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Characterizing the replication and stability regions of Spiroplasma citri plasmids identifies a novel replication protein and expands the genetic toolbox for plant-pathogenic spiroplasmas

机译:表征螺旋肌腱质粒的复制和稳定性区域鉴定了一种新型复制蛋白,并扩大了植物致病螺旋状的遗传工具箱

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Spiroplasma citri strain GII3 contains seven plasmids, pSciA and pSci1–6, that share extensive regions of sequence homology and display a mosaic gene organization. Plasmid pSci2 comprises 12 coding sequences (CDS), three of which encode polypeptides homologous to proteins Soj/ParA, involved in chromosome partitioning, and TrsE and Mob/TraG, implicated in the type IV secretion pathway. One CDS encodes the adhesin-like protein ScARP3d whereas the other eight encode polypeptides with no homology to known proteins. The pSci2 CDS pE and soj have counterparts in all seven plasmids. Through successive deletions, various pSci2 derivatives were constructed and assessed for their ability to replicate by transformation of S. citri 44, a strain which has no plasmid. The smallest functional replicon was found to contain a single CDS (pE) and its flanking intergenic regions. Shuttle (S. citri/Escherichia coli) plasmids, in which CDS pE was disrupted, failed to replicate in S. citri, suggesting that PE is the replication protein of the S. citri plasmids. Successive propagations of pSci2-derived transformed spiroplasmas, in the absence of selection pressure, revealed that only pSci2 derivatives having an intact soj gene were stably maintained, indicating that the soj-encoded polypeptide is most likely involved in plasmid partitioning. Upon transformation, pSci2 derivatives, including shuttle (S. citri/E. coli) plasmids, were shown to replicate in all S. citri strains tested regardless of whether the strain possesses endogenous plasmids, such as strain GII3, or not, such as strain R8A2. In addition, the pSci replicons were introduced efficiently into the plant-pathogenic spiroplasmas Spiroplasma kunkelii and Spiroplasma phoeniceum, the transformation of which had never, to our knowledge, been described before. These studies show that, besides their implications for the biology of S. citri, the pSci plasmids hold considerable promise as vectors of general use for genetic studies of plant-pathogenic spiroplasmas. As an example, a HA-tagged S. citri protein was expressed in S. kunkelii. Detection of pE-hybridizing sequences in various group I spiroplasma species indicated that pE replicating plasmids were not restricted to the three plant-pathogenic spiroplasmas.
机译:螺旋肌菌菌株GII3含有七种质粒,pscia和psci1-6,其份数是序列同源性的广泛区域,并显示马赛克基因组织。质粒pSCI2包含12个编码序列(CDS),其中三种编码多肽与蛋白质SOJ / PARA同源的多肽,参与染色体分配,以及TRSE和MOB / TRAG,涉及IV型分泌途径。一个CD编码粘附蛋白样蛋白质Scarp3d,而另外八个编码多肽没有与已知蛋白质没有同源性。 PSCI2 CDS PE和SOJ在所有七种质粒中都有对应物。通过连续的缺失,构建和评估各种PSCI2衍生物,以通过转化的S. Citri 44,一种没有质粒的菌株来复制的能力。发现最小的功能性复制子包含单个CD(PE)及其侧翼的基因区域。班车(CITRI / eScherichia Coli)质粒,其中CDS PE被破坏,未被在S.Citri中复制,表明PE是S. Citri质粒的复制蛋白。在没有选择压力的情况下,PSCI2衍生转化的螺旋状物的连续传播揭示只有稳定地保持具有完整的SOJ基因的PSCI2衍生物,表明SOJ编码的多肽最有可能参与质粒分配。在转化后,PSCI2衍生物,包括梭子,包括育核苷酸的梭藻,包括在所有S.菌株是否具有内源性质粒,例如菌株,例如菌株R8A2。此外,PSCI复制品有效地引入植物致病螺旋状螺旋状螺旋状和螺旋状肺血症,其在之前从未如此知识过的转变。这些研究表明,除了对S. Citri的生物学的影响之外,PSCI质粒是否认为植物致病螺旋瘤的遗传研究的一般用途是相当大的。例如,在S.Kunkelii中表达了HA标记的S. Citri蛋白。检测各种群中的PE杂交序列螺旋状物种表明PE复制质粒不限于三种植物病原螺旋状斑块。

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