Immune Response on the Administration of Recombinant Protein Antibodies Ag-38 Kda Mycobacterium Tuberculosis and Rifampicin Ex-Vivo.

Raras, Tri Yudhani Mardining; Fahrinda, Almira; Yuliati, Yuliati; Nurhidayati, Dwi Yuni; Sujuti, Hidayat; Prawiro, Sumarno Reto

doi:10.21010/ajid.v16i2.8

AJID

2022

DOI: 10.21010/ajid.v16i2.8

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Immune Response on the Administration of Recombinant Protein Antibodies Ag-38 Kda Mycobacterium Tuberculosis and Rifampicin Ex-Vivo.

Tri Yudhani Mardining Raras

Almira Fahrinda²,

Yuliati Yuliati³

et al.

Abstract: Background: Development a granuloma model resembling latent tuberculosis in vitro is needed with a fast and efficient time to be used as an effective therapy. This study aimed to form efficient granulomas, increase cellular immunity and humoral immunity, and evaluate growth on media using recombinant protein antibody Ag38kDa, Rifampicin, and a combination of both. Peripheral Blood Mononuclear Cell (PBMC) in vitro is derived from a healthy individual separated from monocytes and lymphocytes. Materials and meth… Show more

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2024

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Cited by 2 publications

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Preliminary Test of Candidate Rapid Diagnostic Test for the Detection of 38 kDa Mycobacterium Tuberculosis Antigen in Saliva

Mardining Raras,

Rahmadani,

Arthamin

et al. 2024

TOBIOTJ

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Background and Objectives Identifying tuberculosis (TB) in pediatric cases is a major challenge in developing countries, as children have problems with expelling sputum, making specific diagnostics crucial. The objective of the study was to develop a rapid test using polyclonal antibodies to detect antigen 38kDa from Mycobacterium tuberculosis in the saliva of TB patients. Materials and Methods The recombinant protein Ag38 was purified using the Ni-NTA purification kit. Polyclonal antibodies were generated in BALB-c mice using 50 µg/ml of purified Ag38 recombinant protein. A Lateral Flow Assay (LFA) was constructed, employing 5 mg/mL colloidal gold-labelled polyclonal antibody anti-Ag38 in the test line to capture the conjugates, while goat anti-mouse IgG was used in the control line. The LFA was tested in 5 TB patients and 7 healthy person served as negative control . Results The recombinant protein achieved 95% purity. The rapid test kit, with a detection limit of 5.3 µg/mL, successfully identified Ag38 protein in TB patient saliva (positive control) and not in healthy human serum (negative control). While reproducibility was confirmed for TB patients, results were inconsistent for healthy individuals. Conclusion The Lateral Flow Assay using polyclonal antibody Ag38 displays promise in detecting M tuberculosis antigen in the saliva of TB patients. Further validation with more TB patient saliva samples is needed to determine LFA sensitivity and specificity.

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Preliminary Test of Candidate Rapid Diagnostic Test for the Detection of 38 kDa Mycobacterium Tuberculosis Antigen in Saliva

Mardining Raras,

Rahmadani,

Arthamin

et al. 2024

TOBIOTJ

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Detection of Recombinant Antigen 38 and Epitope Antigen 38 Antibody as Humoral Immune Response of Tuberculosis as a New Marker of Tuberculous Meningitis

Munir,

Santosaningsih,

Nur Hidayati

et al. 2024

RJPT

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Antigen 38(PstS-1), is a lipoprotein secreted by M. tb and capable of enhancing B and T cell responses with high specificity. Previous study of recombinantantigen 38(RecAg38) from Mycobacterium tuberculosis local strain showed high homology of M.tb. Epitope is playinga significant role in the diagnosis of TB and TB meningitis. Previous study, antigen 38 could be detected in liquor cerebrospinal (LCS) tuberculosis meningitis in children. The purpose of this study was to prove recombinant antigen 38 and epitope antigen 38 can induce IgG and IgM antibodies. RecAg38 was overexpressed in E. coli BL21-(DE-3) strains. The purity of antigen was verified using SDS-PAGE and Western Blot. Using bioinformatic two dominant epitope antigen 38 was identified: QGTIKTWDDPQIAALNPGVNLP and Both antigen 38 and two dominant epitopes were used to immunize mice. As many as 12 male mice were divided into two groups. Group 1 received 50ug/0,3ml Antigen 38 intra peritoneal, whereas group 2 received 50ug/0,3 ml epitope. Booster at week 2,3, and 4. Detection of antibodies was conducted using ELISA assay. The results showed that Ag38 rec as well as epitopes of Ag38 rec could induce the synthesis of antibody IgG and IgM. the highest OD (Optical Density) value of IgG and IgM antibodies was 3,508 and 1,368 upon induction with Ag38 protein. Groups with an antibody concentration of 1/1000 and an antigen concentration of 10ug/mL. The highest OD IgM antibodies it was 1,368 in the peptide epitope dominant group 2 with an antibody concentration of 1/5000 and an antigen concentration of 10ug/mL. The conclusion is that recombinant protein and epitope antigen 38 has capacity to induce IgG antibodies, IgM in in vivo a hence potential to be used as a marker tuberculosis diagnosis test and candidate a biomarker for the diagnosis of TB meningitis.

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Immune Response on the Administration of Recombinant Protein Antibodies Ag-38 Kda Mycobacterium Tuberculosis and Rifampicin Ex-Vivo.

Cited by 2 publications

References 28 publications

Preliminary Test of Candidate Rapid Diagnostic Test for the Detection of 38 kDa Mycobacterium Tuberculosis Antigen in Saliva

Preliminary Test of Candidate Rapid Diagnostic Test for the Detection of 38 kDa Mycobacterium Tuberculosis Antigen in Saliva

Detection of Recombinant Antigen 38 and Epitope Antigen 38 Antibody as Humoral Immune Response of Tuberculosis as a New Marker of Tuberculous Meningitis

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