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使用微阵列杂交和信号模式识别技术从血液中分离出人类病原体的鉴定。

Identification of human pathogens isolated from blood using microarray hybridisation and signal pattern recognition.

作者信息

Wiesinger-Mayr Herbert, Vierlinger Klemens, Pichler Rudolf, Kriegner Albert, Hirschl Alexander M, Presterl Elisabeth, Bodrossy Levente, Noehammer Christa

机构信息

Molecular Diagnostics, Austrian Research Centers GmbH - ARC, Mendelstrasse 1, A-2444 Seibersdorf, Austria.

出版信息

BMC Microbiol. 2007 Aug 14;7:78. doi: 10.1186/1471-2180-7-78.

Abstract

BACKGROUND

Pathogen identification in clinical routine is based on the cultivation of microbes with subsequent morphological and physiological characterisation lasting at least 24 hours. However, early and accurate identification is a crucial requisite for fast and optimally targeted antimicrobial treatment. Molecular biology based techniques allow fast identification, however discrimination of very closely related species remains still difficult.

RESULTS

A molecular approach is presented for the rapid identification of pathogens combining PCR amplification with microarray detection. The DNA chip comprises oligonucleotide capture probes for 25 different pathogens including Gram positive cocci, the most frequently encountered genera of Enterobacteriaceae, non-fermenter and clinical relevant Candida species. The observed detection limits varied from 10 cells (e.g. E. coli) to 10(5) cells (S. aureus) per mL artificially spiked blood. Thus the current low sensitivity for some species still represents a barrier for clinical application. Successful discrimination of closely related species was achieved by a signal pattern recognition approach based on the k-nearest-neighbour method. A prototype software providing this statistical evaluation was developed, allowing correct identification in 100 % of the cases at the genus and in 96.7 % at the species level (n = 241).

CONCLUSION

The newly developed molecular assay can be carried out within 6 hours in a research laboratory from pathogen isolation to species identification. From our results we conclude that DNA microarrays can be a useful tool for rapid identification of closely related pathogens particularly when the protocols are adapted to the special clinical scenarios.

摘要

背景

临床常规中的病原体鉴定基于微生物培养,随后进行形态学和生理学特征鉴定,这至少需要24小时。然而,早期准确鉴定是快速且进行最佳靶向抗菌治疗的关键前提条件。基于分子生物学的技术能够实现快速鉴定,但区分亲缘关系极近的物种仍然困难。

结果

本文介绍了一种将PCR扩增与微阵列检测相结合的病原体快速鉴定分子方法。该DNA芯片包含针对25种不同病原体的寡核苷酸捕获探针,这些病原体包括革兰氏阳性球菌、肠杆菌科最常见的属、非发酵菌以及临床相关的念珠菌属。在人工加标的血液中,观察到的检测限从每毫升10个细胞(如大肠杆菌)到10⁵个细胞(金黄色葡萄球菌)不等。因此,目前某些物种的低灵敏度仍然是临床应用的障碍。通过基于k近邻法的信号模式识别方法成功区分了亲缘关系极近的物种。开发了一款提供这种统计评估的原型软件,在属水平上100%的病例以及种水平上96.7%的病例(n = 241)能够正确鉴定。

结论

新开发的分子检测方法在研究实验室中从病原体分离到物种鉴定可在6小时内完成。根据我们的结果,我们得出结论,DNA微阵列可以成为快速鉴定亲缘关系极近病原体的有用工具,特别是当方案适用于特殊临床情况时。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/673e/1994958/12b8f5f8c752/1471-2180-7-78-1.jpg

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