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141.
Disha Shah Elisabeth Jonckers Jelle Praet Greetje Vanhoutte Rafael Delgado y Palacios Christian Bigot Dany V. D’Souza Marleen Verhoye Annemie Van der Linden 《PloS one》2013,8(12)
Introduction
Functional connectivity (FC) studies have gained immense popularity in the evaluation of several neurological disorders, such as Alzheimer’s disease (AD). AD is a complex disorder, characterised by several pathological features. The problem with FC studies in patients is that it is not straightforward to focus on a specific aspect of pathology. In the current study, resting state functional magnetic resonance imaging (rsfMRI) is applied in a mouse model of amyloidosis to assess the effects of amyloid pathology on FC in the mouse brain.Methods
Nine APP/PS1 transgenic and nine wild-type mice (average age 18.9 months) were imaged on a 7T MRI system. The mice were anesthetized with medetomidine and rsfMRI data were acquired using a gradient echo EPI sequence. The data were analysed using a whole brain seed correlation analysis and interhemispheric FC was evaluated using a pairwise seed analysis. Qualitative histological analyses were performed to assess amyloid pathology, inflammation and synaptic deficits.Results
The whole brain seed analysis revealed an overall decrease in FC in the brains of transgenic mice compared to wild-type mice. The results showed that interhemispheric FC was relatively preserved in the motor cortex of the transgenic mice, but decreased in the somatosensory cortex and the hippocampus when compared to the wild-type mice. The pairwise seed analysis confirmed these results. Histological analyses confirmed the presence of amyloid pathology, inflammation and synaptic deficits in the transgenic mice.Conclusions
In the current study, rsfMRI demonstrated decreased FC in APP/PS1 transgenic mice compared to wild-type mice in several brain regions. The APP/PS1 transgenic mice had advanced amyloid pathology across the brain, as well as inflammation and synaptic deficits surrounding the amyloid plaques. Future studies should longitudinally evaluate APP/PS1 transgenic mice and correlate the rsfMRI findings to specific stages of amyloid pathology. 相似文献142.
143.
Memory of Social Partners in Hermit Crab Dominance 总被引:3,自引:0,他引:3
Francesca Gherardi & Jelle Atema† 《Ethology : formerly Zeitschrift fur Tierpsychologie》2005,111(3):271-285
We investigated the possibility that invertebrates recognize conspecific individuals by studying dominance relationships in the long‐clawed hermit crab, Pagurus longicarpus. We conducted three sets of laboratory experiments to define the time limits for acquiring and maintaining memory of an individual opponent. The results reveal two characteristics that make individual recognition in this species different from standard associative learning tasks. Firstly, crabs do not require training over many repeated trials; rather, they show evidence of recognition after a single 30‐min exposure to a stimulus animal. Secondly, memory lasts for up to 4 d of isolation without reinforcement. A third interesting feature of individual recognition in this species is that familiar opponents are recognized even before the formation of a stable hierarchical rank. That is, recognition seems to be relatively independent of repeated wins (rewards) or losses (punishments) in a dominance hierarchy. The experimental protocol allowed us to show that this species is able to classify conspecifics into two ‘heterogeneous subgroups’, i.e. familiar vs. unfamiliar individuals, but not to discriminate one individual of a group from every other conspecific from ‘a unique set of cues defining that individual’. In other words, we demonstrated a ‘binary’– and not a ‘true’– individual recognition. However, 1 d of interactions with different crabs did not erase the memory of a former rival, suggesting that P. longicarpus uses a system of social partner discrimination more refined than previously shown. 相似文献
144.
Yolande F. M. Ramos Wouter den Hollander Judith V. M. G. Bovée Nils Bomer Ruud van der Breggen Nico Lakenberg J. Christiaan Keurentjes Jelle J. Goeman P. Eline Slagboom Rob G. H. H. Nelissen Steffan D. Bos Ingrid Meulenbelt 《PloS one》2014,9(7)
Objective
Identify gene expression profiles associated with OA processes in articular cartilage and determine pathways changing during the disease process.Methods
Genome wide gene expression was determined in paired samples of OA affected and preserved cartilage of the same joint using microarray analysis for 33 patients of the RAAK study. Results were replicated in independent samples by RT-qPCR and immunohistochemistry. Profiles were analyzed with the online analysis tools DAVID and STRING to identify enrichment for specific pathways and protein-protein interactions.Results
Among the 1717 genes that were significantly differently expressed between OA affected and preserved cartilage we found significant enrichment for genes involved in skeletal development (e.g. TNFRSF11B and FRZB). Also several inflammatory genes such as CD55, PTGES and TNFAIP6, previously identified in within-joint analyses as well as in analyses comparing preserved cartilage from OA affected joints versus healthy cartilage were among the top genes. Of note was the high up-regulation of NGF in OA cartilage. RT-qPCR confirmed differential expression for 18 out of 19 genes with expression changes of 2-fold or higher, and immunohistochemistry of selected genes showed a concordant change in protein expression. Most of these changes associated with OA severity (Mankin score) but were independent of joint-site or sex.Conclusion
We provide further insights into the ongoing OA pathophysiological processes in cartilage, in particular into differences in macroscopically intact cartilage compared to OA affected cartilage, which seem relatively consistent and independent of sex or joint. We advocate that development of treatment could benefit by focusing on these similarities in gene expression changes and/or pathways. 相似文献145.
cIAP1/2 are direct E3 ligases conjugating diverse types of ubiquitin chains to receptor interacting proteins kinases 1 to 4 (RIP1-4) 总被引:1,自引:0,他引:1
Bertrand MJ Lippens S Staes A Gilbert B Roelandt R De Medts J Gevaert K Declercq W Vandenabeele P 《PloS one》2011,6(9):e22356
The RIP kinases have emerged as essential mediators of cellular stress that integrate both extracellular stimuli emanating from various cell-surface receptors and signals coming from intracellular pattern recognition receptors. The molecular mechanisms regulating the ability of the RIP proteins to transduce the stress signals remain poorly understood, but seem to rely only partially on their kinase activities. Recent studies on RIP1 and RIP2 have highlighted the importance of ubiquitination as a key process regulating their capacity to activate downstream signaling pathways. In this study, we found that XIAP, cIAP1 and cIAP2 not only directly bind to RIP1 and RIP2 but also to RIP3 and RIP4. We show that cIAP1 and cIAP2 are direct E3 ubiquitin ligases for all four RIP proteins and that cIAP1 is capable of conjugating the RIPs with diverse types of ubiquitin chains, including linear chains. Consistently, we show that repressing cIAP1/2 levels affects the activation of NF-κB that is dependent on RIP1, -2, -3 and -4. Finally, we identified Lys51 and Lys145 of RIP4 as two critical residues for cIAP1-mediated ubiquitination and NF-κB activation. 相似文献
146.
147.
148.
149.
Memory and dementia are often topics of educational activities, however there is only limited information about the effectiveness of this education. In this study the effectiveness of a lecture, as part of a series of lectures about dementia, has been evaluated. The results showed an improvement in knowledge after the lecture and the participants were satisfied afterwards. Finally, it showed that there is a need for this kind of education; for professionals and for people who were worried about their memory or their partners' memory. 相似文献
150.
Jelle Hendrix Viola Baumg?rtel Waldemar Schrimpf Sergey Ivanchenko Michelle A. Digman Enrico Gratton Hans-Georg Kr?usslich Barbara Müller Don C. Lamb 《The Journal of cell biology》2015,210(4):629-646
Assembly of the Gag polyprotein into new viral particles in infected cells is a crucial step in the retroviral replication cycle. Currently, little is known about the onset of assembly in the cytosol. In this paper, we analyzed the cytosolic HIV-1 Gag fraction in real time in live cells using advanced fluctuation imaging methods and thereby provide detailed insights into the complex relationship between cytosolic Gag mobility, stoichiometry, and interactions. We show that Gag diffuses as a monomer on the subsecond timescale with severely reduced mobility. Reduction of mobility is associated with basic residues in its nucleocapsid (NC) domain, whereas capsid (CA) and matrix (MA) domains do not contribute significantly. Strikingly, another diffusive Gag species was observed on the seconds timescale that oligomerized in a concentration-dependent manner. Both NC- and CA-mediated interactions strongly assist this process. Our results reveal potential nucleation steps of cytosolic Gag fractions before membrane-assisted Gag assembly. 相似文献