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HERQ-9 Is a New Multiplex PCR for Differentiation and Quantification of All Nine Human Herpesviruses

机译:HERQ-9是一种新的多重PCR,用于分化和定量所有九个人疱疹病毒

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Infections with the nine human herpesviruses (HHVs) are globally prevalent and characterized by lifelong persistence. Reactivations can potentially manifest as life-threatening conditions for which the demonstration of viral DNA is essential. In the present study, we developed HERQ-9, a pan-HHV quantitative PCR designed in triplex reactions to differentiate and quantify each of the HHV-DNAs: (i) herpes simplex viruses 1 and 2 and varicella-zoster virus; (ii) Epstein-Barr virus, human cytomegalovirus, and Kaposi’s sarcoma-associated herpesvirus; and (iii) HHV-6A, -6B, and -7. The method was validated with prequantified reference standards as well as with mucocutaneous swabs and cerebrospinal fluid, plasma, and tonsillar tissue samples. Our findings highlight the value of multiplexing in the diagnosis of many unsuspected, yet clinically relevant, herpesviruses. In addition, we report here frequent HHV-DNA co-occurrences in clinical samples, including some previously unknown. HERQ-9 exhibited high specificity and sensitivity (LOD 95 s of ~10 to ~17 copies/reaction), with a dynamic range of 10 1 to 10 6 copies/μl. Moreover, it performed accurately in the coamplification of both high- and low-abundance targets in the same reaction. In conclusion, we demonstrated that HERQ-9 is suitable for the diagnosis of a plethora of herpesvirus-related diseases. Besides its significance to clinical management, the method is valuable for the assessment of hitherto-unexplored synergistic effects of herpesvirus coinfections. Furthermore, its high sensitivity enables studies on the human virome, often dealing with minute quantities of persisting HHVs. IMPORTANCE By adulthood, almost all humans become infected by at least one herpesvirus (HHV). The maladies inflicted by these microbes extend beyond the initial infection, as they remain inside our cells for life and can reactivate, causing severe diseases. The diagnosis of active infection by these ubiquitous pathogens includes the detection of DNA with sensitive and specific assays. We developed the first quantitative PCR assay (HERQ-9) designed to identify and quantify each of the nine human herpesviruses. The simultaneous detection of HHVs in the same sample is important since they may act together to induce life-threatening conditions. Moreover, the high sensitivity of our method is of extreme value for assessment of the effects of these viruses persisting in our body and their long-term consequences on our health.
机译:患有九九人疱疹病毒(HHV)的感染是全球普遍的,并以终身持久性为特征。再激活可能表现为病毒DNA的证明至关重要的生命威胁性条件。在本研究中,我们开发了HERQ-9,一种在三重反复反应中设计的PAN-HHV定量PCR,以区分HHV-DNA:(i)单纯疱疹病毒1和2和Varicella-Zoster病毒; (ii)Epstein-Barr病毒,人巨细胞病毒和Kaposi的肉瘤相关的Herpesvirus; (iii)HHV-6a,-6b和-7。该方法验证了预压缩的参考标准以及粘膜皮下拭子和脑脊液,血浆和扁桃体组织样品。我们的研究结果突出了多路复用在许多未经用途,临床相关的Herpesviruses诊断中的价值。此外,我们在此报告频繁出现在临床样本中的HHV-DNA共同发生,包括一些先前未知的。 HERQ-9表现出高特异性和灵敏度(LOD 95s〜10至17拷贝/反应),动态范围为10 1至10 6拷贝/μl。此外,它在相同反应中精确地在高度和低丰度靶的基础上进行。总之,我们证明HERQ-9适用于诊断血腥与血疱相关疾病的诊断。除了对临床管理的重要性外,该方法对于评估Herpesvirus辛纤维的迄今为止的协同效应是有价值的。此外,它的高灵敏度使得能够研究人体病毒,通常处理微小量的持续性HHV。成年期的重要性,几乎所有人类都被至少一种疱疹病毒(HHV)感染。这些微生物造成的疾病延伸到初始感染之外,因为它们留在我们的细胞内部,可以重新激活,引起严重疾病。这些无处不在的病原体的活性感染的诊断包括检测具有敏感和特异性测定的DNA。我们开发了第一定量PCR测定(HERQ-9),旨在识别和量化九个人疱疹病毒中的每一个。同一样品中HHV的同时检测是重要的,因为它们可以共同起来引起危及生命的条件。此外,我们的方法的高灵敏度是评估这些病毒持续存在于我们的身体的影响以及对我们健康的长期后果的极端值。

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