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      A rapid diagnostic test for human Visceral Leishmaniasis using novel Leishmania antigens in a Laser Direct-Write Lateral Flow Device

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          ABSTRACT

          Visceral Leishmaniasis (VL) causes high morbidity and mortality in low-to-middle-income countries worldwide. In this study, we used Laser Direct-Write (LDW) technology to develop a new Lateral Flow Device (LFD) with double-channel geometry on a low-cost paper platform as a rapid and accurate serodiagnostic assay for human VL. This Duplex VL-LFD was based on a laser-patterned microfluidic device using two recombinant Leishmania proteins, β-tubulin and LiHyp1, as novel diagnostic antigens. The VL-LFD assay was tested with blood/serum samples from patients diagnosed with VL, Tegumentary Leishmaniasis, Leishmaniasis of unknown identity, other parasitic diseases with similar clinical symptoms, i.e. Leprosy Disease and Chagas Disease, and blood from healthy donors, and compared in parallel with commercial rK39 IT-LEISH ® Kit. Clinical diagnosis and real-time Polymerase Chain Reaction assay were used as reference standards. VL-LFD Sensitivity (S ± 95% Confidence Intervals (CI)) of 90.9 (78.9-100) and Specificity (Sp ± 95% CI) of 98.7 (96.1-100) outperformed the IT-LEISH ® Kit [ S = 77.3 (59.8-94.8), Sp = 94.7 (89.6-99.8)]. This is the first study reporting successful development of an LFD assay using the LDW technology and the VL-LFD warrants comparative testing in larger patient cohorts and in areas with endemic VL in order to improve diagnosis and disease management.

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          Visceral leishmaniasis: what are the needs for diagnosis, treatment and control?

          Visceral leishmaniasis (VL) is a systemic protozoan disease that is transmitted by phlebotomine sandflies. Poor and neglected populations in East Africa and the Indian sub-continent are particularly affected. Early and accurate diagnosis and treatment remain key components of VL control. In addition to improved diagnostic tests, accurate and simple tests are needed to identify treatment failures. Miltefosine, paromomycin and liposomal amphotericin B are gradually replacing pentavalent antimonials and conventional amphotericin B as the preferred treatments in some regions, but in other areas these drugs are still being evaluated in both mono- and combination therapies. New diagnostic tools and new treatment strategies will only have an impact if they are made widely available to patients.
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            A Historical Overview of the Classification, Evolution, and Dispersion of Leishmania Parasites and Sandflies

            Background The aim of this study is to describe the major evolutionary historical events among Leishmania, sandflies, and the associated animal reservoirs in detail, in accordance with the geographical evolution of the Earth, which has not been previously discussed on a large scale. Methodology and Principal Findings Leishmania and sandfly classification has always been a controversial matter, and the increasing number of species currently described further complicates this issue. Despite several hypotheses on the origin, evolution, and distribution of Leishmania and sandflies in the Old and New World, no consistent agreement exists regarding dissemination of the actors that play roles in leishmaniasis. For this purpose, we present here three centuries of research on sandflies and Leishmania descriptions, as well as a complete description of Leishmania and sandfly fossils and the emergence date of each Leishmania and sandfly group during different geographical periods, from 550 million years ago until now. We discuss critically the different approaches that were used for Leishmana and sandfly classification and their synonymies, proposing an updated classification for each species of Leishmania and sandfly. We update information on the current distribution and dispersion of different species of Leishmania (53), sandflies (more than 800 at genus or subgenus level), and animal reservoirs in each of the following geographical ecozones: Palearctic, Nearctic, Neotropic, Afrotropical, Oriental, Malagasy, and Australian. We propose an updated list of the potential and proven sandfly vectors for each Leishmania species in the Old and New World. Finally, we address a classical question about digenetic Leishmania evolution: which was the first host, a vertebrate or an invertebrate? Conclusions and Significance We propose an updated view of events that have played important roles in the geographical dispersion of sandflies, in relation to both the Leishmania species they transmit and the animal reservoirs of the parasites.
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              FLASH: a rapid method for prototyping paper-based microfluidic devices.

              This article describes FLASH (Fast Lithographic Activation of Sheets), a rapid method for laboratory prototyping of microfluidic devices in paper. Paper-based microfluidic devices are emerging as a new technology for applications in diagnostics for the developing world, where low cost and simplicity are essential. FLASH is based on photolithography, but requires only a UV lamp and a hotplate; no clean-room or special facilities are required (FLASH patterning can even be performed in sunlight if a UV lamp and hotplate are unavailable). The method provides channels in paper with dimensions as small as 200 microm in width and 70 microm in height; the height is defined by the thickness of the paper. Photomasks for patterning paper-based microfluidic devices can be printed using an ink-jet printer or photocopier, or drawn by hand using a waterproof black pen. FLASH provides a straightforward method for prototyping paper-based microfluidic devices in regions where the technological support for conventional photolithography is not available.
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                Author and article information

                Journal
                Emerg Microbes Infect
                Emerg Microbes Infect
                TEMI
                temi20
                Emerging Microbes & Infections
                Taylor & Francis
                2222-1751
                2019
                5 August 2019
                : 8
                : 1
                : 1178-1185
                Affiliations
                [a ]Neisseria Research Group, Molecular Microbiology, School of Clinical and Experimental Sciences, University of Southampton Faculty of Medicine, Southampton General Hospital , Southampton, England
                [b ]Programa de Pós-Graduação em Ciências da Saúde: Infectologia e Medicina Tropical, Faculdade de Medicina, Universidade Federal de Minas Gerais , Belo Horizonte, Brazil
                [c ]Optoelectronics Research Centre, University of Southampton , Southampton, England
                [d ]Departamento de Patologia Clínica, COLTEC, Universidade Federal de Minas Gerais , Belo Horizonte, Brazil
                Author notes
                [CONTACT ] Myron Christodoulides mc4@ 123456soton.ac.uk Neisseria Research Group, Molecular Microbiology, School of Clinical and Experimental Sciences, University of Southampton Faculty of Medicine, Southampton General Hospital , Southampton SO16 6YD, England
                [*]

                These authors contributed equally to the experimental work.

                [†]

                These authors are equal principal investigators on this work.

                Supplemental data for this article can be accessed https://doi.org/10.1080/22221751.2019.1635430.

                Article
                1635430
                10.1080/22221751.2019.1635430
                6713177
                31381478
                b65143bb-b523-4cf5-beca-c2df474b21c8
                © 2019 The Author(s). Published by Informa UK Limited, trading as Taylor & Francis Group on behalf of Shanghai Shangyixun Cultural Communication Co., Ltd

                This is an Open Access article distributed under the terms of the Creative Commons Attribution License ( http://creativecommons.org/licenses/by/4.0/), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

                History
                : 25 April 2019
                : 19 June 2019
                : 20 June 2019
                Page count
                Figures: 2, Tables: 2, Equations: 0, References: 41, Pages: 8
                Funding
                Funded by: Conselho Nacional de Desenvolvimento Científico e Tecnológico, Brazil
                Award ID: APQ-408675/2018-7
                Funded by: Coordenadoria de Aperfeiçoamento de Pessoal de Nível Superior, Brazil
                Funded by: Engineering and Physical Sciences Research Council, UK
                Award ID: EP/PO25757/1
                Award ID: EP/N004388/1
                Award ID: EP/M027260/1
                This work was supported by funding from the Network for Anti-Microbial Resistance and Infection Prevention (Engineering and Physical Sciences Research Council, UK, reference EP/M027260/1) to MC, EAFC, CS and MVH; from the Engineering and Physical Sciences Research Council, UK, to IK and CS via the grants EP/PO25757/1, EP/N004388/1 and EP/M027260/1; from Conselho Nacional de Desenvolvimento Científico e Tecnológico, Brazil, to EAFC and LEC via grant APQ-408675/2018-7. EAFC receives a scholarship from Conselho Nacional de Desenvolvimento Científico e Tecnológico, Brazil, and LEC was a visiting postdoctoral research fellow funded by Coordenadoria de Aperfeiçoamento de Pessoal de Nível Superior, Brazil.
                Categories
                Article

                leishmania infantum,visceral leishmaniasis,laser direct-write,lateral flow device,immunochromatographic test

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