• 한국버섯학회지
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• 제19권4호
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• pp.272-278
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• 2021

Bacillus velezensis HKB-1가 표고버섯 수확후배지 퇴비로부터 분리되었으며 고추역병균(Phythopthora capsici), 인삼모잘록병균(Rhizoctonia solani), 고추탄저병균(Collectotrichum coccodes) 및 시들음병(Fusarium oxysporium)의 균사체 성장을 70% 이상 억제하는 항 진균 활성을 보였다. B. velezensis HKB-1은 표고버섯 수확후배지 퇴비 물 추출물과 당밀 1% 첨가배지에서 다른 상업용 세균배지보다 10~100배 더 높은 세균증식률을 보였으며 고추 역병균의 균사체 생장을 90% 억제하였으며 고추생육 촉진효과 및 고추역병에 대하여 70% 이상의 방제효과가 있었다.

• 한국작물학회지
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• 제65권4호
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• pp.314-326
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• 2020

본 연구는 유전자의 확대와 집적을 통해 벼 흰잎마름병균 K3a에 대응하는 저항성 계통을 육성하였고 육성계통에 대한 육종과정, 병 저항성반응을 분석하여 저항성 계통의 기초자료와 재배 효과를 제공하여 우수한 벼 흰잎마름병 저항성 품종 개발에 활용하고자 실험을 수행하였다. 벼 흰잎마름병 저항성 Xa3 유전자를 가지고 있는 중만생 자포니카 품종 황금누리를 반복친으로, Xa21 유전자를 가진 중만생 인디카 근동질유전자계통 IRBB21을 수여친으로 인공교배 후 3번 여교배하여 ABLs21을 얻었다. 생물검정과 분자표지검정을 활용하여 저항성 유전자 Xa3, Xa21이 집적을 확인하였다. ABLs21이 보유한 저항성 유전자는 분자표지 9643.T4 (Xa3), U1/I1 (Xa21)로 PCR 한 결과 모두 증폭되어 저항성 유전자를 가지는 것으로 확인되었다. ABLs21과 모부본의 벼 흰잎마름병 레이스에 대한 저항성 반응은 황금누리, IRBB3가 K1, K2, K3 레이스에 저항성 반응을 보였지만 K3a, K4, K5에는 감수성 반응을 나타냈다. IRBB21은 K1에 감수성 반응이었고 K2~K5에는 저항성 반응이었다. K3a 레이스 균주 접종 시 유묘단계에서 황금누리, IRBB21, ABL21-1, 분얼단계에서 황금누리, IRBB21, 성체단계에서 황금누리가 감수성 반응이었다. ABL21-1은 분얼단계에서 중도저항성을, 성체단계에서 저항성 반응을 나타냈다. K3a 레이스 18개 균주 접종 결과 ABL21-1은 각각의 수여친보다 병반길이와 표준편차가 작아 안정적인 저항성을 보여주었다. 18개 균주 각각의 반복간 병반길이의 유의차는 없어 균주의 병원성은 안정적이었으며 군집분석 결과 HB4032 균주의 병원력이 가장 큰 것으로 나타났다. ABLs21의 분자표지 다형성은 63.2%이며 평균 86.1 cM의 염색체단편이 이입되었다. ABLs21의 Xa21 유전자 부위로 추정되는 곳에 수여친의 염색체단편 이입이 일어났다.

• Journal of Plant Biotechnology
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• 제33권4호
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• pp.309-313
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• 2006

본 연구는 흰잎마름병 K1 레이스에 감수성인 상주찰벼와 저항성인 HR13721-53-3-1-3-3-2-2를 인공교배하여 육성된 F2, F3를 재료로 하천 Kl 레이스에 대한 저항성 검정과 SNP 마커를 이용한 유전자형 분석 및 저항성과의 연관성을 분석하였다. Kl 레이스에 대한 저항성 검정 결과 $F_2,\;F_3$에서 각각 이론적 분리비인 3:1, 1:1의 분리비를 나타냈으며 SNP 마커를 이용한 유전자형 분석은 16PFXa1 primer를 이용하여 유전자를 증폭한 후 Eco RV 제한효소 처리하여 다형성을 분석하여 저항성 및 유전자형을 확인할 수 있었다. K1 레이스에 대한 저항성 검정과SNP마커를 이용한 유전자형의 연관분석 결과 저항성과 마커간에 연관성이 일치하였으며, 특히 SNP 마커를 이용한 유전자형 분석에서는 K1 레이스에 대한 저항성 검정에서 알 수 없었던 $F_2$ 개체가 동형접합체인지 이형접합체인지를 판별할 수 있어 저항성 품종 육종을 위한 선발 효율을 높일 수 있었다.

• 한국육종학회지
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• 제41권3호
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• pp.314-318
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• 2009

"진백"은 국립식량과학원 벼맥류부에서 2008년도에 육성한 중만생 고품질 벼흰잎마름병 신균계, K3a 저항성 품종으로 주요특성과 수량성을 요약하면 다음과 같다. 1. 남서해안지, 호남 및 영남평야지 보통기 보비재배에서 평균 출수기가 8월 18일로 남평벼보다 1일 늦은 중만생종이다. 2. 간장은 71 cm로 '남평벼'에 비해 8 cm 정도 작고 주당 수수는 남평벼와 비슷하며 수당립수는 적고 등숙비율이 다소 높은 중립종에 속한다. 3. 위조현상은 나타나지 않았으며 성숙기 하엽노화가 늦고 수발아는 남평벼보다 잘 안되는 편이다. 춘천 내냉성 검정 결과 '남평벼'에 비해 유묘기 내냉성은 비슷하나 출수가 6일 정도 지연되며 내냉성 임실율이 낮은 편이다. 4. 진백은 Xa3, xa5 저항성 유전자가 집적된 품종으로 벼흰잎마름병(K1~K3, K3a)에는 강한 저항성 반응을 보였다. 5. 입형은 현미장폭비가 1.76으로 단원형이며 심복백은 거의 없고 남평벼 수준으로 맑고 투명하다. 아밀로스 및 단백질 함량은 남평벼에 비해 낮고 밥맛은 양호하며 제현율, 현백율 및 도정율은 남평벼와 비슷하나 백미완전미율은 다소 낮다. 6. 쌀수량은 보통기 보비재배에서 5.30 MT/ha로 남평벼보다 5% 낮았으나 벼흰잎마름병 발병상습지에서는 이병성인 남평벼에 비해 높은 수량을 보였다.

• The Plant Pathology Journal
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• 제33권4호
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• pp.434-439
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• 2017

Incidence rates of diseases in kiwiberry orchards were investigated monthly from late June to late September in Gwangyang and Boseong in 2015 and 2016. The impact of postharvest fruit rot was investigated during ripening after harvest. Bacterial canker was only observed on one single tree in 2015, but black rot, powdery mildew, leaf spot and blight, and postharvest fruit rot diseases were problematic throughout the study period in both 2015 and 2016. Incidence rates of the diseases varied with kiwiberry cultivar, region and sampling time. Incidence rates of powdery mildew, leaf spot and blight diseases increased significantly during the late growing stages near fruit harvest, while black rot peaked in late August. Incidence rate of postharvest fruit rot on fruit without fruit stalks was less than half of fruit with fruit stalks, regardless of kiwiberry cultivars. Among the four cultivars, Mansu was relatively resistant to black rot and postharvest fruit rot diseases. In our knowledge, this is the first report of various potential pathogens of kiwiberry in Korea.

• The Plant Pathology Journal
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• 제37권4호
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• pp.404-412
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• 2021

Despite the plant microbiota plays an important role in plant health, little is known about the potential interactions of the flower microbiota with pathogens. In this study, we investigated the microbial community of apple blossoms when infected with Erwinia amylovora. The long-read sequencing technology, which significantly increased the genome sequence resolution, thus enabling the characterization of fire blight-induced changes in the flower microbial community. Each sample showed a unique microbial community at the species level. Pantoea agglomerans and P. allii were the most predominant bacteria in healthy flowers, whereas E. amylovora comprised more than 90% of the microbial population in diseased flowers. Furthermore, gene function analysis revealed that glucose and xylose metabolism were enriched in diseased flowers. Overall, our results showed that the microbiome of apple blossoms is rich in specific bacteria, and the nutritional composition of flowers is important for the incidence and spread of bacterial disease.

• The Plant Pathology Journal
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• 제25권1호
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• pp.62-69
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• 2009

In this study, we characterized the bacterial strain KJ2C12 in relation with its biocontrol activity against Phytophthora capsici on pepper, and identified this strain using morphological, physiological, biochemical, fatty acid methyl ester, and 16S rRNA gene sequence analyses. Strain KJ2C12 significantly (P=0.05) reduced both final disease severity and areas under the disease progress curves of 5-week-old pepper plants inoculated with P. capsici compared to buffer-treated controls. As for the production of antibiotics, biofilms, biosurfactant, extracellular enzyme, HCN, and swarming activity, strain KJ2C12 produced an extracellular enzyme with protease activity, but no other productions or swarming activity. However, Escherichia coli produced weak biofilm only. Strain KJ2C12 could colonize pepper roots more effectively in a gnotobiotic system using sterile quartz sand compared to E. coli over 4 weeks after treatments. However, no bacterial populations were detected in 10 mM $MgSO_4$ buffer-treated controls. Strain KJ2C12 produced significantly higher microbial activity than the $MgSO_4$-treated control or E. coli over 4 weeks after treatments. Bacterial strain KJ2C12 was identified as Bacillus luciferensis based on morphological, physiological, and biochemical characteristics as well as FAME and 16S rRNA gene sequence analyses. In addition, these results suggested that B. luciferensis strain KJ2C12 could reduce Phytophthora blight of pepper by protecting infection courts through enhanced effective root colonization with protease production and an increase of soil microbial activity.

• Mycobiology
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• 제29권4호
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• pp.218-223
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• 2001

A rapid radicle assay for prescreening antagonistic bacteria to Phytophthora capsic4 causal agent of Phytophthora blight of pepper was developed. Sixty-four bacterial strains with in vitro antifungal activity selected out of 1,400 strains isolated from soils of Ansung, Chunan, Koyang, and Paju, Korea in 1998 were used for development of the bioassay. Uniformly germinated pepper seeds dipped in bacterial cells for 3 hours were placed near the edges of growing mycelia of P. capsici on water agar containing 0.02% glucose. Five-week-old pepper plants(cv. Nockwang) were inoculated to compare with results of the radicle assay developed in this study. For plant inoculation, pepper seeds were sown in potting mixtures incorporated with the bacterial strains, then transplanted into steam-sterilized soils 3 weeks later. Plants were hole-inoculated with zoospores of P. capsici 2 weeks after transplanting. Disease incidence and severity were determined in radicle and plant assessments, respectively. In radicle assay, six strains, GK-B15, GK-B25, OA-B26, OA-B36, PK-B09, and VK-B14 consistently showed the significant(P=0.05) disease reduction against radicle infection by the fungus, four of which also did in plant assessments. Strains OA-B36 and GK-B15 consistently reduced the fungal infection in both the radicle assay and the plant assessment. Therefore, prescreening strains using the radicle assay developed in this study followed by plant assay could reduce time and labor, and improved the possibility of selecting antagonistic bacteria for control of Phytophthora blight of peppers.

• 한국미생물·생명공학회지
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• 제50권4호
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• pp.563-573
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• 2022

Xanthomonas arboricola pv. juglandis (Xaj) is a globally important bacterial pathogen of walnut trees that causes substantial economic losses in commercial walnut production. Although prophages are common in bacterial plant pathogens and play important roles in bacterial diversity and pathogenicity, there has been limited investigation into the distribution and function of prophages in Xaj. In this study, we identified and characterized 13 predicted prophages from the genomes of 12 Xaj isolates from around the globe. These prophages ranged in length from 11.8 kb to 51.9 kb, with between 11-75 genes and 57.82-64.15% GC content. The closest relatives of these prophages belong to the Myoviridae and Siphoviridae families of the Caudovirales order. The phylogenetic analysis allowed the classification of the prophages into five groups. The gene constitution of these predicted prophages was revealed via Roary analysis. Amongst 126 total protein groups, the most prevalent group was only present in nine prophages, and 22 protein groups were present in only one prophage (singletons). Also, bioinformatic analysis of the 13 identified prophages revealed the presence of 431 genes with an average length of 389.7 bp. Prokka annotation of these prophages identified 466 hypothetical proteins, 24 proteins with known function, and six tRNA genes. The proteins with known function mainly comprised prophage integrase IntA, replicative DNA helicase, tyrosine recombinase XerC, and IS3 family transposase. There was no detectable insertion site specificity for these prophages in the Xaj genomes. The identified Xaj prophage genes, particularly those of unknown function, merit future investigation.

• The Plant Pathology Journal
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• 제39권1호
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• pp.123-135
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• 2023

Previously, Pseudomonas plecoglossicida YJR13 and Pseudomonas putida YJR92 from a sequential screening procedure were proven to effectively control Phytophthora blight caused by Phytophthora capsici. In this study, we further investigated the anti-oomycete activities of these strains against mycelial growth, zoospore germination, and germ tube elongation of P. capsici. We also investigated root colonization ability of the bacterial strains in square dishes, including cell motility (swimming and swarming motilities) and biofilm formation. Both strains significantly inhibited mycelial growth in liquid and solid V8 juice media and M9 minimal media, zoospore germination, and germ tube elongation compared with Bacillus vallismortis EXTN-1 (positive biocontrol strain), Sphingomonas aquatilis KU408 (negative biocontrol strain), and MgSO₄ solution (untreated control). In diluted (nutrient-deficient) V₈ juice broth, the tested strain populations were maintained at >10⁸ cells/ml, simultaneously providing mycelial inhibitory activity. Additionally, these strains colonized pepper roots at a 10⁶ cells/ml concentration for 7 days. The root colonization of the strains was supported by strong swimming and swarming activities, biofilm formation, and chemotactic activity towards exudate components (amino acids, organic acids, and sugars) of pepper roots. Collectively, these results suggest that strains YJR13 and YJR92 can effectively suppress Phytophthora blight of pepper through direct anti-oomycete activities against mycelial growth, zoospore germination and germ tube elongation. Bacterial colonization of pepper roots may be mediated by cell motility and biofilm formation together with chemotaxis to root exudates.