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人类疱疹病毒 6B 转录组的 RNA 测序,以鉴定用于区分潜伏和活跃感染的临床检测的靶标。

RNA Sequencing of the Human Herpesvirus 6B Transcriptome To Identify Targets for Clinical Assays Distinguishing between Latent and Active Infections.

机构信息

Department of Medicine, University of Washington, Seattle, Washington, USA

Vaccine and Infectious Disease Division, Fred Hutchinson Cancer Research Center, Seattle, Washington, USA.

出版信息

J Virol. 2019 Jan 17;93(3). doi: 10.1128/JVI.01419-18. Print 2019 Feb 1.

Abstract

Human herpesvirus 6B (HHV-6B) DNA is frequently detected in human samples. Diagnostic assays distinguishing HHV-6B reactivation from latency are limited. This has impaired strategies to diagnose and treat HHV-6B-associated diseases. We used RNA sequencing to characterize and compare the HHV-6B transcriptome in multiple sample types, including (i) whole blood from hematopoietic cell transplant (HCT) recipients with and without HHV-6B plasma viremia, (ii) tumor tissue samples from subjects with large B cell lymphoma infected with HHV-6B, (iii) lymphoblastoid cell lines (LCLs) from subjects with inherited chromosomally integrated HHV-6B or latent infection with HHV-6B, and (iv) HHV-6B Z29 infected SupT1 CD4 T cells. We demonstrated substantial overlap in the HHV-6B transcriptome observed in and samples, although there was variability in the breadth and quantity of gene expression across samples. The HHV-6B viral polymerase gene U38 was the only HHV-6B transcript detected in all next-generation RNA sequencing (RNA-seq) data sets and was one of the most highly expressed genes. We developed a novel reverse transcription-PCR assay targeting HHV-6B U38, which identified U38 mRNA in all tested whole-blood samples from patients with concurrent HHV-6B viremia. No HHV-6B U38 transcripts were detected by RNA-seq or reverse transcription-real-time quantitative PCR (RT-qPCR) in whole-blood samples from subjects without HHV-6B plasma detection or from latently infected LCLs. A RT-qPCR assay for HHV-6B U38 may be useful to identify lytic HHV-6B infection in nonplasma samples and samples from individuals with inherited chromosomally integrated HHV-6B. This study also demonstrates the feasibility of transcriptomic analyses for HCT recipients. Human herpesvirus 6B (HHV-6B) is a DNA virus that infects most children within the first few years of life. After primary infection, HHV-6B persists as a chronic, latent infection in many cell types. Additionally, HHV-6B can integrate into germ line chromosomes, resulting in individuals with viral DNA in every nucleated cell. Given that PCR to detect viral DNA is the mainstay for diagnosing HHV-6B infection, the characteristics of HHV-6B infection complicate efforts to distinguish between latent and active viral infection, particularly in immunocompromised patients who have frequent HHV-6B reactivation. In this study, we used RNA sequencing to characterize the HHV-6B gene expression profile in multiple sample types, and our findings identified evidence-based targets for diagnostic tests that distinguish between latent and active viral infection.

摘要

人类疱疹病毒 6B(HHV-6B)DNA 在人类样本中经常被检测到。用于区分 HHV-6B 再激活与潜伏的诊断检测方法有限。这阻碍了诊断和治疗 HHV-6B 相关疾病的策略。我们使用 RNA 测序来描述和比较多种样本类型中的 HHV-6B 转录组,包括(i)造血细胞移植(HCT)受者的全血,这些受者有或没有 HHV-6B 血浆病毒血症,(ii)感染 HHV-6B 的大 B 细胞淋巴瘤患者的肿瘤组织样本,(iii)具有遗传性染色体整合 HHV-6B 或潜伏性 HHV-6B 感染的淋巴母细胞系(LCL),和(iv)HHV-6B Z29 感染的 SupT1 CD4 T 细胞。我们证明了在 和 样本中观察到的 HHV-6B 转录组有很大的重叠,尽管在跨样本的基因表达的广度和数量上存在差异。HHV-6B 病毒聚合酶基因 U38 是所有下一代 RNA 测序(RNA-seq)数据集中检测到的唯一 HHV-6B 转录本,也是表达量最高的基因之一。我们开发了一种针对 HHV-6B U38 的新型逆转录-PCR 检测方法,该方法在所有同时伴有 HHV-6B 病毒血症的患者的全血样本中鉴定出了 U38 mRNA。在没有 HHV-6B 血浆检测或潜伏性感染的 LCL 的全血样本中,RNA-seq 或逆转录实时定量 PCR(RT-qPCR)均未检测到 HHV-6B U38 转录本。HHV-6B U38 的 RT-qPCR 检测可能有助于识别非血浆样本和遗传性染色体整合 HHV-6B 的个体中的裂解性 HHV-6B 感染。本研究还证明了对 HCT 受者进行转录组分析的可行性。人类疱疹病毒 6B(HHV-6B)是一种 DNA 病毒,在生命的头几年内感染大多数儿童。初次感染后,HHV-6B 在许多细胞类型中持续存在慢性潜伏感染。此外,HHV-6B 可以整合到生殖系染色体中,导致每个有核细胞中都有病毒 DNA。鉴于检测病毒 DNA 的 PCR 是诊断 HHV-6B 感染的主要方法,HHV-6B 感染的特征使得区分潜伏和活跃的病毒感染变得复杂,尤其是在经常发生 HHV-6B 再激活的免疫功能低下的患者中。在这项研究中,我们使用 RNA 测序来描述多种样本类型中的 HHV-6B 基因表达谱,我们的研究结果确定了有针对性的诊断测试靶点,用于区分潜伏和活跃的病毒感染。

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