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New England Biolabs
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myPOLS Biotec
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Image Search Results
Journal: Molecular Medicine
Article Title: Glabridin improves autoimmune disease in Trex1-deficient mice by reducing type I interferon production
doi: 10.1186/s10020-023-00754-y
Figure Lengend Snippet: Glab inhibits the activation of the cGAS-STING pathway by disrupting the STING-IRF3 interaction. A Transfection of Flag-tagged plasmids (Flag-MAVS, Flag-STING, Flag-TBK1 and Flag-IRF3) into HEK-293 cells for 12 h, and then treated with vehicle, Glab (20 μM) for 6 h. Whole cell lysates were collected and immunoblotted with the indicated antibody. Samples for qPCR were detected by qPCR assay for the expression of IFN-β mRNA. B BMDMs were first treated with DMSO or Glab (20 μM) for 1 h and then stimulated with cGAMP for 2 h. The expression of STING and the oligomerization of SITNG in the cell lysate were analyzed by Western blot with the indicated antibodies. C and D HEK-293 T cells were transfected with Flag-tagged plasmids (Flag-Vector, Flag-IRF3 and Flag-TBK1) and HA-tagged plasmids (HA-Vector and HA-STING) for 20 h, then treated with Glab (20 μM) for 6 h and immunoprecipitated with Anti-FLAG® M2 Affinity Gel, as shown by Western Blots analysis. Data in A are expressed as mean ± SEM (n = 3/group, from three biological replicates.). one-way ANOVA and Dunnett’s post hoc test were used to assess differences among groups, * p < 0.05, ** p < 0.01 and *** p < 0.001 vs. the control, NS, not significant
Article Snippet:
Techniques: Activation Assay, Transfection, Expressing, Western Blot, Plasmid Preparation, Immunoprecipitation, Control
Journal: Molecular Medicine
Article Title: Glabridin improves autoimmune disease in Trex1-deficient mice by reducing type I interferon production
doi: 10.1186/s10020-023-00754-y
Figure Lengend Snippet:
Article Snippet:
Techniques: Protease Inhibitor, Enzyme-linked Immunosorbent Assay, Transfection, SYBR Green Assay
Journal: medRxiv
Article Title: Detection of SARS-CoV-2 from raw patient samples by coupled high temperature reverse transcription and amplification
doi: 10.1101/2020.05.19.20103150
Figure Lengend Snippet: Schematic overview of the SARS-CoV-2 genome. The target sequences for the N1 primers and probe are marked in red and green, respectively. The R2 primer binding sequence is underlined. Sequences divergence between SARS-CoV-2 and SARS-CoV-1 genomes are highlighted in blue. B) Performance of Volcano3G polymerase was compared to Taq polymerase using plasmid DNA or in vitro transcribed RNA as template (5000 viral genome equivalents). C) Determination of the linear dynamic range for the Volcano3G protocol with or without an additional primer (R2) for optimized reverse transcription at a final concentration of 250 nM. In vitro transcribed RNA containing the Sars-CoV-2 N amplicon was serially diluted in the range from 1×10 6 copies to 10 copies. D) Limit of detection (LOD) was assessed with serial dilutions ranging from 20 to 1 copy per reaction (n = 6 for each dilution). The fraction of positive reactions (y-axis) were plotted against the log-transformed number of RNA copies per reaction. Addition of R2 primer enhances the performance at lower copy-numbers. E) Amplification curves showing the performance of Volcano3G on isolated RNA from two COVID-19 patients in presence or absence of R2.
Article Snippet: AM, RK are founders of and employed by
Techniques: Binding Assay, Sequencing, Plasmid Preparation, In Vitro, Concentration Assay, Amplification, Transformation Assay, Isolation
Journal: medRxiv
Article Title: Detection of SARS-CoV-2 from raw patient samples by coupled high temperature reverse transcription and amplification
doi: 10.1101/2020.05.19.20103150
Figure Lengend Snippet: A ) RNA was isolated from nasopharyngeal- and throat swab samples (n = 43) and SARS-CoV-2 and RNAseP were detected using the Volcano3G protocol. N1 amplicon (blue), RNaseP gene (gray). Water was used as a non-template control (light gray). B) Identical samples were processed in parallel in an accredited diagnostic lab using the Allplex 2019-nCoV assay from Seegene. Direct comparison of assay results reveals 100% concordance of Volcano3G with the reference assay. C) Cq values obtained with Volcano3G were lower than those obtained with the reference assay (ΔCq = 6.4 +/− 0.78). D) For each positive patient sample, the Cq values obtained with both assays were plotted against each other for linear regression analysis. A highly significant correlation of Volcano3G with the reference assay was observed (r 2 = 0.98, p<0.0001).
Article Snippet: AM, RK are founders of and employed by
Techniques: Isolation, Amplification, Diagnostic Assay
Journal: medRxiv
Article Title: Detection of SARS-CoV-2 from raw patient samples by coupled high temperature reverse transcription and amplification
doi: 10.1101/2020.05.19.20103150
Figure Lengend Snippet: A) Nasopharyngeal- and throat swab samples (prepared in water) were added directly as template for RT-qPCR using the Volcano3G protocol. Representative amplification curves of patients with high (dark blue), medium (medium blue) and low Cq as well as negative patients (light blue) are shown. B) RNA was isolated from the remaining patient material and analysed in an accredited diagnostic lab using the Allplex 2019-nCoV assay from Seegene. C) The Cq values of each patient sample are compared between the reference protocol and the Volcano3G direct approach. Dotted red line indicates the cut-off, were the assay loses sensitivity. D) For each positive patient sample, the Cq values obtained with both assays were plotted against each other for linear regression analysis (r 2 = 0.779, p<0.0001) E) RTPCR analysis of 100 copies of in vitro transcribed RNA spiked with varying amounts of pooled patient material from 5 confirmed negative patients. F) RT-PCR analysis of confirmed COVID-19 patient samples with high Cq values were analysed in a larger volume. G) Four confirmed COVID-19 patient samples and one negative control were used directly as in A). The reference cq-values obtained by standard RT-PCR from purified RNA (upper row) and the cq-values obtained by high temperature RT-PCR with Volcano3G polymerase (loer row) are given. After completion of PCR cycling, the reaction tubes were photographed on a blue light transilluminator (470 nm). Positive samples emitted a distinct green fluorescence visible by the naked eye.
Article Snippet: AM, RK are founders of and employed by
Techniques: Quantitative RT-PCR, Amplification, Isolation, Diagnostic Assay, Reverse Transcription Polymerase Chain Reaction, In Vitro, Negative Control, Purification, Fluorescence