首页> 美国卫生研究院文献>Experimental and Therapeutic Medicine >A novel method of combining Periodic Acid Schiff staining with Wright-Giemsa staining to identify the pathogens Penicillium marneffei Histoplasma capsulatum Mucor and Leishmania donovani in bone marrow smears
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A novel method of combining Periodic Acid Schiff staining with Wright-Giemsa staining to identify the pathogens Penicillium marneffei Histoplasma capsulatum Mucor and Leishmania donovani in bone marrow smears

机译:结合高碘酸希夫氏染色和赖特-吉姆萨染色的新方法以鉴定骨髓涂片中的马尔尼菲青霉菌荚膜组织胞浆菌Mucor和多形利什曼原虫

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摘要

Penicillium marneffei, Histoplasma capsulatum, Mucor and Leishmania donovani can lead to penicilliosis marneffei, histoplasmosis, mucormycosis and leishmaniasis, respectively, which, to a certain extent, share similar clinical manifestations. These pathogens are approximately the same size, therefore it is relatively difficult to rapidly diagnose the diseases. The aim of the present study was to explore a novel method that attempts to rapidly identify the pathogens of these diseases. In the Wright-Giemsa staining, the four pathogens were approximately the same size and mainly existed in macrophages. The multiplying P. marneffei had two nuclei, which were on both sides of the fungus, and had light cross-walls in the middle. H. capsulatum had a purplish nucleus, which occupied between one-third and one-half of the spore. The cytoplasm was light blue. Peripheral spores were observed in the form of an empty, bright ring without color, like a capsule. Generally, Mucor were observed to have a long and lightly stained area, which could be easily confused with the Wright staining of dinuclear P. marneffei. L. donovani exhibited a deep-staining kinetoplast near the nucleus. In the Periodic Acid Schiff (PAS) staining, the pathogens of P. marneffei and H. capsulatum were distinct and stained red. Differentiation between P. marneffei and H. capsulatum relied on their modes of reproduction: P. marneffei depends on fission, when the pathogens stretch into sausage-shapes and are split by a cross-wall, while H. capsulatum depends on budding so that narrow-necked, single spores can be formed. With PAS staining, the cell walls and intracellular contents of Mucor and L. donovani were not stained, lightly stained or granulated and discontinuous. In conclusion, this method, combining PAS and Wright-Giemsa staining, is simple and rapid, and may contribute to the effective identification of the four pathogens.
机译:马尔尼菲青霉菌,荚膜组织胞浆菌,Mucor和多发性利什曼原虫可以分别导致马尔尼菲青霉菌,组织胞浆菌病,粘膜霉菌病和利什曼病,它们在一定程度上具有相似的临床表现。这些病原体的大小大致相同,因此快速诊断疾病相对困难。本研究的目的是探索一种尝试快速识别这些疾病的病原体的新方法。在赖特-吉姆萨染色中,四种病原体的大小大致相同,主要存在于巨噬细胞中。繁殖中的P. marneffei有两个核,位于真菌的两侧,中间有轻质的隔壁。荚膜H.有一个紫色的核,占据了孢子的三分之一到一半。细胞质为浅蓝色。观察到的外围孢子呈空的,明亮的,无颜色的环状,如胶囊。通常,观察到Mucor具有长而浅的染色区域,该区域很容易与双核马尼菲假单胞菌的Wright染色相混淆。 L. donovani在细胞核附近表现出深染的动塑料。在高碘酸希夫(PAS)染色中,P。marneffei和H.荚膜菌的病原体明显且呈红色。马尔尼菲假单胞菌和荚膜H.荚膜之间的区别取决于它们的繁殖方式:马尔尼菲假单胞菌依赖于裂变,当病原体伸展成香肠形状并被横壁分裂时,而荚膜H.荚膜则取决于出芽从而狭窄颈可形成单孢子。用PAS染色,Mucor和donovani的细胞壁和细胞内内容物未染色,轻度染色或颗粒化且不连续。总之,该方法结合了PAS和Wright-Giemsa染色,简便,快速,可有助于有效鉴定四种病原体。

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