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1
Represents a New Host of the 16SrI Group of Phytoplasma Associated with Yellow Leaf Symptoms in China.代表中国与黄叶症状相关的植原体16SrI组的一个新寄主。
Plant Dis. 2023 Nov 3. doi: 10.1094/PDIS-09-23-1820-PDN.

代表中国与黄叶症状相关的植原体16SrI组的一个新寄主。

Represents a New Host of the 16SrI Group of Phytoplasma Associated with Yellow Leaf Symptoms in China.

作者信息

Cao Lu, Deng Wenqiao, Lin Yu-Feng, Zhu Xiuxiu, Xu Xiumei, Zhang Zheng Bing, Li Xin Wen, Li Yi, Wang Fang, Qin Jingjing, Yu Xiaoying, Xu Jian Ping, Cheng Yi

机构信息

Hunan Agricultural University, College of Horticulture,, Changsha, China;

Changsha Academy of Agricultural Sciences, Changsha, China;

出版信息

Plant Dis. 2023 Nov 3. doi: 10.1094/PDIS-09-23-1820-PDN.

DOI:10.1094/PDIS-09-23-1820-PDN
PMID:37923979
Abstract

Ampelopsis grossedentata, commonly known as "Vine Tea" and well-recognized for its rich flavonoid content, is mainly distributed in the southern regions of the Yangtze River basin in China. These regions include Hunan, Hubei, Jiangxi, and Guizhou provinces. Vine Tea is mainly consumed as an herbal tea and has garnered attention for its reported health benefits, including antioxidant, anti-inflammatory, anti-tumor, anti-diabetic, and neuroprotective properties. It has been used to alleviate coughs and sore throats (Zhang et al., 2021; Wang et al., 2017; Gao et al., 2009). In the Zhangjiajie region of Hunan province alone, the Vine Tea planting area reached 7,670.5 hectares and produced commercial goods worth 1.417 billion RMB in 2022. In May 2021, leaf margins and veins fading to yellowing mottling, and crumpling of leaf blades in the shape of a boat symptoms were found in ~16% of Vine Tea plants in the Sanjiakuan Township, Yongding District, Zhangjiajie region (29°15'E, 110°30' N) (Figure 1a, b, c). (Figure 1a, b, c). Phytoplasma-like microbial cells (small oval shaped bacterial cells, around 1000 nm in size) were observed in sieve tube cells in the phloem of diseased leaves using transmission electron microscopy. No such cell was observed in the phloem of healthy leaves (Figure 2a, b). To investigate the potential association between phytoplasma and the observed symptoms of the diseased plants, total DNA was isolated from ten diseasedeaves and compared with ten healthy leaves from the same field using SteadyPure Plant Genomic DNA Extraction Kit. The isolated DNAs were analyzed first in a direct PCR using universal phytoplasma primer pair R16mF2/R16mR1 targeting the 16S rRNA gene (Gundersen and Lee 1996) and specific pair rpF1/rpR1 (Lee et al. 1998) targeting the DNA fragment encoding partial ribosomal proteins (rp) L22 (complete) and S3 and S19 (partial). The initial amplified products were used as templates and further amplified by nested PCR respectively with primer pair R16F2n/R16R2 for the 16S rRNA gene (Lee et al. 1998) and the rpF2/rpR2 primer pair for the rp gene (Martini et al. 2007). No amplification was obtained with DNA from healthy leaf samples using any of the four primer pairs. The amplified fragments from diseased leaves by nested PCR were cloned and sequenced (Qingke Biotech, China). The obtained sequences have been deposited in GenBank with accession numbers OR282806 for the 16S rRNA gene and GenBank OR353012 for the rp gene. BLASTn analysis revealed that the partial 16S rRNA gene sequence in our sample shared 99.4% nucleotide sequence identity with 'Candidatus Phytoplasma sp.' (MW364378) and 'Peony yellows phytoplasma' (KY814723) of the 16SrI group. Similarly, our rp gene sequence shared 99.6% nucleotide identity with the rpI group of phytoplasma such as the 'Balsamine virescence phytoplasma' (JN572890) and 'Paulownia witches'-broom phytoplasma' (HM146079). Phylogenetic analysis of the 16S rRNA and rp sequences using MEGA version 7.0 revealed that the phytoplasma strain associated with A. grossedentata yellow leaf syndrome in our study site belonged to the 16SrI (Candidatus Phytoplasma asteris) group of phytoplasma (Figure 3a, b). Using the interactive online phytoplasma classification tool iPhyClassifier (Zhao et al., 2009), virtual restriction fragment length polymorphism (RFLP) analysis of the 16S rRNA gene sequences showed our strain having a distinct RFLP map but was closest to that of the onion yellow phytoplasma 16SrI-B subgroup (GenBank accession number: AP006628), with a similarity coefficient of 0.94 (Figure 4a, b). To confirm phytoplasma transmission, healthy plants were inoculated with three scions of infected plants of A. grossedentata. After 16 days, the new leaves of the inoculated A. grossedentata showed yellow leaf symptoms (Figure 5a, b, c), akin to the symptoms originally observed in the field, and the outer contour of the leaf margin appeared chlorotic. After 26 days, primer pairs R16mF2/R16R1 and R16F2n/R16R2 were used for nested PCR detection of phytoplasma in symptomatic A. grossedentata leaves. Phytoplasma was detected in the first and second leaves of symptomatic branches and leaves while negative control showed no amplification. Sequencing of the amplified fragments showed 100% nucleotide identity to the strain from the grafting source. Our results indicated that the pathogen and the disease can be transmitted by tissue grafting, consistent with the biological characteristics of phytoplasma, and further confirmed that the phytoplasma was the pathogen of yellow leaf syndrome of A. grossedentata. Toour knowledge, this is the first report of phytoplasma of group 16SrI affecting A. grossedentata.

摘要

显齿蛇葡萄,俗称“藤茶”,因其富含黄酮类化合物而闻名,主要分布在中国长江流域的南部地区。这些地区包括湖南、湖北、江西和贵州省。藤茶主要作为草药茶饮用,并因其所报道的健康益处而受到关注,这些益处包括抗氧化、抗炎、抗肿瘤、抗糖尿病和神经保护特性。它已被用于缓解咳嗽和喉咙痛(Zhang等人,2021年;Wang等人,2017年;Gao等人,2009年)。仅在湖南省张家界地区,2022年藤茶种植面积就达到7670.5公顷,商业产值达14.17亿元人民币。2021年5月,在张家界地区永定区三家馆乡(东经29°15′,北纬110°30′)约16%的藤茶植株中发现叶片边缘和叶脉褪绿变黄斑驳,叶片呈船形皱缩症状(图1a、b、c)。(图1a、b、c)。使用透射电子显微镜在患病叶片韧皮部的筛管细胞中观察到类植原体微生物细胞(小椭圆形细菌细胞,大小约1000纳米)。在健康叶片的韧皮部未观察到此类细胞(图2a、b)。为了研究植原体与患病植株所观察到症状之间的潜在关联,使用SteadyPure植物基因组DNA提取试剂盒从十个患病叶片中分离总DNA,并与同一田地的十个健康叶片进行比较。首先使用通用植原体引物对R16mF2/R16mR1靶向16S rRNA基因(Gundersen和Lee,1996年)以及特异性引物对rpF1/rpR1(Lee等人,1998年)靶向编码部分核糖体蛋白(rp)L22(完整)和S3及S19(部分)的DNA片段,对分离的DNA进行直接PCR分析。最初的扩增产物用作模板,分别用引物对R16F2n/R16R2对16S rRNA基因(Lee等人,1998年)和rpF2/rpR2引物对rp基因(Martini等人,2007年)进行巢式PCR进一步扩增。使用任何四对引物对健康叶片样本的DNA均未获得扩增。通过巢式PCR从患病叶片扩增的片段进行克隆和测序(中国擎科生物)。获得的序列已存入GenBank,16S rRNA基因的登录号为OR282806,rp基因的登录号为GenBank OR353012。BLASTn分析显示,我们样本中的部分16S rRNA基因序列与16SrI组的“‘Ca. Phytoplasma sp.’”(MW364378)和“牡丹黄化植原体”(KY814723)具有99.4%的核苷酸序列同一性。同样,我们的rp基因序列与植原体的rpI组如“凤仙花变绿植原体”(JN572890)和“泡桐丛枝植原体”(HM146079)具有99.6%的核苷酸同一性。使用MEGA 7.0版本对16S rRNA和rp序列进行系统发育分析表明,我们研究地点与显齿蛇葡萄黄叶综合征相关的植原体菌株属于植原体的16SrI(‘Ca. Phytoplasma asteris’)组(图3a、b)。使用交互式在线植原体分类工具iPhyClassifier(Zhao等人,2009年),对16S rRNA基因序列进行虚拟限制性片段长度多态性(RFLP)分析表明,我们的菌株具有独特的RFLP图谱,但最接近洋葱黄化植原体16SrI - B亚组(GenBank登录号:AP006628),相似系数为0.94(图4a、b)。为了确认植原体传播情况,用三株感染显齿蛇葡萄的接穗接种健康植株。16天后,接种的显齿蛇葡萄新叶出现黄叶症状(图5a、b、c),类似于最初在田间观察到的症状,叶缘外轮廓出现黄化。26天后,使用引物对R16mF2/R16R1和R16F2n/R16R2对有症状的显齿蛇葡萄叶片进行植原体巢式PCR检测。在有症状的枝条和叶片的第一片和第二片叶子中检测到植原体,而阴性对照未显示扩增。扩增片段的测序显示与嫁接源菌株具有100%的核苷酸同一性。我们的结果表明,病原体和疾病可以通过组织嫁接传播,这与植原体的生物学特性一致,并进一步证实植原体是显齿蛇葡萄黄叶综合征的病原体。据我们所知,这是16SrI组植原体影响显齿蛇葡萄的首次报道。