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Molecular coevolution among cryptically simple expansion segments of eukaryotic 26S/28S rRNAs 总被引:16,自引:4,他引:12
The set of "expansion segments" of any eukaryotic 26S/28S ribosomal RNA
(rRNA) gene is responsible for the bulk of the difference in length between
the prokaryotic 23S rRNA gene and the eukaryotic 26S/28S rRNA gene. The
expansion segments are also responsible for interspecific fluctuations in
length during eukaryotic evolution. They show a consistent bias in base
composition in any species; for example, they are AT rich in Drosophila
melanogaster and GC rich in vertebrate species. Dot-matrix comparisons of
sets of expansion segments reveal high similarities between members of a
set within any 28S rRNA gene of a species, in contrast to the little or
spurious similarity that exists between sets of expansion segments from
distantly related species. Similarities among members of a set of expansion
segments within any 28S rRNA gene cannot be accounted for by their
base-compositional bias alone. In contrast, no significant similarity
exists within a set of "core" segments (regions between expansion segments)
of any 28S rRNA gene, although core segments are conserved between species.
The set of expansion segments of a 26S/28S gene is coevolving as a unit in
each species, at the same time as the family of 28S rRNA genes, as a whole,
is undergoing continual homogenization, making all sets of expansion
segments from all ribosomal DNA (rDNA) arrays in a species similar in
sequence. Analysis of DNA simplicity of 26S/28S rRNA genes shows a direct
correlation between significantly high relative simplicity factors (RSFs)
and sequence similarity among a set of expansion segments. A similar
correlation exists between RSF values, overall rDNA lengths, and the
lengths of individual expansion segments. Such correlations suggest that
most length fluctuations reflect the gain and loss of simple sequence
motifs by slippage-like mechanisms. We discuss the molecular coevolution of
expansion segments, which takes place against a background of slippage-like
and unequal crossing-over mechanisms of turnover that are responsible for
the accumulation of interspecific differences in rDNA sequences.
相似文献
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An experimental system was developed in which the majority of all lymphocyte cell-surface proteins, regardless of antigenic specificity, could be cross-linked and redistributed in the membrane to determine whether this would induce a corresponding redistribution of intramembrane particles (IMP). Mouse spleen cells were treated with P-diazoniumphenyl- β-D-lactoside (lac) to modify all exposed cell-surface proteins. Extensive azo- coupling was achieved without significantly reducing cell viability or compromising cellular function in mitogen- or antigen-stimulated cultures. When the lac-modified cell- surface proteins were capped with a sandwich of rabbit antilactoside antibody and fluorescein-goat anti-rabbit Ig, freeze-fracture preparations obtained from these cells revealed no obvious redistribution of IMP on the majority of fracture faces. However, detailed analysis showed a statistically significant 35 percent decrease (P less than 0.01) in average IMP density in the E face of the lac-capped spleen cells compared with control cells, whereas a few E-face micrographs showed intense IMP aggregation. In contrast, there was no significant alteration of P-face IMP densities or distribution. Apparently, the majority of E-face IMP and virtually all P-face IMP densities or distribution. Apparently, the majority of E-face IMP and virtually all P-face IMP do not present accessible antigenic sites on the lymphocyte surface and do not associate in a stable manner with surface protein antigens. This finding suggests that IMP, as observed in freeze-fracture analysis, may not comprise a representative reflection of lymphocyte transmembrane protein molecules and complexes because other evidence establishes: (a) that at least some common lymphocyte surface antigens are indeed exposed portions of transmembrane proteins and (b) that the aggregation of molecules of any surface antigen results in altered organization of contractile proteins at the cytoplasmic face of the membrane. 相似文献
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Deuterostome phylogeny and the sister group of the chordates: evidence from molecules and morphology 总被引:13,自引:3,他引:10
Complete coding regions of the 18S rRNA gene of an enteropneust
hemichordate and an echinoid and ophiuroid echinoderm were obtained and
aligned with 18S rRNA gene sequences of all major chordate clades and four
outgroups. Gene sequences were analyzed to test morphological character
phylogenies and to assess the strength of the signal. Maximum- parsimony
analysis of the sequences fails to support a monophyletic Chordata; the
urochordates form the sister taxon to the hemichordates, and together this
clade plus the echinoderms forms the sister taxon to the cephalochordates
plus craniates. Decay, bootstrap, and tree-length distribution analyses
suggest that the signal for inference of dueterostome phylogeny is weak in
this molecule. Parsimony analysis of morphological plus molecular
characters supports both monophyly of echinoderms plus enteropneust
hemichordates and a sister group relationship of this clade to chordates.
Evolutionary parsimony does not support chordate monophyly.
Neighbor-joining, Fitch-Margoliash, and maximum-likelihood analyses support
a chordate lineage that is the sister group to an
echinoderm-plus-hemichordate lineage. The results illustrate both the
limitations of the 18S rRNA molecule alone for high- level phylogeny
inference and the importance of considering both molecular and
morphological data in phylogeny reconstruction.
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