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胡萝卜软腐果胶杆菌巴西亚种在肯尼亚引起马铃薯软腐病和黑胫病的首次报道

First Report of Pectobacterium carotovorum subsp. brasiliense Causing Soft Rot and Blackleg of Potatoes in Kenya.

作者信息

Onkendi E M, Maluleke L N, Moleleki L N

机构信息

Forestry Agriculture and Biotechnology Institute (FABI), Department of Microbiology and Plant Pathology, University of Pretoria, South Africa.

出版信息

Plant Dis. 2014 May;98(5):684. doi: 10.1094/PDIS-09-13-0988-PDN.

Abstract

During the 2012/2013 growing season, potato tubers and stems showing rotting tissue and black discoloration, respectively, were obtained for analysis from Nyandarua and Mau Narok areas of Kenya, where potatoes are widely grown. During this period, more than 50% of the farms across Kenya reported cases of soft rot and blackleg diseases. Soft rot and blackleg diseases account for as much as 1/4 of the annual potato losses in Kenya. Bacteria from infected potato tuber and stem samples were isolated on nutrient agar then transferred to crystal violet polypectate medium (CVP) according to established standard procedures (3). All pit-forming (n = 48) strains were purified on nutrient agar and stored in 30% glycerol at -80°C for further use. All strains grew at 28°C and 37°C. PCR with pel gene specific primers (Y1/Y2) produced a 434-bp product and confirmed that all 48 strains have the gene sequence coding for pectate lyase specific for Pectobacterium spp. (1). Primers (Br1f/L1r) identified 1/3 of these strains as Pectobacterium carotovorum subsp. brasiliense based on their characteristic 322 bp (2). The other Pectobacterium spp. are currently undergoing further characterization. To further identify these pectolytic strains, a multi locus sequence typing (MLST) approach was employed (4). To this end, partial nucleotide sequences of the housekeeping genes mdh and gapA (accession nos. KF72004 to KF72009) showed 92% similarity to the Pcb1692 reference strain in GenBank. These results were in agreement with those obtained by species-specific primers. Phylogenetic analysis of the 679-bp concatenated partial gene sequences grouped strains collected in this study together with Pectobacterium subsp. brasiliense strains identified in other parts of the world with a 98% bootstrap support value. Three randomly selected Kenyan strains and Pcb1692 reference strain were inoculated into potato tubers in our research laboratory by making 1-cm holes into the tubers using a sterile pipette tip and thereafter injecting 10 μl (at 1.0 × 10 cfu/ml) into the tuber for pathogenicity assays. A negative control of 10 mM MgSO was included and all the inoculated holes sealed with petroleum jelly to avoid contamination. This experiment consisted of five potato tubers per strain in three independent assays. All three representative strains induced water soaked soft symptoms similar to the symptoms previously observed on infected potato tubers. Furthermore, when bacterial suspensions of 1.0 × 10 cfu/ml isolated strains and the Pcb1692 reference strain were inoculated onto potato stems maintained at 28°C, blackleg and wilting of the stems occurred within a period of 3 to 21 days. No symptoms were observed in potato tubers or stems inoculated with the negative control (MgSO). PCR with Br1f/L1r primers confirmed that the re-isolated bacteria were P. carotovorum subsp. brasiliense. To our knowledge, this is the first occurrence of P. carotovorum subsp. brasiliense on potatoes in Kenya. References: (1) A. Darrasse et al. Appl. Environ. Microbiol. 60:1437, 1994. (2) V. Duarte et al. J. Appl. Microbiol. 96:535, 2004. (3) L. J. Hyman et al. Potato Res. 44:265, 2001. (4) Ma et al. Phytopathology 97:1150, 2007.

摘要

在2012/2013生长季,从肯尼亚广泛种植马铃薯的尼亚达鲁阿和莫纳罗克地区获取了分别表现出腐烂组织和黑色变色的马铃薯块茎及茎用于分析。在此期间,肯尼亚超过50%的农场报告了软腐病和黑胫病病例。软腐病和黑胫病占肯尼亚马铃薯年损失的多达四分之一。按照既定标准程序(3),从受感染的马铃薯块茎和茎样本中分离出细菌,接种于营养琼脂上,然后转移至结晶紫聚果胶酸盐培养基(CVP)。所有形成凹陷的(n = 48)菌株在营养琼脂上纯化,并保存在-80°C的30%甘油中以备进一步使用。所有菌株在28°C和37°C下均能生长。使用果胶酸裂解酶基因特异性引物(Y1/Y2)进行PCR产生了一个434 bp的产物,并证实所有48个菌株都具有编码果胶杆菌属特异性果胶酸裂解酶的基因序列(1)。引物(Br1f/L1r)根据其特征性的322 bp确定这些菌株中有三分之一为胡萝卜软腐果胶杆菌巴西亚种(2)。其他果胶杆菌属目前正在进行进一步鉴定。为进一步鉴定这些果胶分解菌株,采用了多位点序列分型(MLST)方法(4)。为此,管家基因mdh和gapA的部分核苷酸序列(登录号KF72004至KF72009)与GenBank中的Pcb1692参考菌株显示出92%的相似性。这些结果与通过种特异性引物获得的结果一致。对679 bp串联部分基因序列的系统发育分析将本研究收集的菌株与在世界其他地区鉴定出的胡萝卜软腐果胶杆菌巴西亚种菌株归为一组,并具有98%的自展支持值。在我们的研究实验室中,通过使用无菌移液器吸头在马铃薯块茎上打1 cm的孔,然后向块茎中注射10 μl(1.0×10 cfu/ml),将三个随机选择的肯尼亚菌株和Pcb1692参考菌株接种到马铃薯块茎中进行致病性测定。包括10 mM MgSO的阴性对照,所有接种孔用凡士林密封以避免污染。该实验在三个独立试验中每个菌株使用五个马铃薯块茎。所有三个代表性菌株均诱导出类似于先前在受感染马铃薯块茎上观察到的水渍状软腐症状。此外,当将1.0×10 cfu/ml的分离菌株和Pcb1692参考菌株的细菌悬液接种到保持在28°C的马铃薯茎上时,茎在3至21天内出现黑胫病和萎蔫。接种阴性对照(MgSO)的马铃薯块茎或茎未观察到症状。使用Br1f/L1r引物进行PCR证实重新分离出的细菌为胡萝卜软腐果胶杆菌巴西亚种。据我们所知,这是胡萝卜软腐果胶杆菌巴西亚种在肯尼亚马铃薯上的首次出现。参考文献:(1)A. Darrasse等人,《应用与环境微生物学》60:1437,1994年。(2)V. Duarte等人,《应用微生物学杂志》96:535,2004年。(3)L. J. Hyman等人,《马铃薯研究》44:265,2001年。(4)Ma等人,《植物病理学》97:1150,2007年。

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