新疆农业科学 ›› 2024, Vol. 61 ›› Issue (7): 1766-1771.DOI: 10.6048/j.issn.1001-4330.2024.07.024
洪飞1,2(), 贾丰莲1, 刘易2, 吴燕2, 杨茹薇2(
), 孙慧2, 李广悦1(
)
收稿日期:
2024-01-05
出版日期:
2024-07-20
发布日期:
2024-09-04
通信作者:
李广悦(1983-),男,河北沧州人,研究员,博士生导师,研究方向为植物病害生物防治,(E-mail)liguangyue@caas.cn;作者简介:
沈洪飞(1989-),男,云南昆明人,助理研究员,研究方向为马铃薯育种及病害防治,(E-mail)hongfeiscience@163.com
基金资助:
SHEN Hongfei1,2(), JIA Fenglian1, LIU Yi2, WU Yan2, YANG Ruwei2(
), SUN Hui2, LI Guangyue1(
)
Received:
2024-01-05
Published:
2024-07-20
Online:
2024-09-04
Supported by:
摘要:
【目的】分离鉴定引起新疆马铃薯黑痣病病原菌,为筛选防治该病药剂奠定基础。【方法】从新疆吉木萨尔县、奇台县、乌鲁木齐市达坂城区和昭苏县等马铃薯种植区采集马铃薯块茎,通过组织分离法从带有马铃薯黑痣病的块茎分离病原菌,利用电子显微镜观察病原菌的形态特征,进行对峙培养和ITS序列分析,鉴定融合群。【结果】从新疆吉木萨尔县、奇台县、乌鲁木齐市达坂城区和昭苏县分离的4株病原菌均能使马铃薯块茎出现马铃薯黑痣病症状,分离菌株均为AG3融合群。【结论】AG3融合群是新疆马铃薯黑痣病的主要致病群。
中图分类号:
洪飞, 贾丰莲, 刘易, 吴燕, 杨茹薇, 孙慧, 李广悦. 新疆马铃薯黑痣病病原菌的分离及定[J]. 新疆农业科学, 2024, 61(7): 1766-1771.
SHEN Hongfei, JIA Fenglian, LIU Yi, WU Yan, YANG Ruwei, SUN Hui, LI Guangyue. Isolation and identification of the pathogen for potato black scurf in Xinjiang[J]. Xinjiang Agricultural Sciences, 2024, 61(7): 1766-1771.
引物名称 Primer name | 引物序列(5'-3') Primer sequence(5'-3') |
---|---|
ITS1 | TCCGTAGGTGAACCTGCGG |
ITS4 | TCCTCCGCTTATTGATATGC |
AG-2-1-F | CAAAGGCAATGGGTTATTGGAC |
AG-2-1-R | CCTGATTTGAGATCAGATCATAAAG |
Rs1F2 | TTGGTTGTAGCTGGTCTATTT |
AG-3PR2 | ACACTGAGATCCAGCTAATA |
表1 病原菌鉴定引物
Tab.1 Primers for pathogen identification
引物名称 Primer name | 引物序列(5'-3') Primer sequence(5'-3') |
---|---|
ITS1 | TCCGTAGGTGAACCTGCGG |
ITS4 | TCCTCCGCTTATTGATATGC |
AG-2-1-F | CAAAGGCAATGGGTTATTGGAC |
AG-2-1-R | CCTGATTTGAGATCAGATCATAAAG |
Rs1F2 | TTGGTTGTAGCTGGTCTATTT |
AG-3PR2 | ACACTGAGATCCAGCTAATA |
图1 病薯样品中分离出病原菌在不同时间点的形态特征的变化 注:A~C为菌丝生长特征;E为72 h菌落形态,F为96 h菌落形态,G为168 h菌落形态
Fig.1 Changes of morphological characteristics of pathogen isolated from potato sample infected with R.solani Note: A-C is the hyphal growth characteristic; E is the colony of pathogen incubatedon in PDA media for 72 hours, F is the colony of pathogen incubatedon in PDA media for 96 hours, and G is the colony of pathogen incubatedon in PDA media for 168 hours
图2 分离菌株的致病性验证 注:CK为不接带菌土壤,收获的块茎;XJ1-4为回接带分离菌株毒土,收获的块茎
Fig.2 Verification of pathogenicity of the isolated strains Note: CK is harvested tuber from soil without tuber; XJ1-4 was a tieback strain isolated from tuber and harvested tuber
图3 特异性引物PCR扩增的凝胶电泳图 注:A图为原始病原菌的ITS区通用引物ITS1/IT4的PCR扩增的电泳图,M为Star Marker D2000 PlusⅡ,1~4为新疆马铃薯分离的菌株XJ1-4;B图为回接后重新分离的病原菌的PCR扩增验证的电泳图,1~4是通用引物ITS1/IT4;5-8是特异性引物AG-2-1-F/R,9-12是特异性引物Rs1F2/AG-3PR2
Fig.3 Gel electrophoresis of the PCR amplification with specific primer Note: A is the electrophoretic PCR amplification of universal primer ITS1/IT4 in ITS region of the original pathogen, M is Star Marker D2000 PlusⅡ, 1-4 is strain XJ1-4 isolated from Xinjiang potato.The B diagram is an electrophoretic diagram of PCR amplification verification of pathogens reisolated after tieback.1-4 are universal primers ITS1/IT4.5-8 is the specific primer AG-2-1-F/R, and 9-12 is the specific primer Rs1F2/AG-3PR2
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