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Evaluation of In Situ Methods Used To Detect Mycobacterium avium subsp. paratuberculosis in Samples from Patients with Crohn's Disease

机译:评价用于检测鸟分枝杆菌亚种的原位方法。克罗恩病患者样本中的副结核病

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摘要

In common with other diagnostic tests, detection of mycobacteria in tissue by microscopic examination is susceptible to spectrum bias. Since Crohn's disease is defined by the absence of detectable pathogenic organisms, the use of in situ techniques to search for Mycobacterium avium subsp. paratuberculosis in Crohn's disease samples requires validation of methods in a paucibacillary setting. To generate paucibacillary infection, C57BL/6 mice were artificially infected with Mycobacterium avium subsp. paratuberculosis strain K10 and M. tuberculosis H37Rv, yielding tissues harboring fewer than one bacillus per oil immersion field. Serial sections of organs were then studied by cell wall-based staining techniques (Ziehl-Neelsen and auramine rhodamine) and nucleic acid-based staining techniques (in situ hybridization [ISH] and indirect in situ PCR [IS PCR]). Microscopic examination and measurement of morphometric parameters of bacilli revealed that for all methods, Mycobacterium avium subsp. paratuberculosis bacilli were observed to be shorter, smaller, and less rod shaped than M. tuberculosis bacilli. Ziehl-Neelsen, auramine rhodamine stains, ISH targeting rRNA, and IS-PCR targeting the IS900 element afforded comparable sensitivities, but for all methods, visualization of individual bacterial forms required magnification ×1,000. Auramine rhodamine staining and IS-PCR generated positive signals in negative controls, indicating the nonspecificity of these assays. Together, our results indicate that detection of Mycobacterium avium subsp. paratuberculosis bacilli in tissue requires oil immersion microscopy, that rRNA-ISH provides sensitivity and specificity comparable to those of Ziehl-Neelsen staining, and that the microscopic detection limit for Mycobacterium avium subsp. paratuberculosis in tissue is governed more by bacterial burden than by staining method.
机译:与其他诊断测试一样,通过显微镜检查检测组织中的分枝杆菌容易受到光谱偏差的影响。由于克罗恩氏病是由于缺乏可检测的病原生物而引起的,因此使用原位技术搜索鸟分枝杆菌亚种。克罗恩病样品中的副结核病需要在睑板菌环境中验证方法。为了产生脓杆菌感染,将C57BL / 6小鼠用鸟分枝杆菌亚种人工感染。副油杆菌菌株K10和结核分枝杆菌H37Rv,每个油浸场产生的组织中含有少于一株杆菌。然后通过基于细胞壁的染色技术(Ziehl-Neelsen和金胺罗丹明)和基于核酸的染色技术(原位杂交[ISH]和间接原位PCR [IS PCR])研究器官的连续切片。显微镜检查和细菌形态参数的测量表明,对于所有方法,鸟分枝杆菌亚种都可以。观察到副结核杆菌比结核分枝杆菌更短,更小并且杆形更少。 Ziehl-Neelsen,金胺罗丹明染色,ISH靶向rRNA和IS-PCR靶向IS900元件都具有相当的灵敏度,但是对于所有方法,单个细菌形式的可视化都需要放大1000倍。金胺罗丹明染色和IS-PCR在阴性对照中产生阳性信号,表明这些测定的非特异性。在一起,我们的结果表明,鸟分枝杆菌亚种的检测。组织中的副结核杆菌需要油浸显微镜检查,rRNA-ISH的敏感性和特异性可与Ziehl-Neelsen染色相媲美,禽分枝杆菌亚种的显微镜检出限。组织中的副结核病更多地是由细菌负担而不是染色方法所控制。

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