A Real Time PCR strategy for the detection and quantification of Candida albicans in human blood.
Felipe Delatorre BusserVivian Caso CoelhoClaudia de Abreu FonsecaGilda Maria Barbaro Del NegroMaria Aparecida Shikanai-YasudaMarta Heloisa LopesMarcello Mihailenko Chaves MagriVera Lúcia Teixeira de FreitasPublished in: Revista do Instituto de Medicina Tropical de Sao Paulo (2020)
Candidemia is a significant cause of bloodstream infections (BSI) in nosocomial settings. The identification of species can potentially improve the quality of care and decrease human mortality. Quantitative PCR (qPCR) was evaluated for Candida albicans detection using culture suspensions containing C. albicans , spiked human blood, the cloned qPCR target fragment (ITS2 region) and the results of these assays were compared. The assays showed a good detection limit: C. albicans DNA extracted from yeast (sensitivity 0.2 CFU/µL), spiked human blood (sensitivity 10 CFU/mL), and cloned fragment of ITS2 region (sensitivity 20 target copies/μL). The efficiency of ITS2 fragment-qPCR ranged from 89.67 to 97.07, and the linearity (R2) of the standard curve ranged from 0.992 to 0.999. The results showed that this ITS2-qPCR has a great potential as a molecular prototype model for the development of a test to be applied in clinical practice, greatly reducing the time of candidemia diagnosis, which is extremely important in this clinical setting.
Keyphrases
- candida albicans
- real time pcr
- endothelial cells
- biofilm formation
- induced pluripotent stem cells
- high throughput
- type diabetes
- palliative care
- high resolution
- cardiovascular disease
- cystic fibrosis
- label free
- drug resistant
- single molecule
- risk assessment
- chronic pain
- staphylococcus aureus
- multidrug resistant
- cardiovascular events
- quality improvement
- mass spectrometry
- pain management
- nucleic acid