4.7 Article

Serum Antibody Signature Directed against Candida albicans Hsp90 and Enolase Detects Invasive Candidiasis in Non-Neutropenic Patients

期刊

JOURNAL OF PROTEOME RESEARCH
卷 13, 期 11, 页码 5165-5184

出版社

AMER CHEMICAL SOC
DOI: 10.1021/pr500681x

关键词

diagnosis; biomarkers; immunoproteomics; immunome; invasive candidiasis; hsp90; enolase; serological proteome analysis; antibody response; sensitivity and specificity

资金

  1. Community of Madrid [S2010/BMD-2414 PROMPT-CM]
  2. Ministry of Economy and Competitiveness [BIO-2012-31767]
  3. Marie Curie Initial Training Networks (FP7-PEOPLE-ITN ImResFun)
  4. National Plan of I+D+i
  5. ISCIII, Spanish Network for Research in Infectious Diseases [REIPI RD12/0015/0004]
  6. European Development Regional Fund Away to achieve Europe ERDF
  7. Ramon Areces Foundation
  8. MSD Special Chair in Genomics and Proteomics, Spain

向作者/读者索取更多资源

Invasive candidiasis (IC) adds significantly to the morbidity and mortality of non-neutropenic patients if not diagnosed and treated early. To uncover serologic biomarkers that alone or in combination could reliably detect IC in this population, IgG antibodyreactivity profiles to the Candida albicans intracellular proteome were examined by serological proteome analysis (SERPA) and data mining procedures in a training set of 24 non-neutropenic patients. Despite the high interindividual molecular heterogeneity, unsupervised clustering analyses revealed that serum 22-IgG antibodyreactivity patterns differentiated IC from non-IC patients. Univariate analyses further highlighted that 15 out of the 22 SERPA-identified IgG antibodies could be useful candidate IC biomarkers. The diagnostic performance of one of these candidates (anti-Hsp90 IgG antibodies) was validated using an ELISA prototype in a test set of 59 non-neutropenic patients. We then formulated an IC discriminator based on the combined immunoproteomic fingerprints of this and another SERPA-detected and previously validated IC biomarker (anti-Eno1 IgG antibodies) in the training set. Its consistency was substantiated using their ELISA prototypes in the test set. Receiver-operating-characteristic curve analyses showed that this two-biomarker signature accurately identified IC in non-neutropenic patients and provided better IC diagnostic accuracy than the individual biomarkers alone. We conclude that this serum IgG antibody signature directed against C. albicans Hsp90 and Eno1, if confirmed prospectively, may be useful for IC diagnosis in non-neutropenic patients.

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