Escherichia coli 8624 and the isogenic mutants in qseE, qseF and qseG are compared to determine the role that each of the genes play in regulation of the transcriptome. These results are verified by qRT-PCR and reveal the important role of this three-component signaling system.
The two-component system QseEF and the membrane protein QseG link adrenergic and stress sensing to bacterial pathogenesis.
No sample metadata fields
View SamplesPre-stimulation of MDMs with LPS (signals via MyD88 and TRIF dependent pathways) and PolyI:C (signals via a TRIF dependent pathway) leads to a reduced viral infection. In contrast, pre-stimulation with P3C (signals via MyD88 dependent pathway) does not lead to a reduced viral infection. This microarray was performed to find genes that are specifically upregulated in LPS and PolyI:C stimulated MDMs but not P3C stimulated MDMs. So to give us leads into the mechanism involved in the reduction of viral infection.
Bacterial lipopolysaccharide inhibits influenza virus infection of human macrophages and the consequent induction of CD8+ T cell immunity.
Specimen part, Treatment, Subject
View SamplesReports that low-intensity microwave radiation can induce heat-shock reporter gene expression in the nematode, Caenorhabditis elegans, have recently been reinterpreted as a subtle thermal effect caused by very slight heating. This study used a microwave exposure system (1.0 GHz, 0.5 W power input; SAR 0.9-3 mW kg-1 for 6-well plates) that minimises the temperature differential between sham and exposed conditions to 0.1C. Comparable measurement and simulation studies of SAR distribution within this exposure system are presented. We compared 5 Affymetrix gene-arrays of pooled triplicate RNA populations from sham-exposed L4/adult worms against 5 gene-arrays of pooled RNA from microwave-exposed worms (taken from the same source population in each run). Few genes showed consistent expression changes across all 5 comparisons, and all such expression changes appeared modest after applying standard normalisation procedures ( 30% up- or down-regulated). The number of statistically significant differences in gene expression (846) was less than the false-positive rate expected by chance (1131). As one example, an apparent up-regulation of the vit-3 vitellogenin gene by microwave exposure was not mirrored by similar changes affecting the other co-regulated members of the same vit gene family. We conclude that the pattern of gene expression in L4/adult C elegans is not substantially perturbed by low-intensity microwave radiation, and that the minor changes observed in this study may well be explicable as false positives. As a check on the sensitivity of the Affymetrix gene-arrays used, we also compared RNA samples from N2 worms subjected to a sub-heat-shock treatment (28C) against controls kept at 26 C (but using only 2 gene arrays per condition). After similar normalisation, many more genes (3712) showed substantial expression changes (i.e. > 2-fold at p < 0.05), including a group of six heat-shock genes which were strongly but unexpectedly down-regulated (by > 10-fold). However, further replication and confirmation by real-time RT-PCR would be needed to establish how many of these changes might also be false positives.
Low-intensity microwave irradiation does not substantially alter gene expression in late larval and adult Caenorhabditis elegans.
No sample metadata fields
View SamplesAirway epithelial cells and macrophages differ markedly in their responses to influenza A virus (IAV) infection. To investigate transcriptional responses underlying these differences, purified subsets of type II airway epithelial cells (ATII) and alveolar macrophages (AM) recovered from the lungs of mock- or IAV-infected mice were subjected to RNA sequencing. In the absence of infection, AM predominantly expressed genes related to immunity whereas ATII expressed genes consistent with their physiological roles in the lung. Following IAV infection, AM almost exclusively activated cell-intrinsic antiviral pathways that were dependent on interferon regulatory factor (IRF)3/7 and/or type I interferon (IFN) signaling. In contrast, IAV-infected ATII activated a broader range of physiological responses, including cell-intrinsic antiviral pathways, which were both independent and dependent on IRF3/7 and/or type I IFN. These data suggest that transcriptional profiles hardwired during development could be a major determinant underlying the different responses of ATII and AM to IAV infection. Overall design: 96 samples were analyzed: (A) 4 replicates of HA+ Alveolar Macrophage (AM) and 4 replicates of CD103+ Dendritic cells (DC) isolated from the lung lobes of C57/BL6 mice on 9 h p.i. with PR8. 4 replicates of mock-infected (HA-) AM and 4 replicates of mock-infected (HA-) CD103+ DC isolated from the lung lobes of mock-infected C57/BL6 mice on 9 h p.i. with allantoic fluid of equal dilution as PR8. 4 replicates of HA+ Airway epithelial cell Type II (ATII) and 4 replicates of HA+ Ciliated Cell (CC) isolated from the lung lobes of C57/BL6 mice on 9 h p.i. with PR8. 4 replicates of mock-infected (HA-) ATII and 4 replicates of mock-infected (HA-) CC isolated from the lung lobes of mock-infected C57/BL6 mice on 9 h p.i. with allantoic fluid of equal dilution as PR8. (B) 4 replicates of HA+ AM and 4 replicates of CD103+ DC isolated from the lung lobes of IFNAR2-/- mice on 9 h p.i. with PR8. 4 replicates of mock-infected (HA-) AM and 4 replicates of mock-infected (HA-) CD103+ DC isolated from the lung lobes of mock-infected IFNAR2-/- mice on 9 h p.i. with allantoic fluid of equal dilution as PR8. 4 replicates of HA+ ATII and 4 replicates of HA+ CC isolated from the lung lobes of IFNAR2-/- mice on 9 h p.i. with PR8. 4 replicates of mock-infected (HA-) ATII and 4 replicates of mock-infected (HA-) CC isolated from the lung lobes of mock-infected IFNAR2-/- mice on 9 h p.i. with allantoic fluid of equal dilution as PR8. (C) 4 replicates of HA+ AM and 4 replicates of CD103+ DC isolated from the lung lobes of IRF3/7-/- mice on 9 h p.i. with PR8. 4 replicates of mock-infected (HA-) AM and 4 replicates of mock-infected (HA-) CD103+ DC isolated from the lung lobes of mock-infected IRF3/7-/- mice on 9 h p.i. with allantoic fluid of equal dilution as PR8. 4 replicates of HA+ ATII and 4 replicates of HA+ CC isolated from the lung lobes of IRF3/7-/- mice on 9 h p.i. with PR8. 4 replicates of mock-infected (HA-) ATII and 4 replicates of mock-infected (HA-) CC isolated from the lung lobes of mock-infected IRF3/7-/- mice on 9 h p.i. with allantoic fluid of equal dilution as PR8.
Unique Transcriptional Architecture in Airway Epithelial Cells and Macrophages Shapes Distinct Responses following Influenza Virus Infection <i>Ex Vivo</i>.
Specimen part, Subject
View SamplesGoal was to detect differences in response to TLR7 versus TLR8 agonists in human monocytes from healthy donors
Granzyme B expression is enhanced in human monocytes by TLR8 agonists and contributes to antibody-dependent cellular cytotoxicity.
Specimen part, Treatment, Subject
View SamplesThere are currently no biological tests that differentiate patients with bipolar disorder (BPD) from healthy controls. While there is evidence that peripheral gene expression differences between patients and controls can be utilized as biomarkers for psychiatric illness, it is unclear whether current use or residual effects of antipsychotic and mood stabilizer medication drives much of the differential transcription. We therefore tested whether expression changes in first-episode, never-medicated bipolar patients, can contribute to a biological classifier that is less influenced by medication and could potentially form a practicable biomarker assay for BPD.
Utilization of never-medicated bipolar disorder patients towards development and validation of a peripheral biomarker profile.
Sex, Age, Specimen part
View SamplesWe are examining the genes that control initiation and progression of murine medulloblastomas that result from loss of patched. Approximately 25% of human medulloblastomas have mutations in patched or in other elements of the sonic hedgehog pathway. However, the cells from which these tumors originate (neural progenitors or stem cells), the cells that are responsible for tumor propagation (cancer stem cells), and the genes that are required for tumor progression are poorly understood. To address these questions, we have developed conditional patched knockout mice in which the gene is deleted in neural stem cells or progenitors. In addition, we have isolated a population of tumor-propagating cells from these tumors. By studying these models we will gain insight into the mechanisms of tumorigenesis and identify new targets for therapy.
Identification of CD15 as a marker for tumor-propagating cells in a mouse model of medulloblastoma.
No sample metadata fields
View SamplesSUMMARY
Loss of patched and disruption of granule cell development in a pre-neoplastic stage of medulloblastoma.
No sample metadata fields
View SamplesCD14+ monocytes sorted from the synovial fluid or peripheral blood of rheumatoid arthritis patients were analyzed by full transcriptome microarray analysis. Monocytes from healthy control samples (peripheral blood) were also profiled.
MicroRNA-155 contributes to enhanced resistance to apoptosis in monocytes from patients with rheumatoid arthritis.
Specimen part, Disease, Disease stage, Subject
View SamplesDystonia is characterized by involuntary muscle contractions. Its many forms are genetically, phenotypically and etiologically diverse and it is unknown whether their pathogenesis converges on shared pathways. Mutations in THAP1, a zinc-finger transcription factor, cause DYT6, but its neuronal targets and functions are unknown. We used RNA-Seq to assay the in vivo effect of a heterozygote Thap1C54Y or ?Exon2 allele on the gene transcription signatures in neonatal mouse striatum and cerebellum. Enriched pathways and gene ontology terms include eIF2a Signaling, Mitochondrial Dysfunction, Neuron Projection Development, Axonal Guidance Signaling, and Synaptic Long Term Depression pathways, which are dysregulated in a genotype and tissue-dependent manner. Electrophysiological and neurite outgrowth assays confirmed the functional significance of those findings. Notably, several of these pathways were recently implicated in other forms of inherited dystonia, including DYT1. We conclude that dysfunction of these pathways may represent a point of convergence on the pathogenesis of unrelated forms of inherited dystonia. Overall design: We used RNA-Seq to assay the in vivo effect of a heterozygote Thap1C54Y or deltaExon2 allele on the gene transcription signatures in neonatal mouse striatum and cerebellum
Mutations in THAP1/DYT6 reveal that diverse dystonia genes disrupt similar neuronal pathways and functions.
Specimen part, Cell line, Subject
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