WT at 48 and 72 hpi but was similar to that of the WT at 72 hpi. Furthermore, the low vertical transmission rate of FgV1 and continually growing of virus-free sectors in the colonies of FgV1-infected gene deletion mutant suggesting that FgHal2 might be required for stable maintenance of FgV1 infection. Together, these results indicate that the putative 3'(2'), 5'-bisphosphate nucleotidase gene, FgHal2, has diverse biological functions in the host fungus and might affect the viral RNA accumulation and transmission of FgV1.
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dc.description.tableofcontentsABSTRACT i
CONTENTS iv
LIST OF TABLES vi
LIST OF FIGURES vii

GENERAL INTRODUCTION 1
LITERATURE CITED 6
CHAPTER I. Molecular characterization of Fusarium graminearum virus 2-4 isolated from Fusarium graminearum strain 98-8-60 and DK3. 10
ABSTRACT 11
INTRODUCTION 13
MATERIALS AND METHODS 16
I.Fungal strain and culture conditions 16
II. Double-strand RNA extraction 16
III.cDNA synthesis, amplification, cloning 17
IV.5' and 3' RACE 18
V.Northern blot hybridization 19
VI.Sequence alignment and phylogenetic analysis 19
RESULTS 21
I. Genome organization of FgV2 21
II. Genome organization of FgV3 and FgV4 27
III. Phylogenetic analysis 33
DISCUSSION 37
LITERATURE CITED 41
CHAPTER II. Characterization of the FgHal2 gene required for host defense against Fusaruim graminearum virus-1 infection. 44
ABSTRACT 45
INTRODUCTION 47
MATERIALS AND METHODS 53
I. Fungal strains and media 53
II. Sequence analysis 53
III. Construction of FgHal2 gene deletion, over-expression, complementation mutant 54
IV. DNA extraction and Southern blot hybridization 55
V. Mycelial growth, colony morphology 57
VI. Microscopic observation of conidial and hyphal morphology 58
VII. Virulence assay on flowering wheat heads 59
VIII. Total RNA extraction and gene expression level analysis 59
IX. Vertical transmission 60
RESULTS 63
I. Sequence analysis of FgHal2 63
II. Generation of mutant 67
III. Impact of FgV1 infection on FgHal2 gene expression level 70
IV. Involvement of FgHAL2 on vegetative growth and pigmentation 72
V. Effects of FgHal2 on hydrophobicity of the cell surface 76
VI. Involvement of FgHal2 on conidiation and conidial morphology 78
VII. Impact of FgHal2 on virulence of F. graminearum 78
VIII. Involvement of FgHal2 on transmission of FgV1 79
IX.Effect of FgHal2 on accumulation of FgV1 RNA 82
X. Effect of FgHal2 on silencing related genes 85
DISCUSSION 87
LITERATURE CITED 95
ABSTRACT IN KOREAN 105
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dc.formatapplication/pdf-
dc.format.extent4049476 bytes-
dc.format.mediumapplication/pdf-
dc.language.isoen-
dc.publisher서울대학교 대학원-
dc.subjectmycovirus-
dc.subject.ddc630-
dc.titleCharacterization of Fusarium viruses and host factor fghal2 required for host defense against Fusarium graminearum virus 1 infection-
dc.title.alternative붉은 곰팡이에 감염하는 바이러스의 분자 생물학적 특성 및 방어 반응 관련 기주 요인의 특성 구명-
dc.typeThesis-
dc.contributor.AlternativeAuthorJisuk Yu-
dc.description.degreeDoctor-
dc.citation.pagesviii, 106-
dc.contributor.affiliation농업생명과학대학 농생명공학부-
dc.date.awarded2015-02-
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