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Image Search Results
Journal: Frontiers in Microbiology
Article Title: A Multiplex Immunosensor for Detecting Perchlorate-Reducing Bacteria for Environmental Monitoring and Planetary Exploration
doi: 10.3389/fmicb.2020.590736
Figure Lengend Snippet: PRBCHIP, an antibody microarray for detecting perchlorate reducing bacteria. (A) Schematic of the antibody printing pattern layout (by triplicate) in the PRBCHIP as indicated in and in Section “Materials and Methods.” Empty circles correspond to a serial dilution of a fluorescent antibody printed as a control for fluorescence (marked with a yellow dashed line); circles 1–20 represent antibodies raised against different strains; circles 21–24 indicate antibodies produced against proteins (red rectangles); P1–P20 indicate their corresponding pre-immune antibodies (marked with a continuous yellow line); circles labeled as B (BSA) and PP (Protein Printing Buffer) were used as negative control spots. (B,C) Images obtained after fluorescence sandwich microarray immunoassay (FSMI) with PRBCHIP by using cell lysates of Magnetospirillum bellicus VDY (B) and Dechlorobacter hydrogenophilus LT-1 (C) strains as sample. Immunoassays were revealed with anti- M. bellicus VDY (L2C1) and anti- D. hydrogenophilus LT- 1 (L4C1) antibodies, respectively. (D,E) Images obtained for the same samples and revealed with TOP-PRB fluorescent mix, made up of all anti-PRB antibodies shown in plus A-Cld and A-PCR antibodies. Red and white spots are fluorescence signals corresponding to positive immunodetections.
Article Snippet: The
Techniques: Microarray, Bacteria, Serial Dilution, Control, Fluorescence, Produced, Labeling, Negative Control
Journal: Frontiers in Microbiology
Article Title: A Multiplex Immunosensor for Detecting Perchlorate-Reducing Bacteria for Environmental Monitoring and Planetary Exploration
doi: 10.3389/fmicb.2020.590736
Figure Lengend Snippet: Testing the PRBCHIP sensitivity by fluorescent sandwich microarray immunoassay (FSMI). We assayed serial dilutions of cell cultures as samples for FSMI using their corresponding fluorescent antibodies or the TOP-PRB mix. The fluorescent signals in the microarray were quantified and plotted against the sample concentration. (A) Example of the calibration curve for antibody L1C1 raised against Azospira suillum PS and revealed with its tracer antibody and (B) with the TOP-PRB mix, respectively. When Azospira suillum PS was used as tested sample, besides L1C1 (black circles) and L1S2 (white circles), also L8C1 (triangles) showed a comparable signal at high sample concentrations. (C) Calibration curve for the antibody L4C1 raised against D. hydrogenophilus LT-1 revealed with its tracer antibody and (D) revealed with the TOP-PRB mix. In this case, only L4C1 showed positive immunodetections.
Article Snippet: The
Techniques: Microarray, Concentration Assay
Journal: Frontiers in Microbiology
Article Title: A Multiplex Immunosensor for Detecting Perchlorate-Reducing Bacteria for Environmental Monitoring and Planetary Exploration
doi: 10.3389/fmicb.2020.590736
Figure Lengend Snippet: Testing the specificity of the antibodies with the PRBCHIP. Immunogens corresponding to whole-cell extracts of each perchlorate reducing strain, its EPS fractions and proteins were tested by FSMI with its corresponding fluorescent antibody at its appropriate working dilution (see section “Materials and Methods”). (A) Specificities and cross-reactions between different antibodies and immunogens. Microarray images were scanned for fluorescence, quantified and plotted in a heatmap. Each column corresponds to a single PRBCHIP assay with the corresponding strain or protein tested (see section “Materials and Methods”) as the immunogen, while each row represents the antibody code for each printed antibody (as in ) on the microarray. (B) Antibody graph G of 16 nodes (antibodies with low performance were not considered for this analysis) and 28 links associated with our antibody microarray. Each node represents one antibody. The link (arrow) from antibody j to antibody i represents cross-reactivity of weight G ij , where G ij is the extent of cross-reactivity between antibodies i and j referred to the cognate immunogen of antibody j . Self-loops ( G jj = 1) are not shown for clarity.
Article Snippet: The
Techniques: Microarray, Fluorescence
Journal: Frontiers in Microbiology
Article Title: A Multiplex Immunosensor for Detecting Perchlorate-Reducing Bacteria for Environmental Monitoring and Planetary Exploration
doi: 10.3389/fmicb.2020.590736
Figure Lengend Snippet: Deconvolution method applied to two complex natural samples by sandwich microarray immunoassay (FSMI). (A) Deconvolution of the American Pacific sample 140-10_07/07 and (B) deconvolution of the Lost Hammer sediment sample (LH-Sed) after performing both immunoassays with the mixture of all fluorescent-labeled tracer antibodies (TOP-PRB mix). Filled black bars represent the experimental fluorescence intensities F and red bars represent the deconvoluted signals F ′ [see (40–41) for details on obtaining F ′ from F and the matrix G associated to the antibody graph G]. Note that the experimental fluorescence intensities are ≥0 (as they were directly obtained from the FSMI), while the deconvoluted signals might be positive, zero or negative. Analyzing whether the experimental signal of each antibody is positive or close to zero and whether its deconvoluted signal is positive, zero or negative, we obtain a code for each organism (in bold) that yields reliable information about its existence or not in the sample [see supporting information of ].
Article Snippet: The
Techniques: Microarray, Labeling, Fluorescence
Journal: Ecotoxicology (London, England)
Article Title: Application of physiologically based modelling and transcriptomics to probe the systems toxicology of aldicarb for Caenorhabditis elegans (Maupas 1900)
doi: 10.1007/s10646-010-0591-z
Figure Lengend Snippet: Scores plot for PC1 and PC2 from a PCA of normalised whole genome microarray data for C. elegans exposed to control or 16 mg/l aldicarb
Article Snippet: Acquired
Techniques: Microarray, Control
Journal:
Article Title: A protein multiplex microarray substrate with high sensitivity and specificity
doi: 10.1016/j.jim.2010.10.005
Figure Lengend Snippet: The Multiplex Microarray format is as follows: A1= Hepatitis B Core, A2 = Hepatitis C Core, A3 = HTLV-I, A4 = HTLV-II, B1 = T. Palladium, B2 = HIV-1 IIIB, B3 = HIV-2, B4 = Human Serum Albumin, 25 μg/μl packed colloid C1 = Human IgG, 25 μg/μl packed colloid, C2 = Human IgG, 12 μg/μl packed colloid, C3 = Human IgG, 6μg/μl packed colloid and C4 = Human Serum Albumin, 25 μg/μl packed colloid
Article Snippet: Presented in , are developed
Techniques: Multiplex Assay, Microarray
Journal:
Article Title: A protein multiplex microarray substrate with high sensitivity and specificity
doi: 10.1016/j.jim.2010.10.005
Figure Lengend Snippet: Light microscope (40X) images of developed colloidal microarrays. The multiplex microarray format is as follows: Each spot in triplicate, Row 1 = anti-norovirus, Row 2 = anti-adenovirus 41 (type specific), Row 3 = anti-adenovirus 40 (type specific), Row 4 = anti-hexon of adenovirus (group specific), Row 5 anti-astrovirus and Row 6 anti-rotavirus.
Article Snippet: Presented in , are developed
Techniques: Light Microscopy, Multiplex Assay, Microarray
Journal: Journal of Cancer
Article Title: Construction and validation of a comprehensive metabolism-associated prognostic model for predicting survival and immunotherapy benefits in ovarian cancer
doi: 10.7150/jca.100796
Figure Lengend Snippet: The comparison of levels of signature genes expression in tumor and normal controls. (A) Differences of expression levels of the four signature genes among the normal ovarian tissues and Ovarian cancer tissues (TCGA and GTEx database). (B) The relative mRNA levels of the four signature genes between normal ovarian cell lines and OV cell lines. (C) The prognostic value of a 4 sigurenaure gene for patients in TCGA has been confirmed through Kaplan-Meier analysis. (D) The immunohistochemical staining of tissue microarray shows 4 signature genes expressions on protein level between OV and normal control tissues.
Article Snippet: OV and
Techniques: Comparison, Expressing, Immunohistochemical staining, Staining, Microarray, Control