AUTHOR=Mesquita Silvia Gonçalves , Lugli Elena Birgitta , Matera Giovanni , Fonseca Cristina Toscano , Caldeira Roberta Lima , Webster Bonnie 

TITLE=Development of real-time and lateral flow recombinase polymerase amplification assays for rapid detection of Schistosoma mansoni

JOURNAL=Frontiers in Microbiology

VOLUME=13

YEAR=2022

URL=https://www.frontiersin.org/journals/microbiology/articles/10.3389/fmicb.2022.1043596

DOI=10.3389/fmicb.2022.1043596

ISSN=1664-302X

ABSTRACT=<sec><title>Background</title><p>Accurate diagnosis followed by timely treatment is an effective strategy for the prevention of complications together with reducing schistosomiasis transmission. Recombinase Polymerase Amplification (RPA) is a simple, rapid, sensitive, and specific isothermal method with low resource needs. This research aimed at the development and optimisation of a real-time (RT) and a lateral flow (LF) RPA assay for the detection of <italic>Schistosoma mansoni</italic>.</p></sec><sec><title>Methodology</title><p>Recombinase Polymerase Amplification reactions were performed at full- (as recommended) and half-volumes (to reduce costs), with RT or LF detection systems targeting the <italic>S</italic>. <italic>mansoni</italic> mitochondrial minisatellite region. The specificity was assessed using gDNA from other <italic>Schistosoma</italic> species, helminths co-endemic with <italic>S</italic>. <italic>mansoni</italic>, human stool, and urine, and <italic>Biomphalaria</italic> snail hosts. The analytical sensitivity was evaluated using serial dilutions of gDNA, synthetic copies of the target, and single eggs. The ability of both assays to detect the <italic>S</italic>. <italic>mansoni</italic> DNA in human urine and stool samples was also tested. The long-term stability of the RT-RPA reagents was evaluated by storing the reaction components in different temperature conditions for up to 3  weeks.</p></sec><sec><title>Results</title><p>The RT- and the LF-RPA (SmMIT- and SmMIT-LF-RPA, respectively) presented similar results when used full- and half-volumes, thus the latter was followed in all experiments. The SmMIT-RPA was 100% specific to <italic>S</italic>. <italic>mansoni</italic>, able to detect a single egg, with a limit of detection (LOD) of down to 1  fg of gDNA and one synthetic copy of the target. The assay was able to detect <italic>S</italic>. <italic>mansoni</italic> DNA from stool containing 1 egg/g and in spiked urine at a concentration of 10  fg/μl. SmMIT-RPA reagents were stable for up to 3  weeks when kept at 19°C, and 2  weeks when stored at 27°C. The SmMIT-LF-RPA cross-reacted with Clinostomidae, presented the LOD of 10  fg and one synthetic copy of the target, being able to detect a single egg and 1 egg/g in a stool sample. The LOD in spiked urine samples was 10  pg/μl.</p></sec><sec><title>Conclusion</title><p>The half-volume SmMIT-RPA is a promising method to be used in the field. It is specific, sensitive, robust, and tolerant to inhibitors, with a long-term stability of the reaction components and the real-time visualisation of results.</p></sec>