海南长春花黄化病植原体的16S rDNA序列分析研究

 Periwinkle(Catharanthus roseus) yellows is a common disease in Hainan. Periwinkle's leaf tissue with symptoms was assayed for phytoplasma infection by using PCR assay employing phytoplasma universal 16S rRNA gene primers (Rl6mF2/Rl6mR1). A PCR product (about 1.4 kb) was amplified from periwinkle showed yellows. Nucleotide sequencing and phylogenetic tree analysis showed that the amplified 16S rDNA contained 1 432 nucleotides, the most homology was 98.1% with the members of elm yellows group (16S r Ⅴ) and clustered in the same clade, while it was under 96.1% with other phytoplasma groups. Our results suggested that the phytoplasma sample belonged to 16S rⅤgroup and was tentatively named as Hainan periwinkle yellows phytoplasma (PY-Hn). This is the first report of existence of 16S r Ⅴ group phytoplasma in naturally infected periwinkle.     

Increased plant tolerance against chrysanthemum yellows phytoplasma (‘Candidatus Phytoplasma asteris’) following double inoculation with Glomus mosseae BEG12 and Pseudomonas putida S1Pf1Rif

The aim of this work was to assess the effects of a combined inoculum of a rhizobacterium and an arbuscular mycorrhizal (AM) fungus on plant responses to phytoplasma infection, and on phytoplasma multiplication and viability in Chrysanthemum carinatum plants infected by chrysanthemum yellows phytoplasma (CY). Combined inoculation with Glomus mosseae BEG12 and Pseudomonas putida S1Pf1Rif resulted in some resistance to phytoplasma infection (about 30%), delayed symptom expression in nonresistant plants, improved growth of the aerial part of the infected plants (+68·1%), and altered root morphology (root tip number: +49·9%; branching degree: +82·8%). Combined inoculation with the two beneficial microorganisms did not alter CY multiplication and viability. In inoculated and infected plants, phytoplasma morphology was typical of senescent cells. A more active and efficient root system in double‐inoculated plants probably mediated the effects of the two rhizospheric microorganisms in the infected plants. The practical application of rhizospheric microorganisms for mitigating phytoplasma damage, following evaluation under field conditions, represents an additional tool for the integrated management of phytoplasmosis.     

榆树黄化病植原体的分子检测与鉴定

 利用植原体16SrRNA基因的通用引物R16rrLF2/R16mR1和R16F2n/R16R2对山东泰山上发生的榆树(Ulmus parvifolia)黄化病感病植株总DNA进行巢式PCR扩增,得到了约1.2kb的特异性片段,从分子水平证实了榆树黄化病的病原(EY-China)为植原体。将扩增到的片段测序,并进行一致性和系统进化树分析。结果表明,该分离物属于植原体榆树黄化组(Candidatus Phytoplasma ulmi),与该组成员16SrRNA序列的一致性均在98.2%以上,其中与16SrV-B亚组中的纸桑丛枝(Paper mulberry wiches'-broom)和枣疯病(Jujube witches'-broom)植原体一致性最高,达到99.4%,在系统进化树中与该亚组成员聚类到同一个分支,说明该分离物属于植原体16SrV-B亚组。本研究首次对在中国引致榆树黄化病的植原体进行了分子检测,并通过核酸序列分析将其鉴定到亚组水平。     

嵌套引物P1/P7-U3/U5检测葡萄黄化(stolbur)植原体时扩增出的额外片段分析

 当采用嵌套引物P1/P7(U5/P7) U3/U5的巢式PCR检测植原体时,伴随着正常的0.85kb片段还经常扩增出一条额外片段。与其它常见的非特异性片段不同,该额外片段十分稳定,与正常片段总是同步出现,二者的强度呈正比。经测定,额外片段的大小为0.36kb。迄今,这一现象仅在采用P1/P7(U5/P7)-U3/U5引物的巢式PCR中出现。在采用P1/P7、U5/P7或-U3/U5引物的常规PCR中从未出现过。另外,已知这一现象至少在葡萄黄化stolbur和榆黄化植原体的检测过程中出现。对该现象产生的原因进行了深入研究,方法是将额外片段从凝胶中分离出来,用不同的引物在不同的条件下进行重新扩增,同时结合已知的植原体16SrRNA基因序列进行综合分析判断。结果表明,该额外片段源于植原体16SrRNA基因上存在的一个与U5引物部分互补的位点。对额外片段的测序结果进一步证实了分析的正确性。据此,指出了该额外片段在植原体检测中的可能用途。     

Detection and characterization of a phytoplasma associated with annual blue grass (Poa annua) white leaf disease in southern Italy

A phytoplasma was detected in annual blue grass (Poa annua L. Fienardo), exhibiting white leaf symptoms, that was grown in the fields near Caserta in southern Italy. Based on restriction fragment length polymorphism analysis of PCR-amplified 16S rDNA sequences, the phytoplasma associated with annual blue grass white leaf disease was identified as a new member of phytoplasma 16S rRNA group XI (16SrXI) (type strain, rice yellow dwarf phytoplasma). The annual blue grass white leaf phytoplasma is most closely related to Bermuda grass white leaf phytoplasma found in Asia. Annul blue grass white leaf and Bermuda grass white leaf phytoplasmas were designated as the third subgroup (16SrXI-C) of group XI. This is the first report that a plant pathogenic phytoplasma belonging to group 16SrXI is present on the European continent.     

瓜类褪绿黄化病毒(Cucurbit chlorotic yellows virus)在湖南省的首次报道及其流行动态研究

正瓜类褪绿黄化病毒Cucurbit chlorotic yellows virus(CCYV)属长线形病毒科(closteroviridae)毛形病毒属(crinivirus)~([1]),在世界范围内给蔬菜生产造成了严重危害,病毒侵染造成果实重量减轻10%~33%,产量减少10%~12%~([2])。CCYV不能靠摩擦接毒,只能由烟粉虱以半持久方式传播,其     

Genetic and serological analyses of elongation factor EF‐Tu of paulownia witches’‐broom phytoplasma (16SrI‐D)

This study determined the tuf gene sequence of the phytoplasma specific to paulownia witches’‐broom from Nanyang, China (hereby designated PaWB‐Ny). The PaWB‐Ny tuf gene was 1185 nucleotides in length and confirmed that the phytoplasma belongs to subgroup 16SrI‐D of aster yellows. Three characteristic GTP‐binding protein motifs were identified based on the peptide deduced from the tuf gene sequence. Results suggested that the elongation factor EF‐Tu was localized in the cytoplasm and lacked hydrophobic transmembrane domains. Antibodies against PaWB‐Ny EF‐Tu were prepared by rabbit immunization with glutathione‐S‐transferase (GST)‐tagged EF‐Tu fusion protein expressed in Escherichia coli. EF‐Tu exhibited a molecular weight of ～43 kDa and was detected in PaWB‐infected paulownia plants by western blot analysis. Indirect enzyme‐linked immunosorbent assays (ELISA) and dot blotting analyses were performed with freezing and thawing treatments during antigen preparation. Dilution of extracts to an appropriate scale significantly reduced non‐specific reactions. The resultant PaWB EF‐Tu antibody reacted with antigens from plants infected with periwinkle virescence and chinaberry tree witches’‐broom phytoplasmas, but not those infected with jujube witches’‐broom or bishopwood witches’‐broom phytoplasma. The EF‐Tu was characteristically localized within the phytoplasmal cytoplasm of infected plant phloem tissues.     

Aster yellows subgroup (Candidatus Phytoplasma sp. AY 16S-group,AY-sg) phytoplasma associated with porcelain vine showing witches' broom symptoms in South Korea

 This is the first report of a phytoplasma in porcelain vine [Ampelopsis brevipedunculata var. heterophylla (Thunb.) Hara.] with severe witches' broom symptoms in Korea. On the basis of the polymerase chain reaction-amplified ribosomal DNA, the phytoplasma infecting porcelain vine was classified as a member of the aster yellows subgroup. Received: October 21, 2002 / Accepted: December 20, 2002     

Phytoplasma [Stolbur-subgroup (Bois Noir-BN)] infection inhibits photosynthetic pigments, ribulose-1,5-bisphosphate carboxylase and photosynthetic activities in field grown grapevine (Vitis vinifera L. cv. Chardonnay) leaves

In this work we have studied the influence of phytoplasma-induced grapevine yellows (yellowing) on some features of the thylakoids from field grown grapevine (Vitis vinifera L. cv. Chardonnay) leaves. Changes in photosynthetic pigments, soluble proteins, ribulose-1,5-bisphosphate carboxylase, photosynthetic activities and thylakoid membrane proteins were investigated. The level of total chlorophyll and carotenoids, on a unit fresh weight basis, showed a progressive decrease in phytoplasma infected leaves. Similar results were also observed for total soluble proteins and ribulose-1,5-bisphosphate carboxylase activity. When various photosynthetic activities were followed in isolated thylakoids, phytoplasma infection caused marked inhibition of whole chain and photosystem (PS) II activity. Smaller inhibition of PSI activity was observed even in severely infected leaves. The artificial exogenous electron donors, DPC and NH₂OH significantly restored the PSII activity in both mild and severely infected leaves. The same results were obtained when F_v/ F_m was evaluated by Chl fluorescence measurements. The marked loss of PS II activity in infected leaves was evidently due to the loss of 33, 28–25, 23, 17 and 10 kDa polypeptides. This conclusion was confirmed by immunological studies showing that the content of the 33 kDa protein of the water-splitting complex was diminished significantly in infected leaves. Phytoplasma infection induced a fast degradation of LHCP II which became visible as yellowish colour in leaves.