ML0405 and ML2331 Are Antigens of<i>Mycobacterium leprae</i>with Potential for Diagnosis of Leprosy

Reece, Stephen T.; Ireton, Greg C.; Mohamath, Raodoh; Guderian, Jeffrey A.; Goto, Wakako; Gelber, Robert H.; Groathouse, Nathan A.; Spencer, John S.; Brennan, Patrick J.; Reed, Steven G.

doi:10.1128/cvi.13.3.333-340.2006

Cited by 62 publications

(59 citation statements)

References 30 publications

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“…The titres of IgG antibodies to protein antigens generally correlate with the bacterial load and strong responses in MB patients can rival anti-PGL-I responses. The best protein candidates to assess the IgG response include ML0405, ML2331, ML2055 (Reece et al 2006, Duthie et al 2007), ML2028 (Launois et al 1994) and ML2038 , Kai et al 2008. A bioinformatics analysis predicted ML0405 to be one of the most promiscuous M. leprae proteins studied to date and to contain T cell epitopes predicted to be recognised by 50 out of 51 human leukocyte antigen-DR alleles along with seven potential T cell epitopes and 39 potential B cell epitopes, whereas ML2331 contained 24 potential B cell epitopes (Sampaio et al 2011).…”

Section: Discussionmentioning

confidence: 99%

“…Cloning and purification of recombinant M. leprae proteins -DNA sequences encoding 12 full-length M. leprae proteins were cloned from genomic DNA as previously described (Spencer et al 2005, Reece et al 2006. Purified recombinant proteins were produced by the Infectious Disease Research Institute (IDRI), Seattle, WA or Colorado State University (CSU), Fort Collins, CO, USA.…”

Section: Subjects Materials and Methodsmentioning

confidence: 99%

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Identification of serological biomarkers of infection, disease progression and treatment efficacy for leprosy

Spencer

Duthie

Geluk

et al. 2012

Mem. Inst. Oswaldo Cruz

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Section: Discussionmentioning

confidence: 99%

Section: Subjects Materials and Methodsmentioning

confidence: 99%

Identification of serological biomarkers of infection, disease progression and treatment efficacy for leprosy

Spencer

Duthie

Geluk

et al. 2012

Mem. Inst. Oswaldo Cruz

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“…The expressed TR-containing proteins were analyzed for seroreactivity using panels of patient and control sera. L. infantum soluble lysate antigen (SLA) was used as a positive control and a Mycobacterium leprae antigen ML2331 was used as an irrelevant antigen (26). Proteins were diluted in an enzyme-linked immunosorbent assay (ELISA) coating buffer, and 96-well plates were coated with 1 g of L. infantum SLA or 200 ng of individual recombinant antigens, followed by blocking with phosphate-buffered saline containing 0.05% Tween 20 and 1% bovine serum albumin.…”

Section: Methodsmentioning

confidence: 99%

“…rLinJ11.0070r2 and rLinJ25.1100TR showed intermediate reactivity to the VL patient sera; none of the four antigens were recognized by sera from healthy donors. VL patient sera showed only a weak antibody response to an irrelevant Mycobacterium leprae antigen ML2331 (26). Compared to the reactivity of the irrelevant antigen, rLinJ11.0070r2, rLinJ25.1100TR, rLinJ27.0400r2, and rLinJ29.29.0110TR, as well as L. infantum SLA, showed significantly stronger reactivity to the VL patient sera, whereas rLinJ21.2010TR or LinJ32.3710TR did not detect VL-specific antibodies (P Ͻ 0.05 on rLinJ11.0070r2, P Ͻ 0.01 on rLinJ25.1100TR, and P Ͻ 0.001 on rLinJ27.0400r2, rLinJ29.29.0110TR, and L. infantum SLA by unpaired t test).…”

Section: Identification Of Tr Genes From a L Infantum Gene Databasementioning

confidence: 99%

Bioinformatic Identification of Tandem Repeat Antigens of the Leishmania donovani Complex

2007

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With large amounts of parasite gene sequence available, additional bioinformatic tools to screen these sequences for identifying genes encoding antigens are needed. Proteins containing tandem repeat (TR) domains are often B-cell antigens, and antibody responses toward TR domains of the proteins are dominant in human infected with certain parasites. We hypothesized that antigens of serological significance could be identified with a search for TR domains. Here we show the result of bioinformatic screening of the gene sequence database of the parasitic protozoan Leishmania infantum. Of 8,191 genes scanned, 64 genes contained TR domains. Of the 64 genes, 22 encoded previously characterized antigens; the remaining 42 genes were previously uncharacterized. By using sera from Sudanese visceral leishmaniasis patients, we confirmed that the TR domains of LinJ11.0070, LinJ25.1100, LinJ27.0400, and LinJ29.0110, which were from the 42 uncharacterized proteins, are also antigenic. The results suggest the validity of this approach for identifying leishmanial antigens of serological significance.

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“…Recombinant forms of some of the more significant native proteins were subsequently created and tested (22,27,37). Recently, several groups have also used a postgenomic approach to discover new antigens for leprosy diagnosis (1,2,28,36,37). These studies all exploited genomic sequence for the identification of M. leprae-specific proteins or peptides that may be suitable for serodiagnosis of different disease states of leprosy.…”

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confidence: 99%

Use of Protein Microarrays To Define the Humoral Immune Response in Leprosy Patients and Identification of Disease-State-Specific Antigenic Profiles

Groathouse¹,

Amin²,

Marques³

et al. 2006

Infect Immun

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Although the global prevalence of leprosy has decreased over the last few decades due to an effective multidrug regimen, large numbers of new cases are still being reported, raising questions as to the ability to identify patients likely to spread disease and the effects of chemotherapy on the overall incidence of leprosy. This can partially be attributed to the lack of diagnostic markers for different clinical states of the disease and the consequent implementation of differential, optimal drug therapeutic strategies. Accordingly, comparative bioinformatics and Mycobacterium leprae protein microarrays were applied to investigate whether leprosy patients with different clinical forms of the disease can be categorized based on differential humoral immune response patterns. Evaluation of sera from 20 clinically diagnosed leprosy patients using native protein and recombinant protein microarrays revealed unique disease-specific, humoral reactivity patterns. Statistical analysis of the serological patterns yielded distinct groups that correlated with phenolic glycolipid I reactivity and clinical diagnosis, thus demonstrating that leprosy patients, including those diagnosed with the paucibacillary, tuberculoid form of disease, can be classified based on humoral reactivity to a subset of M. leprae protein antigens produced in recombinant form.

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ML0405 and ML2331 Are Antigens ofMycobacterium lepraewith Potential for Diagnosis of Leprosy

Cited by 62 publications

References 30 publications

Identification of serological biomarkers of infection, disease progression and treatment efficacy for leprosy

Identification of serological biomarkers of infection, disease progression and treatment efficacy for leprosy

Bioinformatic Identification of Tandem Repeat Antigens of the Leishmania donovani Complex

Use of Protein Microarrays To Define the Humoral Immune Response in Leprosy Patients and Identification of Disease-State-Specific Antigenic Profiles

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