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51.
52.
Eric Dumonteil Ardem Elmayan Alicia Majeau Weihong Tu Brandy Duhon Preston Marx Wendy Wolfson Garry Balsamo Claudia Herrera 《PLoS neglected tropical diseases》2020,14(12)
BackgroundChagas disease is a neglected zoonosis of growing concern in the southern US, caused by the parasite Trypanosoma cruzi. We genotyped parasites in a large cohort of PCR positive dogs to shed light on parasite transmission cycles and assess potential relationships between parasite diversity and serological test performance.Methodology/principal findingsWe used a metabarcoding approach based on deep sequencing of T. cruzi mini-exon marker to assess parasite diversity. Phylogenetic analysis of 178 sequences from 40 dogs confirmed the presence of T. cruzi discrete typing unit (DTU) TcI and TcIV, as well as TcII, TcV and TcVI for the first time in US dogs. Infections with multiple DTUs occurred in 38% of the dogs. These data indicate a greater genetic diversity of T. cruzi than previously detected in the US. Comparison of T. cruzi sequence diversity indicated that highly similar T. cruzi strains from these DTUs circulate in hosts and vectors in Louisiana, indicating that they are involved in a shared T. cruzi parasite transmission cycle. However, TcIV and TcV were sampled more frequently in vectors, while TcII and TcVI were sampled more frequently in dogs.Conclusions/significanceThese observations point to ecological host-fitting being a dominant mechanism involved in the diversification of T. cruzi-host associations. Dogs with negative, discordant or confirmed positive T. cruzi serology harbored TcI parasites with different mini-exon sequences, which strongly supports the hypothesis that parasite genetic diversity is a key factor affecting serological test performance. Thus, the identification of conserved parasite antigens should be a high priority for the improvement of current serological tests. 相似文献
53.
Emilie Boulanger Alicia Dalongeville Marco Andrello David Mouillot Stéphanie Manel 《Ecography》2020,43(8):1167-1179
Current approaches that compare spatial genetic structure of a given species and the dispersal of its mobile phase can detect a mismatch between both patterns mainly due to processes acting at different temporal scales. Genetic structure result from gene flow and other evolutionary and demographic processes over many generations, while dispersal predicted from the mobile phase often represents solely one generation on a single time-step. In this study, we present a spatial graph approach to landscape genetics that extends connectivity networks with a stepping-stone model to represent dispersal between suitable habitat patches over multiple generations. We illustrate the approach with the case of the striped red mullet Mullus surmuletus in the Mediterranean Sea. The genetic connectivity of M. surmuletus was not correlate with the estimated dispersal probability over one generation, but with the stepping-stone estimate of larval dispersal, revealing the temporal scale of connectivity across the Mediterranean Sea. Our results highlight the importance of considering multiple generations and different time scales when relating demographic and genetic connectivity. The spatial graph of genetic distances further untangles intra-population genetic structure revealing the Siculo-Tunisian Strait as an important corridor rather than a barrier for gene flow between the Western- and Eastern Mediterranean basins, and identifying Mediterranean islands as important stepping-stones for gene flow between continental populations. Our approach can be easily extended to other systems and environments. 相似文献
54.
Eric Dumonteil Henry Pronovost Eli F. Bierman Anna Sanford Alicia Majeau Ryan Moore Claudia Herrera 《Molecular ecology》2020,29(19):3747-3761
Integrating how biodiversity and infectious disease dynamics are linked at multiple levels and scales is highly challenging. Chagas disease is a vector‐borne disease, with specificities of the triatomine vectors and Trypanosoma cruzi parasite life histories resulting in a complex multihost and multistrain life cycle. Here, we tested the hypothesis that T. cruzi transmission cycles are shaped by triatomine host communities and gut microbiota composition by comparing the integrated interactions of Triatoma sanguisuga in southern Louisiana with feeding hosts, T. cruzi parasite and bacterial microbiota in two habitats. Bugs were collected from resident's houses and animal shelters and analysed for genetic structure, blood feeding sources, T. cruzi parasites, and bacterial diversity by PCR amplification of specific DNA markers followed by next‐generation sequencing, in an integrative metabarcoding approach. T. sanguisuga feeding host communities appeared opportunistic and defined by host abundance in each habitat, yielding distinct parasite transmission networks among hosts. The circulation of a large diversity of T. cruzi DTUs was also detected, with TcII and TcV detected for the first time in triatomines in the US. The bacterial microbiota was highly diverse and varied significantly according to the DTU infecting the bugs, indicating specific interactions among them in the gut. Expanding such studies to multiple habitats and additional triatomine species would be key to further refine our understanding of the complex life cycles of multihost, multistrain parasites such as T. cruzi, and may lead to improved disease control strategies. 相似文献
55.
H. Lisle Gibbs Libia Sanz Alicia Prez Alexander Ochoa Alyssa T.B. Hassinger Matthew L. Holding Juan J. Calvete 《Molecular ecology》2020,29(15):2871-2888
Understanding how interspecific interactions mould the molecular basis of adaptations in coevolving species is a long‐sought goal of evolutionary biology. Venom in predators and venom resistance proteins in prey are coevolving molecular phenotypes, and while venoms are highly complex mixtures it is unclear if prey respond with equally complex resistance traits. Here, we use a novel molecular methodology based on protein affinity columns to capture and identify candidate blood serum resistance proteins (“venom interactive proteins” [VIPs]) in California Ground Squirrels (Otospermophilus beecheyi) that interact with venom proteins from their main predator, Northern Pacific Rattlesnakes (Crotalus o. oreganus). This assay showed that serum‐based resistance is both population‐ and species‐specific, with serum proteins from ground squirrels showing higher binding affinities for venom proteins of local snakes compared to allopatric individuals. Venom protein specificity assays identified numerous and diverse candidate prey resistance VIPs but also potential targets of venom in prey tissues. Many specific VIPs bind to multiple snake venom proteins and, conversely, single venom proteins bind multiple VIPs, demonstrating that a portion of the squirrel blood serum “resistome” involves broad‐based inhibition of nonself proteins and suggests that resistance involves a toxin scavenging mechanism. Analyses of rates of evolution of VIP protein homologues in related mammals show that most of these proteins evolve under purifying selection possibly due to molecular constraints that limit the evolutionary responses of prey to rapidly evolving snake venom proteins. Our method represents a general approach to identify specific proteins involved in co‐evolutionary interactions between species at the molecular level. 相似文献
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57.
Christophe J. Queval Antony Fearns Laure Botella Alicia Smyth Laura Schnettger Morgane Mitermite Esen Wooff Bernardo Villarreal-Ramos Waldo Garcia-Jimenez Tiaan Heunis Matthias Trost Dirk Werling Francisco J. Salguero Stephen V. Gordon Maximiliano G. Gutierrez 《PLoS pathogens》2021,17(3)
The Mycobacterium tuberculosis complex (MTBC) is a group of related pathogens that cause tuberculosis (TB) in mammals. MTBC species are distinguished by their ability to sustain in distinct host populations. While Mycobacterium bovis (Mbv) sustains transmission cycles in cattle and wild animals and causes zoonotic TB, M. tuberculosis (Mtb) affects human populations and seldom causes disease in cattle. The host and pathogen determinants underlying host tropism between MTBC species are still unknown. Macrophages are the main host cell that encounters mycobacteria upon initial infection, and we hypothesised that early interactions between the macrophage and mycobacteria influence species-specific disease outcome. To identify factors that contribute to host tropism, we analysed blood-derived primary human and bovine macrophages (hMϕ or bMϕ, respectively) infected with Mbv and Mtb. We show that Mbv and Mtb reside in different cellular compartments and differentially replicate in hMϕ whereas both Mbv and Mtb efficiently replicate in bMϕ. Specifically, we show that out of the four infection combinations, only the infection of bMϕ with Mbv promoted the formation of multinucleated giant cells (MNGCs), a hallmark of tuberculous granulomas. Mechanistically, we demonstrate that both MPB70 from Mbv and extracellular vesicles released by Mbv-infected bMϕ promote macrophage multinucleation. Importantly, we extended our in vitro studies to show that granulomas from Mbv-infected but not Mtb-infected cattle contained higher numbers of MNGCs. Our findings implicate MNGC formation in the contrasting pathology between Mtb and Mbv for the bovine host and identify MPB70 from Mbv and extracellular vesicles from bMϕ as mediators of this process. 相似文献
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59.
Isolated mitochondria respiring on physiological substrates, both in state 4 and 3, are reported to be or not to be a source of reactive oxygen species (ROS). The cause of these discrepancies has been investigated. As protein concentration was raised in in vitro assays at 37°C, the rate of H2O2 release by rat heart mitochondria supplemented with pyruvate/malate or with succinate (plus rotenone) was shown to increase (0.03–0.15?mg?protein/ml), to decrease (0.2–0.5?mg?protein/ml) and to be negligible (over 0.5?mg?protein/ml). The inhibition of mitochondrial respiration (with rotenone or antimycin A) or the increase in the oxygen concentration dissolved in the assay medium allowed an enhancement of ROS production rate throughout the studied range of protein concentrations. In mitochondria respiring in state 3 on pyruvate/malate or on succinate (plus rotenone), ROS release vanished for protein concentrations over 0.5 or 0.2?mg/ml, respectively. However, ROS production rates measured with low protein concentrations (below 0.1?mg/ml) or in oxygen-enriched media were similar or even slightly higher in the active respiratory state 3 than in the resting state 4 for both substrates. Consequently, these findings indicate that isolated mitochondria, respiring in vitro under conditions of forward electron transport, release ROS with Complex I- and II-linked substrates in the resting condition (state 4) and when energy demand is maximal (state 3), provided that there is sufficient oxygen dissolved in the medium. 相似文献
60.
Alicia L. Richards Catherine E. Vincent Adrian Guthals Christopher M. Rose Michael S. Westphall Nuno Bandeira Joshua J. Coon 《Molecular & cellular proteomics : MCP》2013,12(12):3812-3823
We report the use of neutron-encoded (NeuCode) stable isotope labeling of amino acids in cell culture for the purpose of C-terminal product ion annotation. Two NeuCode labeling isotopologues of lysine, 13C615N2 and 2H8, which differ by 36 mDa, were metabolically embedded in a sample proteome, and the resultant labeled proteins were combined, digested, and analyzed via liquid chromatography and mass spectrometry. With MS/MS scan resolving powers of ∼50,000 or higher, product ions containing the C terminus (i.e. lysine) appear as a doublet spaced by exactly 36 mDa, whereas N-terminal fragments exist as a single m/z peak. Through theory and experiment, we demonstrate that over 90% of all y-type product ions have detectable doublets. We report on an algorithm that can extract these neutron signatures with high sensitivity and specificity. In other words, of 15,503 y-type product ion peaks, the y-type ion identification algorithm correctly identified 14,552 (93.2%) based on detection of the NeuCode doublet; 6.8% were misclassified (i.e. other ion types that were assigned as y-type products). Searching NeuCode labeled yeast with PepNovo+ resulted in a 34% increase in correct de novo identifications relative to searching through MS/MS only. We use this tool to simplify spectra prior to database searching, to sort unmatched tandem mass spectra for spectral richness, for correlation of co-fragmented ions to their parent precursor, and for de novo sequence identification.The ability to make de novo sequence identifications directly from tandem mass spectra has long been a holy grail of the proteomic community. Such a capability would wean the field from its reliance upon sequenced genome databases. Even for organisms with fully annotated genomes, events such as single nucleotide polymorphisms, alternative splicing, gene fusion, and a host of other genomic transformations can result in altered proteomes. These alterations can vary from cell to cell and individual to individual. Thus, one could argue that the most valuable proteomic information, the individual and cellular proteome variation from the genome, remains elusive (1). This problem has received considerable attention; that said, it is not easy to de novo correlate spectrum to sequence in a large-scale, automated fashion (2–6). Improvements in mass accuracy have helped, but routine, reliable de novo sequencing without database assistance is not standard (7–10).A primary means to facilitate de novo spectral interpretation is the simple annotation of m/z peaks in tandem mass spectra as either N- or C-terminal. We and others have investigated this seemingly simple first step. Real-world spectra, however, are complex. Difficulties often arise in determining the charge state of the fragment or in differentiating between fragment ions and peaks arising from neutral loss, internal fragmentation, or spectral noise, both electronic and chemical. Several strategies have focused on product ion annotation. These approaches have included manipulation of the N-terminus basicity combined with electron transfer dissociation (ETD)1 (11–13). This approach can yield mostly N-terminal fragments for peptides having only two charges. However, it requires both ETD and the protease LysN. Other methods have used differential labeling of N- and C-terminal peptides to shift either one or the other product ion series, by either metabolic or chemical means (14–18). Metabolic incorporation of amino acids is an efficient method of introducing distinctive labels that eliminates in vitro labeling, but this method requires that the sample be amenable to cell culture (19, 20). Additionally, it may be difficult to achieve complete labeling in complex systems. Several other approaches used to introduce heavy isotopes onto one terminus have been investigated, including trypsin digestion in 18O water (21–23), differential isotopic esterification (24, 25), derivatization of the C-terminal carboxylate by p-bromophenethylamine (8, 26), N-terminal derivatization with sulfonic acid groups (27, 28), and formaldehyde labeling via reductive amination (29–31). These chemical modifications are introduced after cell lysis, often immediately prior to analysis. Although chemical labeling strategies can be used with a variety of samples, difficulties can arise from differences in labeling efficiency between samples, and often a clean-up step is required following labeling, which may lead to sample loss. No matter the labeling method, in this regime, the two precursors must be separately isolated, fragmented, and analyzed either together or separately. The recognition and selection of the broadly spaced doublet in real time also are necessary. These requirements have limited the utility of these approaches. Our own laboratory discovered that the c- and ●z-type product ions generated from either electron capture dissociation or ETD have distinct chemical formulae and therefore can always be distinguished based on accurate mass alone (32). The problem with this approach is that extremely high mass accuracy (<500 ppb) is required in order to distinguish these product ion types above ∼600 Da in mass. Thus, the majority of the product ions within a spectrum cannot be readily mapped to either terminus with high confidence.Despite these difficulties, we assert that robust de novo sequencing methodology would benefit greatly from a simple method that could be used to distinguish N- and C-terminal product ions with high accuracy and precision. Ideally, the approach would work regardless of the choice of proteolytic enzyme or dissociation method. Recently, we described a new technology for protein quantification called neutron encoding (NeuCode) (33). NeuCode embeds millidalton mass differences into peptides and proteins by exploiting the mass defect induced by differences in the nuclear binding energies of the various stable isotopes of common elements such as C, N, H, and O. For example, consider the amino acid lysine, which has eight additional neutrons (+8 Da). One way to synthesize this amino acid is to add six 13C atoms and two 15N atoms (+8.0142 Da). Another isotopologue could be constructed by adding eight 2H atoms (+8.0502). These two isotopologues differ by only 36 mDa; peptide precursors containing both of these amino acids would appear as a single, unresolved precursor m/z peak at a mass resolving power of less than ∼100,000. However, under high resolving powers (i.e. greater than ∼100,000 at m/z 400), this doublet is resolved. We first developed this NeuCode concept in the context of metabolic labeling, akin to stable isotope labeling with amino acids in cell culture (SILAC), except that instead of the precursor partners being separated by 4 to 8 Da, they are separated by only 6 to 40 mDa. For quantitative purposes, NeuCode promises to deliver ultraplexed SILAC (>12) without increasing spectral complexity.We reasoned that the isotopologues of Lys that permit NeuCode SILAC would generate a distinct fingerprint on C-terminal product ions. Specifically, peptides that have been labeled with NeuCode SILAC and digested with LysC uniformly contain Lys at the C terminus. Upon MS/MS, all C-terminal product ions should present as doublets (with duplex NeuCode), whereas N-terminal products will be detected as a single m/z peak. The very close m/z spacing of the NeuCode SILAC partners will ensure that each partner is always co-isolated and that the signatures are visible only upon high-resolving-power mass analysis. Here we investigate the combination of NeuCode SILAC and high-resolving-power MS/MS analysis to allow the straightforward identification of C-terminal product ions.