Your search keyword '"Tonge Ebai"' showing total 3 results

1. Accurate detection of Newcastle disease virus using proximity‐dependent DNA aptamer ligation assays

Author

Felipe Marques Souza de Oliveira, Tonge Ebai, Masood Kamali-Moghaddam, Issam Hmila, Boutheina Marnissi, Khouloud Khalfaoui, and Abdeljelil Ghram

Subjects

0301 basic medicine, rRT‐PCR, medicine.drug_class, Aptamer, Newcastle Disease, aptamers, Newcastle disease virus, Medical Biotechnology (with a focus on Cell Biology (including Stem Cell Biology), Molecular Biology, Microbiology, Biochemistry or Biopharmacy), Monoclonal antibody, Real-Time Polymerase Chain Reaction, Sensitivity and Specificity, sandwich ELAA, General Biochemistry, Genetics and Molecular Biology, Virus, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, medicine, Animals, Medicinsk bioteknologi (med inriktning mot cellbiologi (inklusive stamcellsbiologi), molekylärbiologi, mikrobiologi, biokemi eller biofarmaci), lcsh:QH301-705.5, Research Articles, Detection limit, proximity ligation assays, Biochemistry and Molecular Biology, Reproducibility of Results, Amplicon, Aptamers, Nucleotide, Molecular biology, Reverse transcription polymerase chain reaction, 030104 developmental biology, rRT&#8208, PCR, chemistry, lcsh:Biology (General), 030220 oncology & carcinogenesis, Ligation, Nucleic Acid Amplification Techniques, DNA, Biokemi och molekylärbiologi, Research Article

Abstract

Detecting viral antigens at low concentrations in field samples can be crucial for early veterinary diagnostics. Proximity ligation assays (PLAs) in both solution and solid‐phase formats are widely used for high‐performance protein detection in medical research. However, the affinity reagents used, which are mainly poly‐ and monoclonal antibodies, play an important role in the performance of PLAs. Here, we have established the first homogeneous and solid‐phase proximity‐dependent DNA aptamer ligation assays for rapid and accurate detection of Newcastle disease virus (NDV). NDV is detected by a pair of extended DNA aptamers that, upon binding in proximity to proteins on the envelope of the virus, are joined by enzymatic ligation to form a unique amplicon that can be sensitively detected using real‐time PCR. The sensitivity, specificity, and reproducibility of the assays were validated using 40 farm samples. The results demonstrated that the developed homogeneous and solid‐phase PLAs, which use NDV‐selective DNA aptamers, are more sensitive than the sandwich enzymatic‐linked aptamer assay (ELAA), and have a comparable sensitivity to real‐time reverse transcription PCR (rRT‐PCR) as the gold standard detection method. In addition, the solid‐phase PLA was shown to have a greater dynamic range with improved lower limit of detection, upper‐ and lower limit of quantification, and minimal detectable dose as compared with those of ELAA and rRT‐PCR. The specificity of PLA is shown to be concordant with rRT‐PCR., Newcastle disease virus is detected by a pair of extended DNA aptamers that, upon binding in proximity to proteins on the envelope of the virus, are joined by enzymatic ligation to form a unique amplicon that can be sensitively detected using real‐time PCR.

Published

2021

2. Analytically Sensitive Protein Detection in Microtiter Plates by Proximity Ligation with Rolling Circle Amplification

Author

Johannes Haybaeck, Liza Löf, Ulrich Keilholtz, Ulf Landegren, Masood Kamali-Moghaddam, Lotta Wik, Caroline Schweiger, Tonge Ebai, Anders Larsson, and Felipe Marques Souza de Oliveira

Subjects

Male, 0301 basic medicine, Clinical Biochemistry, Enzyme-Linked Immunosorbent Assay, Protein detection, Growth Differentiation Factor 1, 03 medical and health sciences, 0302 clinical medicine, Limit of Detection, Neoplasms, Humans, Early Detection of Cancer, Volume concentration, Detection limit, Chromatography, Chemistry, Clinical Laboratory Medicine, Interleukins, Biochemistry (medical), Prostatic Neoplasms, Proteins, Nucleic acid amplification technique, Clinical routine, Molecular biology, 3. Good health, Klinisk laboratoriemedicin, 030104 developmental biology, Rolling circle replication, Ligation, Antibodies, Immobilized, Nucleic Acid Amplification Techniques, 030217 neurology & neurosurgery

Abstract

BACKGROUND Detecting proteins at low concentrations in plasma is crucial for early diagnosis. Current techniques in clinical routine, such as sandwich ELISA, provide sensitive protein detection because of a dependence on target recognition by pairs of antibodies, but detection of still lower protein concentrations is often called for. Proximity ligation assay with rolling circle amplification (PLARCA) is a modified proximity ligation assay (PLA) for analytically specific and sensitive protein detection via binding of target proteins by 3 antibodies, and signal amplification via rolling circle amplification (RCA) in microtiter wells, easily adapted to instrumentation in use in hospitals. METHODS Proteins captured by immobilized antibodies were detected using a pair of oligonucleotide-conjugated antibodies. Upon target recognition these PLA probes guided oligonucleotide ligation, followed by amplification via RCA of circular DNA strands that formed in the reaction. The RCA products were detected by horseradish peroxidase-labeled oligonucleotides to generate colorimetric reaction products with readout in an absorbance microplate reader. RESULTS We compared detection of interleukin (IL)-4, IL-6, IL-8, p53, and growth differentiation factor 15 (GDF-15) by PLARCA and conventional sandwich ELISA or immuno-RCA. PLARCA detected lower concentrations of proteins and exhibited a broader dynamic range compared to ELISA and iRCA using the same antibodies. IL-4 and IL-6 were detected in clinical samples at femtomolar concentrations, considerably lower than for ELISA. CONCLUSIONS PLARCA offers detection of lower protein levels and increased dynamic ranges compared to ELISA. The PLARCA procedure may be adapted to routine instrumentation available in hospitals and research laboratories.

Published

2017

3. Detecting individual extracellular vesicles using a multicolor in situ proximity ligation assay with flow cytometric readout

Author

K. Göran Ronquist, Tonge Ebai, Ulf Landegren, Lotta Wik, Louise Dubois, Olivia Nolander, Masood Kamali-Moghaddam, Liza Löf, Ola Söderberg, and Emma Lundin

Subjects

0301 basic medicine, In situ, Multidisciplinary, medicine.diagnostic_test, Cell- och molekylärbiologi, Proximity ligation assay, Biology, Extracellular vesicles, Molecular medicine, Article, Flow cytometry, Cell biology, 03 medical and health sciences, Cell and molecular biology, 030104 developmental biology, 0302 clinical medicine, Qualitative analysis, Flow (mathematics), 030220 oncology & carcinogenesis, medicine, Cell and Molecular Biology

Abstract

Flow cytometry is a powerful method for quantitative and qualitative analysis of individual cells. However, flow cytometric analysis of extracellular vesicles (EVs) and the proteins present on their surfaces has been hampered by the small size of the EVs – in particular for the smallest EVs, which can be as little as 40 nm in diameter, the limited number of antigens present and their low refractive index. We addressed these limitations for detection and characterization of EV by flow cytometry through the use of multiplex and multicolor in situ proximity ligation assays (in situ PLA), allowing each detected EV to be easily recorded over background noise using a conventional flow cytometer. By targeting sets of proteins on the surface that are specific for distinct classes of EVs, the method allows for selective recognition of populations of EVs in samples containing more than one type of EVs. The method presented herein opens up for analyses of EVs using flow cytometry for their characterization and quantification.

Published

2016