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Molecular diagnosis of rhino-orbital mucormycosis in a COVID-19 setting.
Khapuinamai, Agimanailiu; Sharma, Savitri; Dave, Tarjani Vivek; Kapoor, Anasua Ganguly; Joseph, Joveeta.
  • Khapuinamai A; LVPEI Network, Jhaveri Microbiology Centre, Brien Holden Eye Research Centre, L. V. Prasad Eye Institute, Kallam Anji Reddy Campus, L V Prasad Marg, Hyderabad, Telangana, 500 034, India.
  • Sharma S; The Ramoji Foundation for Ocular Infections, L. V. Prasad Eye Institute, Hyderabad, Telangana, India.
  • Dave TV; LVPEI Network, Jhaveri Microbiology Centre, Brien Holden Eye Research Centre, L. V. Prasad Eye Institute, Kallam Anji Reddy Campus, L V Prasad Marg, Hyderabad, Telangana, 500 034, India.
  • Kapoor AG; The Ramoji Foundation for Ocular Infections, L. V. Prasad Eye Institute, Hyderabad, Telangana, India.
  • Joseph J; Ophthalmic Plastic Surgery Service, LV Prasad Eye Institute, Kallam Anji Reddy Campus, Hyderabad, India.
Int Ophthalmol ; 2022 Nov 21.
Article in English | MEDLINE | ID: covidwho-2324069
ABSTRACT

PURPOSE:

Mucormycosis is a severe fungal infection caused by species of the order Mucorales. Early and accurate diagnosis is a prerequisite in the management of the disease. In the present study, we evaluated and compared two PCR-based techniques for the diagnosis and identification of mucormycosis in patients with rhino-orbital mucormycosis (ROM) post-COVID-19.

METHODS:

Diagnosed clinically and radiologically, 25 patients of ROM were included in the study and endoscopically or blind collected nasal swabs or orbital tissues were submitted for microbiological evaluation (direct microscopy + culture) and PCR using primers targeting two different loci (ITS and 28S rDNA region) for diagnosis. All PCR products were further processed for species identification using Sanger sequencing whenever possible.

RESULT:

Of the 25 samples included in the study, 16 samples were positive for presence of fungal filaments by Smear suggestive of Mucorales sp., but only 7/25 grew in culture. ITS-based PCR was able to identify mucormycosis in 7/25 (28%) samples and 28S rDNA PCR showed positivity for 19/25 (76%) samples. Rhizopus oryzae was found to be the predominant species in our study. The sensitivity and specificity of 28S rDNA PCR compared to culture were found to be 85.71% and 27.78%, respectively, while for ITS-based PCR, they were 42.86% and 77.78%, respectively.

CONCLUSIONS:

28S rDNA-based PCR is a reliable and sensitive method for early diagnosis of mucormycosis. Molecular techniques have shown a promising future to provide quick and effective treatment by accurately identifying the aetiologic agent.
Keywords

Full text: Available Collection: International databases Database: MEDLINE Type of study: Diagnostic study / Etiology study / Experimental Studies / Prognostic study Topics: Long Covid Language: English Year: 2022 Document Type: Article Affiliation country: S10792-022-02577-y

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Full text: Available Collection: International databases Database: MEDLINE Type of study: Diagnostic study / Etiology study / Experimental Studies / Prognostic study Topics: Long Covid Language: English Year: 2022 Document Type: Article Affiliation country: S10792-022-02577-y