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271.
The activities of enzymes involved in lipid metabolism—phospholipase A2 (PLA2) and phosphatidylethanolamine N-methyltransferase (PE N-MTase)—were found to be differently affected by pre-incubation of rod outer segments (ROS) under protein phosphorylating or dephosphorylating conditions. Exposure to cAMP-dependent protein kinase (PKA), under dark or light conditions, produced a significant increase in PE N-MTase activity, whereas PLA2 activity decreased. Under standard protein kinase C (PKC) phosphorylating conditions in light, PE N-MTase activity was stimulated and PLA2 activity was not affected. When the assays were performed in the dark, both enzymatic activities were unaffected when compared to the corresponding controls. Incubation of ROS membranes in light in the presence of PKC activators phorbol 12,13-dibutyrate (PDBu) and dioctanoylglycerol (DOG) resulted in the same pattern of changes in enzyme activities as described for standard PKC phosphorylating condition. Pre-incubation of membranes with the PKC inhibitor H-7 reduced the stimulation of PDBu on PE N-MTase activity, and had no effect on PLA2 activity in ROS membranes incubated with the phorbol ester. Pre-treatment of isolated ROS with alkaline phosphatase resulted in decreased PE N-MTase activity and produced a significant stimulation of PLA2 activity under dark as well as under light conditions when compared to the corresponding controls. These findings suggest that ROS protein phosphorylation and dephosphorylation modulates PE N-MTase and PLA2 activities in isolated ROS, and that these activities are independently and specifically modulated by particular kinases. Furthermore, dephosphorylation of ROS proteins has the opposite effect to that produced by protein phosphorylation on the enzymes studied.  相似文献   
272.
Protein-tyrosine phosphatases (PTPases) form a novel and important class of cell regulatory proteins. We evaluated the expression of PTPases in mouse brain by polymerase chain amplification of cDNA segments that encode the catalytic domains of these enzymes. Degenerate primer pairs devised on the basis of conserved protein motifs were used to generate a series of distinct PCR-derived clones. In this way, murine homologues of the human PTPases LRP, PTP, PTP, PTP and LAR were obtained. Corresponding regions in their catalytic domains were used to reveal the evolutionary relationships between all currently known mammalian PTPase protein family members. Phylogenetic reconstruction displayed considerable differences in mutation rates for closely related PTPases.  相似文献   
273.
H. M. Helal 《Plant and Soil》1990,123(2):161-163
This paper presents results of a comparative study of phosphorus utilization from inositol hexaphosphate by various varieties of Phaseolus vulgaris in relation to the activity and characteristics of their root phosphatases. Bean varieties show significant differences in their uptake of phosphorus from inositol hexaphosphate with a clear dependency on the phosphatase activity of their roots at pH 5. The results which are discussed in connection with the phosphorus turnover in the rhizosphere suggest that root phosphatase activity is a significant factor of nutritional efficiency under limited mineral phosphorus supply.  相似文献   
274.
Acid phosphatase activities have been partially purified from an aqueous extract of an acetone powder from orange flavedo. The use of a gel filtration step with an ionic gradient allowed a dissociation of proteins from pigments, thus facilitating purification and stabilization of the enzymes. The enzymes do not require metals for full activity, and they hydrolysed a wide spectrum of phosphorylated substrates. C10–C20 allylic pyrophosphates and monophosphates were hydrolysed sequentially by these ‘prenylphosphatases’. The final product was the corresponding unrearranged prenyl alcohol. This demonstrated the absence of E-Z isomerization and suggested an OP bond cleavage. Prenylphosphatases exhibited a certain degree of chain length specificity. Although the E or Z conformation of the C-2 double bond was not important, its presence was required for full activity. Excess prenylpyrophosphate inhibited the rate of formation of alcohols, most likely through the inhibition of phosphomonoesterase activity. These prenylphosphatases generated the alcoholic components of essential oils from the corresponding pyrophosphates and removed them from the chain lengthening process.  相似文献   
275.
In Escherichia coli chemosensory arrays, transmembrane receptors, a histidine autokinase CheA, and a scaffolding protein CheW interact to form an extended hexagonal lattice of signaling complexes. One interaction, previously assigned a crucial signaling role, occurs between chemoreceptors and the CheW-binding P5 domain of CheA. Structural studies showed a receptor helix fitting into a hydrophobic cleft at the boundary between P5 subdomains. Our work aimed to elucidate the in vivo roles of the receptor–P5 interface, employing as a model the interaction between E. coli CheA and Tsr, the serine chemoreceptor. Crosslinking assays confirmed P5 and Tsr contacts in vivo and their strict dependence on CheW. Moreover, the P5 domain only mediated CheA recruitment to polar receptor clusters if CheW was also present. Amino acid replacements at CheA.P5 cleft residues reduced CheA kinase activity, lowered serine response cooperativity, and partially impaired chemotaxis. Pseudoreversion studies identified suppressors of P5 cleft defects at other P5 groove residues or at surface-exposed residues in P5 subdomain 1, which interacts with CheW in signaling complexes. Our results indicate that a high-affinity P5–receptor binding interaction is not essential for core complex function. Rather, P5 groove residues are probably required for proper cleft structure and/or dynamic behavior, which likely impact conformational communication between P5 subdomains and the strong binding interaction with CheW that is necessary for kinase activation. We propose a model for signal transmission in chemotaxis signaling complexes in which the CheW–receptor interface plays the key role in conveying signaling-related conformational changes from receptors to the CheA kinase.  相似文献   
276.
Es wird über Ergebnisse und Probleme beim Transport in Markstrahlen, insbesondere beim Siebelement-Baststrahl-Übergang, beim eigentlichen Radialtransport in den Markstrahlen und beim Stoffaustausch mit den Gefäßen berichtet. Zahlreiche Resultate über die Stoffwechselaktivität, die Feinstruktur und den DNA/RNA-Gehalt von Strasburger Zellen weisen auf deren besondere Rolle beim Stoffübertritt zwischen Siebzellen und Baststrahlzellen hin. Die Entstehung der Saccharose in den Strasburger Zellen, das Beladen in Vesikel und die möglichen Transportwege werden anhand eines Modells diskutiert. Aufgrund von Messungen der Stärkedeposition im Holzstrahlgewebe (etwa 5,2 mg/mg TG/Monat) und der zur Verfügung stehenden tangentialen Lumenfläche wird eine radiale Fluxrate von minimal 2,1 bis 4,2 nmol cm?2 min?1 (in Glucoseeinheiten) erhalten, die deutlich über den bekannten Membran-fluxraten liegt und damit für das Vorliegen eines symplastischen Transportes in den Holzstrahlen spricht. Cytochemische Befunde und eine deutlich polare Phosphatanreicherung in den Holzstrahlzellen zur Zeit intensiven Radialtransportes führen zu einem hypothetischen Modell, in dem eine polar erfolgende Beladung von Vesikel mit Saccharose aus dem Cytosol als Antrieb eines symplastischen Transportes in die Nachbarzelle erörtert wird. Den Stoffaustausch zwischen Holzstrahlen und Gefäßen beleuchten Ergebnisse über den Eintritt von Zuckern und Aminosäuren in das Gefäßwasser und Experimente über die Zuckeraufnahme aus dem Gefäßwasser sowie bei Gewebsschnitten in vitro. Beide lassen auf eine Trägervermittelte Glucoseaufnahme nach extraplasmatischer Spaltung der Saccharose schließen. Den Kontakttüpfeln als Orte stark erhöhter Nucleosidtriphosphatspaltung kommt dabei möglicherweise eine besondere Rolle zu. Frau Patrizia schekahn danke ich herzlich für wertvolle technische Assistenz bei der Durchführung der Untersuchungen, Frau A. Gabriel und Frau P. Zimmerma nn für die Assistenz bei der Benutzung des Zucker- und Aminosäureanalysators.  相似文献   
277.
Summary The ultrastructural localisation of acid phosphatases (AcPhs) during the normal daily breakdown of rhabdomere membrane in Dinopis has been examined using -glycerophosphate and p-nitrophenyl phosphate as substrates. Results are related to the classification of organelles in the receptors given by Blest, Powell and Kao (1978). Weak and infrequent reactions are obtained in multivesicular bodies (mvbs) and multilamellar bodies (mlbs) derived from them. Residual bodies (rbs) begin to react strongly as they lyse. Source of AcPhs is endoplasmic reticulum which has barely differentiated towards the GERL configuration; it becomes reactive as it is incorporated into secondary lysosomes. GERL tubules, Y-bodies and vesicles respond erratically and weakly, and are also incorporated into rbs. No evidence was found for a significant participation of Golgi bodies in these processes, and acid phosphatase cytochemistry fails to reveal a topographical relationship between GERL in these cells and Golgi saccules. Coated vesicle clusters found in the predawn receptive segments are AcPh-negative; this implies that their previous identification as GERL-derived Nebenkerne carrying hydrolytic enzymes to newly-formed mvbs (Blest, Kao and Powell, 1978) is dubious. Isolation bodies and autophagic vacuoles enclosing other organelles in pathological receptors give strong reactions while adjacent secondary lysosomes derived from rhabdomere membrane and associated GERL give weak ones. It is concluded that rhabdomere-derived rb lysis is more tightly regulated than other autophagic processes, and it is suggested that a high degree of control is necessary in a receptor which may repeat the autophagy of a large mass of transductive membrane at least 60–100 times in the course of its working life.The authors thank Professor D.T. Anderson F.R.S. for the use of field facilities at the Crommelin Biological Field Station of Sydney University at Warrah, Pearl Beach, New South Wales throughout all these studies; Dr. Gary Griffiths (EMBO, Heidelberg) and Dr. Alex Pyliotis (Biochemistry, SGS, Australian National University) for some helpful comments on acid phosphatase histochemistry; Sally J. Stowe for help in the field; and Rod Whitty and the staff on the Electron Microscopy Unit for advice and support. Figure 28 was prepared by Chris Snoek  相似文献   
278.
CDC25 phosphatases play key roles in cell proliferation by activating cell cycle-specific cyclin-dependent kinases (CDKs). We identified four new splice variants in the amino-terminal regulatory region of human cdc25C and one in cdc25A. All variants except one retain an intact catalytic domain. Alternative splicing results in loss of phosphorylation sites for kinases like CDK and the calcium/calmodulin-dependent kinase II (CaMKII), which influence CDC25 activity and compartmental localization. In NT2 teratocarcinoma cells, induced for nerve cell differentiation, the smaller sized variant of cdc25C was upregulated. At the protein level both phosphorylation state and isoform distribution differed between cell lines and cell cycle phases.  相似文献   
279.
Soluble and wall-bound acid phosphatases isolated from rape seed pollen showed similar properties except for the pH optimum curve which was elevated for the cell wall enzyme. About 50 % of the phosphatase activity of washed pollen wall preparations could be solubilized with Triton X-100, compared with only ca 20% for the corresponding preparation from lily pollen. A comparison of the wall-bound acid phosphatase of rape seed and lily pollen showed a marked difference in specificity towards fructose-6-phosphate and glucose-6-phosphate. A Mg2+-dependent alkaline pyrophosphatase was obtained from rape seed pollen but this activity could not be detected in cell wall preparations.  相似文献   
280.
Wiskott-Aldrich Syndrome (WAS) is a severe X-linked disorder characterised by immune deficiency, thrombocytopenia and eczema, resulting from abnormalities in a range of haematopoietic cell types. The protein that is defective in WAS, named WASP, appears to be involved in regulating changes in the cytoskeletal organisation of haematopoietic cells in response to external stimuli. In support of this idea, WASP has been found to be physically associated in haematopoietic cells in vivo with a number of SH3 domain-containing proteins involved in signal transduction, including the cytoplasmic protein-tyrosine kinase Fyn. Here, we have used a baculovirus expression system to explore the biochemical consequences of the interaction between WASP and Fyn. We find that the kinase activity of Fyn is stimulated as a result of binding to WASP, and that a cellular protein, which may be WASP itself, becomes phosphorylated on tyrosine as a result of the binding of WASP to Fyn.  相似文献   
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