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  falciparum. Transactions of theRoyal Socieg of TropicalMedicine       Roeffen, W., Geeraedts, F., Eling, W., Beckers, I’., Wizel, B.,
    and Hygiene, 74,738-742.                                              Kumar, N., Lensen, T. & Sauerwein, R. (1995). Transmis-
Graves, I’. M., Burkot, T. R., Carter, R., Cattani, J. A., Lagog,         sion blockade of Plasmodium falciparum malaria by anti-
   M., Parker, J., Brabin, B. J., Gibson, F. D., Bradley, D. J. &         Pfs230-specific antibodies is isotype dependent. Infection
   AlDers, M. P. (1988). Measurement of malaria infectivitv of            and Immunity, 63,467-471.
   himan populations to mosquitoes in the Madang area, Papua            Rutledge, L. C., Ward, R. A. & Gould, D. J. (1964). Studies on
   New Guinea. Parasitology, 96,251-263.                                  the feeding response of mosquitoes to nutritive solutions in a
Jeffery, G. & Eyles, D. E. (1955). Infectivity to mosquitoes of           new membrane feeder. Mosquito New!, 24, 407-419.
   Plasmodium falcioarum as related to aametocvte densitv and           Tchuinkam, T., Mulder, B., Dechermg, K., Stoffels, H.,
   duration of ‘mfection. American Jot&al of Tiopical Me&&e               Verhave, J. P., Cot, M., Carnevale, I’., Meuwissen, J. H. E.
   and Hygiene, 4, 781-789.                                               T. & Robert, V. (1993). Experimental infections of Anopheles
Kaslow, D. C. (1993). Transmission-blocking             immunity          gambiae with Plasmodium falciparum of naturally infected
   against malaria and other vector-borne diseases. Current               gametocvte carriers in Cameroon: factors influencing the
   Opinion in Immunology, 5, 557-565.                                     hfectiv&    to mosquitoes. Tropical Medicine and Parasitology,
Lensen, A., Vandruten, J., Bolmer, M., Vangemert, G., Eling,              44,271-276.
   W. & Sauerwein, R. (1996). Measurement by membrane                   Vanderberg, J. P. & Gwadz, R. W. (1980). The transmission by
   feeding of reduction in Plasmodium falciparum transmission             mosquitoes of plasmodia in the laboratory. In: Malaria,
   induced by endemic sera. Transactions of the Royal Society of          Kreier, J. I’. (editor). New York: Academic Press, pp. 154-
    Tropical Medicine and Hygiene, 90, 20-22.                             218.
Muirhead-Thomson,       R. C. (1957). The malarial infectivity of       Yoeli, M. (1938). Note on the experimental infection of
   an African village population to mosquitoes (Anopheles gam-            Anopheles elutus with Plasmodium falciparum by feeding
   biae) American Journal of Tropical Medicine and Hygiene, 6,            through a prepared animal membrane. Rivista diMaZariologia,
   971-979.                                                               17,62-66.
Ponnudurai, T., Lensen, A. H. W., Gemert Van, G. J. A.,
  Bensink, M. P. E., Bolmer, M. & Meuwissen, J. H. E. T.
   (1989). Infectivity of cultured Plasmodium falciparum game-          Received 25 May 1999; revised 18 3;11y 1999; accepted for
  tocytes to mosquitoes. Parasitology,98, 165-173.                      publication 3 August 1999




TRANSACTIONS        OF THE ROYAL     SOCIETY   OF TROPICAL   MEDICINE     AND HYGIENE     (2000) 94,106-107



                                                                         Amapi, Rondbnia and Roraima States). The same num-
1 Short Report             1                                             ber of mosquitoes known to be negative for human
I                          I                                             malaria parasites was also tested.
                                                                             The source of PZusmodium DNA was the same material
Infectivity of malaria vector                                            used for the ELISA test [triturated mosquitoes-head
                                                                          and thorax ground in a blocking buffer containing 0.05%
mosquitoes:    correlation of positivity                                 nonidet P-40 (WIRTZ et al., 1987)], either 20 @spotted
between ELBA and PCR-ELISA tests                                         on a glass fibre membrane (GFM) prepared for PCR,
                                                                         using l/8 of the spot as DNA source directly into the PCR
                                                                         mixture as described by WARHURST et al. (1991), or
Marinete     M. l%voa’*,     Ricardo L. D. Machado’,                     extracted as follows: 40 & of ELISA solution was
Maria     N. 0. Segura’,       Giselle M. R. Vianna’,                    centrifuged for 10 min at 22 500 g, the pellet was lysed
Adenildo S. Vasc&celds’         and Jan E. Conn3 ‘Pro:                   by adding 25 &of lysis buffer and incubating at 65°C for
wama    de Malhia.   Instituto Evandro ChaPaslFAWMS.                     30 min, afterwards adding potassium acetate and placing
k. Almirante Bakroso, 492, 66.090-000, -Bel&m, Park,                     on ice for at least 60 min. The isolated DNA (obtained by
Brazil; ‘Institute Oswald0 Cruz, FIOCRUZ, Av. Brasil,                    ethanol precipitation)     was dissolved in 15 pL of TE-
436.5, 210 45-900, Rio deyaneiro, RJ, Brazil; 3Department                buffer containing ribonuclease WILSON et al., 1998).
of Biology, Marsh Life Sciences Building, University of                  The DNA was amplified as described by MACHADO           et al.
Vermont, Burlington, VT, 054050460, USA                                   (1998) using primer sequence, concentrations and reac-
                                                                         tion conditions indicated by OLIVEIRA et al. (1995). For
                                                                         the identification of the human malaria parasites we used
Keywords:     malaria transmission, anopheline mosquitoes, in-           the liquid-phase,      non-isotopic hybridization    ELISA
fectivity, ELISA, PCR-ELISA,      Brazil                                 technique, following the protocol of OLIVEIRA et al.
                                                                         (1995). For negative controls we used distilled water,
    Studies on the infectivity of malaria vector mosquitoes              male anopheline      and culicine mosquitoes, and human
using the enzyme-linked immunosorbent assay (ELISA)                      DNA. Positive controls included strain Kl of I? fulcipar-
described by WIRTZ et al. (1987) have been carried out                   urn, and mosquitoes experimentally infected with l?
worldwide for several years. SOMBOON et al. (1993)                      falciparum and l? vivax.
reported false-positive results for the ELISA associated                     Our PCR results confirmed the ELISA test results for
with bovine and swine blood. In order to avoid these                     all positive and all negative mosquitoes, and in 5 (15.6%)
false-positive results it is advisable either to use only the            of the positive mosquitoes (3 An. albitursis and 2 An.
anterior part of the mosquito (head and thorax) which,                   darlingi) the PCR-ELISA          technique detected other
normally, is not contaminated by the ingested animal                     species of human Plasmodium that were not found by
blood (WIRTZ      et al., 1987). or to confirm     the ELISA             the ELISA test alone (Table). The DNA source was
result by another method’such          as polymerase chain               obtained only by DNA extraction, which means that the
reaction (PCR).                                                          GFM technique is not applicable for this tvpe of material.
    We have carried out the PCR-ELISA          to confirm the           These results indicate-&at        the PCR-&ISA      is more
detection of human malaria parasites in mosquitoes                       sensitive than a simnle ELISA test which. however. still
already recorded as positive by ELISA alone. Thirty                     remains a very goodand useful tool for testing mo&ito
two such mosquitoes were tested, belonging to different                 infectivity.
species of the genus Anopheles and collected during field
trips to different areas of the Amazonia Region (Pari,                  Acknowledgements
                                                                           We thank the staff of the Malaria Entomology Laboratory at
                                                                        the Evandro Chagas Institute for technical assistance and
*Author   for correspondence;   fax +55 91226 1284 or 2114417.          Professor Ralph Lainson for reviewing the manuscript. This
lXA.SMODIUM     DETECTION       IN MOSQUITOES                                                                                     107



                    Table. Comparison     between            ELISA and PCR-ELISA      results for human
                    malaria parasites in Anopheles           mosquitoes from several areas ofthe Amazon
                    region in Brazil

                    Species                          State              ELISA                PCR-ELISA
                    An.   (NY.) albitarsis          Roraima             PVIPf                PvllwPm
                    An.   (Nys.) albitarsis                                                  PvlPj
                    An.   (Nys.) albitarsis         Roraima                                  filpf
                    An.   (N&.j albitarsis          Roraima                                  PvlPf
                    An.   fNvs. ) braziliensis      Roraima                                  PvlPf
                    An.   &$.j    nuneztovari       Roraima                                  Pvlps
                    An.   (Nys.) darlingi           Rondbnia
                    An.   (Nys.) darlingi           Rondhnia                                 g
                    An.   (Nys.) albitarsis         Amap                                     y&k
                    An.   (Nys.) albitarsis         Amapi
                    An.   (Nys.) albitarsis         Amapi                                    rym
                    An.   (Nys.) albitarsis         Amaph                                    Pv
                    An.   (Nys.) albitarsis         AmapL                                    l%
                    An.   (Nys.) albitarsis         Amapk                                    Pm
                    An.   (Nys.) albitarsis         Amapi                                    Pv
                    An.   (Nys.) braziliensis       Amapi                                    Pv
                    An.   (Nys.) darlingi           Amapi
                    An.   (Nys.) darlingi           Amapi                                    x
                    An.   (Nys.) aquasalis          ParP
                    An.   (Nys.) aquasalis          Pari
                    An.   (Nys.) aquasalis          Pari
                    An.   (Nys.) darlingi           Pari                                     Pv
                    An.   (Nys.) darling’           Pari                                     PV
                    An.   (Nys.) darlingi           Pari
                    An.   (Nys.) darlingi           Pari
                    An.   (Nys.) nuneztovari        Pari
                    An.   (Nys.) nuneztovari        Pari
                    An.   (Nys.) nuneztovari        Pari
                    An. (Nys.) nuneztovan’          Pari
                    An. (Nys.) nuneztovari          Pa&
                    An. (Nys.) nuneztovari          Pari                                     Pm
                    An. (Nys.) nuneztovari          Pari                                     Pm
                    Pv, Plasmodium vivax; pf, l? falciparum; Pm, I? malariae.

study received financial support from a National     Institute of     Warhurst, D. C., Awad-el-Karien,   F. M. & Miles, M. A. (199 1).
Health Grant (A140116) to J.E.C. and Evandro         Chagas In-         Simplified preparation of malaria blood samples for polymer-
stitute/FNS.                                                            ase chain reaction. Lancet, 337, 303-304.
                                                                      Wilson, M. D., Ofosu-Okyere, A., Okoli, A. U., McCall, P. J. &
References                                                              Snounou, G. (1998). Direct comparison of microscopy and
Machado, R. L. D., Garret, D. O., Adagu, I. S., Warhurst, D. C.         polymerase chain reaction for the detection of Plasmodium
   & I%voa, M. M. (1998). Simolified diagnosis of malaria               sporozoites in salivary glands of mosquitoes. Transactions of
   infection: GFM/PC&E&A,           a-simplified-nucleic  acid am-      the Royal Society of Tropical Medicine and Hvpiene, 92,
   plification technique by PClUELISA. Revista do Institute de          482-483.
   Medicina Tropical de SLio Paulo, 40, 333-334.                      Wirtz, R. A., Zavala, F., Charoenvit, Y., Campell, G. H.,
Oliveira, D. A., Holloway, B. P., Durigon, E. L., Collins, W. E.        Burkot, T. R., Scheneider, I., Esser, K. M., Beaudoin, R. L.
   & Lal, A. A. (1995). Polymerase chain reaction and liquid-           & Andr& R. G. (1987). Comparative testing of monoclonal
   phase, nonisotopic hybridization      for species-specific and       antibody against Plasmodiumfalciparum sporozoite for ELISA
   sensitive detection of malaria infection. American Journal of        development. Bulletin of the World Health Organization, 65,
   Tropical Medicine and Hygiene, 52, 139- 144.                         39-45.
Somboon, I’., Morakote, N., Koottathep, S. & Trisanarom, U.
   (1993). Detection of sporozoites of Plasmodium vivax and
   Plasmodium falciparum in mosquitoes by ELISA: false posi-
   tivity associated with bovine and swine blood. Transactions of
   the Royal Society of Tropical Medicine and Hygiene, 87,             Received ISJune 1999; revised 28 September 1999; accepted
   322-324.                                                           for publication 1 October 1999

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2000 infectivity of malaria vector mosquitoes

  • 1. 106 S.BONNETETAL falciparum. Transactions of theRoyal Socieg of TropicalMedicine Roeffen, W., Geeraedts, F., Eling, W., Beckers, I’., Wizel, B., and Hygiene, 74,738-742. Kumar, N., Lensen, T. & Sauerwein, R. (1995). Transmis- Graves, I’. M., Burkot, T. R., Carter, R., Cattani, J. A., Lagog, sion blockade of Plasmodium falciparum malaria by anti- M., Parker, J., Brabin, B. J., Gibson, F. D., Bradley, D. J. & Pfs230-specific antibodies is isotype dependent. Infection AlDers, M. P. (1988). Measurement of malaria infectivitv of and Immunity, 63,467-471. himan populations to mosquitoes in the Madang area, Papua Rutledge, L. C., Ward, R. A. & Gould, D. J. (1964). Studies on New Guinea. Parasitology, 96,251-263. the feeding response of mosquitoes to nutritive solutions in a Jeffery, G. & Eyles, D. E. (1955). Infectivity to mosquitoes of new membrane feeder. Mosquito New!, 24, 407-419. Plasmodium falcioarum as related to aametocvte densitv and Tchuinkam, T., Mulder, B., Dechermg, K., Stoffels, H., duration of ‘mfection. American Jot&al of Tiopical Me&&e Verhave, J. P., Cot, M., Carnevale, I’., Meuwissen, J. H. E. and Hygiene, 4, 781-789. T. & Robert, V. (1993). Experimental infections of Anopheles Kaslow, D. C. (1993). Transmission-blocking immunity gambiae with Plasmodium falciparum of naturally infected against malaria and other vector-borne diseases. Current gametocvte carriers in Cameroon: factors influencing the Opinion in Immunology, 5, 557-565. hfectiv& to mosquitoes. Tropical Medicine and Parasitology, Lensen, A., Vandruten, J., Bolmer, M., Vangemert, G., Eling, 44,271-276. W. & Sauerwein, R. (1996). Measurement by membrane Vanderberg, J. P. & Gwadz, R. W. (1980). The transmission by feeding of reduction in Plasmodium falciparum transmission mosquitoes of plasmodia in the laboratory. In: Malaria, induced by endemic sera. Transactions of the Royal Society of Kreier, J. I’. (editor). New York: Academic Press, pp. 154- Tropical Medicine and Hygiene, 90, 20-22. 218. Muirhead-Thomson, R. C. (1957). The malarial infectivity of Yoeli, M. (1938). Note on the experimental infection of an African village population to mosquitoes (Anopheles gam- Anopheles elutus with Plasmodium falciparum by feeding biae) American Journal of Tropical Medicine and Hygiene, 6, through a prepared animal membrane. Rivista diMaZariologia, 971-979. 17,62-66. Ponnudurai, T., Lensen, A. H. W., Gemert Van, G. J. A., Bensink, M. P. E., Bolmer, M. & Meuwissen, J. H. E. T. (1989). Infectivity of cultured Plasmodium falciparum game- Received 25 May 1999; revised 18 3;11y 1999; accepted for tocytes to mosquitoes. Parasitology,98, 165-173. publication 3 August 1999 TRANSACTIONS OF THE ROYAL SOCIETY OF TROPICAL MEDICINE AND HYGIENE (2000) 94,106-107 Amapi, Rondbnia and Roraima States). The same num- 1 Short Report 1 ber of mosquitoes known to be negative for human I I malaria parasites was also tested. The source of PZusmodium DNA was the same material Infectivity of malaria vector used for the ELISA test [triturated mosquitoes-head and thorax ground in a blocking buffer containing 0.05% mosquitoes: correlation of positivity nonidet P-40 (WIRTZ et al., 1987)], either 20 @spotted between ELBA and PCR-ELISA tests on a glass fibre membrane (GFM) prepared for PCR, using l/8 of the spot as DNA source directly into the PCR mixture as described by WARHURST et al. (1991), or Marinete M. l%voa’*, Ricardo L. D. Machado’, extracted as follows: 40 & of ELISA solution was Maria N. 0. Segura’, Giselle M. R. Vianna’, centrifuged for 10 min at 22 500 g, the pellet was lysed Adenildo S. Vasc&celds’ and Jan E. Conn3 ‘Pro: by adding 25 &of lysis buffer and incubating at 65°C for wama de Malhia. Instituto Evandro ChaPaslFAWMS. 30 min, afterwards adding potassium acetate and placing k. Almirante Bakroso, 492, 66.090-000, -Bel&m, Park, on ice for at least 60 min. The isolated DNA (obtained by Brazil; ‘Institute Oswald0 Cruz, FIOCRUZ, Av. Brasil, ethanol precipitation) was dissolved in 15 pL of TE- 436.5, 210 45-900, Rio deyaneiro, RJ, Brazil; 3Department buffer containing ribonuclease WILSON et al., 1998). of Biology, Marsh Life Sciences Building, University of The DNA was amplified as described by MACHADO et al. Vermont, Burlington, VT, 054050460, USA (1998) using primer sequence, concentrations and reac- tion conditions indicated by OLIVEIRA et al. (1995). For the identification of the human malaria parasites we used Keywords: malaria transmission, anopheline mosquitoes, in- the liquid-phase, non-isotopic hybridization ELISA fectivity, ELISA, PCR-ELISA, Brazil technique, following the protocol of OLIVEIRA et al. (1995). For negative controls we used distilled water, Studies on the infectivity of malaria vector mosquitoes male anopheline and culicine mosquitoes, and human using the enzyme-linked immunosorbent assay (ELISA) DNA. Positive controls included strain Kl of I? fulcipar- described by WIRTZ et al. (1987) have been carried out urn, and mosquitoes experimentally infected with l? worldwide for several years. SOMBOON et al. (1993) falciparum and l? vivax. reported false-positive results for the ELISA associated Our PCR results confirmed the ELISA test results for with bovine and swine blood. In order to avoid these all positive and all negative mosquitoes, and in 5 (15.6%) false-positive results it is advisable either to use only the of the positive mosquitoes (3 An. albitursis and 2 An. anterior part of the mosquito (head and thorax) which, darlingi) the PCR-ELISA technique detected other normally, is not contaminated by the ingested animal species of human Plasmodium that were not found by blood (WIRTZ et al., 1987). or to confirm the ELISA the ELISA test alone (Table). The DNA source was result by another method’such as polymerase chain obtained only by DNA extraction, which means that the reaction (PCR). GFM technique is not applicable for this tvpe of material. We have carried out the PCR-ELISA to confirm the These results indicate-&at the PCR-&ISA is more detection of human malaria parasites in mosquitoes sensitive than a simnle ELISA test which. however. still already recorded as positive by ELISA alone. Thirty remains a very goodand useful tool for testing mo&ito two such mosquitoes were tested, belonging to different infectivity. species of the genus Anopheles and collected during field trips to different areas of the Amazonia Region (Pari, Acknowledgements We thank the staff of the Malaria Entomology Laboratory at the Evandro Chagas Institute for technical assistance and *Author for correspondence; fax +55 91226 1284 or 2114417. Professor Ralph Lainson for reviewing the manuscript. This
  • 2. lXA.SMODIUM DETECTION IN MOSQUITOES 107 Table. Comparison between ELISA and PCR-ELISA results for human malaria parasites in Anopheles mosquitoes from several areas ofthe Amazon region in Brazil Species State ELISA PCR-ELISA An. (NY.) albitarsis Roraima PVIPf PvllwPm An. (Nys.) albitarsis PvlPj An. (Nys.) albitarsis Roraima filpf An. (N&.j albitarsis Roraima PvlPf An. fNvs. ) braziliensis Roraima PvlPf An. &$.j nuneztovari Roraima Pvlps An. (Nys.) darlingi Rondbnia An. (Nys.) darlingi Rondhnia g An. (Nys.) albitarsis Amap y&k An. (Nys.) albitarsis Amapi An. (Nys.) albitarsis Amapi rym An. (Nys.) albitarsis Amaph Pv An. (Nys.) albitarsis AmapL l% An. (Nys.) albitarsis Amapk Pm An. (Nys.) albitarsis Amapi Pv An. (Nys.) braziliensis Amapi Pv An. (Nys.) darlingi Amapi An. (Nys.) darlingi Amapi x An. (Nys.) aquasalis ParP An. (Nys.) aquasalis Pari An. (Nys.) aquasalis Pari An. (Nys.) darlingi Pari Pv An. (Nys.) darling’ Pari PV An. (Nys.) darlingi Pari An. (Nys.) darlingi Pari An. (Nys.) nuneztovari Pari An. (Nys.) nuneztovari Pari An. (Nys.) nuneztovari Pari An. (Nys.) nuneztovan’ Pari An. (Nys.) nuneztovari Pa& An. (Nys.) nuneztovari Pari Pm An. (Nys.) nuneztovari Pari Pm Pv, Plasmodium vivax; pf, l? falciparum; Pm, I? malariae. study received financial support from a National Institute of Warhurst, D. C., Awad-el-Karien, F. M. & Miles, M. A. (199 1). Health Grant (A140116) to J.E.C. and Evandro Chagas In- Simplified preparation of malaria blood samples for polymer- stitute/FNS. ase chain reaction. Lancet, 337, 303-304. Wilson, M. D., Ofosu-Okyere, A., Okoli, A. U., McCall, P. J. & References Snounou, G. (1998). Direct comparison of microscopy and Machado, R. L. D., Garret, D. O., Adagu, I. S., Warhurst, D. C. polymerase chain reaction for the detection of Plasmodium & I%voa, M. M. (1998). Simolified diagnosis of malaria sporozoites in salivary glands of mosquitoes. Transactions of infection: GFM/PC&E&A, a-simplified-nucleic acid am- the Royal Society of Tropical Medicine and Hvpiene, 92, plification technique by PClUELISA. Revista do Institute de 482-483. Medicina Tropical de SLio Paulo, 40, 333-334. Wirtz, R. A., Zavala, F., Charoenvit, Y., Campell, G. H., Oliveira, D. A., Holloway, B. P., Durigon, E. L., Collins, W. E. Burkot, T. R., Scheneider, I., Esser, K. M., Beaudoin, R. L. & Lal, A. A. (1995). Polymerase chain reaction and liquid- & Andr& R. G. (1987). Comparative testing of monoclonal phase, nonisotopic hybridization for species-specific and antibody against Plasmodiumfalciparum sporozoite for ELISA sensitive detection of malaria infection. American Journal of development. Bulletin of the World Health Organization, 65, Tropical Medicine and Hygiene, 52, 139- 144. 39-45. Somboon, I’., Morakote, N., Koottathep, S. & Trisanarom, U. (1993). Detection of sporozoites of Plasmodium vivax and Plasmodium falciparum in mosquitoes by ELISA: false posi- tivity associated with bovine and swine blood. Transactions of the Royal Society of Tropical Medicine and Hygiene, 87, Received ISJune 1999; revised 28 September 1999; accepted 322-324. for publication 1 October 1999