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用于结膜炎的无偏病原体检测和宿主基因分析。

Unbiased Pathogen Detection and Host Gene Profiling for Conjunctivitis.

机构信息

Department of Ocular Microbiology, Aravind Eye Hospital, Madurai, Tamil Nadu, India.

Francis I. Proctor Foundation, San Francisco, California; Department of Ophthalmology, University of California, San Francisco, California.

出版信息

Ophthalmology. 2019 Aug;126(8):1090-1094. doi: 10.1016/j.ophtha.2019.03.039. Epub 2019 Apr 4.

Abstract

PURPOSE

The etiology of conjunctivitis is often misdiagnosed. An ideal diagnostic test would identify all possible infectious causes. In this study, we apply unbiased metagenomic RNA deep sequencing (MDS) to identify pathogens causing conjunctivitis.

DESIGN

Molecular study of prospectively collected conjunctival swabs from patients with presumed infectious conjunctivitis.

PARTICIPANTS

Patients with presumed acute infectious conjunctivitis.

METHODS

Conjunctival swabs were collected from patients presenting with acute conjunctivitis. Swabs were processed for MDS. Pathogens were identified using a rapid computational pipeline to analyze the nonhost sequences obtained from MDS. Differential gene expression analysis was performed to evaluate for host transcriptome signatures for infectious types. Clinical samples were deidentified, and laboratory personnel handling the samples and interpreting the data were masked.

MAIN OUTCOME MEASURES

Pathogens and differential transcripts identified by MDS.

RESULTS

Metagenomic RNA deep sequencing detected pathogens in 86% (12/14) of the patients tested. Swabs from 10 of 14 patients were positive for human adenovirus (HAdV) while swabs from 2 of 14 patients were positive for Vittaforma corneae (a parasitic fungal species of the microsporidia group). Samples positive for HAdV by RNA-seq were independently verified in a CLIA-certified laboratory. Pathogen-directed polymerase chain reaction confirmed the presence of V. corneae genome in the samples positive by RNA-seq. Local host transcriptome analysis identified 12 differentially expressed genes that provided distinct expression signatures for patients infected with HAdV compared with V. corneae.

CONCLUSIONS

Metagenomic RNA deep sequencing can reliably detect and quantify common and rare pathogens causing conjunctivitis, and identify strains. The unbiased nature of metagenomic RNA deep sequencing allowed an expanded scope of pathogen detection, including fungal species not commonly associated with acute conjunctivitis. In addition, the identification of infection type-specific local host transcriptome signatures may allow for pathogen detection even when the pathogen load is too low for direct identification.

摘要

目的

结膜炎的病因常常被误诊。理想的诊断测试应该能够识别所有可能的感染原因。在本研究中,我们应用无偏倚的宏基因组 RNA 深度测序(MDS)来鉴定引起结膜炎的病原体。

设计

对疑似传染性结膜炎患者的前瞻性收集的结膜拭子进行分子研究。

参与者

疑似急性传染性结膜炎患者。

方法

从患有急性结膜炎的患者中采集结膜拭子。对拭子进行 MDS 处理。使用快速计算管道来分析从 MDS 获得的非宿主序列来鉴定病原体。进行差异基因表达分析,以评估感染类型的宿主转录组特征。临床样本被去识别,处理样本和解释数据的实验室人员被屏蔽。

主要观察指标

MDS 鉴定的病原体和差异转录本。

结果

宏基因组 RNA 深度测序检测到 86%(12/14)测试患者的病原体。14 名患者中有 10 名的拭子检测到人类腺病毒(HAdV)阳性,而 14 名患者中有 2 名的拭子检测到 Vittaforma corneae(一种微孢子虫组的寄生真菌物种)阳性。通过 RNA-seq 检测到 HAdV 的样本在经过 CLIA 认证的实验室中得到了独立验证。针对病原体的聚合酶链反应证实了 RNA-seq 阳性样本中存在 V. corneae 基因组。局部宿主转录组分析确定了 12 个差异表达基因,这些基因为感染 HAdV 与 V. corneae 的患者提供了独特的表达特征。

结论

宏基因组 RNA 深度测序可以可靠地检测和定量引起结膜炎的常见和罕见病原体,并鉴定菌株。无偏倚的宏基因组 RNA 深度测序的性质允许扩大病原体检测范围,包括与急性结膜炎不常相关的真菌物种。此外,即使病原体负荷太低而无法直接鉴定,感染类型特异性的局部宿主转录组特征的鉴定也可能允许进行病原体检测。

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