首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Diagnosis of disseminated microsporidian Encephalitozoon hellem infection by PCR-Southern analysis and successful treatment with albendazole and fumagillin.
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Diagnosis of disseminated microsporidian Encephalitozoon hellem infection by PCR-Southern analysis and successful treatment with albendazole and fumagillin.

机译:通过PCR-Southern分析诊断弥散性的小孢子虫脑性乙脑感染并用阿苯达唑和烟曲霉素成功治疗。

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摘要

A 37-year old AIDS patient presented with foreign body sensation. Microsporidia were detected in smears from a conjunctival swab and urine sediment stained with calcofluor and a modified trichrome blue stain and by indirect fluorescent-antibody staining with murine polyclonal antiserum raised against Encephalitozoon hellem. This antiserum cross-reacted with other Encephalitozoon species, so PCR was performed to amplify the microsporidian ribosomal DNA (rDNA) with pan-Encephalitozoon primers. The PCR DNA products from the urine and conjunctival clinical specimens, along with the tissue culture-derived microsporidian controls, were assayed by Southern analysis with oligonucleotide probes specific for Encephalitozoon cuniculi, E. hellem, and Encephalitozoon (Septata) intestinalis. The PCR product amplified from the urine specimen hybridized with the E. hellem probe only, while insufficient DNA was amplified from the conjunctiva specimen for detection by Southern analysis. For corroboration of the PCR-Southern analysis results, aliquots of the urine and conjunctiva specimens were seeded onto RK-13 cell monolayers. The rDNA extracts of the cultured microsporidia were amplified by PCR with pan-Encephalitozoon primers, and the PCR DNA products were subjected to digestion with restriction endonuclease FokI. The amplified rDNA of both the urine and conjunctiva isolates generated digestion patterns that were identified to the E. hellem PCR rDNA digestion pattern. In addition, double-stranded heteroduplex mobility shift analysis with these PCR products indicated that the urine and conjunctiva isolates were identical to each other and to E. hellem. The patient was treated with albendazole and topical fumagillin and responded rapidly, with no recurrence of ophthalmologic signs. The results of this study demonstrate that PCR-Southern analysis provides a basis for distinguishing E. cuniculi, E. hellem, and E. intestinalis in clinical specimens.
机译:一名37岁的AIDS患者出现异物感。在结膜拭子和尿沉渣的涂片中检测到微孢子虫,用钙氟荧光素和改良的三色蓝色染料染色,并通过间接荧光抗体染色,用鼠抗Encephalitozoon hellem的多克隆抗血清进行染色。该抗血清与其他脑型虫交叉反应,因此进行了PCR反应,以泛型脑型虫引物扩增微孢子虫核糖体DNA(rDNA)。尿液和结膜临床标本的PCR DNA产物,以及组织培养衍生的微孢子虫质控品,通过Southern检验,使用对Encephalitozoon cuniculi,E。hellem和Encephalitozoon(Septata)小肠具有特异性的寡核苷酸探针进行分析。从尿液样本扩增的PCR产物仅与埃里希氏大肠杆菌探针杂交,而从结膜样本扩增的DNA不足,无法通过Southern分析进行检测。为了证实PCR-Southern分析结果,将尿液和结膜样本的等分试样接种到RK-13​​细胞单层上。培养的小孢子虫的rDNA提取物通过泛脑头虫引物通过PCR扩增,并将PCR DNA产物用限制性核酸内切酶FokI消化。尿液和结膜分离株的扩增rDNA均产生了消化模式,该消化模式已被鉴定为大肠杆菌(E. hellem)PCR rDNA消化模式。此外,用这些PCR产物进行的双链异源双链迁移率迁移分析表明,尿液和结膜分离株彼此相同,与大肠杆菌一样。该患者接受了阿苯达唑和局部烟曲霉素的治疗,反应迅速,没有眼科症状的复发。这项研究的结果表明,PCR-Southern分析为区分临床标本中的E. cuniculi,E。hellem和E. intestinalis提供了基础。

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