Multi-centric evaluation of a stage-specific reverse transcriptase-polymerase chain reaction assay as a xenomonitoring tool for the detection of infective (L3) stage Wuchereria bancrofti in vectors

Venkatesan Vasuki; Sugeerappa Laxmanappa Hoti; Swaminathan Subramanian; Abdul Mabood Khan; Velayudham Thenmozhi; Nagarajan Shriram Ananganallur; Namita Mahapatra; Ramalingam Balasubramaniyan

doi:10.4103/ijmr.IJMR_713_19

Multi-centric evaluation of a stage-specific reverse transcriptase-polymerase chain reaction assay as a xenomonitoring tool for the detection of infective (L₃) stage Wuchereria bancrofti in vectors

Indian J Med Res. 2021 Jul;154(1):132-140. doi: 10.4103/ijmr.IJMR_713_19.

Authors

Venkatesan Vasuki¹, Sugeerappa Laxmanappa Hoti², Swaminathan Subramanian¹, Abdul Mabood Khan³, Velayudham Thenmozhi⁴, Nagarajan Shriram Ananganallur⁵, Namita Mahapatra⁶, Ramalingam Balasubramaniyan¹

Affiliations

¹ ICMR-Vector Control Research Centre, Puducherry, India.
² ICMR-National Institute of Traditional Medicine, Belagavi, Karnataka, India.
³ ICMR-Regional Medical Research Centre, Dibrugarh, Assam, India.
⁴ ICMR-Centre for Research in Medical Entomology, Madurai, Tamil Nadu, India.
⁵ ICMR-Regional Medical Research Centre, Port Blair, Andaman & Nicobar Islands, India.
⁶ ICMR-Regional Medical Research Centre, Bhubaneswar, Odisha, India.

Abstract

Background & objectives: An infective stage specific reverse transcriptase-polymerase chain reaction (RT-PCR) assay utilizing the abundant larval transcript-3 (Alt-3) gene of Wuchereria bancrofti was developed at ICMR-VCRC, Puducherry and found to be stage specific, and sensitive upon validation in the laboratory. This study was aimed at independently evaluating this assay for its utility as a monitoring/surveillance tool in the operational programme for elimination of lymphatic filariasis (LF) by four national research laboratories.

Methods: Evaluation of the assay was carried out in a multi-centric mode in three phases. In phase I, a workshop was conducted to impart hands-on training to the scientists from the collaborating centres on the RT-PCR assay and in Phase II the assay was evaluated for specificity and sensitivity in detecting the infective (L₃) stage larvae of W. bancrofti in its vector, Culex quinquefasciatus, using 50 coded pooled samples. Phase III evaluation was done on wild-caught mosquito vectors from selected endemic areas of Assam and Bhubaneswar States and Andaman Nicobar islands.

Results: Phase I data indicated that the assay was able to detect all the pools of mosquito samples contaning L₃ stage larvae of W. bancrofti as positive, even in the presence of other vector stages of the parasite indicating its stage specificity (100%). The assay was found highly sensitive (100%), detecting all the infected pools as positive and specific detecting all uninfected pools as negative. The results of phase II showed inter-laboratory variation. Phase III evaluation from all the centres suggested that the infectivity rate determined for pooled mosquitoes by the RT-PCR assay (0.5%) was comparable to that by dissection method (1.2%) (95% confidence interval overlaps).

Interpretation & conclusions: Overall, the results from three of the four participating centres indicated that the assay is at least as sensitive and stage specific as the conventional mosquito dissection technique, and hence, may be useful as a xenomonitoring tool for Transmission Assessment Survey in Mass Drug Administration programmes for LF.

Keywords: Infective (L3) stage; L3 specific reverse transcriptase-polymerase chain reaction assay; Wuchereria bancrofti; multi-centric evaluation.

MeSH terms

Animals
Culex*
Elephantiasis, Filarial* / diagnosis
Elephantiasis, Filarial* / epidemiology
RNA-Directed DNA Polymerase
Reverse Transcriptase Polymerase Chain Reaction
Wuchereria bancrofti / genetics

Substances

RNA-Directed DNA Polymerase