<?xml version="1.0" encoding="ISO-8859-1"?><article xmlns:mml="http://www.w3.org/1998/Math/MathML" xmlns:xlink="http://www.w3.org/1999/xlink" xmlns:xsi="http://www.w3.org/2001/XMLSchema-instance">
<front>
<journal-meta>
<journal-id>0037-8682</journal-id>
<journal-title><![CDATA[Revista da Sociedade Brasileira de Medicina Tropical]]></journal-title>
<abbrev-journal-title><![CDATA[Rev. Soc. Bras. Med. Trop.]]></abbrev-journal-title>
<issn>0037-8682</issn>
<publisher>
<publisher-name><![CDATA[Sociedade Brasileira de Medicina Tropical - SBMT]]></publisher-name>
</publisher>
</journal-meta>
<article-meta>
<article-id>S0037-86822003000400010</article-id>
<article-id pub-id-type="doi">10.1590/S0037-86822003000400010</article-id>
<title-group>
<article-title xml:lang="en"><![CDATA[Serological and parasitological study and report of the first case of human babesiosis in Colombia]]></article-title>
<article-title xml:lang="pt"><![CDATA[Estudo sorológico e parasitológico e relato do primeiro caso de babesiose humana na Colômbia]]></article-title>
</title-group>
<contrib-group>
<contrib contrib-type="author">
<name>
<surname><![CDATA[Ríos]]></surname>
<given-names><![CDATA[Leonardo]]></given-names>
</name>
<xref ref-type="aff" rid="A01"/>
</contrib>
<contrib contrib-type="author">
<name>
<surname><![CDATA[Alvarez]]></surname>
<given-names><![CDATA[Gonzalo]]></given-names>
</name>
<xref ref-type="aff" rid="A01"/>
</contrib>
<contrib contrib-type="author">
<name>
<surname><![CDATA[Blair]]></surname>
<given-names><![CDATA[Silvia]]></given-names>
</name>
<xref ref-type="aff" rid="A01"/>
</contrib>
</contrib-group>
<aff id="A01">
<institution><![CDATA[,Universidad de Antioquia Grupo Malaria ]]></institution>
<addr-line><![CDATA[Medellín ]]></addr-line>
<country>Colombia</country>
</aff>
<pub-date pub-type="pub">
<day>00</day>
<month>07</month>
<year>2003</year>
</pub-date>
<pub-date pub-type="epub">
<day>00</day>
<month>07</month>
<year>2003</year>
</pub-date>
<volume>36</volume>
<numero>4</numero>
<fpage>493</fpage>
<lpage>498</lpage>
<copyright-statement/>
<copyright-year/>
<self-uri xlink:href="http://www.scielo.br/scielo.php?script=sci_arttext&amp;pid=S0037-86822003000400010&amp;lng=en&amp;nrm=iso&amp;tlng=en"></self-uri><self-uri xlink:href="http://www.scielo.br/scielo.php?script=sci_abstract&amp;pid=S0037-86822003000400010&amp;lng=en&amp;nrm=iso&amp;tlng=en"></self-uri><self-uri xlink:href="http://www.scielo.br/scielo.php?script=sci_pdf&amp;pid=S0037-86822003000400010&amp;lng=en&amp;nrm=iso&amp;tlng=en"></self-uri><abstract abstract-type="short" xml:lang="en"><p><![CDATA[A study on the presence of Babesia in humans was performed in Puerto Berrío (Latitude 6.50deg. Longitude: -74.38deg. River: Magdalena. Area: 74.410km², Colombia-South America). Indirect immunofluorescence, thin and thick blood smears were used to study 194 individuals. Patients were grouped according to their risk-factors for Babesia infection: (group 1) individuals with fever, chills, sweating and other malaria-type symptoms; (group 2) symptomatic and asymptomatic individuals from local cattle ranches, which were enrolled in an active form, and (group 3) workers from the local slaughterhouse. Seven individuals were serologically positive for Babesia: Three individuals presented IgM antibodies against B. bovis, while one had IgG against this species; one individual had IgM against B. bigemina, another had IgG and a third both IgM and IgG against this species. Only one individual was parasitologically positive for Babesiaand serologically positive for Babesia bovis (IgM 1:64)]]></p></abstract>
<abstract abstract-type="short" xml:lang="pt"><p><![CDATA[O estudo realizado avaliou a presença de Babesia em pessoas do município de Puerto Berrío (Latitude: 6.50 graus. Longitude: -74,38 graus. Rio: Madalena. Área: 74.410km², Colômbia, América do Sul). Utilizou-se a inmunofluorescência indireta, a gota espessa e o esticado de sangue para avaliar 194 indivíduos. As pessoas foram distribuidas em grupos segundo seus fatores de risco à infecção com Babesia. Grupo1: indivíduos com febre, calafrio, sudorese e outros sintomas associados à malária; Grupo 2: indivíduos residentes em fazendas de gado e que apresentavam ou não, sintomas associados à infecção; Grupo 3: trabalhadores do abatedouro da localidade. Os resultados mostraram sete pessoas com sorologia positiva para Babesia, das quais três tinham anticorpos IgM contra B. bovis, uma apresentou anticorpos IgG contra dita espécie; um indivíduo teve anticorpos IgM contra B. bigemina, outro teve anticorpos IgG e um terceiro apresentou tanto anticorpos IgM quanto IgG contra essa espécie. Só em uma das pessoas avaliadas houve resultados parasitológicos e sorológicos positivos para Babesia bovis (IgM 1:64).]]></p></abstract>
<kwd-group>
<kwd lng="en"><![CDATA[Babesia]]></kwd>
<kwd lng="en"><![CDATA[Indirect immunofluorescence antibody test (IFA)]]></kwd>
<kwd lng="en"><![CDATA[Blood smear]]></kwd>
<kwd lng="en"><![CDATA[Malaria]]></kwd>
<kwd lng="en"><![CDATA[Human babesiosis]]></kwd>
<kwd lng="pt"><![CDATA[Babesia]]></kwd>
<kwd lng="pt"><![CDATA[Inmunoflourescência indireta]]></kwd>
<kwd lng="pt"><![CDATA[Gota espessa]]></kwd>
<kwd lng="pt"><![CDATA[Malária]]></kwd>
<kwd lng="pt"><![CDATA[Babesiose humana]]></kwd>
</kwd-group>
</article-meta>
</front><body><![CDATA[ <p align="right"><b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">ARTIGO    </font></b></p>     <p>&nbsp;</p>     <p><b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="4"><a name="top"></a>Serological    and parasitological study and report of the first case of human babesiosis in    Colombia</font></b></p>     <p>&nbsp;</p>     <p><b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="3">Estudo    sorol&oacute;gico e parasitol&oacute;gico e relato do primeiro caso de babesiose    humana na Col&ocirc;mbia</font></b></p>     <p>&nbsp;</p>     <p>&nbsp;</p>     <p><b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Leonardo    R&iacute;os; Gonzalo Alvarez; Silvia Blair</font></b></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Grupo Malaria,    Universidad de Antioquia, Medell&iacute;n-Colombia</font></p>     <p><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><a href="#back10">Correspondence</a></font></p>     ]]></body>
<body><![CDATA[<p>&nbsp;</p>     <p>&nbsp;</p> <hr size="1" noshade>     <p><b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">ABSTRACT</font></b></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">A study    on the presence of <i>Babesia</i> in humans was performed in Puerto Berr&iacute;o    (Latitude 6.50deg. Longitude: -74.38deg. River: Magdalena. Area: 74.410km<sup>2</sup>,    Colombia-South America). Indirect immunofluorescence, thin and thick blood smears    were used to study 194 individuals. Patients were grouped according to their    risk-factors for <i>Babesia</i> infection: (group 1) individuals with fever,    chills, sweating and other malaria-type symptoms; (group 2) symptomatic and    asymptomatic individuals from local cattle ranches, which were enrolled in an    active form, and (group 3) workers from the local slaughterhouse. Seven individuals    were serologically positive for <i>Babesia: </i>Three individuals presented    IgM antibodies against <i>B. bovis</i>, while one had IgG against this species;    one individual had IgM against <i>B. bigemina</i>, another had IgG and a third    both IgM and IgG against this species. Only one individual was parasitologically    positive for Babesiaand serologically positive for <i>Babesia bovis</i> (IgM    1:64)</font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2"><b>Keywords:</b>    Babesia. Indirect immunofluorescence antibody test (IFA). Blood smear. Malaria.    Human babesiosis.</font></p> <hr size="1" noshade>     <p><b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">RESUMO</font></b></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">O estudo    realizado avaliou a presen&ccedil;a de <i>Babesia</i> em pessoas do munic&iacute;pio    de Puerto Berr&iacute;o (Latitude: 6.50 graus. Longitude: -74,38 graus. Rio:    Madalena. &Aacute;rea: 74.410km<sup>2</sup>, Col&ocirc;mbia, Am&eacute;rica    do Sul). Utilizou-se a inmunofluoresc&ecirc;ncia indireta, a gota espessa e    o esticado de sangue para avaliar 194 indiv&iacute;duos. As pessoas foram distribuidas    em grupos segundo seus fatores de risco &agrave; infec&ccedil;&atilde;o com    <i>Babesia</i>. Grupo1: indiv&iacute;duos com febre, calafrio, sudorese e outros    sintomas associados &agrave; mal&aacute;ria; Grupo 2: indiv&iacute;duos residentes    em fazendas de gado e que apresentavam ou n&atilde;o, sintomas associados &agrave;    infec&ccedil;&atilde;o; Grupo 3: trabalhadores do abatedouro da localidade.    Os resultados mostraram sete pessoas com sorologia positiva para <i>Babesia</i>,    das quais tr&ecirc;s tinham anticorpos IgM contra <i>B. bovis, </i>uma apresentou    anticorpos IgG contra dita esp&eacute;cie; um indiv&iacute;duo teve anticorpos    IgM contra <i>B. bigemina</i>, outro teve anticorpos IgG e um terceiro apresentou    tanto anticorpos IgM quanto IgG contra essa esp&eacute;cie. S&oacute; em uma    das pessoas avaliadas houve resultados parasitol&oacute;gicos e sorol&oacute;gicos    positivos para <i>Babesia bovis</i> (IgM 1:64).</font></p>     <p><b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Palavras-chaves:</font></b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">    Babesia. Inmunoflouresc&ecirc;ncia indireta. Gota espessa. Mal&aacute;ria. Babesiose    humana.</font></p> <hr size="1" noshade>     <p>&nbsp;</p>     <p>&nbsp;</p>     ]]></body>
<body><![CDATA[<p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Babesiosis    is an infection produced by protozoan parasites of the genus <i>Babesia</i>,    which naturally infect mammals, birds, reptiles and amphibians. Bovine babesiosis    is a prevalent disease in the malaria endemic regions of Colombia, and is produced    by <i>Babesia bigemina</i> and <i>Babesia bovis</i><sup>4 10 21</sup>.</font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">In medical    history, the first case of human babesiosis was described in 1957 by Skrabalo    and Deanovic in Yugoslavia, in a splenectomized farm-worker who presented malaria    symptoms. The patient died and afterwards a bovine <i>Babesia</i> was confirmed    in blood smears<sup>23</sup> .</font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Human babesiosis    is a zoonosis clinically similar to malaria, it is transmitted by a tick-bite<sup>3    23</sup>. The etiological agent and laboratory diagnosis are notoriously similar    to those of human malaria<sup>1 9 17 19 20 28 29 30</sup>. This created confusion    when the first cases of human babesiosis were diagnosed and reported<sup>5 12    20 23</sup>.</font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">In Colombia,    there are areas where eco-epidemiologic risk-factors for malaria and human babesiosis    converge and overlap. Furthermore, there is an important percentage of patients    with malaria symptoms and negative blood smears for malaria. Therefore, the    main purpose of our work was to study the presence of infection by<i> Babesia    bovis</i> and <i>Babesia bigemina</i> in humans in a malaria and bovine babesiosis    endemic region using an epidemiological, parasitological and serological approach<i>.</i></font></p>     <p>&nbsp;</p>     <p><b><font face="Verdana, Arial, Helvetica, sans-serif" size="3">MATERIAL AND    METHODS</font></b></p>     <p><b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Groups    studied.</font></b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">    The study was carried out using a descriptive and transversal design. 194 inhabitants    of Puerto Berr&iacute;o (locality of Colombia) were included. Participants were    distributed in three groups according to their epidemiological risk-factors    for human babesiosis; the first group consisted of 10 male adults with symptoms    of malaria who sought treatment at the local hospital presenting fever, chills,    sweating, and headache. The second group comprised 134 male adults, with or    without malaria symptoms. All individuals of these two groups were working at    local farms and had direct contact with cattle for a year or more. All individuals    from the second group were enrolled in an active form. A third group was constituted    by 50 individuals, of which 45 were employed at the local slaughterhouse, where    they were in close contact with tissues, secretions, blood and viscera of cattle    originating from local ranches. The remaining 5 individuals were veterinarians    working in the area and in close contact with cattle during palpation, birth,    surgery, and other work. All procedures performed in this study were in accordance    with the standards of the ethical committee of Universidad de Antioquia, defining    human experimentation and based on the 1975 Helsinki Declaration, as revised    in 52<sup>nd</sup> The World Medical association General Assembly, Edinburgh,    Scotland, October 2000.</font></p>     <p><b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Babesiosis    diagnosis.</font></b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">    Parasitological diagnosis of <i>Babesia</i> was based on the finding of compatible    forms in thin blood smear. Indirect immunofluorescence antibody (IFA) was used    for serological diagnosis.</font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Diagnosis    of active babesiosis was based on positive results in both tests. The diagnosis    of previous contact with <i>Babesia,</i> was based on the presence of antibody    titers <u>&gt;</u> 1:32 for IgG<sup>15 27</sup>.</font></p>     <p><b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Parasitological    study.</font></b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">    Capillary blood was obtained in triplicate and thick and thin blood smears were    Field and Giemsa stained respectively<sup>19 26</sup>. Samples were evaluated    at the Laboratorio de Hemopar&aacute;sitos of Universidad de Antioquia. All    slides were negative for malaria. Slides with suspected babesiosis were evaluated    by experts in bovine babesiosis at CORPOICA (Corporaci&oacute;n del Instituto    Colombiano Agropecuario Santaf&eacute; de Bogot&aacute;, Colombia). The presence    of pyriform parasites in pairs or tetrads without pigment was considered as    positive for <i>Babesia.</i> Likewise, detection of circular or ovoid forms    with differentiated chromatin and cytoplasm without pigment was also considered    positive.</font></p>     ]]></body>
<body><![CDATA[<p><b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Serological    study.</font></b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">    Antigen preparation for IFA test for <i>Babesia bovis</i> and <i>Babesia bigemina</i>    was obtained from &lt;1 year old splenectomized calves, some of which were infected    with the Australian strain of <i>Babesia bovis</i> and others with the Bv V1    strain of <i>B. bigemina</i>, donated by the Epivet germ plasm (CORPOICA). At    peak parasitemia, blood was collected in test tubes with heparin, then washed    with PBS (pH 7.2-7.3), and the layer of white blood cells was removed. Hematocrit    was adjusted to 30% using 4% bovine albumin, and then parasitemia was adjusted    to 25% in the case of <i>B. bovis</i> and 35% for <i>B. bigemina</i>. Thin blood    smears were prepared and air-dried at 30<sup>o</sup>C for 30 to 45 minutes,    these were then covered with aluminum foil and stored at -20&deg;C.</font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2"><i>Conjugate    titration:</i> due to lack of a positive human serum for <i>Babesia bovis</i>    and <i>Babesia bigemina</i> a direct immunofluorescence technique was used for    the titration of the conjugate. Concentrated human red blood cells were used    as antigen. The slides were air-dried and an IgG or IgM conjugate was added.    Fluorescein was added at different dilutions from 1/20 to 1/400, optimal dilutions    were 1/200 for IgM, and 1/100 for IgG.</font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2"><i>Antibody    titration</i>: IFA test for IgG and IgM was performed following the technique    of Hijmans <i>et al</i> 1970<sup>14</sup>; serum dilution started at 1:16<sup>6    7</sup>. IgG and IgM titers were considered positive when dilution <u>&gt;</u>    1:32 showed a clear fluorescence of the antigen within red blood cells<sup>15    27</sup>. Immunofluorescence was read using the simple-blind method, in which    researchers were not aware of the patient's condition and had access only to    serum samples and to thick and thin blood films. In order to exclude cross-reactions,    IFA and ELISA tests for malaria were performed in all positive <i>Babesia bovis</i>    and <i>Babesia bigemina</i> samples.</font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2"><i>Malaria    IFA</i>: the technique of Hijmans et al 1970<sup>14</sup> was used. <i>P. falciparum</i>    schizonts (FCB-2 strain) were used as antigen. They were separated by Percoll.    Samples were read in a Leitz fluorescence microscope. Titers higher than 1:16    for IgG and 1:32 for IgM<sup>6 7</sup> were considered as positive.</font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2"><i>Malaria    ELISA</i>: crude <i>P. falciparum</i> schizont extracts was obtained after 2    minutes of sonication at 25W (Branson Sonifier Mod. 200). Protein concentration    was measured using 1000&#181;g/mL of Bradford reactive (Bio-Rad, Hercules, California).    Standardization of the technique was performed at 1.0, 2.5, 5.0, 7.5 and 10&#181;g/mL    of the reactive in carbonate buffer (concentration of 1000&#181;g/mL) on 96    wells U button plates (Nuclon, Denmark), and a concentration of 5&#181;g/mL    was chosen for performance of the ELISA test. 100&#181;g/mL of the antigen were    plated and incubated for one hour at 37&ordm;C and then overnight at 4<sup>o</sup>C.    The wells were washed with PBS and 0.05% Tween 20 (J.T.Baker, Deventer, Holland).    100&#181;g/mL of PBS/5% bovine albumin were added and incubated for one hour    at 37<sup>o</sup>C. Finally, plates were washed with PBS 0.05% Tween 20 (J.T.Baker).</font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Negative    and positive controls were evaluated as a pure sample and at dilution of 1:32    in two fold dilutions in PBS 1% bovine albumin (BSA). The antigen on 96 well    U-bottom plates was incubated for an hour at 37<sup>o</sup>C. Plates were washed    5 times with PBS 0.05% Tween 20 (JT Baker) and the anti-IgM alkaline phosphatase    conjugated was added at a dilution of 1:20000 in PBS 1% BSA. The anti-IgG alkaline    phosphatase conjugated at 1:1000 in PBS 1% BSA. Samples were incubated for an    hour at 37<sup>o</sup>C and washed 5 times with PBS 0.05% Tween 20 (JT Baker).    P-Nitrophenyl Phosphate (Sigma, St. Louis, USA) was added as substrate and incubated    for 45 minutes at room temperature. Reaction was stopped with NaOH 2N and absorption    was measured in an ELISA reader (Titertek-Uniskan II) at 405nm. The cutoff point    of reactivity was determined at titers <u>&gt;</u> 1:32.</font></p>     <p>&nbsp;</p>     <p><b><font face="Verdana, Arial, Helvetica, sans-serif" size="3">RESULTS</font></b></p>     <p><b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Parasitological    findings.</font></b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">    One individual out of 194, presented parasite forms compatible with <i>Babesia,</i>    described as follows: A pyriform parasite, resembling a trophozoite, which was    found in a 100X microscopic field, although differentiation of the chromatin    was insufficient, it was compatible with <i>Babesia.</i> An aggregate was observed    in another field, corresponding to four parasites within a red blood cell, each    one had a pear-shaped trophozoite; with adequate chromatin differentiation;    this form is known as Maltese Cross and is considered to confirm the diagnosis    of infection by <i>Babesia.</i> (<a href="#figura1">Figures 1</a> and <a href="#figura2">2</a>)</font></p>     <p align="center"><a name="figura1"></a></p>     ]]></body>
<body><![CDATA[<p align="center">&nbsp;</p>     <p align="center"><img src="/img/revistas/rsbmt/v36n4/16728f1.jpg"></p>     <p align="center"><a name="figura2"></a></p>     <p align="center">&nbsp;</p>     <p align="center">&nbsp;</p>     <p align="center"><img src="/img/revistas/rsbmt/v36n4/16728f2.jpg"></p>     <p align="center">&nbsp;</p>     <p><b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Serological    findings.</font></b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">    Seven individuals (3.6%) had positive titers, two for IgG, four for IgM and    one for both IgG and IgM. Titers varied between 1:32 and 1:128 (<a href="#tabela1">Table    1</a>). The most relevant features of these patients are shown in <a href="#tabela1">Tables    1</a> and <a href="/img/revistas/rsbmt/v36n4/16728t2.gif">2</a>.</font></p>     <p align="center"><a name="tabela1"></a></p>     <p align="center">&nbsp;</p>     ]]></body>
<body><![CDATA[<p align="center"><img src="/img/revistas/rsbmt/v36n4/16728t1.gif"></p>     <p align="center">&nbsp;</p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">The IFA    test for malaria was positive in patient number 4, who was also positive for    <i>Babesia bovis</i> IgG (1:64) The other six individuals seropositive for <i>Babesia    bovis</i> and/or <i>B. bigemina</i> were negative for malaria antibodies. In    the ELISA test, all tested individuals were negative for malaria IgM (<a href="#tabela3">Table    3</a>).</font></p>     <p align="center"><a name="tabela3"></a></p>     <p align="center">&nbsp;</p>     <p align="center"><img src="/img/revistas/rsbmt/v36n4/16728t3.gif"></p>     <p align="center">&nbsp;</p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2"><i>Clinical    and epidemiological description in patient number 1 with</i> Babesia bovis<b><i>:</i></b>    the patient was a 37-year-old male, who presented at the local hospital with    intermittent fever (without periodicity), chills, sweating, weakness and bone    ache; a thick smear was negative for malaria. The patient worked for 20 years    as a chainsaw operator. At the time of consultation, he was working at a cattle    ranch located in the rural area. He reported remembering tick bytes on three    occasions, and he did not have history of malaria (<a href="/img/revistas/rsbmt/v36n4/16728t2.gif">Table    2</a>). His serological study showed antibodies for <i>Babesia bovis</i> IgM    (1:64), negative anti-malarial IgM antibodies by ELISA and negative by IFA (<a href="#tabela3">Table    3</a>).</font></p>     <p>&nbsp;</p>     <p><b><font face="Verdana, Arial, Helvetica, sans-serif" size="3">DISCUSSION</font></b></p>     ]]></body>
<body><![CDATA[<p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">We report    the first case of human babesiosis in Colombia which was parasitologically confirmed    by positive blood films for <i>Babesia</i> and antibody titers positive for    <i>Babesia bovis</i> (IgM 1:64)<i>,</i> in a patient who presented intermittent    fever, chills and sweating lasting several days. These findings have been reported    in the medical literature as characteristic of the acute phase of the disease,    as confirmed by positive IgM titers<sup>15 27</sup>.</font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Six other    individuals were positive by serology for <i>Babesia,</i> three for <i>Babesia    bovis</i> and three for <i>Babesia bigemina.</i> Two of those patients (patients    number 4 and number 7) were IgG positive and asymptomatic, which can be explained    by a possible prior infection; two were IgM positive and symptomatic (patients    number 3 and 5) and two patients had positive IgM titers and absence of symptoms    (patients number 2 and 6), which can be explained by a subacute phase of the    infection (<a href="#tabela1">Table 1</a>).</font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Coexistence    of positive anti-<i>Babesi</i>a antibodies and positive anti-<i>Plasmodium</i>    antibodies suggest the possibility of co-infection by both parasites<i>.</i>    This has been reported previously in humans in the case of <i>Babesia microti</i>    and <i>Borrelia burdogferi</i><sup>2 16 20</sup>. Similarly, cross-reactivity    by IFA among parasites of the phylum Apicomplexa, including <i>Babesia bovis</i>    and <i>Plasmodium falciparum</i> has been reported<sup>8 18 24</sup>. Patients    number 4 could have either a cross reactivity or co-existing antibody IgG for    both <i>Babesia</i> and <i>Plasmodium</i> parasites.</font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Suarez et    al conducted the first study on seroprevalence of human <i>Babesia bovis</i>    and <i>Babesia bigemina</i> in the province of Ciego de Avila, Cuba. Suarez    used the IFA test in 781 samples. Titers for IgG positive antibodies were established    as (1:64), 7% positivity was found in workers of cattle ranches and 3.9% in    blood donors coming from the same area, compared to 3.6% seroprevalence for    antibabesia antibodies in the studied population comprising cattle ranch workers<sup>27</sup>.</font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Working    in close contact with organic fluids and viscera of possibly infected animals,    can not be defined as a direct risk-factor for infection by <i>Babesia bovis</i>    and/or <i>Babesia bigemina,</i> since in this study no positive individuals    were found in group 3.</font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Worldwide,    the IFA test is the most used technique, to determine evidence of contact between    humans and <i>Babesia</i><sup>2 12 15 24 25</sup>. It is necessary, however,    to use molecular techniques to identify the species, since it is known that    the morphological features alone do not offer accurate criteria and that the    changes in the parasite's morphology are variable in the infected host<sup>11    13 22 23</sup>.</font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Human babesiosis    is present in Puerto Berr&iacute;o. The first case of human babesiosis in Colombia    is presented here and confirmed by parasitological and serological studies.    Furthermore, we have reported the first six cases of human babesiosis detected    by the IFA test.</font></p>     <p>&nbsp;</p>     <p><b><font face="Verdana, Arial, Helvetica, sans-serif" size="3">ACKNOWLEDGEMENTS</font></b></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">These study    was supported by Direcci&oacute;n Seccional de Salud de Antioquia (DSSA) and    the Universidad de Antioquia. We are grateful to the Committee of ranchers of    Puerto Berr&iacute;o, the Colombian Institute for farming and animal husbandry    (Instituto Colombiano agropecuario ICA, CORPOICA) and inhabitants of Puerto    Berr&iacute;o. Special thanks to Mrs. Adriana Pab&oacute;n and her family, to    Claudia Milena Brito, Efra&iacute;n Benavides and Juan M. Castillo.</font></p>     ]]></body>
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Parasitology Today 4:214-218, 1988.</font>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;[&#160;<a href="javascript:void(0);" onclick="javascript: window.open('/scielo.php?script=sci_nlinks&ref=000104&pid=S0037-8682200300040001000030&lng=','','width=640,height=500,resizable=yes,scrollbars=1,menubar=yes,');">Links</a>&#160;]<!-- end-ref --><p>&nbsp;</p>     <p>&nbsp;</p>     <p><b><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><a name="back10"></a><a href="#top"><img src="/img/revistas/rsbmt/v36n4/seta.gif" border="0"></a>Correspondence    to    <br>   </font></b><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Dra.    Silvia Blair    <br>   T. Kra 51-D # 62-29, AA: 1226, Medell&iacute;n Colombia    <br>   </font><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Telephone:    (574) 510-6058, Fax (574) 263-3509    <br>   </font><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">e-mail:    <a href="mailto:sblair@catios.udea.edu.co">sblair@catios.udea.edu.co</a></font></p>     <p><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Recebido    para publica&ccedil;&atilde;o em 10/9/2003    ]]></body>
<body><![CDATA[<br>   </font><font face="Verdana, Arial, Helvetica-Normal, sans-serif" size="2">Aceito    em 12/6/2003</font></p>      ]]></body><back>
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