RESUMO
Anaplasma marginale (A. marginale), es una bacteria del orden de las Rickettsias que ocasiona la anaplasmosis bovina en regiones tropicales y subtropicales del mundo. Esta enfermedad, trasmitida principalmente por tábanos y garrapatas, se desarrolla típicamente en una etapa inicial aguda con manifestaciones clínicas caracterizadas principalmente por anemia y fiebre. Después de un par de meses, los animales recuperan su condición física y se hacen asintomáticos, siendo incapaces de eliminar completamente la bacteria, convirtiéndose en animales persistentemente infectados. Esto se debe a la capacidad de A. marginale para evadir el sistema inmune. En este sentido, se ha demostrado la existencia de un mecanismo de variación antigénica en las proteínas MSP1, MSP2 y MSP3 de la bacteria. Al evaluar la familia multigénica que codifica para la MSP2, se determinó que está conformada por dos regiones conservadas que flanquean una región central hipervariable. De esta manera, al expresarse cada una de las 52 variables de la MSP2, se expresa un epítope diferente. Cuando se describió el genoma completo de este hemotrópico, se encontró también la presencia de 16 pseudogenes msp2, los cuales pueden ser recombinados dentro del sitio de expresión del operón de la MSP2, constituyendo un segundo mecanismo de variación. Además de ello, los fragmentos hipervaribles y los pseudogenes se pueden combinar entre sí, en un proceso denominado conversión génica, creando nuevos epítopes recombinantes, confiriendo una capacidad de variabilidad antigénica casi infinita al A. marginale (tercer mecanismo). Un cuarto mecanismo de variación antigénica, lo constituye la dimerización de la MSP2 sobre la superficie del A. marginale, debido a que la expresión simultánea de variantes conforman epítopes únicos. En conclusión, la recombinación génica de la MSP2 y su dimerización en la membrana, constituye un mecanismo muy eficiente de variación antigénica para eludir el sistema inmunológico del hospedador.
Anaplasma marginale (A. marginale) is a bacterium of the Rickettsiales order that causes bovine anaplasmosis in tropical and subtropical regions worldwide. This disease, mainly transmitted by ticks and horseflies, typically develops in an initial acute stage, with clinical signs characterized by anemia and fever. After two months, animals recover their original physical condition and become asymptomatic, being unable to completely eliminate the bacterium, turning into persistently infected animals. This is due to the ability of A.marginale to evade the immune system. In this regard, the existence of a mechanism for antigenic variation in proteins of the bacterium, such as MSP1, MSP2, and MSP3, has been demonstrated. When assessing the multigenic family which encodes for MSP2, it was determined that it consists of two conserved regions flanking a central hypervariable region. Thus, when expressing each of the 52 MSP2 variables, a different epitope is also expressed. When the entire genome of this parasite was decoded, the presence of 16 pseudogenes for MSP2 was also discovered. These pseudogenes can be recombined within the operon expression site of MSP2, providing a second mechanism of variation. Moreover, both the hypervariable fragments and pseudogenes can combine among them, in a process called gene conversion, creating new recombinant epitopes, conferring the A. marginale with an almost infinite capacity for antigenic variability (third mechanism). A fourth mechanism of antigentic variation consists of the dimerization of MSP2 on the surface of A. marginale, because the simultaneous expression of variants creates unique epitopes. In conclusion, gene recombination of MSP2 along with the dimerization of MSP2 on the membrane provides a very efficient mechanism for antigenic variation for evading the hosts immune system.
RESUMO
Animal trypanosomiasis is a disease caused by parasites of the genus Trypanosome. This malady is widely distributed in many countries, located in tropical and subtropical areas of the world where blood-sucking flies are present. Water buffaloes are important domestic animals used for meat and milk production, and draught power. Buffalo herds are raised in areas where trypanosomiasis is endemic. In Venezuela, the buffalo industry is becoming a very important and common livestock. However, animals imported from non-endemic areas may suffer severe infections. The development of methods which ensure an efficient epidemiological surveillance against this disease is of great relevance. The immunological tests are of great importance for this purpose, because of the low sensitivity of the current parasitological methods, due to the low parasite burden that occur in subclinical and chronic infections caused by trypanosomes. To estimate the serological prevalence of trypanosome in water buffaloes, an enzyme-linked immunosorbent assay (ELISA) was used in buffalo samples of healthy animals from the municipalities of Rómulo Gallegos, Ricaurte and Girardot, in the State of Cojedes, Venezuela. Additionally, samples were also assessed with the indirect fluorescence antibody test (IFAT) and the microhematocrit test (MHCT). A total of 180 blood samples, none of which had an active parasitemia by TMC, were assessed. The prevalence determined by ELISA was 45.56%, which was significantly (P<0.05) higher than that obtained by IFAT (28.89%). The results of the experiments showed a moderate Kappa index of concordance of 0.45 (95% CI: 0.31-0.58); whereas the concordance value for both tests was 73.33%. Both the sensitivity and specificity of ELISA, compared to the IFAT, was 82.69% and 69.53%, respectively. The predictive positive and negative values were 52.44% and 90.82%, respectively. The findings suggest an endemic condition, with moderate infection values caused by Trypanosoma spp. in buffaloes from these regions of Venezuela and show, for the first time, the usefulness of ELISA for epidemiological studies of trypanosomiasis.
RESUMO
La anaplasmosis, es una enfermedad producida por la bacteria Anaplasma marginale que está ampliamente distribuida en Venezuela, originando efectos negativos en la salud y productividad de los rebaños bovinos. Hasta el presente se han caracterizado 6 proteínas mayoritarias de superficie (MSP) de esta bacteria, de las cuales la MSP5, ha sido señalada como un excelente polipéptido para el diagnóstico de la enfermedad, debido a que esta proteína es altamente conservada e inmunogénica. Esto ha motivado su clonamiento e inserción en un plásmido de E. coli, para usarla purificada como antígeno en ensayos inmunoenzimáticos. Sin embargo, estudios posteriores, indican que proteínas de E. coli recombinante que eluyen conjuntamente con la MSP5 durante el proceso de purificación, interfieren en el ELISA originando falsos positivos. En el presente trabajo se estandarizó un ELISA indirecto, utilizando la MSP5 como antígeno y se logró disminuir las uniones inespecíficas a las proteínas contaminantes de E. coli, por adición de un suero de conejo anti E. coli que bloquea los epítopes de estas proteínas. A través de un cuadro de contingencia de doble entrada, se determinaron los parámetros de validación del ELISA al compararla con la técnica de naranja de acridina-bromuro de etídio, obteniéndose como resultado que la técnica de ELISA mejorada es 96,1 por ciento sensible, 9 por ciento específica y presenta un valor predictivo del 88,6 por ciento. Además, se estudió una población bovina de 48 mautes de la Estación Experimental La Iguana (estado Guárico), utilizando ambas técnicas, obteniendo una seroprevalencia de 93,7 por ciento por ELISA y una prevalencia de 54,1 por ciento por naranja de acridina-bromuro de etidio. Estos resultados muestran que el bloqueo de los epítopes de las proteínas de E. coli contaminates, utilizando para ello un suero de conejo anti-E. coli, permite disminuir los falsos negativos cuando se utilizan proteínas recombinantes.
Anaplasmosis, is a disease produced by Anaplasma marginale widely distributed in Venezuela, causing negative effects on the health and productivity of bovine herds. Until now, 6 constitutive Anaplasma marginale Mayor Surface Proteins (MSPs) have been characterized, including MSP5 which appears to be an excellent polypeptide for the diagnosis of this disease since it is highly conserved and immunogenic. This has motivated its cloning and insertion into a plasmid in E. coli and the use of the purified antigen in immunoenzymatic assays. However, subsequent indicated that E. coli recombinant proteins, that copurify with MSP5, interfere with the ELISA giving rise to false positives. In the present study, it was accomplished the standardization of an indirect ELISA, using MSP5 as the antigen and it was also diminishing the non-specific unions to the contaminating proteins of E. coli by adding anti-E. coli rabbit serum that blocks the epitopes of these proteins. With the use of a double entry contingency table, the parameters of validation of the ELISA were determined, comparing it to the acridine orange-ethidium bromide technique. The result indicate that the improve MSP5 indirect ELISA has a 96.1% sensitivity, 9% specificity and a predictive value of 88.6%. It was also studied a bovine population of 48 cattle from the Experimental Station La Iguana (Guárico State), using both techniques, obtaining a seroprevalence of 93.7% with ELISA and a prevalence of 54.1% with orange acridine-ethidium bromide. These results show that the blockage of the contaminating E. coli protein epitopes using an anti-E. coli rabbit serum permits the diminishment of false negatives when using recombinant proteins.
Assuntos
Bovinos , Animais , Laranja de Acridina , Anaplasma marginale , Ensaio de Imunoadsorção Enzimática , Escherichia coli , Etídio , Medicina VeterináriaRESUMO
Two different ELISAs were routinely performed in our laboratory to detect bovine trypanosomosis and anaplasmosis. The ELISA test for trypanosomosis involved the adsorption of a soluble fraction of parasites as the antigen; and, the ELISA for anaplasmosis was performed with a purified recombinant protein MSP5r adsorbed to the plate. With the purpose of assessing the merit of ABTS and TMB, we compared the absorbance obtained from positive and negative control sera from both assays. The results obtained, suggest that TMB is more adequate for recombinant antigens and that ABTS is preferred when partially purified antigenic extracts are used in the ELISA test.