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511.
Cheuk-Lun Lee Poh-Choo Pang William S. B. Yeung Bérangère Tissot Maria Panico Terence T. H. Lao Ivan K. Chu Kai-Fai Lee Man-Kin Chung Kevin K. W. Lam Riitta Koistinen Hannu Koistinen Markku Sepp?l? Howard R. Morris Anne Dell Philip C. N. Chiu 《The Journal of biological chemistry》2009,284(22):15084-15096
Glycodelin is a human glycoprotein with four reported glycoforms, namely
glycodelin-A (GdA), glycodelin-F (GdF), glycodelin-C (GdC), and glycodelin-S
(GdS). These glycoforms have the same protein core and appear to differ in
their N-glycosylation. The glycosylation of GdA is completely
different from that of GdS. GdA inhibits proliferation and induces cell death
of T cells. However, the glycosylation and immunomodulating activities of GdF
and GdC are not known. This study aimed to use ultra-high sensitivity mass
spectrometry to compare the glycomes of GdA, GdC, and GdF and to study the
relationship between the immunological activity and glycosylation pattern
among glycodelin glycoforms. Using MALDI-TOF strategies, the glycoforms were
shown to contain an enormous diversity of bi-, tri-, and tetra-antennary
complex-type glycans carrying Galβ1–4GlcNAc (lacNAc) and/or
GalNAcβ1–4GlcNAc (lacdiNAc) antennae backbones with varying levels
of fucose and sialic acid substitution. Interestingly, they all carried a
family of Sda (NeuAcα2–3(GalNAcβ1–4)Gal)-containing
glycans, which were not identified in the earlier study because of less
sensitive methodologies used. Among the three glycodelins, GdA is the most
heavily sialylated. Virtually all the sialic acid on GdC is located on the Sda
antennae. With the exception of the Sda epitope, the GdC N-glycome
appears to be the asialylated counterpart of the GdA/GdF glycomes. Sialidase
activity, which may be responsible for transforming GdA/GdF to GdC, was
detected in cumulus cells. Both GdA and GdF inhibited the proliferation,
induced cell death, and suppressed interleukin-2 secretion of Jurkat cells and
peripheral blood mononuclear cells. In contrast, no immunosuppressive effect
was observed for GdS and GdC.Glycodelin is a member of the lipocalin family. It consists of 180 amino
acid residues (1) with two
sites of N-linked glycosylation. There are four reported glycodelin
isoforms, namely glycodelin-A (amniotic fluid isoform,
GdA),4 glycodelin-F
(follicular fluid, GdF), glycodelin-C (cumulus matrix, GdC) and glycodelin-S
(seminal plasma, GdS)
(2–5).
Among the four glycodelin isoforms, only the N-glycan structures of
GdA and GdS have been previously determined. This was achieved using fast atom
bombardment mass spectrometry
(6,
7). The glycan structures of
GdA and GdS are completely different. In GdA, the Asn-28 site carries high
mannose, hybrid, and complex-type structures, whereas the second Asn-63 site
is exclusively occupied by complex-type glycans
(6). The major non-reducing
epitopes characterized in the complex-type glycans are
Galβ1–4GlcNAc (lacNAc), GalNAcβ1–4GlcNAc (lacdiNAc),
NeuAcα2–6Galβ1–4GlcNAc (sialylated lacNAc),
NeuAcα2–6GalNAcβ1–4GlcNAc (sialylated lacdiNAc),
Galβ1–4(Fucα1–3)GlcNAc (Lewis-x), and
GalNAcβ1–4(Fucα1–3)GlcNAc (lacdiNAc analog of the blood
group substance Lewis-x) (6).
Many of these oligosaccharides are rare in other human glycoproteins. GdS
glycans are unusually fucose-rich, and the major complex type glycan
structures are bi-antennary glycans with Lewis-x and Lewis-y antennae.
Glycosylation of GdS is highly site-specific. Asn-28 contains only high
mannose structures, whereas Asn-63 contains only complex type glycans. More
than 80% of the complex glycans have 3–5 fucose residues/glycan, and
none of the glycans is sialylated, which is unusual for a secreted human
glycoprotein (7). The glycan
structures of GdF and GdC are not known, although they differ in
lectin-binding properties and isoelectric point from the other two glycodelin
isoforms (5).Glycans are involved in various intracellular, intercellular, and
cell-matrix recognition events
(8,
9). Glycosylation determines
the biological activities of the glycodelin isoforms
(2,
10). For example, both GdA and
GdF inhibit the spermatozoa-zona pellucida binding
(11) via fucosyltransferase-5
(12), but only the latter
inhibits progesterone-induced acrosome reaction, thus preventing a premature
acrosome reaction of the spermatozoa. There is evidence that cumulus cells can
convert exogenous GdA and -F to GdC, the physicochemical properties of which
suggest that it is differently glycosylated compared with GdA/F
(5). Moreover, GdC stimulated
spermatozoa-zona pellucida binding in a dose-dependent manner, and it
effectively displaced sperm-bound GdA and -F
(4,
5). GdS suppresses capacitation
probably via its inhibitory activity on cholesterol efflux from spermatozoa
(13).Except for the effects on fertilization, GdA is involved in fetomaternal
defense. This glycodelin isoform suppresses proliferation and induces
apoptosis of T cells (2) and
inhibits natural killer cell
(14) and B-cell
(15) activities. Glycosylation
is involved in the binding of GdA to receptors on T cells
(16). The sialic acid of GdA
contributes to the apoptotic activity in T cells
(17,
18) and binding to CD45, a
potential GdA receptor (16).
The importance of glycosylation in glycodelin is further shown by the absence
of immunosuppressive activities in GdS with different glycosylation
(18). The immunomodulating
activities of GdF and GdC are unknown.Our previous work showed that glycans are indispensable for the different
glycodelins to exhibit their binding activities and biological effects
(13,
19,
20). The present study aims to
identify the effect of all four glycodelin isoforms on lymphocyte viability,
cell death, and interleukin-2 (IL-2) secretion and to correlate these
bioactivities with their glycosylation patterns determined by mass
spectrometry. 相似文献
512.
Plantation forestry with exotic trees in south China needs compatible symbionts to improve the growth of seedlings in nurseries and to enhance establishment and growth in the field. Scleroderma, a potentially suitable symbiont for inoculation, is not being used in containerized nurseries in the region due to poor knowledge of its host range. The ability of 15 collections of Scleroderma, nine from Australia and six from Asia, to colonize and promote growth of four important exotic plantation trees (Eucalyptus globulus Labill., Eucalyptus urophylla ST Blake, Pinus elliottii Engl., and Pinus radiata D. Don) was examined in a nursery potting mix. There was generally low host specificity of Scleroderma between tree genera. At 12 weeks after inoculation, 13 to 14 of the 15 spore collections formed ectomycorrhizas on seedlings of eucalypts or pines. The extent of colonization differed between spore treatments with two or four collections forming abundant mycorrhizas (>50% fine roots colonized) on E. globulus or E. urophylla, respectively, and three or five on P. radiata or P. elliottii, respectively. Three collections from Australia strongly colonized all hosts resulting in 26 to 100% of short roots being colonized. Chinese Scleroderma collections resulted in fewer mycorrhizas on eucalypts than on pines. Inoculation stimulated the growth (shoot height and dry weight) of eucalypt and pine seedlings by up to 105% where Scleroderma mycorrhizas developed. The results suggest that there is a need to source Scleroderma from outside China for inoculating eucalypts in Chinese nurseries whereas Chinese collections of Scleroderma could be used in pine nurseries. Further screening of Australian and Chinese Scleroderma should be performed in Chinese nurseries and in the field before final commercial decisions are made. 相似文献
513.
Parry S Hanisch FG Leir SH Sutton-Smith M Morris HR Dell A Harris A 《Glycobiology》2006,16(7):623-634
The MUC1 mucin is an important tumor-associated antigen that shows extensive glycosylation in vivo. The O-glycosylation of this molecule, which has been well characterized in many cell types and tissues, is important in conferring the unusual biochemical and biophysical properties on a mucin. N-Glycosylation is crucial to the folding, sorting, membrane trafficking, and secretion of many proteins. Here, we evaluated the N-glycosylation of MUC1 derived from two sources: endogenous MUC1 isolated from human milk and a recombinant epitope-tagged MUC1F overexpressed in Caco2 colon carcinoma cells. N-Glycans on purified MUC1F/MUC1 were analyzed by matrix-assisted laser desorption/ionization time-of-flight mass spectrometry (MALDI-TOF-MS), gas chromatography-mass spectrometry (GC-MS), and CAD-ESI-MS/MS. The spectra indicate that MUC1F N-glycans have compositions consistent with high-mannose structures (Hex(5-9)HexNAc(2)) and complex/hybrid-type glycans (NeuAc(0-3)Fuc(0-3)Hex(3-8)HexNAc(3-7)). Many of the N-glycan structures are identical on MUC1F and native MUC1; however, a marked difference is seen between the N-glycans on membrane-bound and secreted forms of the native molecule. 相似文献
514.
The white-tailed deer is the definitive host of the parasitic nematode Parelaphostrongylus tenuis. This parasite also infects a wide variety of domesticated livestock, causing a debilitating neurologic disease. Glycoconjugates are becoming increasingly implicated in nematode strategies to maintain persistent infections in immunologically competent hosts. In this study, we have carried out detailed mass spectrometric analysis together with classical biochemical techniques, including western blotting and immunohistochemical staining with anticarbohydrate monoclonal antibodies and have shown that P. tenuis contains complex-type N-glycans with the antennae capped with Galalpha1-3Galbeta1-4GlcNAc sequence. By mimicking a vertebrate glycan, Galalpha1-3Gal may aid the parasite in evading immunological detection by the host. This is the first report of the Galalpha1-3Gal sequence in a nematode. 相似文献
515.
516.
Wissal M’sehli Marta Dell’Orto Patrizia De Nisi Silvia Donnini Chedly Abdelly Graziano Zocchi Mohamed Gharsalli 《Acta Physiologiae Plantarum》2009,31(4):667-673
Our study investigates the effect of iron deficiency on morpho-physiological and biochemical parameters of two Medicago ciliaris ecotypes (Mateur TN11.11 and Soliman TN8.7). Iron deficiency was imposed by making plants grow, either in an iron free or
by the addition of CaCO3/NaHCO3 to the Hoagland nutrient solution. Our results showed that both true and bicarbonate Fe-deficiency induced the characteristic
iron-chlorosis symptoms, although the intensity of the symptoms was ecotype-dependent. This variability in tolerance to iron
deficiency was also displayed by other morphological parameters such as root biomass and chlorophyll concentration. Besides,
iron chlorosis induced an increase in biochemical parameters: the iron reducing capacity (measured in vivo on root segments
and in vitro on plasma membrane enriched vesicles) and rhizosphere acidification by enhancement of H+-ATPase activity were more pronounced in Mateur ecotype. These findings suggest that Soliman ecotype was more sensitive than
Mateur one to iron chlorosis. 相似文献
517.
Tinya Fleming Shih-Chieh Chien Megan Dell Wayne C. Forrester 《Developmental biology》2010,344(1):94-17713
Ena/VASP proteins mediate the effects of guidance cues on the actin cytoskeleton. The single C. elegans homolog of the Ena/VASP family of proteins, UNC-34, is required for the migrations of cells and growth cones. Here we show that unc-34 mutant alleles also interact genetically with Wnt mutants to reveal a role for unc-34 in the establishment of neuronal polarity along the C. elegans anterior-posterior axis. Our mutant analysis shows that eliminating UNC-34 function results in neuronal migration and polarity phenotypes that are enhanced at higher temperatures, revealing a heat-sensitive process that is normally masked by the presence of UNC-34. Finally, we show that the UNC-34 protein is expressed broadly and accumulates in axons and at the apical junctions of epithelial cells. While most mutants lacked detectable UNC-34, three unc-34 mutants that contained missense mutations in the EVH1 domain produced full-length UNC-34 that failed to localize to apical junctions and axons, supporting the role for the EVH1 domain in localizing Ena/VASP family members. 相似文献
518.
Das A McDowell M O'Dell CM Busch ME Smith JA Ray SK Banik NL 《Neurochemical research》2010,35(12):2175-2183
Injection of rats with kainic acid (KA), a non-N-methyl-D-aspartate (NMDA) type glutamate receptor agonist, induces recurrent (delayed) convulsive seizures and subsequently hippocampal neurodegeneration, which is reminiscent of human epilepsy. The protective effect of anti-epileptic drugs on seizure-induced neuronal injury is well known; however, molecular basis of this protective effect has not yet been elucidated. In this study, we investigated the effect and signaling mediators of voltage-gated Na(+) channel blockers (Lamotrigine, Rufinamide, Oxcarbazepine, Valproic Acid, and Zonisamide) on KA-induced apoptosis in rat primary hippocampal neurons. Exposure of hippocampal neurons to 10 μM KA for 24 h caused significant increases in morphological and biochemical features of apoptosis, as determined by Wright staining and ApopTag assay, respectively. Analyses showed increases in expression and activity of cysteine proteases, production of reactive oxygen species (ROS), intracellular free [Ca(2+)], and Bax:Bcl-2 ratio during apoptosis. Cells exposed to KA for 15 min were then treated with Lamotrigine, Rufinamide, Oxcarbazepine, Valproic Acid, or Zonisamide. Post-treatment with one of these anti-epileptic drugs (500 nM) attenuated production of ROS and prevented apoptosis in hippocampal neurons. Lamotrigine, Rufinamide, and Oxcarbazepine appeared to be less protective when compared with Valproic Acid or Zonisamide. This difference may be due to blockade of T-type Ca(2+) channels also by Valproic Acid and Zonisamide. Our findings thus suggest that the anti-epileptic drugs that block both Na(+) channels and Ca(2+) channels are significantly more effective than agents that block only Na(+) channels for attenuating seizure-induced hippocampal neurodegeneration. 相似文献
519.
Marazziti D Baroni S Fabbrini L Italiani P Catena M Dell'Osso B Betti L Giannaccini G Lucacchini A Cassano GB 《Neurochemical research》2006,31(3):361-365
The dopamine transporter (DAT) is a protein regulating dopamine concentration in the synaptic cleft through the re-uptake mechanism. The DAT is the main target of psychostimulants and seems to play a pivotal role in neuronal degeneration and different neuropsychiatric disorders involving the dopamine system. Exhaustive research, however, regarding the presence of this protein in human platelets is still inconclusive, although it is thought that it might provide a peripheral tool to serve as a mean of exploring the same structure present in the brain. Therefore, we assessed some binding assays in platelets derived from healthy human subjects by means of 3H-WIN 35,428, a compound which is considered a selective ligand for the labelling of this protein, and by means of 125I-RTI-121, another compound with high specificity for DAT. The results showed that the binding of 3H-WIN-35,428 was too low to enable the detection of any structure; the binding of 125I-RTI-121, on the other hand, revealed the presence of two binding sites with pharmacological profiles similar to that of the serotonin transporter (SERT). In conclusions, therefore, platelets would not seem to be a useful model for exploring the DAT, given the prevalence therein of the SERT and the difficulty of labelling the DAT with the currently available ligands. 相似文献
520.