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引入珠磨步骤可改善从选定患者标本中提取真菌DNA的效果。

Introduction of a bead beating step improves fungal DNA extraction from selected patient specimens.

作者信息

Scharf Sebastian, Bartels Anna, Kondakci Mustafa, Pfeffer Klaus, Henrich Birgit, Haas Rainer

机构信息

Institute of Medical Microbiology and Hospital Hygiene, University of Duesseldorf, Germany; Department of Haematology, Oncology and Clinical Immunology, University of Duesseldorf, Medical Faculty, Duesseldorf, Germany.

Department of Haematology, Oncology and Clinical Immunology, University of Duesseldorf, Medical Faculty, Duesseldorf, Germany.

出版信息

Int J Med Microbiol. 2020 Sep;310(6):151443. doi: 10.1016/j.ijmm.2020.151443. Epub 2020 Aug 5.

Abstract

In immunocompromised patients a colonisation with fungi carries the risk to develop serious invasive fungal infection. An early detection is therefore important, but not optimal hitherto. Fortunately, molecular genetic methods have increased the sensitivity of fungal detection and limited the time, until results are available. However, their success depends on an efficient extraction of genomic DNA from the fungal cell in the given diagnostic specimen. To improve the routine DNA preparation method for yeasts and moulds, the impact of bead beating on fungal DNA release was evaluated. PBS, blood and respiratory rinse were spiked with Candida glabrata or Aspergillus fumigatus. DNA was extracted by mechanical bead beating in addition to the different steps of the DNA preparation protocol, which comprised liquid nitrogen treatment, proteinase K digestion and DNA isolation using the EZ1 DNA Tissue Kit and Workstation. In every method variant tested, treatment with liquid nitrogen did not improve the DNA release. Bead beating once followed by proteinase K digestion and EZ1-work-up led to the highest DNA release from fungus, spiked in PBS, and increased the extracted DNA amount of C. glabrata about 100-fold and of A. fumigatus about 10-fold in relation to sole EZ1-work-up. In fungus-spiked respiratory rinse and blood, highest increase in DNA release was measured after triple bead beating with simultaneous proteinase K digestion. Fungal DNA release of C. glabrata increased for >100-fold in respiratory rinse and for >1000-fold in blood and of A. fumigatus for >10-fold in respiratory rinse and about 5- to 10-fold in blood. The data of this study clearly demonstrate that preparation of fungal DNA from human specimens is optimized by introduction of a bead beating step to the conventional DNA-preparation method without the necessity of a liquid nitrogen step.

摘要

在免疫功能低下的患者中,真菌定植有发展为严重侵袭性真菌感染的风险。因此,早期检测很重要,但迄今为止并非最佳。幸运的是,分子遗传学方法提高了真菌检测的灵敏度,并缩短了获得结果的时间。然而,它们的成功取决于从给定诊断标本中的真菌细胞中高效提取基因组DNA。为了改进酵母和霉菌的常规DNA制备方法,评估了珠磨法对真菌DNA释放的影响。将光滑念珠菌或烟曲霉加入磷酸盐缓冲液(PBS)、血液和呼吸道冲洗液中。除了DNA制备方案的不同步骤外,还通过机械珠磨法提取DNA,这些步骤包括液氮处理、蛋白酶K消化以及使用EZ1 DNA组织试剂盒和工作站进行DNA分离。在测试的每种方法变体中,液氮处理均未改善DNA释放。珠磨一次后进行蛋白酶K消化和EZ1处理,导致从加样于PBS中的真菌中释放出的DNA量最高,与单独的EZ1处理相比,光滑念珠菌提取的DNA量增加了约100倍,烟曲霉增加了约10倍。在加样有真菌的呼吸道冲洗液和血液中,经三次珠磨同时进行蛋白酶K消化后,测得的DNA释放增加最多。光滑念珠菌的真菌DNA释放在呼吸道冲洗液中增加了100倍以上,在血液中增加了1000倍以上;烟曲霉的真菌DNA释放在呼吸道冲洗液中增加了10倍以上,在血液中增加了约5至10倍。本研究的数据清楚地表明,通过在传统DNA制备方法中引入珠磨步骤,无需液氮步骤,可优化从人体标本中制备真菌DNA的方法。

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