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Genome analysis of two novel Pseudomonas strains exhibiting differential hypersensitivity reactions on tobacco seedlings reveals differences in nonflagellar T3SS organization and predicted effector proteins

机译:对在烟草幼苗上表现出不同的超敏反应的两种新型假单胞菌菌株的基因组分析揭示了非鞭毛T3SS组织和预期效应蛋白的差异

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摘要

Multilocus sequence analysis (MLSA) of two new biological control strains (S1E40 and S3E12) of Pseudomonas was performed to assess their taxonomic position relative to close lineages, and comparative genomics employed to investigate whether these strains differ in key genetic features involved in hypersensitivity responses (HRs). Strain S3E12, at high concentration, incites HRs on tobacco and corn plantlets while S1E40 does not. Phylogenies based on individual genes and 16S rRNA‐gyrB‐rpoB‐rpoD concatenated sequence data show strains S1E40 and S3E12 clustering in distinct groups. Strain S3E12 consistently clustered with Pseudomonas marginalis, a bacterium causing soft rots on plant tissues. MLSA data suggest that strains S1E40 and S3E12 are novel genotypes. This is consistent with the data of genome‐based DNA‐DNA homology values that are below the proposed cutoff species boundary. Comparative genomics analysis of the two strains revealed major differences in the type III secretion systems (T3SS) as well as the predicted T3SS secreted effector proteins (T3Es). One nonflagellar (NF‐T3SS) and two flagellar T3SSs (F‐T3SS) clusters were identified in both strains. While F‐T3SS clusters in both strains were relatively conserved, the NF‐T3 style="fixed-case">SS clusters differed in the number of core components present. The predicted T3Es also differed in the type and number of style="fixed-case">CDSs with both strains having unique predicted protease‐related effectors. In addition, the T1 style="fixed-case">SS organization of the S3E12 genome has protein‐coding sequences ( style="fixed-case">CDSs) encoding for key factors such as T1 style="fixed-case">SS secreted agglutinin repeats‐toxins (a group of cytolysins and cytotoxins), a membrane fusion protein (LapC), a T1 style="fixed-case">SS ATPase of LssB family (LapB), and T1 style="fixed-case">SS‐associated transglutaminase‐like cysteine proteinase (LapP). In contrast, strain S1E40 has all style="fixed-case">CDSs for the seven‐gene operon (pelA‐pelG) required for Pel biosynthesis but not S3E12, suggesting that biofilm formation in these strains is modulated differently. The data presented here provide an insight of the genome organization of these two phytobacterial strains.
机译:进行了两个新的假单胞菌生物学控制菌株(S1E40和S3E12)的多基因座序列分析(MLSA),以评估其相对于近缘谱系的分类学位置,并采用比较基因组学来研究这些菌株在超敏反应中涉及的关键遗传特征是否不同(人力资源)。高浓度的S3E12菌株会在烟草和玉米苗上引发HR,而S1E40则不会。基于个体基因和16S rRNA-gyrB-rpoB-rpoD串联序列数据的系统发生研究表明,菌株S1E40和S3E12聚集在不同的组中。菌株S3E12始终与边缘假单胞菌聚集在一起,后者是一种在植物组织上引起软腐的细菌。 MLSA数据表明菌株S1E40和S3E12是新的基因型。这与低于临界物种边界的基于基因组的DNA-DNA同源性数据一致。两种菌株的比较基因组学分析显示,III型分泌系统(T3SS)以及预测的T3SS分泌的效应蛋白(T3Es)存在重大差异。在两个菌株中均鉴定出一个非鞭毛(NF-T3SS)和两个鞭毛T3SS(F-T3SS)簇。尽管两个菌株中的F-T3SS簇相对保守,但NF-T3 style =“ fixed-case”> SS 簇的核心成分数量有所不同。预测的T3Es在 style =“ fixed-case”> CDS s的类型和数量上也有所不同,两种菌株均具有独特的预测的蛋白酶相关效应子。此外,S3E12基因组的T1 style =“ fixed-case”> SS 组织具有蛋白质编码序列( style =“ fixed-case”> CDS s)关键因素包括T1 style =“ fixed-case”> SS 分泌的凝集素重复毒素(一组溶细胞素和细胞毒素),膜融合蛋白(LapC),T1 style =“ fixed LssB家族(LapB)的-case“> SS ATP 酶和与T1 style =” fixed-case“> SS 相关的转谷氨酰胺酶样半胱氨酸蛋白酶(LapP)。相反,菌株S1E40具有Pel生物合成所需的7个基因操纵子(pelA-pelG)的所有 style =“ fixed-case”> CDS ,而S3E12没有,这表明这些菌株中的生物膜形成是调制方式不同。此处提供的数据提供了这两个植物细菌菌株的基因组组织的见解。

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