4,946 research outputs found

    Fabia felderi Species Novum, a New Pinnotherid Crab from the Central Eastern Coast of Florida (Crustacea: Decapoda: Brachyura)

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    Fabia felderi, a new species of pinnotherid crab collected from oculinid coral rubble in 80 m of water off the central eastern Florida coast, is described and illustrated from the unique holotypic male. The crab shows morphological similarities to some Pinnotheres species, as well as to two eastern Pacific species in the genus Fabia. All share a more or less subcircular carapace, a produced frontal region rimmed with a heavy fringe of hair, well developed setae along all pereopodal borders, and a generally similar positioning of the palp on the merus of maxilliped 3

    From Florida sand to The City Beautiful : a historical record of Orlando, Florida

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    Book on the history of Orlando by E.H. Gore, which details: early mayors, local newspapers, first churches, hospitals, schools, historical firsts, local industry and shops, early buildings, early pioneers, and the citrus industry

    Amplification and Potential Transformation of Human Syntaxin-17 into Model E. coli

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    Membrane fusion is key to organism homeostasis and occurs when a transport vesicle fuses with a target compartment, merging the two membranes into one while releasing the contents of the transport vesicle into the target compartment. This process is controlled by SNARE proteins. Syntaxin-17 protein plays a crucial role in the fusion of the autophagosome membrane with the lysosome membrane, allowing for degradation of misfolded intracellular components and pathogens. Intriguingly, Syntaxin 17 has been identified as a target of herpesvirus tegument proteins, although the pathological significance of the Syntaxin 17 and tegument protein interaction is unclear. As a first step towards characterizing the biochemical and functional interaction between the tegument proteins and the target SNARE, this study aimed to amplify and introduce the Syntaxin 17 cDNA into a model E. coli for production and purification of Syntaxin 17 protein. Amplified insert and vector cDNA of the correct size were obtained and verified via gel electrophoresis. Future research should focus on the transformation of the chimeric plasmid into competent E. coli. If isolates with the correct size insert were obtained, the next steps would be sequencing to confirm absence of mutation and procee

    Clonal analysis of a human antibody response. Quantitation of precursors of antibody-producing cells and generation and characterization of monoclonal IgM, IgG, and IgA to rabies virus.

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    We quantitated and characterized the changes in the human B cell repertoire, at the clonal level, before and after immunization with rabies virus. Moreover, we generated 10 monoclonal cell lines producing IgM, IgG, and IgA antibodies to the virus. We found that in healthy subjects, not previously exposed to the virus, nearly 2% of the circulating B lymphocytes were committed to the production of antibodies that bound the virus. These B cells expressed the surface CD5 molecule. The antibodies they produced were polyreactive IgM that displayed a relatively low affinity for the virus components (Kd, 1.0-2.4 x 10(-6) g/microliters). After immunization, different anti-virus (IgG and IgA) antibody-producing cells consistently appeared in the circulation and increased from less than 0.005% to greater than 10% of the total B cells committed to the production of IgG and IgA, respectively. Most of such B cells do not express CD5 and produce monoreactive antibodies of high affinity for rabies virus (Kd, 6.5 x 10(-9) to 1.2 x 10(-10) g/microliters). One of these IgG mAbs efficiently neutralized rabies virus in vitro and in vivo, as detailed elsewhere (Dietzschold, B., P. Casali, Y. Ueki, M. Gore, C. E. Rupprecht, A. L. Notkins, and H. Koprowski, manuscript submitted for publication). Hybridization experiments using probes specific for the different human V gene segment families revealed that cell precursors producing low affinity IgM binding to rabies virus utilized a restricted number of VH gene segments (i.e., only members of the VHIIIb subfamily), whereas cell precursors producing high affinity IgG and IgA to rabies virus utilized an assortment of different VH gene segments (i.e., members of the VHI, VHIII, VHIV, and VHVI families and VHIIIb subfamily). In conclusion, our studies show that EBV transformation in conjunction with limiting dilution technology and somatic cell hybridization techniques are useful methods for quantitating, at the B cell clonal level, the human antibody response to foreign Ags and for generating human mAbs of predetermined specificity and high affinity

    Notes

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    Concealment Behavior of the Spanish Lobster, Scyllarides nodifer (Stimpson), with Observations on its Diel Activity. By L. A. Ogren Notes of the Occurrence of the Silver Anchovy, Engraulis eurystole, in the Northern Gulf of Mexico. By R. W. Hastings Studies on Decapod Crustacea from the Indian River Region of Florida VII. A Field Character for Rapid Identification of the Swimming Crabs Callinectes ornatus Ordway, 1863 and C. similis Williams, 1966 (Brachyura, Portunidae). By R.H. Gor

    Investigation and study of a multi-aperture antenna system final report, 1 jan. - 1 apr. 1964

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    Multiple aperture adaptive antenna system for telemetry reception from remote space vehicle

    microRNA-10b enhances pancreatic cancer cell invasion by suppressing TIP30 expression and promoting EGF and TGF-β actions

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    Increased microRNA-10b (miR-10b) expression in the cancer cells in pancreatic ductal adenocarcinoma (PDAC) is a marker of disease aggressiveness. In the present study, we determined that plasma miR-10b levels are significantly increased in PDAC patients by comparison with normal controls. By gene profiling, we identified potential targets downregulated by miR-10b, including Tat-interacting protein 30 (TIP30). Immunoblotting and luciferase reporter assays confirmed that TIP30 was a direct miR-10b target. Downregulation of TIP30 by miR-10b or siRNA-mediated silencing of TIP30 enhanced epidermal growth factor (EGF)-dependent invasion. The actions of miR-10b were abrogated by expressing a modified TIP30 cDNA resistant to miR-10b. EGF-induced EGF receptor (EGFR) tyrosine phosphorylation and extracellular signal–regulated kinase phosphorylation were enhanced by miR-10b, and these effects were mimicked by TIP30 silencing. The actions of EGF in the presence of miR-10b were blocked by EGFR kinase inhibition with erlotinib and by dual inhibition of PI3K (phosphatidylinositol 3′-kinase) and MEK. Moreover, miR-10b, EGF and transforming growth factor-beta (TGF-β) combined to markedly increase cell invasion, and this effect was blocked by the combination of erlotinib and SB505124, a type I TGF-β receptor inhibitor. miR-10b also enhanced the stimulatory effects of EGF and TGF-β on cell migration and epithelial–mesenchymal transition (EMT) and decreased the expression of RAP2A, EPHB2, KLF4 and NF1. Moreover, miR-10b overexpression accelerated pancreatic cancer cell (PCC) proliferation and tumor growth in an orthotopic model. Thus, plasma miR-10b levels may serve as a diagnostic marker in PDAC, whereas intra-tumoral miR-10b promotes PCC proliferation and invasion by suppressing TIP30, which enhances EGFR signaling, facilitates EGF–TGF-β cross-talk and enhances the expression of EMT-promoting genes, whereas decreasing the expression of several metastasis-suppressing genes. Therefore, therapeutic targeting of miR-10b in PDAC may interrupt growth-promoting deleterious EGF–TGF-β interactions and antagonize the metastatic process at various levels

    Genome-Wide Association Study and Pathway-Level Analysis of Kernel Color in Maize.

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    Rapid development and adoption of biofortified, provitamin A-dense orange maize (Zea mays L.) varieties could be facilitated by a greater understanding of the natural variation underlying kernel color, including as it relates to carotenoid biosynthesis and retention in maize grain. Greater abundance of carotenoids in maize kernels is generally accompanied by deeper orange color, useful for distinguishing provitamin A-dense varieties to consumers. While kernel color can be scored and selected with high-throughput, low-cost phenotypic methods within breeding selection programs, it remains to be well established as to what would be the logical genetic loci to target for selection for kernel color. We conducted a genome-wide association study of maize kernel color, as determined by colorimetry, in 1,651 yellow and orange inbreds from the Ames maize inbred panel. Associations were found with y1, encoding the first committed step in carotenoid biosynthesis, and with dxs2, which encodes the enzyme responsible for the first committed step in the biosynthesis of the isoprenoid precursors of carotenoids. These genes logically could contribute to overall carotenoid abundance and thus kernel color. The lcyE and zep1 genes, which can affect carotenoid composition, were also found to be associated with colorimeter values. A pathway-level analysis, focused on genes with a priori evidence of involvement in carotenoid biosynthesis and retention, revealed associations for dxs3 and dmes1, involved in isoprenoid biosynthesis; ps1 and vp5, within the core carotenoid pathway; and vp14, involved in cleavage of carotenoids. Collectively, these identified genes appear relevant to the accumulation of kernel color

    1848 La Fusion (Episode de la vie de Notre Venerable Pere) Deux Actes Avec Prologue

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    Regarding event in 1848. Written in 1949.https://dsc.duq.edu/spiritan-rc/1004/thumbnail.jp
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