They used from these recombinant proteins in serodiagnosis of goat toxoplasmosis (Izatnagar isolate)

They used from these recombinant proteins in serodiagnosis of goat toxoplasmosis (Izatnagar isolate). example, echinococcosis, malaria, leishmaniasis, fascioliasis, and strongyloidiasis were tested of which none showed positive results. Sensitivity and specificity of the generated recombinant IgG ELISA in comparison with commercial ELISA (com ELISA) were 89% and 90%, and the sensitivity and specificity of the generated recombinant IgM ELISA were 96% and 90%, respectively. The results obtained here show that this antigen is useful for diagnostic purposes. Keywords: in MAC13772 humans are asymptomatic although first exposure to the parasite during pregnancy may cause abortion or congenital malformation. The disease is often fatal for immune suppressed patients such as those with acquired immunodeficiency syndrome [1]. The tests presently Rabbit polyclonal to STK6 used for toxoplasmosis diagnosis are based on serological assays. Although they give satisfying results, accurate differentiation between recently acquired and chronic toxoplasmosis remains problematic. False positive reactions with antinuclear antibodies, rheumatoid factors, or naturally occurring human antibodies and false negative reactivity due to competitive inhibition by high levels of specific IgG antibodies have been described [2]. The presence of specific IgM antibodies is not always indicative of an acute infection with is obligatory intracellular parasite therefore, antigens always contaminated with the host cell, various non parasitic materials from culture media in which the parasite is grown. The methods of producing tachyzoites as well as antigen(s) may also vary significantly between laboratories [4]. Therefore, as soon as DNA technology became available for the production of recombinant antigens, they were considered to have the ability to replace natural antigen (s) obtained from lysed whole parasites. The major advantages of recombinant antigens for the diagnosis of infections are (1) the antigen composition of the test is precisely known and caused less false positive and false negative (2) more than one defined antigen can be used and (3) the method can MAC13772 be easily standardized [5]. Dense granule antigens (GRA), secreted in abundance, are major components of both the vacuole surrounding tachyzoites and cyst wall surrounding slower-growing bradyzoites[6]. The dense granules have an essential role in the cell invasion, maintenance of the parasitophorous vacuole, and survival of the parasite after cellular invasion [6]. In almost all nucleated host cells GRA proteins are potent antigens that produce strong T and Bcell responses during infection. Immunological responses to GRA7 may be important in controlling infection, as immunization with the native protein partially protects mice against acute toxoplasmosis [7]. While granule protein 7 produces very strong antibody response in the acute phase of infection , mutant parasites lacking GRA7 exhibit slow growth and pronounced morphological defects when cultured under nutrient-limiting condition [6,7]. In this study, the recombinant protein of dense granule antigen GRA7 of was used for the recognition of acute and chronic phase of toxoplasmosis in human sera [8,9]. The tachyzoites of RH strain were inoculated to the peritoneal cavity of BALB/c mice. After 3 days, the parasites were collected, washed, and resuspended in PBS (pH 7.2). Genomic DNA of RH strain was isolated by the conventional phenol, chloroform, and ethanol precipitation method. Genomic DNA isolated from tachyzoites was used as a template to amplify the GRA7 gene by PCR reaction. A pair of primer based on GRA7 gene sequence was designed with and restriction sites. (GRA Forward: 5′-GGATCCATGGCCCGACACGCAAT-3′), (GRA Reverse: 5′-GCGGCCGCCTGGCGGGCATCCTC-3′). PCR reaction was performed in a total volume of 50 l using 50 ng DNA, 1.5 l forward and reverses primers at 10 pmol, 50 mM Mgcl2, 200 mM dNTP, 10x PCR buffer, 2.5 unit Taq polymerase. PCR reaction was carried out with 30 cycles of denaturation at 94 for 40 sec, annealing at 58 for 60 sec, and extension at 72 for 60 sec. Reaction was incubated at 94 for 5 min before beginning the PCR cycle, and ended with a final extension at 72 for 10 min in a thermal cycler. The amplified DNA of GRA7 gene was visualized on 1% agarose gel MAC13772 stained with syber green. Then,.