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991.
992.
Variability of morphological characters used to separate Pratylenchus penetrans from other species of the genus was studied in a population originating from a single gravid female. Pronounced heteromorphism was observed and characterized. About 30% of females had a crenate-tail terminus. Several shapes of stylet knobs were characterized; 50% of them were anteriorly flattened to indented. The outer margin of the cephalic framework extended into the body from one-half to two annules. The shape of the spermatheca varied from round to oval. A fifth lateral line was observed in many specimens. Environmental factors, and particularly the host plant, influenced such morphometric characters as body length, width, esophagus length, stylet length, V value, a and b'' ratios, as well as qualitative characters such as tail terminus, growth of ovary, and shape of median bulb. Nematodes reared on pea and cabbage had a higher percentage of females with a crenate-tail terminus than those from tomato, rye, beet, and alfalfa callus culture. Nematodes from peas were longer and wider; they often had gonads that extended to esophagi, but they had shorter esophagi amt stylets than those from callus culture. Populations from different geographical locations also exhibited variahility in morphological characters, as did the Cornell population. The validity of many characters used in species identification is discussed, and the possibility that other related Pratylenchus species are conspecific with P. penetrans is suggested. 相似文献
993.
G. Trausch 《Biochemical Systematics and Ecology》1976,4(1):51-54
The fate of D-glucose-6-phosphate and phosphoenolpyruvate in homogenates of tail and claw muscles of the lobster (H vulgaris) has been studied. With both substrates oxygen utilization is higher for the claw than for the tail muscle. Succinate is not an end product of anaerobic D-glucose-6-phosphate-U- 14C degradation in either muscle but L-lactate is the major product of such catabolism in tail muscle whereas both L-lactate and L-alanine are produced in claw muscle. Dihydroxyacetone phosphate production was observed both tissues: this can be related to the known high lipid content of these tissues. 相似文献
994.
Corkidi G Taboada B Wood CD Guerrero A Darszon A 《Biochemical and biophysical research communications》2008,373(1):125-129
Sperm motility, crucial for fertilization, has been mostly studied in two dimensions (2D) by recording their swimming trajectories near a flat surface. However, spermatozoa swim in three-dimensions (3D) to find eggs, with their speed being the main impediment to track them under realistic conditions. Here, we describe a novel method allowing 3D tracking and analysis of the trajectories of multiple free-swimming sperm. The system uses a piezo-electric device displacing a large focal distance objective mounted on a microscope to acquire 70 image stacks per second, each stack composed of 60 images that span a depth of 100 μm. With this method, 3D paths of multiple sperm in the same field could be visualized simultaneously during 1 s . Within the same sample we found that surface-confined sperm swam 25% slower, produced 3-fold fewer circular revolutions per second, and had trajectories of 134% greater radius of curvature than those sperm swimming freely in 3D. 相似文献
995.
Cerná A López-Fernández C Fernández JL Moreno Díaz de la Espina S de la Torre C Gosálvez J 《Chromosoma》2008,117(1):15-24
After applying proper deoxyribonucleic acid (DNA) probes, fluorescence in situ hybridization (FISH) showed that the 8/9 centromeres—one
per chromatid of the male haploid complement (X0) of Pyrgomorpha conica grasshopper—colocalized at the spermatid blunt end, where the spermatozoa flagellum inserts. A bundle of aligned 4′,6-diamidino-2-phenylindole-positive
chromatid scaffolds, which formed the central spermatid core, was observed after DNA breakage detection followed by FISH.
Modular nature of scaffold DNA was occasionally evident. The technique also showed that in the early spermatid, the chromatid
scaffolds lacked any DNA nick, whereas abundant breaks accumulated in the surrounding loops. Moreover, immunodetection showed
that scaffold DNA participated in the formation of triplex DNA, while this configuration was absent from the loops. During
spermatid maturation, triplex DNA disappeared from the scaffold in parallel with loop retraction, while protamines replace
histones. Thus, the presence of triplex DNA in the chromatid scaffold correlates with the anchoring of expanded DNA loops
to it. After loop retraction, the scaffolds of all chromatids coiled as a single unit in the spermatid head. This cooperative
coiling produced enlargement and tilting of the distal telomeric signals, which were distributed along the spermatid head
according to the length of each chromosome. We propose that specific DNA sequences dispersed throughout the whole chromatid
fold forward and backward coaxially to chromatid length, forming individual scaffold modules whose linear assembly accounts
for the minimum length of each individual chromatid. Finally, the core of the grasshopper male spermatid should be considered
as a single chromosome in which the DNA scaffolds of the whole set of the nonhomologous chromosomes of the haploid complement
are interconnected. This pattern of chromatin organization applies probably to other elongated spermatids. 相似文献
996.
997.
The type VI intermediate filament (IF) protein synemin is a unique member of the IF protein superfamily. Synemin associates with the major type III IF protein desmin forming heteropolymeric intermediate filaments (IFs) within developed mammalian striated muscle cells. These IFs encircle and link all adjacent myofibrils together at their Z-lines, as well as link the Z-lines of the peripheral layer of cellular myofibrils to the costameres located periodically along and subjacent to the sarcolemma. Costameres are multi-protein assemblies enriched in the cytoskeletal proteins vinculin, alpha-actinin, and talin. We report herein a direct interaction of human alpha-synemin with the cytoskeletal protein talin by protein-protein interaction assays. The 312 amino acid insert (SNTIII) present only within alpha-synemin binds to the rod domain of talin in vitro and co-localizes with talin at focal adhesion sites within mammalian muscle cells. Confocal microscopy studies showed that synemin co-localizes with talin within the costameres of human skeletal muscle cells. Analysis of the primary sequences of human alpha- and beta-synemins revealed that SNTIII is composed of seven tandem repeats, each containing a specific Ser/Thr-X-Arg-His/Gln (S/T-X-R-H/Q) motif. Our results suggest human alpha-synemin plays an essential role in linking the heteropolymeric IFs to adherens-type junctions, such as the costameres within mammalian striated muscle cells, via its interaction with talin, thereby helping provide mechanical integration for the muscle cell cytoskeleton. 相似文献
998.
Jones AL 《American journal of physical anthropology》2008,137(2):123-144
This study examines how brachiation locomotion evolved in ateline primates using recently-developed molecular phylogenies and character reconstruction algorithms, and a newly-collected dataset including the fossils Protopithecus, Caipora, and Cebupithecia. Fossils are added to two platyrrhine molecular phylogenies to create several phylogenetic scenarios. A generalized least squares algorithm reconstructs ateline and atelin ancestral character states for 17 characters that differentiate between ateline brachiators and nonbrachiators. Histories of these characters are mapped out on these phylogenies, producing two scenarios of ateline brachiation evolution that have four commonalities: First, many characters change towards the Ateles condition on the ateline stem lineage before Alouatta splits off from the atelins, suggesting that an ateline energy-maximizing strategy began before the atelines diversified. Second, the ateline last common ancestor is always reconstructed as an agile quadruped, usually with suspensory abilities. It is never exactly like Alouatta and many characters reverse and change towards the Alouatta condition after Alouatta separates from the atelins. Third, most characters undergo homoplastic change in all ateline lineages, especially on the Ateles and Brachyteles terminal branches. Fourth, ateline character evolution probably went through a hindlimb suspension with tail-bracing phase. The atelines most likely diversified via a quick adaptive radiation, with bursts of punctuated change occurring in their postcranial skeletons, due to changing climatic conditions, which may have caused competition among the atelines and between atelines and pitheciines. 相似文献
999.
1000.
哺乳动物精子质量的评价方法 总被引:15,自引:0,他引:15
精子的各种功能状态反应了精子的受精能力。检测精子质膜完整性的荧光探针有SYBR-14,SYTO-17,CFDA、CDMFDA、CAM、PI、Hoechst33258、Hoechst33342,其中以SYBR-14结合PI使用效果最好,检测线粒体活性的荧光探针有JC-1、MITO、Rh123,JC-1比MITO和Rh123更适用于检测精子线粒体功能,检测顶体状态的荧光探针有PNA-FITC、PSA-FITC、LYSO-G及CTC等。检测获能状态的荧光探针有CTC。此外,还可以通过检测精子与透明带的结合能力、精子穿入去透明带卵子的能力以及使卵子受精的能力和其后胚胎的发育能力等方面来评价精子的功能状态。 相似文献