<?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>1024-0675</journal-id>
<journal-title><![CDATA[Revista de la Sociedad Boliviana de Pediatría]]></journal-title>
<abbrev-journal-title><![CDATA[Rev. bol. ped.]]></abbrev-journal-title>
<issn>1024-0675</issn>
<publisher>
<publisher-name><![CDATA[Sociedad Boliviana de Pediatría]]></publisher-name>
</publisher>
</journal-meta>
<article-meta>
<article-id>S1024-06752004000300002</article-id>
<title-group>
<article-title xml:lang="es"><![CDATA[Caracterización geno-fenotípica de aislados de Escherichia coli AEEC de pacientes pediátricos con procesos diarreicos infecciosos en la ciudad de La Paz: implicancias para el diagnóstico y epidemiología de las enfermedades diarreicas agudas]]></article-title>
<article-title xml:lang="en"><![CDATA[Geno-Phenotypic characterization of aeec Escherichia coli isolated from children with infectious diarrheal diseases in La Paz: relevancy for the diagnosis and epidemiology of acute diarrheal diseases]]></article-title>
</title-group>
<contrib-group>
<contrib contrib-type="author">
<name>
<surname><![CDATA[Sánchez]]></surname>
<given-names><![CDATA[Samanta]]></given-names>
</name>
<xref ref-type="aff" rid="A01"/>
</contrib>
<contrib contrib-type="author">
<name>
<surname><![CDATA[Ropmecin]]></surname>
<given-names><![CDATA[Paola]]></given-names>
</name>
<xref ref-type="aff" rid="A01"/>
</contrib>
<contrib contrib-type="author">
<name>
<surname><![CDATA[Guachalla]]></surname>
<given-names><![CDATA[Luis Miguel]]></given-names>
</name>
<xref ref-type="aff" rid="A01"/>
</contrib>
<contrib contrib-type="author">
<name>
<surname><![CDATA[Iñiguez]]></surname>
<given-names><![CDATA[Volga]]></given-names>
</name>
<xref ref-type="aff" rid="A01"/>
</contrib>
</contrib-group>
<aff id="A01">
<institution><![CDATA[,Universidad Mayor de San Andrés Facultad de Ciencias Puras y Naturales Carrera de Biología]]></institution>
<addr-line><![CDATA[ ]]></addr-line>
</aff>
<pub-date pub-type="pub">
<day>00</day>
<month>08</month>
<year>2004</year>
</pub-date>
<pub-date pub-type="epub">
<day>00</day>
<month>08</month>
<year>2004</year>
</pub-date>
<volume>43</volume>
<numero>3</numero>
<fpage>132</fpage>
<lpage>143</lpage>
<copyright-statement/>
<copyright-year/>
<self-uri xlink:href="http://www.scielo.org.bo/scielo.php?script=sci_arttext&amp;pid=S1024-06752004000300002&amp;lng=en&amp;nrm=iso"></self-uri><self-uri xlink:href="http://www.scielo.org.bo/scielo.php?script=sci_abstract&amp;pid=S1024-06752004000300002&amp;lng=en&amp;nrm=iso"></self-uri><self-uri xlink:href="http://www.scielo.org.bo/scielo.php?script=sci_pdf&amp;pid=S1024-06752004000300002&amp;lng=en&amp;nrm=iso"></self-uri><abstract abstract-type="short" xml:lang="es"><p><![CDATA[En el presente estudio se realizó la caracterización de Escherichia coli Enteropatogénica (EPEC) y Escherichia coli Enterohemorrágica (EHEC), dos categorías patogénicas de E. Coli, causantes de la lesión de adherencia y esfacelación (EAEE), en muestras de heces diarreicas de niños menores a 5 años. El perfil patogénico de EAEE se realizo mediante el análisis por PCR, de los genes intimina (eae), bundlina (bfpA) y toxinas siga (stx1 y stx2). Estas pruebas, se complementaron con ensayos fenotípicos de la resistencia a antibióticos, fermentación de sorbitol y producción de b-D-glucoronidasa. La prevalencia de EAEE fue del 7% con preponderancia de las cepas EPEC (95%) sobre EHEC. Se encontró una mayor proporción (83%) de cepas EPEC atípicas que típicas. Un alto porcentaje de los aislados de EPEC es resistente a más de 5 antibióticos analizados. La frecuencia de multiresistencia a bloques de 5 y 2 antibióticos sugiere que la resistencia es transmisible por vía horizontal. La correlación entre la pertenencia a un serogrupo particular de EPEC y las características genotípicas, mostró heterogeneidad en el perfil de patogenicidad tanto entre un mismo como entre diferentes serogrupos, demostrando que el diagnostico de DEC mediante serotipificación no es útil en nuestro medio. Los aislados de EHEC, se caracterizan por presentar una marcada susceptibilidad a los antibióticos. Se reporta la presencia de los serogrupos O157 y O6. Este estudio, constituye el primer reporte en nuestro medio sobre la determinación y caracterización geno-fenotípica de EPEC y EHEC por métodos moleculares. En conjunto, los datos obtenidos tienen relevancia para el diagnostico, tratamiento y estudio de la epidemiología de AEEC en las EDA en Bolivia.]]></p></abstract>
<abstract abstract-type="short" xml:lang="en"><p><![CDATA[In this study, enteropathogenic (EPEC) and enterohemorrhagic (EHEC) E. Coli, two E. Coli categories causing attaching and effacing lesions, were isolated and characterized from children with diarrhea less than 5 years of age. The AEEC pathogenic profile was analyzed by PCR for the presence of the intimin (eae), bundle-forming pilus (bfpA) and Shiga toxin (stx, stx2) genes. Phenotypic analysis for the presence of antibiotic multi-resistance, sorbitol fermentation and B-D glucoronidase were also performed. AEEC prevalence was 7%. EPEC accounted for 95% of the isolates of which 83% were atypical. A high percentage of EPEC isolates is resistant to more than 5 antibiotics. The multi-resistance frequency to 5 and 2 antibiotics suggest antibiotic resistance transmission by lateral transfer. The lack of correlations between EPEC serogroups and genotypic strain profile demonstrates that serological DEC diagnosis is not useful for local isolates. EHEC isolates were remarkably susceptible to most of the antibiotics tested. The isolation of 0157 and 06 serogroups is reported. This is the first report of EPEC and EHEC molecular strain characterization. The results described are relevant for EAEE diagnosis, treatment and epidemiology of diarrheal diseases in Bolivia.]]></p></abstract>
<kwd-group>
<kwd lng="es"><![CDATA[Adherencia y Esfacelación (EA)]]></kwd>
<kwd lng="es"><![CDATA[Bundlina (BFP)]]></kwd>
<kwd lng="es"><![CDATA[Intimina (EAE)]]></kwd>
<kwd lng="es"><![CDATA[Toxina Shiga (STX)]]></kwd>
<kwd lng="en"><![CDATA[Attaching and Effacing (EA)]]></kwd>
<kwd lng="en"><![CDATA[Bundlina (BFP)]]></kwd>
<kwd lng="en"><![CDATA[Intimin (EAE)]]></kwd>
<kwd lng="en"><![CDATA[Shiga toxin (STX)]]></kwd>
</kwd-group>
</article-meta>
</front><body><![CDATA[ <p align="right"><font size="2"><b><font face="Verdana">ARTICULO ORIGINAL</font></b></font></p>     <p align="justify"><font size="4" face="Verdana"><b>Caracterizaci&oacute;n geno-fenot&iacute;pica de aislados de <i>Escherichia coli </i>AEEC de pacientes pedi&aacute;tricos con procesos diarreicos infecciosos en la ciudad de La Paz: implicancias para el diagn&oacute;stico y epidemiolog&iacute;a de las enfermedades diarreicas agudas</b></font></p>     <p align="justify"><font size="3" face="Verdana, Arial, Helvetica, sans-serif"><b><em>Geno-Phenotypic characterization of aeec Escherichia coli isolated from children with infectious diarrheal diseases in La Paz: relevancy for the diagnosis and epidemiology of acute diarrheal diseases</em></b></font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><strong>Dr: Samanta S&aacute;nchez*, Paola Ropmecin**, Luis Miguel Guachalla*** y Volga I&ntilde;iguez****</strong></font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="1"><em>Instituto de Biolog&iacute;a Molecular y Biotecnolog&iacute;a, Unidad de Biolog&iacute;a Molecular de Enteropat&oacute;genos, Carrera de Biolog&iacute;a. Facultad de Ciencias Puras y Naturales. Universidad Mayor de San Andr&eacute;s</em>    <br>   * Lic. Bioqu&iacute;mica     <br>   ** Lic. Biolog&iacute;a     <br>   *** Lic. Bioqu&iacute;mica     <br>   **** Ph D. Biolog&iacute;a     <br>   * Autor correspondiente. Direcci&oacute;n: Instituto de Biolog&iacute;a Molecular y Biotecnolog&iacute;a, Campus Universitario de Cota-Cota. La Paz, Bolivia. E. mail: <a href="mailto:volgavir@hotmail.com">volgavir@hotmail.com</a>     ]]></body>
<body><![CDATA[<br>       <br> <strong>Art&iacute;culo recibido 1/10/2004 y fue aprobado para publicaci&oacute;n 8/12/2004.</strong></font> </p> <hr> <font size="2" face="Verdana, Arial, Helvetica, sans-serif"><strong>Resumen</strong></font> <font face="Verdana, Arial, Helvetica, sans-serif" size="2">En el presente estudio se realiz&oacute; la caracterizaci&oacute;n de <i>Escherichia coli </i>Enteropatog&eacute;nica (EPEC) y <i>Escherichia coli </i>Enterohemorr&aacute;gica (EHEC), dos categor&iacute;as patog&eacute;nicas de <i>E. Coli</i>, causantes de la lesi&oacute;n de adherencia y esfacelaci&oacute;n (EAEE), en muestras de heces diarreicas de ni&ntilde;os menores a 5 a&ntilde;os. El perfil patog&eacute;nico de EAEE se realizo mediante el an&aacute;lisis por PCR, de los genes intimina (<i>eae</i>), bundlina (<i>bfpA</i>) y toxinas siga (<i>stx1</i> y <i>stx2</i>). Estas pruebas, se complementaron con ensayos fenot&iacute;picos de la resistencia a antibi&oacute;ticos, fermentaci&oacute;n de sorbitol y producci&oacute;n de <i>b-D-glucoronidasa</i>. La prevalencia de EAEE fue del 7% con preponderancia de las cepas EPEC (95%) sobre EHEC. Se encontr&oacute; una mayor proporci&oacute;n (83%) de cepas EPEC at&iacute;picas que t&iacute;picas. Un alto porcentaje de los aislados de EPEC es resistente a m&aacute;s de 5 antibi&oacute;ticos analizados. La frecuencia de multiresistencia a bloques de 5 y 2 antibi&oacute;ticos sugiere que la resistencia es transmisible por v&iacute;a horizontal. La correlaci&oacute;n entre la pertenencia a un serogrupo particular de EPEC y las caracter&iacute;sticas genot&iacute;picas, mostr&oacute; heterogeneidad en el perfil de patogenicidad tanto entre un mismo como entre diferentes serogrupos, demostrando que el diagnostico de DEC mediante serotipificaci&oacute;n no es &uacute;til en nuestro medio. Los aislados de EHEC, se caracterizan por presentar una marcada susceptibilidad a los antibi&oacute;ticos. Se reporta la presencia de los serogrupos O157 y O6. Este estudio, constituye el primer reporte en nuestro medio sobre la determinaci&oacute;n y caracterizaci&oacute;n geno-fenot&iacute;pica de EPEC y EHEC por m&eacute;todos moleculares. En conjunto, los datos obtenidos tienen relevancia para el diagnostico, tratamiento y estudio de la epidemiolog&iacute;a de AEEC en las EDA en Bolivia. </font>     <p align="justify"><font size="2" face="Verdana"><b>Palabras Claves: </b></font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Rev Soc Bol Ped 2004; 43 (3): 132-43: Adherencia y Esfacelaci&oacute;n (EA), Bundlina (BFP), Intimina (EAE), Toxina Shiga (<i>STX</i>).</font></p> <hr> <font size="2" face="Verdana"><b>Abstract </b></font>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">In this study, enteropathogenic (EPEC) and enterohemorrhagic (EHEC) <i>E. Coli</i>, two <i>E. Coli</i> categories causing attaching and effacing lesions, were isolated and characterized from children with diarrhea less than 5 years of age. The AEEC pathogenic profile was analyzed by PCR for the presence of the intimin (<i>eae</i>), bundle-forming pilus (<i>bfpA</i>) and Shiga toxin (<i>stx</i>, <i>stx2</i>) genes. Phenotypic analysis for the presence of antibiotic multi-resistance, sorbitol fermentation and B-D glucoronidase were also performed. AEEC prevalence was 7%. EPEC accounted for 95% of the isolates of which 83% were atypical. A high percentage of EPEC isolates is resistant to more than 5 antibiotics. The multi-resistance frequency to 5 and 2 antibiotics suggest antibiotic resistance transmission by lateral transfer. The lack of correlations between EPEC serogroups and genotypic strain profile demonstrates that serological DEC diagnosis is not useful for local isolates. EHEC isolates were remarkably susceptible to most of the antibiotics tested. The isolation of 0157 and 06 serogroups is reported. This is the first report of EPEC and EHEC molecular strain characterization. The results described are relevant for EAEE diagnosis, treatment and epidemiology of diarrheal diseases in Bolivia. </font></p>     <p align="justify"><font size="2" face="Verdana"><b>Key words: </b></font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Rev Soc Bol Ped 2004; 43 (3): 132-43: Attaching and Effacing (EA), Bundlina (BFP), Intimin (EAE), Shiga toxin (<i>STX</i>). </font></p> <hr> <font size="3" face="Verdana"><b>    <br> Introducci&oacute;n </b></font>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">A nivel mundial, las Enfermedades Diarreicas Agudas (EDAs), son un problema importante de salud de la poblaci&oacute;n infantil, principalmente en los pa&iacute;ses en desarrollo donde se producen anualmente entre 4,6 a 6 millones de muertes constituyendo la segunda causa global de mortalidad infantil. Estas estad&iacute;sticas se reflejan en que se produce un promedio de 3 episodios de diarrea por a&ntilde;o en ni&ntilde;os menores a 5 a&ntilde;os y una tasa global de mortalidad promedio de m&aacute;s de 10.000 ni&ntilde;os por d&iacute;a<sup>1-3</sup>. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">En Bolivia, las EDA constituyen una de las principales causas de mortalidad entre ni&ntilde;os menores de 5 a&ntilde;os de edad, produci&eacute;ndose aproximadamente quince mil muertes por a&ntilde;o<sup>4</sup>. </font></p>     ]]></body>
<body><![CDATA[<p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">La diversidad de enteropat&oacute;genos asociada a las EDA y la falta de acceso a tecnolog&iacute;as sensibles de diagnostico, determinan que, similar a otros pa&iacute;ses en desarrollo, se desconozca la etiolog&iacute;a de una gran parte de los episodios diarreicos infecciosos, los cuales se tratan, por lo general sin conocimiento de la patolog&iacute;a subyacente. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Es as&iacute; que la epidemiolog&iacute;a de los principales pat&oacute;genos asociados a la gastroenteritis infantil y los mecanismos de virulencia, son poco conocidos en nuestro medio. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">En los &uacute;ltimos a&ntilde;os, un n&uacute;mero creciente de pat&oacute;genos bacterianos y virales han sido asociados a las EDA gracias a la progresiva incorporaci&oacute;n de nuevas tecnolog&iacute;as de detecci&oacute;n, que han permitido establecer la relaci&oacute;n causal entre los microorganismos y las EDA, mediante la identificaci&oacute;n y caracterizaci&oacute;n de genes de patogenicidad y virulencia. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Entre las bacterias asociadas a las EDA, <i>Escherichia coli </i>Diarreog&eacute;nica (DEC) esta com&uacute;nmente asociada a formas end&eacute;micas e incluye al menos 6 categor&iacute;as patog&eacute;nicas bien definidas, las cuales comprenden a <i>E. Coli</i> enteropatog&eacute;nica (EPEC), <i>E. Coli</i> enterohemorr&aacute;gica (EHEC), <i>E. Coli</i> enterotoxig&eacute;nica (ETEC), <i>E. Coli</i> enteroagregativa (EAEC), <i>E. Coli</i> enteroinvasiva (EIEC) y <i>E. Coli</i> adherente difusa (DAEC). Estos "patotipos" se distinguen de los simbiontes de la flora normal, por la presencia de factores de virulencia adquiridos principalmente por transferencia horizontal a partir de pl&aacute;smidos, fagos y genomas de otras bacterias"<sup>5</sup>. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">EPEC y EHEC son dos categor&iacute;as patog&eacute;nicas de <i>E. Coli</i> que causan la lesi&oacute;n del tipo de "adherencia y esfacelaci&oacute;n" (A/E) en las c&eacute;lulas intestinales. Esta lesi&oacute;n se caracteriza por la destrucci&oacute;n de las microvellosidades de la membrana, la adherencia intima de la bacteria al epitelio intestinal, el reordenamiento del citoesqueleto de la c&eacute;lula hu&eacute;sped, la formaci&oacute;n de un pedestal y la iniciaci&oacute;n de var&iacute;as se&ntilde;ales de transducci&oacute;n generadoras de la secreci&oacute;n intestinal. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">EPEC es uno de los pat&oacute;genos bacterianos m&aacute;s importantes asociado a la gastroenteritis infecciosa y diarrea espor&aacute;dica en ni&ntilde;os menores a dos a&ntilde;os<sup>6-12</sup>. Adem&aacute;s de producir la lesi&oacute;n A/E, EPEC presenta generalmente un pl&aacute;smido denominado EAF (factor de adherencia de EPEC) relacionado tanto a la adherencia entre bacterias, as&iacute; como a las c&eacute;lulas epiteliales del intestino<sup>13</sup>. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">EHEC, por su parte es un pat&oacute;geno emergente de las &uacute;ltimas d&eacute;cadas, que se caracteriza por producir las citotoxinas Shiga causando diarrea no sanguinolenta, colitis hemorr&aacute;gica y s&iacute;ndrome hemol&iacute;tico ur&eacute;mico (SHU)<sup>14-15</sup>. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Con el prop&oacute;sito de contribuir al conocimiento de la etiolog&iacute;a bacteriana de las EDA, en el presente trabajo, se utilizo un conjunto de ensayos genot&iacute;picos y fenot&iacute;picos para identificar, caracterizar y comparar a EPEC y EHEC, en muestras de heces fecales de pacientes pedi&aacute;tricos con Procesos Diarreicos Infecciosos (PDI). Entre las caracter&iacute;sticas analizadas se incluyen a genes de patogenicidad, patrones de resistencia a antibi&oacute;ticos y marcadores bioqu&iacute;micos. Asimismo, se analizo la validez de la asignaci&oacute;n de EPEC en base a la pertenencia a sus serogrupos caracter&iacute;sticos. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Estos datos, constituyen el primer reporte en Bolivia sobre el aislamiento y an&aacute;lisis de las categor&iacute;as de DEC causantes de la lesi&oacute;n A/E (AEEC) a partir de heces diarreicas de ni&ntilde;os menores a 5 a&ntilde;os. Los resultados obtenidos remarcan una mayor prevalenc&iacute;a de EPEC at&iacute;pica sobre EHEC, heterogeneidad geno-fenot&iacute;pica de cepas EPEC y EHEC, alta proporci&oacute;n de cepas multiresistentes a 7 antibi&oacute;ticos entre aislados de EPEC, en fuerte contraste a EHEC y la discordancia en la clasificaci&oacute;n de EPEC mediante serogrupos con relaci&oacute;n al perfil patog&eacute;nico. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">La diversidad genot&iacute;pica encontrada entre las cepas AEEC, circulantes en los PDI tiene relevancia cl&iacute;nica y epidemiol&oacute;gica para el estudio del rol de EPEC y EHEC en las EDA en nuestro medio. </font></p>     ]]></body>
<body><![CDATA[<p align="justify"><font size="3" face="Verdana"><b>    <br> Material y m&eacute;todos </b></font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>Cepas control y cepas cl&iacute;nicas.</b> Se utilizaron cepas de referencia de <i>E. Coli</i> Diarreog&eacute;nicas (DEC) provenientes del Instituto de Gen&eacute;tica Evolutiva y Molecular, de la Universidad Estatal de Pennsylvania, Estados Unidos de Norte Am&eacute;rica. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Asimismo, se analizaron 31 cepas cl&iacute;nicas de <i>E. Coli</i>, que presentan serogrupo definido, las cuales fueron aisladas en La Paz, Bolivia en 1993 a partir de muestras fecales de ni&ntilde;os con PDI. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>Poblaci&oacute;n de estudio.</b> En el periodo de Febrero del 2001 a Junio del 2002, se recolectaron 882 muestras de heces fecales provenientes de ni&ntilde;os menores a 5 a&ntilde;os de edad, con PDI en tres centros de salud de la ciudad de La Paz (Hospital Materno Infantil, Hospital Militar y Hospital del Ni&ntilde;o Ovidio Aliaga). </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>Aislamiento y caracterizaci&oacute;n fenot&iacute;pica de <i>E. Coli</i>.</b> Las muestras fecales fueron sembradas e incubadas en Agar MacConkey, durante 18 horas a 37&deg; C. Las colonias fermentadoras de lactosa y con morfolog&iacute;a caracter&iacute;stica de <i>E. Coli</i>, fueron luego analizadas por su capacidad de fermentaci&oacute;n de sorbitol (FS) y producci&oacute;n de <i>b-D-glucoronidasa</i> (MUG). </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>Resistencia a antibi&oacute;ticos.</b> Se consideraron para el an&aacute;lisis a los siguientes antibi&oacute;ticos: ampicilina, eritromicina, estrepto-micina, sulfatrimetoprim, &aacute;cido nalidixico, cloranfenicol, tetra-ciclina y gentamicina. La sensibilidad a los ocho antibi&oacute;ticos se evalu&oacute; mediante el m&eacute;todo de difusi&oacute;n de disco acorde a los lineamientos del Comit&eacute; de Control de Laboratorios Cl&iacute;nicos<sup>16</sup>. </font></p>     <p align="justify"><font size="3" face="Verdana"><b>    <br> Caracterizaci&oacute;n genot&iacute;pica </b></font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>Reacci&oacute;n en Cadena de la Polimerasa (PCR).</b> La presencia de los genes <i>eae</i> (regi&oacute;n variable y constante), <i>bfp</i>, <i>stx1</i>, <i>stx2</i> y <i>mdh</i> correspondientes a las prote&iacute;nas Intimina, Bundlina, Shiga toxina 1, Shiga toxina 2 y Malato-deshidrogenasa respectivamente, se realizo en los aislados de <i>E. Coli</i>, mediante el uso de cebadores espec&iacute;ficos (<a href="#c1">Cuadro # 1</a>).</font></p>     ]]></body>
<body><![CDATA[<p align="center"><font size="2" face="Verdana"><b>   <a name="c1"></a><img src="/img/revistas/rbp/v43n3/cuadro_a02_1.gif" width="484" height="431"></b></font></p>     <p align="justify"></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Los productos de PCR se visualizaron por electroforesis en geles de agarosa al 1% con bromuro de etidio, en un transiluminador de luz UV. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>An&aacute;lisis por PCR-RFLP.</b> Los fragmentos amplificados del gen <i>eae</i> y <i>bfp</i> se incubaron con las enzimas de restricci&oacute;n Dra I y Msp I respectivamente, por dos horas a 37&deg;C. Posteriormente, los productos de digesti&oacute;n fueron separados por electroforesis en geles de agarosa (NuSieve) al 4% con bromuro de etidio y visualizados con un transiluminador de luz UV. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>Procesamiento de datos.</b> Los datos fueron analizados por el test exacto de Fisher. La asociaci&oacute;n se considero estad&iacute;sticamente significativa, con un valor de p&lt; 0.05.</font></p>     <p align="justify"><font size="3" face="Verdana"><b>    <br> Resultados </b></font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>Diferenciaci&oacute;n molecular de EPEC y EHEC mediante PCR</b>. En la <a href="#f1">Figura # 1</a>, se observan los productos amplificados mediante PCR, de regiones de los genes <i>eaeA</i>, <i>stx1</i>, mdh, <i>bfpA</i> y <i>stx2</i>, presentes en cepas de referencia. Los ensayos fueron espec&iacute;ficos detectando todos los genes de inter&eacute;s en el 100% de las cepas control de genotipo y fenotipo m&uacute;ltiple (datos no mostrados). El an&aacute;lisis de estos genes en las muestras cl&iacute;nicas permiti&oacute; la identificaci&oacute;n de cepas EPEC y EHEC.</font></p>     <p align="center"><font size="2" face="Verdana"><b><a name="f1"></a><img src="/img/revistas/rbp/v43n3/figura_a02_1.jpg" width="508" height="503"></b></font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">La presencia del gen mdh permiti&oacute; confirmar que las cepas eran de la especie <i>E. Coli</i>.</font><font size="2" face="Verdana"><b>    ]]></body>
<body><![CDATA[<br>       <br> </b></font><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>EPEC: Identificaci&oacute;n y caracterizaci&oacute;n en muestras cl&iacute;nicas.</b> Del total de 882 muestras cl&iacute;nicas, 58 aislados de <i>E. Coli</i> presentaron genotipo <i>eae</i>+ <i>stx</i>- siendo clasificados como EPEC. Esto represento una prevalenc&iacute;a de infecci&oacute;n por EPEC de 6% en el periodo de estudio (<a href="#c2">Cuadro # 2</a>). </font></p>     <p align="center"><font size="2" face="Verdana, Arial, Helvetica, sans-serif"><a name="c2"></a><img src="/img/revistas/rbp/v43n3/cuadro_a02_2.gif" width="472" height="1132"></font></p>     <p align="justify"></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">El producto de amplificaci&oacute;n del gen <i>eaeA</i> (863pb), fue verificado en el total de cepas <i>eaeA</i> + mediante PCR-RFLP. En el 96% de las mismas, se obtuvo el fragmento esperado de 750pb, correspondiente al extremo 3' de la regi&oacute;n amplificada (datos no mostrados). </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">El gen <i>bfpA</i>, codificante de la bundlina o subunidad estructural del pilus BFP fue detectado en el 17% de las cepas <i>eae</i>+ aisladas en el periodo 2001-2002 representando consiguientemente un total de 10 cepas EPEC t&iacute;picas y 48 at&iacute;picas (<a href="#c2">Cuadro # 2</a>). </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">El an&aacute;lisis de las cepas cl&iacute;nicas de <i>E. Coli</i> aisladas en el periodo 1993, mostr&oacute; que 15 de 31 cepas presentaron el gen <i>eaeA</i> (<a href="#c3">Cuadro # 3</a>). En este grupo de muestras, se observ&oacute; un 47% de cepas EPEC t&iacute;picas. </font></p>     <p align="center"><font size="2" face="Verdana, Arial, Helvetica, sans-serif"><a name="c3"></a><img src="/img/revistas/rbp/v43n3/cuadro_a02_3.gif" width="496" height="848"></font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>EPEC: Caracterizaci&oacute;n gen&eacute;tica de las intiminas a, b y g.</b> La identificaci&oacute;n gen&eacute;tica de tres tipos de intimina (a, b y g), se realiz&oacute; mediante PCR de la regi&oacute;n variable del gen <i>eaeA</i> en 72 cepas <i>eae</i>+ que incluyeron a: 15 aislados de 1993 y 57 del per&iacute;odo 2001-2002 (<a href="#f2">Figura # 2</a>). </font></p>     <p align="center"><a name="f2"></a><img src="/img/revistas/rbp/v43n3/figura_a02_2.jpg" width="484" height="469"></p>     ]]></body>
<body><![CDATA[<p align="justify"><font size="2" face="Verdana, Arial, Helvetica, sans-serif">De las cepas analizadas entre el 2001-2002, 3% corresponden al gen de la intimina a, 9% al de la intimina <em>b</em> y 16% al de la intimina <em>g</em>. En el 72% restante, no se observaron productos de amplificaci&oacute;n; por lo cual, estas cepas fueron clasificadas como no tipeables (<a href="#c2">Cuadro # 2</a>). </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Se observa que la proporci&oacute;n de cepas no tipeables fue menor entre los aislados de 1993 (20%) con respecto al periodo 2001-2002. El porcentaje de cepas de intimina tipo g fue mayor que el de las otras variantes de intimina identificadas. No se observaron cepas con intimina a en 1993 (<a href="#c3">Cuadro # 3</a> y <a href="#f3">figura #3</a>). </font></p>     <p align="center"><font size="2" face="Verdana, Arial, Helvetica, sans-serif">  <a name="f3"></a><img src="/img/revistas/rbp/v43n3/figura_a02_3.jpg" width="329" height="340"></font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">La distribuci&oacute;n del tipo de intimina entre las cepas t&iacute;picas y at&iacute;picas aisladas en el 2001-2002, revel&oacute; que las intiminas b y g est&aacute;n presentes en cepas de genotipo <i>bfpA</i>+ y <i>bfpA</i>- aunque con mayor predominio en estas ultimas. Las dos cepas de tipo a encontradas, son at&iacute;picas. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>EPEC: Fermentaci&oacute;n de Sorbitol (FS) y Producci&oacute;n de <i>b-D-glucoronidasa</i> (MUG). </b>El 85% de las cepas EPEC analizadas mostraron ser fermentadoras de sorbitol (FS+) y productoras de -D-glucoronidasa (MUG+). Sin embargo, se observaron asimismo fenotipos FS+/MUG- as&iacute; como FS-/MUG+ en un 14 y 2% respectivamente. No se encontraron cepas FS-/MUG- (<a href="#c2">Cuadro # 2</a>). </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>Resistencia a Antibi&oacute;ticos.</b> El 99% de las cepas EPEC presento resistencia al menos a uno de los 8 antibi&oacute;ticos testados (<a href="#f4a">Figura # 4</a>). </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Se observ&oacute; por una parte, un porcentaje significativo (p&lt;0,05) de cepas resistentes a: ampicilina (89%), tetraciclina (84%), estreptomicina (82%), sulfatrimetoprim (81%) y eritromicina (75%). Por otra, la proporci&oacute;n de cepas resistentes a la gentamicina (40%) y cloranfenicol (40%), y al &aacute;cido nalid&iacute;xico (17%), fue menor pero tambi&eacute;n significativa (p&lt; 0,05) (<a href="#f4a">Figura # 4a</a>). </font></p>     <p align="center"><a name="f4a" id="f4a"></a><img src="/img/revistas/rbp/v43n3/figura_a02_4a.gif" width="332" height="290"></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">En general, se observa baja frecuencia de cepas resistentes a solo un antibi&oacute;tico (5%) mientras que la multiresistencia a 5, 6 y 7 antibi&oacute;ticos, representa en conjunto al 72% de las cepas (<a href="#f4b">Figura # 4b</a>). La resistencia conjunta a 5 antibi&oacute;ticos fue la m&aacute;s frecuentemente encontrada (31%). La asociaci&oacute;n m&aacute;s com&uacute;n entre marcadores de resistencia, fue entre ampicilina y tetraciclina (82%) (p&lt;0,05). </font></p>     <p align="center"><font size="2" face="Verdana, Arial, Helvetica, sans-serif"><a name="f4b"></a><img src="/img/revistas/rbp/v43n3/figura_a02_4b.gif" width="319" height="360"></font></p>     ]]></body>
<body><![CDATA[<p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>EPEC: Asociaci&oacute;n entre serogrupos y factores de patogenicidad (genes <i>eae</i> y <i>bfp</i>).</b> La asociaci&oacute;n entre el serogrupo, con la presencia del gen <i>eaeA</i>, se analizo en 31 cepas de <i>E. Coli</i>, pertenecientes a 15 serogrupos distintos, 8 de los cuales corresponden com&uacute;nmente a aislados de EPEC cl&iacute;nica y epidemiol&oacute;gicamente relevantes (<a href="#c3">Cuadro # 3</a>). El gen <i>eaeA</i> se encontr&oacute; en 15 cepas pertenecientes a 9 serogrupos, observ&aacute;ndose una mayor asociaci&oacute;n con el serogrupo O55 (4/6) (p&lt; 0.05). </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">En general, se observo marcada heterogeneidad en la asociaci&oacute;n entre serogrupos y genotipo <i>eaeA</i>. Por un lado, se observaron diferencias respecto a la presencia del gen </font><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><i>eaeA</i> entre aislados de un mismo serogrupo. Por otro, se encontraron aislados que corresponden a serogrupos prototipo de EPEC (O125, O126), pero que no portan el gene <i>eaeA</i>, as&iacute; como serogrupos no relacionados a EPEC que son de genotipo <i>eae</i>+, (serogrupo O28ac com&uacute;nmente asociado a EIEC). Asimismo, se observan serogrupos comunes a EPEC pero que pueden estar presentes en otras categor&iacute;as patog&eacute;nicas como la cepa 0146 que en otros estudios<sup>17</sup> esta relacionada a VTEC/STEC y que sin embargo, en este estudio no porta genes <i>stx</i>. (<a href="#c3">Cuadro # 3</a>). </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Los aislados <i>eae</i>+ de serogrupo definido fueron luego analizados respecto al tipo de intimina (<a href="#c3">Cuadro 3</a>), observ&aacute;ndose que la cepas con intimina g (9/15) corresponden a seis serogrupos diferentes, siendo O55 y O44 los m&aacute;s frecuentemente encontrados. Las cepas portadoras de intimina b se encontraron asociadas a dos serogrupos diferentes, siendo O119 el m&aacute;s com&uacute;n. Dos de las tres cepas no tipificables, fueron del serogrupo O86. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">7 cepas EPEC t&iacute;picas encontradas en este estudio se observaron tanto en cepas con intimina de tipo g (5/7) y b </font><font face="Verdana, Arial, Helvetica, sans-serif" size="2">(2/7) y pertenecen a 5 diferentes serogrupos, 4 de los cuales son tradicionales de EPEC, siendo O55 el mas frecuentemente asociado. Las cepas at&iacute;picas pertenecen a los serogrupos O1, O44 y O119. Un mismo serogrupo puede estar asociado tanto a una cepa t&iacute;pica como at&iacute;pica (O55, O86) (<a href="#c3">Cuadro # 3</a>). </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>EHEC: Caracterizaci&oacute;n genot&iacute;pica y fenot&iacute;pica. </b>La identificaci&oacute;n de EHEC se realizo a trav&eacute;s del an&aacute;lisis de los genes <i>stx</i> entre las cepas <i>eae</i>+ mdh+. La prevalencia de EHEC (<i>eae</i>+ <i>stx</i>+) fue de 0.34%. Se encontraron tres cepas clasificadas como EHEC que representan el 5% del total de cepas <i>eae</i>+. Una de &eacute;stas pertenece a la categor&iacute;a de intimina g. Las 2 cepas restantes, fueron clasificadas </font><font face="Verdana, Arial, Helvetica, sans-serif" size="2">como no tipeables. Dos de las tres cepas presentaron diferente patr&oacute;n genot&iacute;pico respecto a la distribuci&oacute;n de toxinas <i>Stx1</i> y <i>Stx2</i>. En cuanto a la caracterizaci&oacute;n fenot&iacute;pica; dos de las tres cepas fueron identificadas por serolog&iacute;a como O157 y O6 respectivamente, ambas cepas son FS-/MUG-. La cepa S45 que no present&oacute; serogrupo identificable es FS+/MUG- (<a href="#c4">Cuadro # 4</a>).</font></p>     <p align="center"><a name="c4"></a><img src="/img/revistas/rbp/v43n3/cuadro_a03_4.gif" width="323" height="184"></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">El an&aacute;lisis de la resistencia a antibi&oacute;ticos, mostr&oacute; que a diferencia de los aislados de EPEC, las cepas EHEC, presentaron sensibilidad a siete antibi&oacute;ticos y solo se observ&oacute; resistencia a la eritromicina. </font></p>     <p align="justify"><font size="3" face="Verdana"><b>    <br> Discusi&oacute;n </b></font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">En los pa&iacute;ses en desarrollo, las tasas de mortalidad y morbilidad infantil est&aacute;n com&uacute;nmente asociadas a las EDA<sup>3</sup>. Las complicaciones que se derivan de estas enfermedades incluyen la malnutrici&oacute;n e incremento de los costos de atenci&oacute;n en salud<sup>18</sup>. En este contexto, las EDA asociadas a pat&oacute;genos bacterianos contin&uacute;an siendo muy frecuentes a nivel mundial<sup>19-20</sup>. </font></p>     ]]></body>
<body><![CDATA[<p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Las diversas categor&iacute;as patog&eacute;nicas de <i>E. Coli</i> Diarreog&eacute;nica se cuentan entre los pat&oacute;genos bacterianos m&aacute;s importantes causantes de las EDA<sup>13, 21</sup>. Debido a que la identificaci&oacute;n de DEC, requiere su diferenciaci&oacute;n de la flora normal bacteriana, los m&eacute;todos microbiol&oacute;gicos tradicionales no son &uacute;tiles, siendo necesaria la aplicaci&oacute;n de nuevas herramientas de diagnostico. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">En este trabajo, se utilizaron distintos sistemas de PCR para la caracterizaci&oacute;n del perfil patog&eacute;nico de las cepas de <i>E. Coli</i> causantes de la lesi&oacute;n A/E (AEEC). La detecci&oacute;n por una parte del gen de la intimina (gen <i>eaeA</i>) y por otra, de los genes <i>bfpA</i> y <i>stx</i> permiti&oacute; la caracterizaci&oacute;n de EPEC en cepas t&iacute;picas o at&iacute;picas y su distinci&oacute;n de EHEC respectivamente<sup>22</sup>.</font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Los marcadores fenot&iacute;picos se utilizaron tanto para complementar la caracterizaci&oacute;n genot&iacute;pica definida por PCR como para analizar la validez de su uso en el diagnostico. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>Identificaci&oacute;n y Caracterizaci&oacute;n de cepas EPEC. </b>Los datos obtenidos en el presente trabajo, muestran que la prevalencia de AEEC fue del 7% con predominancia de EPEC (95%) sobre EHEC entre las cepas <i>eae</i>+ (p&lt;0.05). Se observa tambi&eacute;n una alta frecuencia de EPEC at&iacute;pica en relaci&oacute;n a EPEC t&iacute;pica (p&lt;0,05). Por lo tanto, las cepas EPEC at&iacute;picas tendr&iacute;an mayor circulaci&oacute;n entre la poblaci&oacute;n analizada, reflejando por una parte, la relevancia de este grupo aislado de heces diarreicas de ni&ntilde;os que requirieron asistencia hospitalaria y por otra, confirmando el rol del gen <i>eaeA</i> como factor importante de patogenicidad de EPEC. Sin embargo, en vista de la variaci&oacute;n del gen <i>bfpA</i> encontrada en cepas EPEC<sup>23-24</sup> ser&aacute; necesario reconfirmar estos datos con cebadores dirigidos hacia regiones conservadas comunes a los diferentes alelos <i>bfpA</i>. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">La intimina es una prote&iacute;na de membrana externa involucrada en la patogenicidad de EPEC y EHEC. Sus funciones est&aacute;n relacionadas a la adherencia de la bacteria a la c&eacute;lula eucariota a trav&eacute;s de la interacci&oacute;n con la prote&iacute;na receptora Tir, as&iacute; como a la estimulaci&oacute;n de la respuesta inmune de la mucosa intestinal<sup>5</sup>. El gen de la intimina forma parte de los genes codificantes para la lesi&oacute;n AE que est&aacute;n localizados en una isla de patogenicidad (PAI) llamada locus de la esfacelaci&oacute;n del enterocito (LEE). La regi&oacute;n que comprende este locus, es altamente conservada en EPEC y EHEC y contiene 41 y 54 marcos abiertos de lectura respectivamente. Estos genes est&aacute;n localizados en operones policistr&oacute;nicos donde se encuentra el gen del receptor de la intimina (<em>tir</em>) adem&aacute;s de otros asociados al sistema de secreci&oacute;n tipo III y adhesi&oacute;n de prote&iacute;nas<sup>25-27</sup>. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">La importancia de la intimina en la infecci&oacute;n de EPEC y EHEC ha sido documentada en numerosos estudios tanto en cultivos celulares como en voluntarios<sup>28-29</sup>. Por otra parte, se han encontrado altos niveles de anticuerpos antiintimina en el suero de pacientes infectados con EPEC y EHEC<sup>30-32</sup> as&iacute; como en la leche humana<sup>33</sup>. Existen evidencias de que anticuerpos contra intimina de EPEC y EHEC podr&iacute;an tener un efecto protectivo potencial contra la infecci&oacute;n por estos pat&oacute;genos<sup>33</sup>. Dado, que la infecci&oacute;n por EPEC es m&aacute;s com&uacute;n que EHEC, se cree que EPEC conferir&iacute;a protecci&oacute;n inmunitaria de reacci&oacute;n cruzada hacia EHEC, causando la limitaci&oacute;n de su circulaci&oacute;n en la poblaci&oacute;n. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">De forma similar, a lo reportado en este trabajo, otros estudios<sup>34-40</sup> han mostrado entre otros, mayor prevalec&iacute;a de cepas EPEC at&iacute;picas en diferentes regiones geogr&aacute;ficas. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Sin embargo, se ha reportado mayor prevalencia de cepas EPEC t&iacute;picas en pa&iacute;ses en desarrollo, mientras que las at&iacute;picas constituyen los aislados mas frecuentes de EPEC en pa&iacute;ses industrializados<sup>41</sup>. Esta correlaci&oacute;n, no se ajusta a lo observado en el presente estudio, lo que indicar&iacute;a que existe variedad de patrones epidemiol&oacute;gicos asociados a la infecci&oacute;n de EPEC t&iacute;pica y at&iacute;pica en diferentes &aacute;reas geogr&aacute;ficas. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">En vista que EPEC at&iacute;pica, no constituye un grupo homog&eacute;neo<sup>32,42</sup>, su rol en las EDA es aun controversial, por lo que ser&aacute; necesario realizar, por una parte, mayores estudios para definir y precisar su perfil de virulencia y por otra, evaluar su presencia en grupos control. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>EPEC: Serogrupos y factores de virulencia.</b> Previo al conocimiento de los factores de virulencia y patogenicidad de EPEC, su diagn&oacute;stico se basaba en la identificaci&oacute;n de <i>E. Coli</i> perteneciente a determinados serotipos cl&iacute;nica y epidemiol&oacute;gicamen-te asociados a las EDA. En algunos reportes, la serolog&iacute;a es a&uacute;n considerada muy &uacute;til en el diagnostico presuntivo de EPEC<sup>43-44</sup>. En este estudio, se observa sin embargo, que la correlaci&oacute;n entre los aislados de EPEC con diferentes serogrupos es muy heterog&eacute;nea y no se distinguen datos consistentes (<a href="#c3">Cuadro 3</a>). En general se presentan: a) diferencias respecto a la presencia del gen <i>eaeA</i>, entre aislados de un mismo serogrupo caracter&iacute;stico de EPEC (O44, O55 y O111), b) serogrupos de EPEC considerados tradicionales, que no portan el gen <i>eae</i>+ (serogrupo O26, O125), c) cepas EPEC t&iacute;picas y at&iacute;picas en un mismo serogrupo (O44, O55, O86ac), d) serogrupos EPEC que se observan en otras categor&iacute;as patog&eacute;nicas (EHEC y EAEG) y finalmente e) La presencia del gene <i>eaeA</i> en un serogrupo especifico de EIEC. </font></p>     ]]></body>
<body><![CDATA[<p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Estas diferencias podr&iacute;an estar relacionadas al n&uacute;mero de cepas analizadas. Sin embargo, en otros reportes<sup>40, 42, 45-59 </sup>se ha observado discordancia entre el perfil de patogenicidad de esta categor&iacute;a (analizado ya sea a trav&eacute;s de la presencia de genes espec&iacute;ficos o en base a los patrones fenot&iacute;picos de adherencia de las cepas) y la pertenencia a serogrupos y serotipos tradicionalmente caracter&iacute;sticos de EPEC. Asimismo, se han encontrado nuevos serotipos/serogrupos asociados a EPEC<sup>60</sup> y presencia de alta diversidad clonal<sup>53,59</sup>. Estos fen&oacute;menos, probablemente relacionados a la diferencia de origen clonal entre cepas de <i>E. Coli</i> de un mismo serotipo, o a la emergencia de cepas con serogrupos previamente no asociados a EPEC, se evidencian en aislados de diferentes regiones geogr&aacute;ficas<sup>61</sup>. Diferentes factores, como la diversidad de cepas circulantes, eventos de transferencia horizontal, estado nutricional del hu&eacute;sped, uso de antibi&oacute;ticos, condiciones sanitarias (acceso al agua potable, hacinamiento de viviendas, contacto con animales, inadecuado manejo de excretas) entre otros, los cuales var&iacute;an entre una regi&oacute;n a otra, podr&iacute;an afectar a la relaci&oacute;n entre determinados genes de patogenicidad y virulencia y un serogrupo o serotipo dado. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">El grado de discordancia entre determinados serogrupos y categor&iacute;as patog&eacute;nicas puede ser mayor, si como ocurre en nuestro medio, los sistemas de diagnostico, son importados y est&aacute;n basados en estudios de correlaci&oacute;n validos para otras regiones. Los resultados obtenidos, tienen importancia cl&iacute;nica y epidemiol&oacute;gica y remarcan la inespecificidad de los m&eacute;todos basados en la identificaci&oacute;n de serogrupo, en la asignaci&oacute;n de categor&iacute;as patog&eacute;nicas sustentando la necesidad del uso de m&eacute;todos alternativos de diagnostico de DEC y en particular de EPEC. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Al respecto, ser&aacute; importante analizar la presencia de otros genes de virulencia en las cepas (<i>eae</i>+ y <i>eae</i>-) para caracterizarlas m&aacute;s as&iacute; como complementar los perfiles de virulencia con ensayos de adherencia <em>in vitro</em>. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>EPEC: Tipificaci&oacute;n de Intiminas.</b> El an&aacute;lisis de la variaci&oacute;n del gen de la intimina, en cepas EPEC aisladas con PDI, en base a los tres tipos predominantes de intimina (&alpha;, &beta; y &gamma;) mostr&oacute; que las cepas no tipeables representan el mayor porcentaje (72%), seguidas de la intimina g e intimina b. La intimina a es poco frecuente. El alto porcentaje de cepas no tipeables refleja la variaci&oacute;n del gene de la intimina en la regi&oacute;n carboxilo- terminal donde se encuentra el sitio de uni&oacute;n al receptor-la prote&iacute;na Tir cuyo gen presenta tambi&eacute;n polimorfismo. Otros estudios recientes, reportan de forma similar a este estudio alta proporci&oacute;n (70%) de intiminas no tipeables<sup>62</sup>. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Al presente, se han identificado 15 variantes entre tipos y subtipos del gen de la intimina en aislados de humanos y animales de EPEC y EHEC<sup>63-70</sup>. Existen evidencias de que el tipo de intimina tendr&iacute;a influencia sobre los sitios de colonizaci&oacute;n, lo que a su vez reflejar&iacute;a especificidad de tropismo celular o tisular a nivel de la infecci&oacute;n<sup>71</sup>. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">En la <a href="#f3">Figura 3</a>, se distingue la diferencia (p&lt;0.05) en el porcentaje de muestras no tipeables en los per&iacute;odos 1993 y 2001-2002. Aunque el n&uacute;mero total de cepas analizadas es menor en 1993, esta diferencia podr&iacute;a atribuirse a que el gen de la intimina ha adquirido mayor variabilidad a lo largo del tiempo transcurrido y/o a la emergencia de nuevas cepas con variantes diferentes a las analizadas en este estudio. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">En cuanto a la intimina g es interesante observar su asociaci&oacute;n en casi similar proporci&oacute;n tanto a cepas EPEC t&iacute;picas como at&iacute;picas (<a href="#c3">Cuadro # 3</a>) que contrasta fuertemente con lo observado en otros estudios donde este tipo de intimina corresponde com&uacute;nmente a EHEC o a un set limitado de serotipos (O55:[H7] y O111ac:[H8]) de EPEC at&iacute;pica<sup>41, 72</sup>. En este estudio, los 4 aislados <i>eae</i>+ de serogrupo O55 si bien tienen intimina &gamma;, 3 de los cuales son tambi&eacute;n <i>bfpA</i>+. El serogrupo 0111 pertenece a una cepa at&iacute;pica. El resto de las cepas con intimina g est&aacute; distribuido en cuatro serogrupos diferentes que no corresponden a los serogrupos de EPEC epidemiol&oacute;gicamente m&aacute;s comunes. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">La presencia de intimina &beta;, puede tambi&eacute;n estar asociada tanto a cepas t&iacute;picas como at&iacute;picas (<a href="#c3">Cuadro 3</a>) por lo que en este caso tampoco se observa una correlaci&oacute;n entre serogrupos, tipo de intimina y bundlina. Los datos de los aislados del 2001-2002, muestran de forma similar, la distribuci&oacute;n de intimina &beta; y g entre cepas t&iacute;picas como at&iacute;picas aunque dada la preponderancia de cepas at&iacute;picas la asociaci&oacute;n es mayor con esta &uacute;ltimas (<a href="#c2">Cuadro 2</a>). En conjunto, estos datos, demuestran, la diversidad de cepas EPEC aisladas de heces diarreicas, que evidencian la heterogeneidad entre serogrupos, tipo de intimina y presencia de bundlina. En pa&iacute;ses en desarrollo, donde <i>E. Coli</i> Diarreogenica es mas frecuente y donde la proporci&oacute;n de infecciones es mayor, tanto por cepas end&eacute;micas como por aquellas provenientes de reservorios animales, podr&iacute;an existir condiciones potenciales para mayor intercambio gen&eacute;tico por transferencia horizontal, que explicar&iacute;an la heterogeneidad encontrada de combinaciones entre factores de patogenicidad. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Estudios filogen&eacute;ticos sugieren, que el sitio de inserci&oacute;n del locus LEE en el cromosoma bacteriano, est&aacute; directamente relacionado al origen evolutivo de las cepas EPEC del grupo 1 y 2<sup>25, 73-74</sup>. Las cepas caracterizadas como EPEC t&iacute;picas con sus respectivos serotipos, pertenecen a la misma rama evolutiva, que contiene el locus LEE insertado dentro del locus <i>selC</i> del cromosoma bacteriano. En EPEC at&iacute;pica, el LEE es insertado en el locus <i>pheU</i> o en otro sitio<sup>75</sup>. Dado que la regi&oacute;n LEE, es una entidad din&aacute;mica en t&eacute;rminos de la transferencia de genes, que favorecer&iacute;a la aparici&oacute;n de nuevas cepas patog&eacute;nicas, ser&aacute; importante determinar en futuros estudios los sitios de inserci&oacute;n de este locus en el cromosoma bacteriano, las variantes de intimina, as&iacute; como la relaci&oacute;n filogen&eacute;tica entre las cepas EPEC encontradas. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>EPEC: Caracterizaci&oacute;n Fenot&iacute;pica.</b> Si bien las cepas son mayoritariamente del fenotipo FS+/MUG+, existe un porcentaje apreciable de cepas MUG- (14%), que son at&iacute;picas. Estas cepas podr&iacute;an estar filogen&eacute;ticamente m&aacute;s relacionadas a los aislados de EHEC encontrados que presentan este mismo patr&oacute;n. Estas observaciones deber&aacute;n confirmarse en futuros estudios. </font></p>     ]]></body>
<body><![CDATA[<p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>Resistencia a antibi&oacute;ticos.</b> El an&aacute;lisis de la resistencia a antibi&oacute;ticos en los aislados de EPEC mostr&oacute; tres patrones caracter&iacute;sticos. Por una parte, resalta la alta frecuencia de cepas resistentes a ampicilina, tetraciclina, streptomicina, sulfatri-metoprim y eritromicina en un rango entre 75% a 90% seguida de la resistencia a cloranfenicol y gentamicina alrededor del 40% y finalmente la resistencia al &aacute;cido nalidixico en un 17% (<a href="#f4a">Figura # 4a</a>). El primer y segundo patr&oacute;n, donde se observan frecuencias similares de cepas resistentes para bloques de 5 y 2 antibi&oacute;ticos respectivamente (<a href="#f4b">Figura # 4b</a>), estar&iacute;an reflejando la resistencia transmisible mediada por pl&aacute;smidos, transposones o integrones. Este tipo de resistencia estar&iacute;a sujeta a presi&oacute;n de selecci&oacute;n por el uso inadecuado de antibi&oacute;ticos en nuestro medio, para el tratamiento de las EDA y otras enfermedades. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">La amplia distribuci&oacute;n de cepas multiresistentes en las cepas mas prevalentes de AEEC tiene relevancia epidemiol&oacute;gica. Es importante remarcar los datos encontrados donde los fenotipos mas prevalentes comprenden cepas EPEC multiresistentes a entre 5 y 7 antibi&oacute;ticos y donde casi la totalidad de cepas EPEC 57/58 es resistente a por lo menos un antibi&oacute;tico. Los patrones de resistencia encontrados estar&iacute;an reflejando los tipos de antibi&oacute;ticos m&aacute;s frecuentemente usados, la extensi&oacute;n de los mecanismos de transferencia horizontal y la prevalenc&iacute;a de infecci&oacute;n de las cepas pat&oacute;genas en la poblaci&oacute;n. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">En estudios de evaluaci&oacute;n de la multiresistencia a antibi&oacute;ticos de EPEC y otros enteropat&oacute;genos<sup>44, 75-86</sup> en otros pa&iacute;ses, se han encontrado datos similares, aunque en general en menor proporci&oacute;n de cepas multiresistentes. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">El incremento de la prevalenc&iacute;a de la resistencia a antibi&oacute;ticos es un problema de salud publica mundial<sup>87</sup>. La terapia antimicrobiana desde su aplicaci&oacute;n en gran escala hace mas de 50 a&ntilde;os atr&aacute;s, ha generado un incremento creciente de organismos resistentes. Virtualmente todas las especies de bacterias pat&oacute;genas incluyen cepas resistentes a varios antibi&oacute;ticos utilizados para controlarlos. <i>E. Coli</i> como parte de la flora comensal intestinal tiene particularmente un gran potencial para el desarrollo de la resistencia a antimicrobianos y podr&iacute;a constituirse en un reservorio diseminable de genes de multiresistencia a bacterias pat&oacute;genas o viceversa<sup>88</sup>. En este contexto, debe tambi&eacute;n considerarse que gran parte de los factores de patogenicidad y virulencia de DEC, al igual que los genes de multiresistencia a antibioticos, se encuentran asociados a elementos m&oacute;viles. Se estima que las infecciones causadas por bacterias multiresis-tentes a antibi&oacute;ticos estar&iacute;an asociadas a mayores tasas de morbilidad y mortalidad<sup>89</sup>. Este fen&oacute;meno derivado del uso inapropiado de antibi&oacute;ticos estar&iacute;a influenciado por varios factores, como ser la ineficacia de los antibi&oacute;ticos y sus complicaciones en el tratamiento, el incremento de la virulencia microbiana por la asociaci&oacute;n entre genes de virulencia y de resistencia a antibi&oacute;ticos y la ineficiente colonizaci&oacute;n de la microflora intestinal que favorecer&iacute;a la infecci&oacute;n de organismos multiresistentes. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Por lo tanto, los datos reportados en este estudio deber&aacute;n ser considerados en el tratamiento de EDAs y en el desarrollo de programas y estrategias de prevenci&oacute;n que enfoquen el uso racional de antibi&oacute;ticos y el control de la emergencia y diseminaci&oacute;n de cepas multiresistentes. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2"><b>Caracterizaci&oacute;n de cepas EHEC.</b> Las infecciones por EHEC, son un problema de salud p&uacute;blica en pa&iacute;ses como USA, Canad&aacute;, Inglaterra, y Jap&oacute;n<sup>90</sup>. En el hemisferio sur, EHEC es prevalerte en Chile, Argentina<sup>91</sup> y Sud&aacute;frica<sup>90</sup>. Estos datos contrastan con EPEC que es responsable de un n&uacute;mero importante de muertes en ni&ntilde;os menores de cinco a&ntilde;os en pa&iacute;ses en v&iacute;as de desarrollo<sup>13</sup>. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Los datos obtenidos en este estudio muestran la baja prevalenc&iacute;a de las infecciones de EHEC entre las EDA, que coincide con el patr&oacute;n epidemiol&oacute;gico observado en otros pa&iacute;ses<sup>7,9,62,83,92-94</sup>. Sin embargo, se debe tomar en cuenta, que se consideraron solo a las cepas EHEC portadoras del locus LEE por lo que deber&aacute; analizarse en futuros trabajos el rol de las cepas EHEC no asociadas a la lesi&oacute;n A/E.</font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Las tres cepas EHEC encontradas portan el gen <i>stx2</i>. Varios estudios<sup>95</sup> sugieren, que existir&iacute;a sinergismo entre los genes <i>stx2</i> y <i>eaeA</i>, asociado a una mayor virulencia de EHEC. Se observan tambi&eacute;n diferencias en las caracter&iacute;sticas fenot&iacute;picas con respecto a la fermentaci&oacute;n de sorbitol, producci&oacute;n de glucoro-nidasa y serogrupo. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Estos datos reflejar&iacute;an diferencias de origen clonal y se&ntilde;alar&iacute;an de forma preliminar que no existe un patr&oacute;n EHEC circulante predominante como el asociado a la cepa O157H7 (FS-/MUG-). </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Es interesante notar en este n&uacute;mero reducido de muestras, por una parte la presencia del serogrupo O157 caracter&iacute;stico de EHEC (en la cepa FS-/ MUG- de intimina no tipeable). Por otra parte, la presencia del serogrupo O6, caracter&iacute;stico de aislados de ETEC. A nuestro conocimiento, esta cepa representa una nueva variante de EHEC emergente en humanos, que no ha sido reportada previamente en la literatura. Recientemente se ha encontrado a este serogrupo en cepas EHEC de ovinos<sup>69</sup>. </font></p>     ]]></body>
<body><![CDATA[<p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">En conjunto, estos datos deber&aacute;n tomarse en cuenta al considerar lineamientos de diagnostico de EHEC basados en caracter&iacute;sticas fenot&iacute;picas (fermentaci&oacute;n de sorbitol, producci&oacute;n de <i>b-D-glucoronidasa</i>, serogrupo asociado), pues no serian validos para su uso en nuestro medio. Se remarca nuevamente en esta otra categor&iacute;a patog&eacute;nica de DEC, que los patrones de caracterizaci&oacute;n fenot&iacute;pica no son comunes ni extrapolables a distintas regiones geogr&aacute;ficas. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Los resultados obtenidos en los ensayos de multiresistencia a antibi&oacute;ticos en cepas EHEC, contrastan significativamente (P&lt; 0.05) con los datos de EPEC y podr&iacute;an asociarse a la baja prevalec&iacute;a de EHEC encontrada, y a que su circulaci&oacute;n estar&iacute;a reducida en humanos. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Dado que en Bolivia, el uso de antibi&oacute;ticos es mucho m&aacute;s com&uacute;n en h&uacute;manos que en animales, se podr&iacute;a inferir en base al patr&oacute;n de multiresistencia a antibi&oacute;ticos, la emergencia de nuevas cepas a partir de origen animal o humano. Por lo tanto, los contrastes entre los niveles de multiresistencia a antibi&oacute;ticos de EHEC y EPEC reflejar&iacute;an presiones de selecci&oacute;n diferentes determinadas por las frecuencias de infecci&oacute;n y circulaci&oacute;n de estos pat&oacute;genos en humanos y/o animales. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">El presente estudio constituye un an&aacute;lisis preliminar de la caracter&iacute;sticas de dos categor&iacute;as patog&eacute;nicas portadoras del locus LEE, presentes en heces de ni&ntilde;os con PDI, que servir&aacute; de base para futuros estudios epidemiol&oacute;gicos, donde deber&aacute; confirmarse su asociaci&oacute;n a las EDA. </font></p>     <p align="justify"><font size="3" face="Verdana"><b>    <br> Agradecimiento </b></font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Este trabajo fue realizado en el Instituto de Biolog&iacute;a Molecular y Biotecnolog&iacute;a (IBMB) con apoyo parcial del Programa de colaboraci&oacute;n sueca ASDI-SAREC y constituy&oacute; parte de los trabajos de tesis de grado de licenciatura de Samanta S&aacute;nchez y Paola Romec&iacute;n. </font></p>     <p align="justify"><font face="Verdana, Arial, Helvetica, sans-serif" size="2">Los autores agradecen al personal del Hospital del Ni&ntilde;o Ovidio Aliaga y Hospital Materno Infantil. Asimismo a la Dra. Patricia Lada, al Dr. Alberto Ben&iacute;tez y al Sr. Natalio Medrano por la colaboraci&oacute;n prestada. </font></p>     <p align="justify"></p>     <p align="justify"><font size="3" face="Verdana"><b>    ]]></body>
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