Serodiagnosis of toxoplasmosis by using a recombinant form of the 54-kilodalton rhoptry antigen expressed in Escherichia coli

Gelder, Patrick Van; Bosman, Fons; Meuter, F. De; Heuverswyn, Hugo Van; Hérión, Pascal

doi:10.1128/jcm.31.1.9-15.1993

Cited by 45 publications

(29 citation statements)

References 21 publications

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“…The pattern of immunoreactivity observed by Western blotting with human sera varies with the immunoglobulin class and the stage of infection. Several genes have been cloned that encode T. gondii antigens, as follows: the surface antigens P22 (SAG2) (38,46) and P30 (SAG1) (3,12,24); the dense granule antigens P24 (GRA1) (4), P28 (GRA2) (35,45), P29 (GRA7) (2,9,17), P32 (GRA6) (27,47), and P41 (GRA4) (33,55); the rhoptry antigens P54 (ROP2) (31,51,56) and P66 (ROP1) (25,37); and the B10 (36), P25 (22,55), P35, and P68 antigens (25). These recombinant antigens expressed in bacteria have been used to detect antibodies to the parasite in the serum of humans and animals.…”

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confidence: 99%

Recombinant Antigens To DetectToxoplasma gondii-Specific Immunoglobulin G and Immunoglobulin M in Human Sera by Enzyme Immunoassay

et al. 2000

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We have evaluated the diagnostic utility of eleven Toxoplasma gondii recombinant antigens (P22 [SAG2], P24 [GRA1], P25, P28 [GRA2], P29 [GRA7], P30 [SAG1], P35, P41 [GRA4], P54 [ROP2], P66 [ROP1], and P68) in immunoglobulin G (IgG) and IgM recombinant enzyme-linked immunosorbent assays (Rec-ELISAs). Following an initial evaluation, six recombinant antigens (P29, P30, P35, P54, P66, and P68) were tested in the IgG and IgM Rec-ELISAs with four groups of samples which span the toxoplasmosis disease spectrum (negative, chronic infection, acute infection, and recent seroconversion). Our results suggest that the combination of P29, P30, and P35 in an IgG Rec-ELISA and the combination of P29, P35, and P66 in an IgM Rec-ELISA can replace the tachyzoite antigen in IgG and IgM serologic tests, respectively. The relative sensitivity, specificity, and agreement for the IgG P29-P30-P35 Rec-ELISA were 98.4, 95.7, and 97.2%, respectively. The resolved sensitivity, specificity, and agreement for the IgM P29-P35-P66 Rec-ELISA were 93.1, 95.0, and 94.5%, respectively. Relative to the tachyzoite-based immunocapture IgM assay, the IgM P29-P35-P66 Rec-ELISA detects fewer samples that contain IgG antibodies with elevated avidity from individuals with an acute toxoplasmosis.

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confidence: 99%

Recombinant Antigens To DetectToxoplasma gondii-Specific Immunoglobulin G and Immunoglobulin M in Human Sera by Enzyme Immunoassay

et al. 2000

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“…Recombinant proteins therefore possess low antigenicity and show higher background or cross‐reactivity with control sera owing to antibodies directed against these bacterial components, which are unwanted byproducts of recombinant proteins purified from E. coli , whereas the single affinity purification procedure does not remove these components, such as LPS, completely. Thus, the purity of a recombinant protein is inadequate for use as a diagnostic antigen unless further purification procedures or additional purification steps are used 20,21. For example, imidazole, which binds to Ni‐NTA (Qiagen) and competes with His residues in the 6‐His tag, can be used at low concentrations (≤20 mM) to inhibit nonspecific binding, and nonionic detergents can be used to remove background proteins and nucleic acids 22.…”

Section: Discussionmentioning

confidence: 99%

“…The LPS content of pools treated by IMAC was reduced from greater than 800 to 2 ng/mL by the addition of 0.1% triton X‐114 to the elution buffer. In addition, the E. coli lysate should be added to the dilution buffer for Ab1 (serum) detection to reduce interference by antibodies against E. coli that may be present in the sample sera 8,20.…”

Section: Discussionmentioning

confidence: 99%

Expression, purification, and improved antigenic specificity of a truncated recombinant bp26 protein of Brucella melitensis M5‐90: a potential antigen for differential serodiagnosis of brucellosis in sheep and goats

Liu¹,

Hu²,

Qiao³

et al. 2011

Biotech and App Biochem

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Antibodies produced in animals vaccinated using live attenuated vaccines against Brucella spp. are indistinguishable using current conventional serological tests from those produced in infected animals. One potential approach is to develop marker vaccines in which specific genes have been deleted from parental vaccine strains that show good immunogenicity and vaccine efficacy. Corresponding methods of detection for antibodies raised by the marker vaccine should also be developed. A specific fragment of the bp26 gene of Brucella melitensis M5-90 was cloned into vector pQE32 to construct the recombinant plasmid (pQE32-rΔbp26). It was used to transform Escherichia coli M15 (pREP4) host cells, which expressed the rΔbp26 protein. Subsequently, the recombinant protein was purified by immobilized metal affinity chromatography and size-exclusion chromatography. The results of sodium dodecyl sulfate-polyacrylamide gel electrophoresis showed that the purified rΔbp26 protein was represented by only one band, with a molecular weight of 14 kDa, and it showed good antigenic specificity on western blot and enzyme-linked immunosorbent assay (ELISA). The purified rΔbp26 protein was intended to be used as an antigen to develop a novel ELISA to differentiate animals vaccinated with bp26 mutants of Brucella spp. from those infected naturally and those vaccinated with the parental vaccine strains.

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“…The recombinant GRA2 antigen used was the 59 Cterminal amino acids of the protein (GRA2 59aa) expressed as a fusion protein with glutathione-Stransferase (GST) (Cesbron-Delauw et al 1992). Three recombinant fragments of ROP2, each expressed as a fusion protein with a Cro-Lac1 peptide were used; the C-terminal 330 residues (Tg34AR) (Van Gelder et al 1993), the 270 N-terminal amino acids (Tg34EAV) and the 100 N-terminal amino acids (Tg34EB). Soluble T. gondii antigen (STA) was obtained following lysis of purified RH strain tachyzoites by sonication.…”

Section: Methodsmentioning

confidence: 99%

“…ESAs comprise the majority of circulating antigens during the initial stages of infection with T. gondii, and are therefore an early target for the host immune response (Hughes & van Knapen 1982). Around 80% of humans infected with T. gondii had serum antibodies directed against GRA2 59aa (Murray et al 1993), and 90% had antibodies specific for Tg34AR (Van Gelder et al 1993). In the current study, similar percentages of infected sheep had serum antibodies against each of the recombinant antigens.…”

Section: Methodsmentioning

confidence: 99%

Cellular and humoral immune responses to recombinant antigens in sheep infected with Toxoplasma gondii

Coughlan

Saman

Jacobs

et al. 1995

Parasite Immunology

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Immune responses to recombinant fragments of the Toxoplasma gondii antigens ROP2 and GRA2 were investigated in sheep naturally and experimentally infected with T. gondii oocysts. Specific serum antibodies to C-terminal fragments were detected by ELISA. Cell-mediated responses in peripheral blood mononuclear cells were demonstrated by proliferation and interferon-gamma production following in vitro stimulation with the ROP2 fragment. This data indicates the presence of epitopes for sheep B cells in the recombinant GRA2 fragment and for both B and T cells in the ROP2 fragment.

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Serodiagnosis of toxoplasmosis by using a recombinant form of the 54-kilodalton rhoptry antigen expressed in Escherichia coli

Cited by 45 publications

References 21 publications

Recombinant Antigens To DetectToxoplasma gondii-Specific Immunoglobulin G and Immunoglobulin M in Human Sera by Enzyme Immunoassay

Recombinant Antigens To DetectToxoplasma gondii-Specific Immunoglobulin G and Immunoglobulin M in Human Sera by Enzyme Immunoassay

Expression, purification, and improved antigenic specificity of a truncated recombinant bp26 protein of Brucella melitensis M5‐90: a potential antigen for differential serodiagnosis of brucellosis in sheep and goats

Cellular and humoral immune responses to recombinant antigens in sheep infected with Toxoplasma gondii

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