266 resultados para Ehrlich
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Georg Ehrlich
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7 Briefe zwischen Edward Mead Earle, American Committee for International Studies, Princeton N. J. und Max Horkheimer, 1940-1941; 3 Briefe zwischen Margaret Ebert und Margot von Mendelssohn, 1941, 28.08.1941; 6 Briefe zwischen C. C. Eckhardt und Max Horkheimer, 1940; 5 Briefe zwischen Kay Eckstein und Max Horkheimer, 1940; 2 Briefe zwischen George Eckstein und Max Horkheimer, 16.05.1939, 35.05.1939; 1 Brief von F. K. Eden an Max Horkheimer, 02.04.1944; 33 Briefe zwischen Leopold Eder, Frieda Eder, Ruth Eder und Max Horkheimer, 1937-1940; 2 Briefe zwischen Dale Edwards und Max Horkheimer, 16.07.1940; 1 Brief von Hedwig Ehrlich an Max Horkheimer; 1 Brief von Max Horkheimer an Albert Einstein, 20.02.1935; 1 Brief von Max Horkheimer an W. Eisemann, 02.11.1939; 1 Brief von Else Eisner an Max Horkheimer, 09.12.1935; 2 Briefe zwischen Edit Elbogen und Max Horkheimer, 24.03.1942, 26.03.1942; 1 Brief von Käte von Hirsch an Max Horkheimer, 03.08.1941; 2 Briefe von Emmy Elbogen an Margot von Mendelssohn, 1945; 2 Briefe zwischen Paul Elbogen und Max Horkheimer, 02.06.1944, 09.06.1944; 4 Briefe zwischen Norbert Elias und Max Horkheimer, 1934-1935; 1 Brief von Werner B. Ellinger an Max Horkheimer, 16.12.1937; 19 Briefe zwischen dem Emergency Committee in Aid of Displaced Foreign Scholars New York und Max Horkheimer, 1938-1944; 2 Briefe zwischen dem Emergency Rescue Committee New York und Max Horkheimer, 12.06.1941, 14.06.1941; 1 Brief von F.L. Neumann an Emhardt, 13.02.1939; 23 Briefe zwischen Alice Engel und Max Horkheimer, 1937-1941; 9 briefe zwischen Paul Doernberg, Sofie Doernberg und Max Horkheimer, 1940-1942; 3 Briefe zwischen der Hebrew Sheltering and Immigrant Aid Society New York und Max Horkheimer, 05.01.1942, 1942; 1 Brief von der Selfhelp of Emigres from Central Europe, New York an Max Horkheimer, 18.08.1941; 2 Briefe zwischen R. Weissmann und Max Horkheimer, 09.01.1941, 03.02.1941; 5 Briefe zwischen Ernst Engelberg und Max Horkheimer, 1939-1940, 07.06.1939; 1 Brief von Fritz Epstein an Max Horkheimer, 10.04.1937; 1 Brief von Erika Ermel an Max Horkheimer, 15.09.1948; 2 Briefe zwischen Max Ernst und Max Horkheimer, 23.01.1936; 4 Briefe zwischen Margot Esser und Max Horkheimer, 1935-1936; 16 Briefe zwischen Rene Etiemble und Max Horkheimer, 1936-1938; 4 Briefe zwischen L.M. Ettlinger und Max Horkheimer, 1937; 8 Briefe zwischen Walter Fabien und Max Horkheimer, 1937-1941; 1 Brief von Max Horkheimer an Henry Pratt Fairchild, 25.03.1941; 2 Briefe zwischen Marvin Farber und Max Horkheimer, 14.03.1940, 17.05.1940; 4 Briefe zwischen Walter Farley udn Max Horkheimer, 1935, 01.10.1935; 8 Briefe zwischen Alexander Farquharson und Max Horkheimer, 1935-1939;
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In hebr. Schr.
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von Eugen Ehrlich
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von Moriz Ehrlich
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von Arnold B. Ehrlich
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Paul de Kruif is credited with being one of the first popular science writers for the general public. He received his Ph.D. from the University of Michigan in 1916 and worked at the Rockefeller Institute under Simon Flexner. After being fired in 1922 for publishing a scathing article on medical research, de Kruif caught the attention of Sinclair Lewis, who used his scientific background to write his Pulitzer Prize winning novel, Arrowsmith. In 1926, de Kruif published Microbe Hunters which recounted the exploits and discoveries of 14 renowned microbiologists from von Leeuwenhoek to Pasteur, Ross, Paul Ehrlich and Walter Reed. Microbe Hunters became a best seller, was translated into 18 languages, and formed the basis of two Hollywood movies, "Yellow Jack" and "The Magic Bullet." Generations of young readers were captivated by the vivid protrayal of these men and their discoveries.
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We report the development of a practical ultrafast allelic profiling assay for the analysis of short tandem repeats (STRs) by using a highly optimized microfluidic electrophoresis device. We have achieved baseline-resolved electrophoretic separations of single-locus STR samples in 30 sec. Analyses of PCR samples containing the four loci CSF1PO, TPOX, THO1, and vWA (abbreviated as CTTv) were performed in less than 2 min. This constitutes a 10- to 100-fold improvement in speed relative to capillary or slab gel systems. The separation device consists of a microfabricated channel 45 μm × 100 μm in cross section and 26 mm in length, filled with a replaceable polyacrylamide matrix operated under denaturing conditions at 50°C. A fluorescently labeled STR ladder was used as an internal standard for allele identification. Samples were prepared by standard procedures and only 4 μl was required for each analysis. The device is capable of repetitive operation and is suitable for automated high-speed and high-throughput applications.
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We report the genetic organisation of six prophages present in the genome of Lactococcus lactis IL1403. The three larger prophages (36–42 kb), belong to the already described P335 group of temperate phages, whereas the three smaller ones (13–15 kb) are most probably satellites relying on helper phage(s) for multiplication. These data give a new insight into the genetic structure of lactococcal phage populations. P335 temperate phages have variable genomes, sharing homology over only 10–33% of their length. In contrast, virulent phages have highly similar genomes sharing homology over >90% of their length. Further analysis of genetic structure in all known groups of phages active on other bacterial hosts such as Escherichia coli, Bacillus subtilis, Mycobacterium and Streptococcus thermophilus confirmed the existence of two types of genetic structure related to the phage way of life. This might reflect different intensities of horizontal DNA exchange: low among purely virulent phages and high among temperate phages and their lytic homologues. We suggest that the constraints on genetic exchange among purely virulent phages reflect their optimal genetic organisation, adapted to a more specialised and extreme form of parasitism than temperate/lytic phages.
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Biologists should help to guide a process of cultural evolution in which society determines how much effort, if any, is ethically required to preserve options in biological evolution. Evolutionists, conservation biologists, and ecologists should be doing more research to determine actions that would best help to avoid foreclosing evolutionary options.
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Degradation of proteins that, because of improper or suboptimal processing, are retained in the endoplasmic reticulum (ER) involves retrotranslocation to reach the cytosolic ubiquitin-proteasome machinery. We found that substrates of this pathway, the precursor of human asialoglycoprotein receptor H2a and free heavy chains of murine class I major histocompatibility complex (MHC), accumulate in a novel preGolgi compartment that is adjacent to but not overlapping with the centrosome, the Golgi complex, and the ER-to-Golgi intermediate compartment (ERGIC). On its way to degradation, H2a associated increasingly after synthesis with the ER translocon Sec61. Nevertheless, it remained in the secretory pathway upon proteasomal inhibition, suggesting that its retrotranslocation must be tightly coupled to the degradation process. In the presence of proteasomal inhibitors, the ER chaperones calreticulin and calnexin, but not BiP, PDI, or glycoprotein glucosyltransferase, concentrate in the subcellular region of the novel compartment. The “quality control” compartment is possibly a subcompartment of the ER. It depends on microtubules but is insensitive to brefeldin A. We discuss the possibility that it is also the site for concentration and retrotranslocation of proteins that, like the mutant cystic fibrosis transmembrane conductance regulator, are transported to the cytosol, where they form large aggregates, the “aggresomes.”
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Surveys of butterfly and moth diversity in tropical forest fragments suggest that nocturnality confers a dispersal, and possibly a survival, advantage. The butterfly faunas of smaller fragments were depauperate; in contrast, the species richness of nocturnal moths was similar in all fragments and even in pasture. The lack of correlation between butterfly and moth species richness among fragments (r2 = 0.005) is best explained by movements of moths at night when ambient conditions in forest and pasture are most similar; butterflies face substantial daytime temperature, humidity, and solar radiation barriers. This interpretation is supported by information on birds, beetles, and bats.
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During the induction of long-term potentiation (LTP) in hippocampal slices adenosine triphosphate (ATP) is secreted into the synaptic cleft, and a 48 kDa/50 kDa protein duplex becomes phosphorylated by extracellular ATP. All the criteria required as evidence that these two proteins serve as principal substrates of ecto-protein kinase activity on the surface of hippocampal pyramidal neurons have been fulfilled. This phosphorylation activity was detected on the surface of pyramidal neurons assayed after synaptogenesis, but not in immature neurons nor in glial cells. Addition to the extracellular medium of a monoclonal antibody termed mAb 1.9, directed to the catalytic domain of protein kinase C (PKC), inhibited selectively this surface protein phosphorylation activity and blocked the stabilization of LTP induced by high frequency stimulation (HFS) in hippocampal slices. This antibody did not interfere with routine synaptic transmission nor prevent the initial enhancement of synaptic responses observed during the 1-5 min period immediately after the application of HFS (the induction phase of LTP). However, the initial increase in the slope of excitatory postsynaptic potentials, as well as the elevated amplitude of the population spike induced by HFS, both declined gradually and returned to prestimulus values within 30-40 min after HFS was applied in the presence of mAb 1.9. A control antibody that binds to PKC but does not inhibit its activity had no effect on LTP. The selective inhibitory effects observed with mAb 1.9 provide the first direct evidence of a causal role for ecto-PK in the maintenance of stable LTP, an event implicated in the process of learning and the formation of memory in the brain.
