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首页> 外文期刊>Ticks and tick-borne diseases >Transcriptional profiling of Rickettsia prowazekii coding and non-coding transcripts during in vitro host-pathogen and vector-pathogen interactions
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Transcriptional profiling of Rickettsia prowazekii coding and non-coding transcripts during in vitro host-pathogen and vector-pathogen interactions

机译:在体外宿主病原体和载体病原体相互作用期间Rickettia Prowazekii编码和非编码转录物的转录分析

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Natural pathogen transmission of Rickettsia prowazekii, the etiologic agent of epidemic typhus, to humans is associated with arthropods, including human body lice, ticks, and ectoparasites of eastern flying squirrel. Recently, we have documented the presence of small RNAs in Rickettsia species and expression of R. prowazekii sRNAs during infection of cultured human microvascular endothelial cells (HMECs), which represent the primary target cells during human infections. Bacterial noncoding transcripts are now well established as critical post-transcriptional regulators of virulence and adaptation mechanisms in varying host environments. Despite their importance, little is known about the expression profile and regulatory activities of R. prowazekii sRNAs (Rp_sRs) in different host cells encountered as part of the natural life-cycle. To investigate the sRNA expression profile of R. prowazekii during infection of arthropod host cells, we employed an approach combining in vitro infection, bioinformatics, RNA sequencing, and PCR-based quantitation. Global analysis of R. prowazekii transcriptome by strand-specific RNA sequencing enabled us to identify 67 cis-acting (antisense) and 26 trans-acting (intergenic) Rp_sRs expressed during the infection of Amblyomma americanum (AAE2) cells. Comparative evaluation of expression during R. prowazekii infection of HMECs and AAE2 cells by quantitative RT-PCR demonstrated significantly higher expression of four selected Rp_sRs in tick AAE2 cells. Examination of the coding transcriptome revealed differential up-regulation of > 150 rickettsial genes in either HMECs or AAE2 cells and yielded evidence for host cell-dependent utilization of alternative transcription start sites by 18 rickettsial genes. Our results thus suggest noticeable differences in the expression of both Rp_sRs as well as the coding transcriptome and the exploitation of multiple transcription initiation sites for select genes during the infection of human endothelium and tick vector cells as the host and yield new insights into rickettsial virulence and transmission mechanisms.
机译:Rickettsia prowazekii,流行病血管梗死病因症的天然病原体传播与人类有关,包括人体虱子,蜱和东部飞行松鼠的遗传癖。最近,我们在感染培养的人微血管内皮细胞(HMECs)感染期间,我们在Rickettia族物种和R. prowazekii srnas的表达中记录了小RNA的存在。在不同的宿主环境中,该细菌非编码转录物现在被定为毒力和适应机制的关键转录调节因子。尽管重要性,但对于作为自然生命周期的一部分,令人讨厌的是R. Prowazekii SRNA(RP_SRS)的表达剖面和调控活动。为了在感染节肢动物宿主细胞的感染期间研究R. prowazekii的SRNA表达谱,我们采用了一种组合体外感染,生物信息学,RNA测序和基于PCR的定量的方法。通过链状特异性RNA测序对R. prowazekii转录组的全局分析使我们能够鉴定在Amblyomma Americanum(AAE2)细胞感染期间表达的67个顺式作用(反义)和26转作rp_srs。通过定量RT-PCR对HMECS和AAE2细胞进行R. prowazekii感染期间表达的比较评价显示出蜱AAE2细胞中的四种选定的RP_SRS的显着高出表达。对编码转录组的检查显示了HMECs或AAE2细胞中> 150个rickettial基因的差异上调,并产生了18个rickettial基因的宿主细胞依赖性使用的宿主细胞依赖性利用的证据。因此,我们的结果表明,rp_srs的表达以及编码转录组和多个转录起始位点的表达差异明显差异,以及在人体内皮和蜱瘤细胞的感染期间选择基因的多个转录起始位点作为宿主,并产生新的洞察力毒力传输机制。

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