念珠菌血症患者中(1, 3)-β-D-葡聚糖、甘露聚糖及抗甘露聚糖抗体与念珠菌属特异性巢式聚合酶链反应的比较评估
Comparative evaluation of (1, 3)-beta-D-glucan, mannan and anti-mannan antibodies, and Candida species-specific snPCR in patients with candidemia.
作者信息
Alam Fasahat F, Mustafa Abu S, Khan Zia U
机构信息
Department of Microbiology, Faculty of Medicine, Kuwait University, Safat 13110, P, O, Box 24923, Kuwait.
出版信息
BMC Infect Dis. 2007 Sep 4;7:103. doi: 10.1186/1471-2334-7-103.
BACKGROUND
Candidemia is a major infectious complication of seriously immunocompromised patients. In the absence of specific signs and symptoms, there is a need to evolve an appropriate diagnostic approach. A number of methods based on the detection of Candida mannan, nucleic acid and (1,3)-beta- D- glucan (BDG) have been used with varying specificities and sensitivities. In this retrospective study, attention has been focused to evaluate the usefulness of two or more disease markers in the diagnosis of candidemia.
METHODS
Diagnostic usefulness of Platelia Candida Ag for the detection of mannan, Platelia Candida Ab for the detection of anti-mannan antibodies, Fungitell for the detection of BDG, and of a semi-nested PCR (snPCR) for the detection Candida species-specific DNA have been retrospectively evaluated using 32 sera from 27 patients with culture-proven candidemia, 51 sera from 39 patients with clinically suspected candidemia, sera of 10 women with C. albicans vaginitis, and sera of 16 healthy controls.
RESULTS
Using cut-off values recommended by the manufacturers, the sensitivity of the assays for candidemia patients were as follows: Candida snPCR 88%, BDG 47%, mannan 41%, anti-mannan antibodies 47%, respectively. snPCR detected 5 patients who had candidemia due to more than one Candida species. The sensitivities of the combined tests were as follows: Candida mannan and anti-mannan antibodies 75%, and Candida mannan and BDG 56%. Addition of snPCR data improved the sensitivity further to 88%, thus adding 10 sera that were negative by BDG and/or mannan. In clinically suspected, blood culture negative patients; the positivities of the tests were as follows: Candida DNA was positive in 53%, BDG in 29%, mannan in 16%, and anti-mannan antibodies in 29%. The combined detection of mannan and BDG, and mannan, BDG and Candida DNA enhanced the positivity to 36% and 54%, respectively. None of the sera from Candida vaginitis patients and healthy subjects were positive for Candida DNA and mannan.
CONCLUSION
The observations made in this study reinforce the diagnostic value of snPCR in the sensitive and specific diagnosis of candidemia and detection of more than one Candida species in a given patient. Additionally, in the absence of a positive blood culture, snPCR detected Candida DNA in sera of more than half of the clinically suspected patients. While detection of BDG, mannan and anti-mannan antibodies singly or in combination could help enhancing sensitivity and eliminating false positive tests, a more extensive evaluation of these assays in sequentially collected serum samples is required to assess their value in the early diagnosis of candidemia.
背景
念珠菌血症是严重免疫功能低下患者的主要感染并发症。在缺乏特异性体征和症状的情况下,需要制定合适的诊断方法。一些基于检测念珠菌甘露聚糖、核酸和(1,3)-β-D-葡聚糖(BDG)的方法,其特异性和敏感性各不相同。在这项回顾性研究中,重点评估了两种或更多疾病标志物在念珠菌血症诊断中的作用。
方法
回顾性评估了用于检测甘露聚糖的普立泰念珠菌抗原(Platelia Candida Ag)、用于检测抗甘露聚糖抗体的普立泰念珠菌抗体(Platelia Candida Ab)、用于检测BDG的真菌检测试剂盒(Fungitell)以及用于检测念珠菌属特异性DNA的半巢式PCR(snPCR)的诊断价值,使用了来自27例经培养证实为念珠菌血症患者的32份血清、来自39例临床疑似念珠菌血症患者的51份血清、10例白色念珠菌阴道炎女性的血清以及16例健康对照者的血清。
结果
采用制造商推荐的临界值,各检测方法对念珠菌血症患者的敏感性如下:念珠菌snPCR为88%,BDG为47%,甘露聚糖为41%,抗甘露聚糖抗体为47%。snPCR检测出5例由多种念珠菌引起念珠菌血症的患者。联合检测的敏感性如下:念珠菌甘露聚糖和抗甘露聚糖抗体为75%,念珠菌甘露聚糖和BDG为56%。加入snPCR数据后敏感性进一步提高到88%,从而增加了10份BDG和/或甘露聚糖检测为阴性的血清。在临床疑似、血培养阴性的患者中,各检测方法的阳性率如下:念珠菌DNA阳性率为53%,BDG为29%,甘露聚糖为16%,抗甘露聚糖抗体为29%。甘露聚糖和BDG联合检测,以及甘露聚糖、BDG和念珠菌DNA联合检测,阳性率分别提高到36%和54%。念珠菌阴道炎患者和健康受试者的血清中,无一例念珠菌DNA和甘露聚糖检测呈阳性。
结论
本研究的观察结果强化了snPCR在念珠菌血症敏感和特异性诊断以及检测特定患者中多种念珠菌方面的诊断价值。此外,在血培养未阳性的情况下,snPCR在超过一半的临床疑似患者血清中检测到念珠菌DNA。虽然单独或联合检测BDG、甘露聚糖和抗甘露聚糖抗体有助于提高敏感性并消除假阳性检测,但需要对这些检测方法在连续采集的血清样本中进行更广泛的评估,以评估它们在念珠菌血症早期诊断中的价值。
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