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Shotgun-Metagenomics on Positive Blood Culture Bottles Inoculated With Prosthetic Joint Tissue: A Proof of Concept Study

机译:用假体关节组织接种的血液培养瓶上的霰弹枪 - 血液培养瓶:概念研究证明

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摘要

Clinical metagenomics is actively moving from research to clinical laboratories. It has the potential to change the microbial diagnosis of infectious diseases, especially when detection and identification of pathogens can be challenging, such as in prosthetic joint infection (PJI). The application of metagenomic sequencing to periprosthetic joint tissue (PJT) specimens is often challenged by low bacterial load in addition to high level of inhibitor and contaminant host DNA, limiting pathogen recovery. Shotgun-metagenomics (SMg) performed directly on positive blood culture bottles (BCBs) inoculated with PJT may be a convenient approach to overcome these obstacles. The aim was to test if it is possible to perform SMg on PJT inoculated into BCBs for pathogen identification in PJI diagnosis. Our study was conducted as a laboratory method development. For this purpose, spiked samples (positive controls), negative control and clinical tissue samples (positive BCBs) were included to get a comprehensive overview. We developed a method for preparation of bacterial DNA directly from PJT inoculated in BCBs. Samples were processed using MolYsis5 kit for removal of human DNA and DNA extracted with BiOstic kit. High DNA quantity/quality was obtained, and no inhibition was observed during the library preparation, allowing further sequencing process. DNA sequencing reads obtained from the BCBs, presented a low proportion of human reads (<1%) improving the sensitivity of bacterial detection. We detected a 19-fold increase in the number of reads mapping to human in a sample untreated with MolYsis5. Taxonomic classification of clinical samples identified a median of 96.08% (IQR, 93.85–97.07%; range 85.7–98.6%) bacterial reads. Shotgun-metagenomics results were consistent with the results from a conventional BCB culture method, validating our approach. Overall, we demonstrated a proof of concept that it is possible to perform SMg directly on BCBs inoculated with PJT, with potential of pathogen identification in PJI diagnosis. We consider this a first step in research efforts needed to face the challenges presented in PJI diagnoses.
机译:临床偏心组学积极从研究转向临床实验室。它有可能改变传染病的微生物诊断,特别是当病原体的检测和鉴定可能是挑战性的时,例如在假体关节感染(PJI)中。除了高水平的抑制剂和污染物宿主DNA之外,施用聚丙烯元素测序对PeriproSthetth组织(PJT)标本的施用通常是通过低细菌负荷挑战,限制病原体恢复。霰弹枪 - Metagenomics(SMG)直接在接种PJT接种的正血液培养瓶(BCBS)上,可能是克服这些障碍的方便方法。目的是测试是否可以在PJI诊断中接种到BCB的PJT上的SMG进行SMG。我们的研究是作为实验室方法开发的。为此目的,包括尖刺样品(阳性对照),阴性对照和临床组织样品(阳性BCB)以全面概述。我们开发了一种用于将细菌DNA的制备方法直接从BCB中接种的PJT制备。使用莫西5试剂盒处理样品,用于去除用生物溶剂试剂盒提取的人DNA和DNA。获得高DNA量/质量,在文库制剂期间没有观察到抑制,允许进一步测序过程。从BCB获得的DNA测序读数,呈现出低比例的人读取(<1%),提高细菌检测的敏感性。我们检测到在未处理的样品中对人的读取映射的数量增加了19倍的增加。分类样品分类临床样本的分类确定了96.08%的中位数(IQR,93.85-97.07%;范围85.7-98.6%)细菌读数。霰弹枪 - 偏见结果与传统BCB培养方法的结果一致,验证我们的方法。总体而言,我们证明了一种概念证据,即可以直接在接种PJT接种的BCB上进行SMG,具有PJI诊断的病原体鉴定。我们认为这一步需要面对PJI诊断所呈现的挑战所需的研究努力。

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