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[苦楝丛枝植原体一个质粒的全长DNA完整序列及分子特征分析]

[Complete sequence of a full-length DNA and molecular characterization of one plasmid from chinaberry (Melia azedarach Z) witches'-broom phytoplasma].

作者信息

Song Chuansheng, Lin Caili, Tian Guozhong, Zhao Wenjun, Zhu Shuifang, Mou Haiqing, Hu Jiaxu, Wang Xizhuo, Guo Minwei

机构信息

Research Institute of Forest Ecology, Environment and Protection, Chinese Academy of Forestry/The Key Laboratory of Forest Protection, State Forestry Administration, Beijing 100091, China.

出版信息

Wei Sheng Wu Xue Bao. 2011 Sep;51(9):1158-67.

Abstract

OBJECTIVE

To clone plasmid from chinaberry witches'-broom phytoplasma and analyse its molecular characterization.

METHODS

Fragments of one plasmid (pCWBFq) in chinaberry witches'-broom phytoplasma-Fuqing strain (CWBFq) were amplified with primer pairs which were designed according to plasmid sequences published on NCBI. Transmembrane domain and subcellular localization predictions of proteins encoded by the plasmid pCWBFq as well as phylogenetic analysis among the plasmid sequences were completed by using bioinformatic softwares. Southern blot analysis was performed to detect the plasmids existed in CWBFq and several other phytoplasmas with the pCWBFq repA probe.

RESULTS

One complete plasmid was sequenced from CWBFq. pCWBFq comprised 4446 bp and had a nucleotide content of 73.5% A + T and encoded six proteins. Protein P2, P3, P4 and P5 of pCWBFq contained 3, 2, 1 and 2 tranmembrane domains respectively, and their predicted signal peptide values were 0.989, 0.505, 0.918 and 0.914 respectively. Homologous comparison showed that RepA homology between pCWBFq and other phytoplasmas was between 9.6% -85.6% , however, the homology of different SSB proteins was between 74.0% - 89.4%. Southern blotting with pCWBFq repA probe confirmed the existence of the plasmids in CWBFq. In addition, The hybridizations occurred with paulownia witches'-broom phytoplasma-Nanyang strain (PaWBNy), periwinkle virescence phytoplasma-Hainan stanin (PeVHn), chinaberry witches'-broom phytoplasma-Fuzhou strain (CWBFz) and mulberry dwarf phytoplasma - Puyang strain (MDPy), whereas, no hybridizarions occurred with jujube witches'-broom phytoplasma-Beijing strain (JWBBj), cherry lethal yellows phytoplasma-Xichang strain (CLYXc) and Bischofia polycarpa witches'-broom phytoplasma-Nanchang strain (BiWBNc).

CONCLUSION

The plasmid encoded a replication associated protein (RepA) and a single-stranded DNA binding protein (SSB), which were for the replication of plasmid. Four putative proteins encoded by the plasmid were predicted to contain one or more hydrophobic transmembrane domains, respectively, and presumably to be localized to the membrane. The alignment and homology analysis as well as phylogenetic analysis to the DNA and encoded protein amino acid sequences of the whole plasmids and single ORFs on the known phytoplasmal plasmids showed that the different homologous sequences have distinct variation, among which the repA gene with the largest diversity appeared in all the known plasmids while ssb with less variation were only found in 16SrI plasmids. CWBFq, PaWBNy, PeVHn, CWBFz and MDPy possessed distinct plasmids in terms of number and size, whereas there was no plasmid detected in JWBBj, CLYXc and BiWBNc, perhaps as a result of low homology among repA genes in plasmids of JWBBj, CLYXc and BiWBNc.

摘要

目的

克隆苦楝丛枝植原体的质粒并分析其分子特征。

方法

根据NCBI上公布的质粒序列设计引物对,扩增苦楝丛枝植原体福清菌株(CWBFq)中一个质粒(pCWBFq)的片段。利用生物信息学软件完成质粒pCWBFq编码蛋白的跨膜结构域和亚细胞定位预测以及质粒序列间的系统发育分析。用pCWBFq repA探针进行Southern杂交分析,检测CWBFq和其他几种植原体中存在的质粒。

结果

从CWBFq中测序得到一个完整质粒。pCWBFq全长4446 bp,A + T核苷酸含量为73.5%,编码6种蛋白质。pCWBFq的蛋白P2、P3、P4和P5分别含有3、2、1和2个跨膜结构域,其预测的信号肽值分别为0.989、0.505、0.918和0.914。同源性比较显示,pCWBFq与其他植原体的RepA同源性在9.6% - 85.6%之间,而不同SSB蛋白的同源性在74.0% - 89.4%之间。用pCWBFq repA探针进行的Southern杂交证实了CWBFq中质粒的存在。此外,与泡桐丛枝植原体南阳菌株(PaWBNy)、长春花黄化植原体海南菌株(PeVHn)、苦楝丛枝植原体福州菌株(CWBFz)和桑萎缩植原体濮阳菌株(MDPy)发生杂交,而与枣疯植原体北京菌株(JWBBj)、樱桃致死黄化植原体西昌菌株(CLYXc)和重阳木丛枝植原体南昌菌株(BiWBNc)未发生杂交。

结论

该质粒编码一个复制相关蛋白(RepA)和一个单链DNA结合蛋白(SSB),用于质粒复制。该质粒编码的4个推定蛋白预计分别含有一个或多个疏水跨膜结构域,可能定位于膜上。对已知植原体质粒的全质粒和单个开放阅读框的DNA及编码蛋白氨基酸序列进行比对、同源性分析和系统发育分析表明,不同同源序列具有明显差异,其中多样性最大的repA基因出现在所有已知质粒中,而变异较小 的ssb仅在16SrI质粒中发现。CWBFq、PaWBNy、PeVHn、CWBFz和MDPy在质粒数量和大小方面具有不同的质粒,而在JWBBj、CLYXc和BiWBNc中未检测到质粒,这可能是由于JWBBj、CLYXc和BiWBNc质粒中repA基因同源性较低所致。

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