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Experimental annotation of the human pathogen Candida albicans coding and noncoding transcribed regions using high-resolution tiling arrays.

机译:使用高分辨率切片阵列对人类病原体白色念珠菌编码和非编码转录区进行实验注释。

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摘要

Background: Compared to other model organisms and despite the clinical relevance of the pathogenic yeast Candida albicans, no comprehensive analysis has been done to provide experimental support of its in silico-based genome annotation. Results: We have undertaken a genome-wide experimental annotation to accurately uncover the transcriptional landscape of the pathogenic yeast C. albicans using strand-specific high-density tiling arrays. RNAs were purified from cells growing under conditions relevant to C. albicans pathogenicity, including biofilm, lab-grown yeast and seruminduced hyphae, as well as cells isolated from the mouse caecum. This work provides a genome-wide experimental validation for a large number of predicted ORFs for which transcription had not been detected by other approaches. Additionally, we identified more than 2,000 novel transcriptional segments, including new ORFs and exons, noncoding RNAs (ncRNAs) as well as convincing cases of antisense gene transcription. We also characterized the 5' and 3' UTRs of expressed ORFs, and established that genes with long 5' UTRs are significantly enriched in regulatory functions controlling filamentous growth. Furthermore, we found that genomic regions adjacent to telomeres harbor a cluster of expressed ncRNAs. To validate and confirm new ncRNA candidates, we adapted an iterative strategy combining both genome-wide occupancy of the different subunits of RNA polymerases I, II and III and expression data. This comprehensive approach allowed the identification of different families of ncRNAs. Conclusions: In summary, we provide a comprehensive expression atlas that covers relevant C. albicans pathogenic developmental stages in addition to the discovery of new ORF and non-coding genetic elements.
机译:背景:与其他模型生物相比,尽管致病性酵母白色念珠菌具有临床相关性,但尚未进行全面分析以为其基于计算机硅的基因组注释提供实验支持。结果:我们进行了全基因组实验注释,以使用链特异性高密度切片阵列准确揭示病原酵母白色念珠菌的转录情况。从在与白色念珠菌致病性相关的条件下生长的细胞(包括生物膜,实验室生长的酵母和血清诱导的菌丝)以及从小鼠盲肠分离的细胞中纯化RNA。这项工作为尚未通过其他方法检测到转录的大量预测ORF提供了全基因组实验验证。此外,我们鉴定了2,000多个新的转录片段,包括新的ORF和外显子,非编码RNA(ncRNA)以及令人信服的反义基因转录案例。我们还表征了表达的ORF的5'和3'UTR,并确定长5'UTR的基因在控制丝状生长的调节功能中显着丰富。此外,我们发现邻近端粒的基因组区域包含表达的ncRNA簇。为了验证和确认新的ncRNA候选者,我们采用了一种迭代策略,将RNA聚合酶I,II和III的不同亚基的全基因组占有率与表达数据相结合。这种全面的方法允许鉴定不同的ncRNA家族。结论:总之,除了发现新的ORF和非编码遗传元件外,我们还提供了涵盖相关的白色念珠菌致病性发育阶段的综合表达图集。

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