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  • 11
    Publication Date: 2019-06-27
    Description: A coding technique is developed for recording computer generated holograms on a computer controlled CRT in which each resolution cell contains two beam spots of equal size and equal intensity. This provides a binary hologram in which only the position of the two dots is varied from cell to cell. The amplitude associated with each resolution cell is controlled by selectively diffracting unwanted light into a higher diffraction order. The recording of the holograms is fast and simple.
    Keywords: COMMUNICATIONS
    Type: Applied Optics; 11; Nov. 197
    Format: text
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  • 12
    Publication Date: 2019-06-27
    Description: A method for processing multispectral data is provided, which permits an operator to make parameter level changes during the processing of the data. The system is directed to production of a color classification map on a video display in which a given color represents a localized region in multispectral feature space. Interactive controls permit an operator to alter the size and change the location of these regions, permitting the classification of such region to be changed from a broad to a narrow classification.
    Keywords: COMMUNICATIONS AND RADAR
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  • 13
    Publication Date: 2019-08-14
    Description: No abstract available
    Keywords: Plasma Physics
    Type: PLASMA RES. LAB. TECH. REPT. 3 , HQ-E-DAA-TN46324
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  • 14
    Publication Date: 2019-08-14
    Description: No abstract available
    Keywords: Plasma Physics
    Type: HQ-E-DAA-TN45107 , PLASMA RES. LAB. TECH. REPT. 2
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  • 15
    Publication Date: 2019-07-13
    Description: The objective of the present study was to define the optimum conditions for using replication-defective adenovirus (Ad) to transfer the gene for the green fluorescent protein (GFP) to the hypothalamic paraventricular (PVN) and supraoptic (SON) nuclei and cells of the neurohypophysis (NH). As indicated by characterizing cell survival over 15 days in culture and in electrophysiological whole cell patch-clamp studies, viral concentrations up to 2 x 10(7) pfu/coverslip did not affect viability of transfected PVN and NH cultured cells from preweanling rats. At 2 x 10(7) pfu, GFP gene expression was higher (40% of GFP-positive cells) and more sustained (up to 15 days). Using a stereotaxic approach in adult rats, we were able to directly transduce the PVN, SON, and NH and visualize gene expression in coronal brain slices and in the pituitary 4 days after injection of Ad. In animals receiving NH injections of Ad, the virus was retrogradely transported to PVN and SON neurons as indicated by the appearance of GFP-positive neurons in cultures of dissociated cells from those brain nuclei and by polymerase chain reaction and Western blot analyses of PVN and SON tissues. Adenoviral concentrations of up to 8 x 10(6) pfu injected into the NH did not affect cell viability and did not cause inflammatory responses. Adenoviral injection into the pituitary enabled the selective delivery of genes to the soma of magnocellular neurons. The experimental approaches described here provide potentially useful strategies for the treatment of disordered expression of the hormones vasopressin or oxytocin. Copyright 2000 Academic Press.
    Keywords: Life Sciences (General)
    Type: Experimental neurology (ISSN 0014-4886); 167; 2; 260-71
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  • 16
    Publication Date: 2019-07-13
    Description: The present studies used defined cells of the subfornical organ (SFO) and supraoptic nuclei (SON) as model systems to demonstrate the efficacy of replication-deficient adenovirus (Ad) encoding green fluorescent protein (GFP) for gene transfer. The studies investigated the effects of both direct transfection of the SON and indirect transfection (i.e., via retrograde transport) of SFO neurons. The SON of rats were injected with Ad (2 x 10(6) pfu) and sacrificed 1-7 days later for cell culture of the SON and of the SFO. In the SON, GFP fluorescence was visualized in both neuronal and nonneuronal cells while only neurons in the SFO expressed GFP. Successful in vitro transfection of cultured cells from the SON and SFO was also achieved with Ad (2 x 10(6) to 2 x 10(8) pfu). The expression of GFP in in vitro transfected cells was higher in nonneuronal (approximately 28% in SON and SFO) than neuronal (approximately 4% in SON and 10% in SFO) cells. The expression of GFP was time and viral concentration related. No apparent alterations in cellular morphology of transfected cells were detected and electrophysiological characterization of transfected cells was similar between GFP-expressing and nonexpressing neurons. We conclude that (1) GFP is an effective marker for gene transfer in living SON and SFO cells, (2) Ad infects both neuronal and nonneuronal cells, (3) Ad is taken up by axonal projections from the SON and retrogradely transported to the SFO where it is expressed at detectable levels, and (4) Ad does not adversely affect neuronal viability. These results demonstrate the feasibility of using adenoviral vectors to deliver genes to the SFO-SON axis. Copyright 1998 Academic Press.
    Keywords: Life Sciences (General)
    Type: Experimental neurology (ISSN 0014-4886); 154; 2; 353-65
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  • 17
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    In:  Other Sources
    Publication Date: 2019-07-13
    Description: Nomographs for point source holographic imaging, discussing recording and reconstruction geometry
    Keywords: INSTRUMENTATION AND PHOTOGRAPHY
    Type: ; YAL SOCIETY (|FALL MEETING ON NOMOGRAPHS FOR HOLOGRAPHIC IMAGING; Sep 29, 1970 - Oct 02, 1970; HOLLYWOOD, FL
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