Molecular detection of DHFR gene polymorphisms in Pneumocystis jirovecii isolates from Indian patients

Authors

  • Yogita Singh All India institute of Medical Sciences, New Delhi, India
  • Bijay Ranjan Mirdha All India institute of Medical Sciences, New Delhi, India
  • Randeep Guleria All India institute of Medical Sciences, New Delhi, India
  • Shehla Khalil All India institute of Medical Sciences, New Delhi, India
  • Ashutosh Panda All India institute of Medical Sciences, New Delhi, India
  • Rama Chaudhry All India institute of Medical Sciences, New Delhi, India
  • Anant Mohan All India institute of Medical Sciences, New Delhi, India
  • Sushil Kumar Kabra All India institute of Medical Sciences, New Delhi, India
  • Lalit Kumar All India institute of Medical Sciences, New Delhi, India
  • Sanjay Kumar Agarwal All India institute of Medical Sciences, New Delhi, India

DOI:

https://doi.org/10.3855/jidc.6810

Keywords:

Pneumocystis jirovecii, dihydrofolate reductase, trimethoprim-sulfamethoxazole, polymorphisms

Abstract

Introduction: Pneumocystis pneumonia (PCP) is an opportunistic life-threatening infection, especially for immunocompromised individuals. A trimethoprim-sulfamethoxazole (TMP-SMX) combination is commonly used for the treatment of PCP, targeting both dihydrofolate reductase (DHFR) and dihydropteroate synthase (DHPS) enzymes. Several studies have already shown that polymorphisms in the DHPS gene are associated with drug resistance. The present study analyzed DHFR gene polymorphisms in Pneumocystis jirovecii recovered from clinical samples from patients admitted to a tertiary care health center in New Delhi, India.

Methodology: Detection of P. jirovecii was performed using Gomori methenamine silver staining (GMS) and nested polymerase chain reaction (PCR) assay targeting the mitochondrial large subunit ribosomal RNA (mt LSU rRNA) gene. The DHFR gene was amplified using nested PCR protocol and was sequenced for detection of polymorphisms.

Results: Of 180 clinical samples, only 4% (7/180) were positive by GMS staining, and 10% (18/180) were positive by mt LSU rRNA PCR assay. Of these 18 positive samples, only 77% (14/18) were amplified by the DHFR gene PCR assay. A total of 16 nucleotide substitutions were observed in 42% (6/14) samples targeted for the DHFR gene, of which 8 nucleotide substitutions were synonymous and the rest were non-synonymous.

Conclusions: The DHFR gene mutations found in this study may possibly indicate an association of process likely to contribute to therapeutic failure or an evolutionary process, and warrant continuous monitoring.

Author Biographies

Yogita Singh, All India institute of Medical Sciences, New Delhi, India

Department of Microbiology

Bijay Ranjan Mirdha, All India institute of Medical Sciences, New Delhi, India

Professor

Department of Microbiology

Randeep Guleria, All India institute of Medical Sciences, New Delhi, India

Department of Pulmonary Medicine & Sleep Disorders

Shehla Khalil, All India institute of Medical Sciences, New Delhi, India

Department of Microbiology

Ashutosh Panda, All India institute of Medical Sciences, New Delhi, India

Department of Microbiology

Rama Chaudhry, All India institute of Medical Sciences, New Delhi, India

Department of Microbiology

Anant Mohan, All India institute of Medical Sciences, New Delhi, India

Department of Pulmonary Medicine & Sleep Disorders

Sushil Kumar Kabra, All India institute of Medical Sciences, New Delhi, India

Department of Pediatrics

Lalit Kumar, All India institute of Medical Sciences, New Delhi, India

Department of Medical Oncology

 

Sanjay Kumar Agarwal, All India institute of Medical Sciences, New Delhi, India

Department of Nephrology

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Published

2015-11-30

How to Cite

1.
Singh Y, Mirdha BR, Guleria R, Khalil S, Panda A, Chaudhry R, Mohan A, Kabra SK, Kumar L, Agarwal SK (2015) Molecular detection of DHFR gene polymorphisms in Pneumocystis jirovecii isolates from Indian patients. J Infect Dev Ctries 9:1250–1256. doi: 10.3855/jidc.6810

Issue

Vol. 9 No. 11: November 2015

Section

Original Articles

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