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Fungal Typing, Sequencing, and AFLP in Clinical Mycology Lab-Introduction, Purpose, Method, Application, and Conclusion

Introduction to Advanced Molecular Techniques in Clinical Mycology

Clinical mycology laboratories play a crucial role in diagnosing and managing fungal infections. Traditional methods like culture and microscopy are often complemented by advanced molecular techniques to improve the accuracy and speed of fungal identification. Among these techniques, fungal typing, sequencing, and amplified fragment length polymorphism (AFLP) are prominent.

Fig. Various Candida species growth on Chromagar-Candida albicans, Candida krusie, Candida tropicalis, and Candida glabrata

Fungal Typing

Purpose:
Fungal typing is used to differentiate between fungal species and strains. This is essential for epidemiological studies, outbreak investigations, and understanding the distribution of fungal pathogens.

Methods:

  • Phenotypic Typing: Based on morphological characteristics and biochemical tests.
  • Genotypic Typing: Uses DNA-based methods to identify genetic differences. Techniques include:
    • Restriction Fragment Length Polymorphism (RFLP): Analyzes the pattern of DNA fragments produced by restriction enzyme digestion.
    • Random Amplified Polymorphic DNA (RAPD): Uses random primers to amplify DNA and generate unique patterns.

Applications in Clinical Mycology:

  • Tracking the source and spread of infections in hospital settings.
  • Differentiating between relapse and new infection in patients.
  • Understanding the genetic diversity of fungal pathogens.

Sequencing-Based Identification

Purpose:
Sequencing precisely identifies fungal species by analyzing specific regions of the fungal genome.

Methods:

  • Sanger Sequencing: Gold standard for DNA sequencing, particularly useful for small DNA fragments.
  • Next-Generation Sequencing (NGS): Allows high-throughput sequencing of multiple samples simultaneously. Common platforms include Illumina and Ion Torrent.

Target Regions:

  • Internal Transcribed Spacer (ITS): The highly variable region between the rRNA genes, commonly used for fungal identification.
  • D1/D2 Region of 28S rRNA: Useful for identifying a wide range of fungi.
  • 18S rRNA Gene: Provides broad taxonomic resolution.

Applications in Clinical Mycology:

  • Identifying fungal species directly from clinical samples.
  • Detecting mixed fungal infections.
  • Identifying non-culturable or slow-growing fungi.
  • Confirming results from phenotypic and other genotypic methods.

Amplified Fragment Length Polymorphism (AFLP)

Purpose:
AFLP is used for genotyping and fingerprinting of fungal isolates. It combines the specificity of restriction enzymes with the sensitivity of PCR amplification.

Fig. Aspergillus fumigatus-bluish green pigment of conidia on SDA after 4 days of incubation at

Method:

  1. DNA Extraction: Fungal DNA is extracted from clinical isolates.
  2. Restriction Digestion: DNA is digested with restriction enzymes (e.g., EcoRI, MseI).
  3. Adaptor Ligation: Short DNA adaptors are ligated to the ends of restriction fragments.
  4. Selective Amplification: PCR amplifies a subset of these fragments using primers that match the adaptors.
  5. Fragment Analysis: The amplified fragments are separated by gel or capillary electrophoresis to generate a unique pattern.

Applications in Clinical Mycology:

  • Differentiating closely related fungal strains.
  • Studying population genetics and epidemiology of fungal pathogens.
  • Identifying genetic markers associated with antifungal resistance.

Integration of Techniques in Clinical Mycology Labs

Workflow:

  1. Sample Collection and Preparation: Clinical samples (e.g., blood, CSF, tissue) are collected and DNA is extracted.
  2. Preliminary Identification: Initial identification using culture, microscopy, and basic biochemical tests.
  3. Molecular Typing: RFLP, RAPD, or AFLP is used to differentiate strains.
  4. Sequencing: Sequencing of ITS, D1/D2, or 18S regions for precise species identification.
  5. Data Analysis: Bioinformatics tools analyze sequencing and AFLP data to generate reports.

Benefits of Fungal Typing, Sequencing, and AFLP in Clinical Mycology Lab

  • Accuracy: Molecular techniques provide precise and accurate identification, reducing diagnostic errors.
  • Speed: Faster turnaround time compared to traditional methods, enabling prompt treatment decisions.
  • Sensitivity: Higher sensitivity in detecting low-level or mixed infections.
  • Resistance Detection: Identifying genetic mutations associated with antifungal resistance, guiding effective therapy.

Conclusion for Fungal Typing, Sequencing, and AFLP in Clinical Mycology Lab

The integration of fungal typing, sequencing, and AFLP in clinical mycology labs enhances diagnostic capabilities, leading to better patient management and outcomes. These advanced molecular techniques provide detailed insights into the epidemiology, diversity, and resistance patterns of fungal pathogens, making them indispensable tools in modern clinical mycology.

Medical Lab Notes

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