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81.
J Cronshaw 《The journal of histochemistry and cytochemistry》1980,28(4):375-377
A cytochemical study using a lead precipitation technique has been made of the distribution of adenosine triphosphatase (ATPase) in mature and differentiating phloem and xylem cells of Nicotiana tabacum and Pisum sativum. The sites of ATPase localization in tobacco phloem were the plasma membrane, endoplasmic reticulum, mitochondria, dictyosomes, plasmodesmata, and the dispersed P proteins of mature sieve elements. In pea phloem sieve elements ATPase was localized in the endoplasmic reticulum, but was not associated with the P proteins or plasma membranes at any stage of their differentiation. In pea transfer cells ATPase activity was associated with the endoplasmic reticulum at all stages of their differentiation and with the plasma membrane of transfer cells that had formed wall ingrowths. In xylem cells of both tobacco and pea the patterns of ATPase activity was similar. At early stages of differentiation ATPase activity was associated with the plasma membrane and the endoplasmic reticulum. At intermediate stages of differentiation ATPase activity continued to be associated with the endoplasmic reticulum, but was no longer associated with the plasma membrane. At later stages of xylem element differentiation ATPase activity was associated with disintegrating organelles and with the hydrolyzing cell walls. 相似文献
82.
The effect of relaxed functional constraints on the photosynthetic gene rbcL in photosynthetic and nonphotosynthetic parasitic plants 总被引:1,自引:0,他引:1
The photosynthetic gene rbcL has been lost or dramatically altered in some
lineages of nonphotosynthetic parasitic plants, but the dynamics of these
events following loss of photosynthesis and whether rbcL has sustained
functionally significant changes in photosynthetic parasitic plants are
unknown. To assess the changes to rbcL associated with the loss of
functional constraints for photosynthesis, nucleotide sequences from
nonparasitic and parasitic plants of Scrophulariales were used for
phylogeny reconstruction and character analysis. Plants in this group
display a broad range of parasitic abilities, from photosynthetic
("hemiparasites") to nonphotosynthetic ("holoparasites"). With the
exception of Conopholis (Orobanchaceae), the rbcL locus is present in all
parasitic plants of Scrophulariales examined. Several holoparasitic genera
included in this study, including Boschniakia, Epifagus, Orobanche, and
Hyobanche, have rbcL pseudogenes. However, the holoparasites Alectra
orobanchoides, Harveya capensis, Harveya purpurea, Lathraea clandestina,
Orobanche corymbosa, O. fasciculata, and Striga gesnerioides have intact
open reading frames (ORFs) for the rbcL gene. Phylogenetic hypotheses based
on rbcL are largely in agreement with those based on sequences of the
nonphotosynthetic genes rps2 and matK and show a single origin of
parasitism, and loss of photosynthesis and pseudogene formation have been
independently derived several times in Scrophulariales. The mutations in
rbcL in nonparasitic and hemiparasitic plants would result in largely
conservative amino acid substitutions, supporting the hypothesis that
functional proteins can experience only a limited range of changes, even in
minimally photosynthetic plants. In contrast, ORFs in some holoparasites
had many previously unobserved missense substitutions at functionally
important amino acid residues, suggesting that rbcL genes in these plants
have evolved under relaxed or altered functional constraints.
相似文献
83.
Alternative splicing and protein function 总被引:1,自引:0,他引:1
AD?Neverov II?Artamonova RN?Nurtdinov D?Frishman MS?GelfandEmail author AA?Mironov 《BMC bioinformatics》2005,6(1):266
Background
Alternative splicing is a major mechanism of generating protein diversity in higher eukaryotes. Although at least half, and probably more, of mammalian genes are alternatively spliced, it was not clear, whether the frequency of alternative splicing is the same in different functional categories. The problem is obscured by uneven coverage of genes by ESTs and a large number of artifacts in the EST data. 相似文献84.
Dubois T Howell S Zemlickova E Learmonth M Cronshaw A Aitken A 《Biochemical and biophysical research communications》2003,302(2):186-192
CPI-17 is a protein phosphatase 1 (PP1) inhibitor that has been shown to act on the myosin light chain phosphatase. CPI-17 is phosphorylated on Thr-38 in vivo, thus enhancing its ability to inhibit PP1. Thr-38 has been shown to be the target of several protein kinases in vitro. Originally, the expression of CPI-17 was proposed to be smooth muscle specific. However, it has recently been found in platelets and we show in this report that it is endogenously phosphorylated in brain on Ser-128 in a domain unique to CPI-17. Ser-128 is within a consensus phosphorylation site for protein kinase A (PKA) and calcium calmodulin kinase II. However, these two kinases do not phosphorylate Ser-128 in vitro but phosphorylate Ser-130 and Thr-38, respectively. The kinase responsible for Ser-128 phosphorylation remains to be identified. CPI-17 has strong sequence similarity with PHI-1 (which is also a phosphatase inhibitor) and LimK-2 kinase. The novel in vivo and in vitro phosphorylation sites (serines 128 and 130) are in a region/domain unique to CPI-17, suggesting a specific interaction domain that is regulated by phosphorylation. 相似文献
85.
Proteomic analysis of the mammalian nuclear pore complex 总被引:35,自引:0,他引:35
Cronshaw JM Krutchinsky AN Zhang W Chait BT Matunis MJ 《The Journal of cell biology》2002,158(5):915-927
As the sole site of nucleocytoplasmic transport, the nuclear pore complex (NPC) has a vital cellular role. Nonetheless, much remains to be learned about many fundamental aspects of NPC function. To further understand the structure and function of the mammalian NPC, we have completed a proteomic analysis to identify and classify all of its protein components. We used mass spectrometry to identify all proteins present in a biochemically purified NPC fraction. Based on previous characterization, sequence homology, and subcellular localization, 29 of these proteins were classified as nucleoporins, and a further 18 were classified as NPC-associated proteins. Among the 29 nucleoporins were six previously undiscovered nucleoporins and a novel family of WD repeat nucleoporins. One of these WD repeat nucleoporins is ALADIN, the gene mutated in triple-A (or Allgrove) syndrome. Our analysis defines the proteome of the mammalian NPC for the first time and paves the way for a more detailed characterization of NPC structure and function. 相似文献
86.
The components of hard tissues including dentin, enamel, cementum, bone and other calcified deposits, and mature and immature collagen pose problems for identification in routine hematoxylin and eosin (H & E) stained sections. Use of combinations of stains can demonstrate the components of hard tissues and soft tissues distinctly. We assessed the efficacy of the Verde Luz-orange G-acid fuchsin (VOF) stain for differentiating hard and soft connective tissues and compared results with other histochemical staining techniques. Eighty tissue sections comprising developing tooth (30), ossifying fibroma (30) and miscellaneous pathologies (20) expected to contain varying types of calcified tissues were stained with H & E, VOF, and Masson's trichrome (MT). In developing tooth, VOF demonstrated better differentiation of hard tissues, while it was comparable to MT for ossifying fibroma and miscellaneous pathologies. The intensity of staining was greater with VOF than with the other stains studied. VOF stains hard tissue components distinctly and gives good contrast with the surrounding connective tissue. VOF is comparable to MT, but has added advantages including single step staining, rapid and easy procedures, and it distinguishes the maturity of the tissues. 相似文献
87.
The method of affinity coelectrophoresis was used to study the binding of
nine representative glycosaminoglycan (GAG)-binding proteins, all thought
to play roles in nervous system development, to GAGs and proteoglycans
isolated from developing rat brain. Binding to heparin and non-neural
heparan and chondroitin sulfates was also measured. All nine
proteins-laminin-1, fibronectin, thrombospondin-1, NCAM, L1, protease
nexin-1, urokinase plasminogen activator, thrombin, and fibroblast growth
factor-2-bound brain heparan sulfate less strongly than heparin, but the
degree of difference in affinity varied considerably. Protease nexin-1
bound brain heparan sulfate only 1.8- fold less tightly than heparin
(Kdvalues of 35 vs. 20 nM, respectively), whereas NCAM and L1 bound heparin
well (Kd approximately 140 nM) but failed to bind detectably to brain
heparan sulfate (Kd>3 microM). Four proteins bound brain chondroitin
sulfate, with affinities equal to or a few fold stronger than the same
proteins displayed toward cartilage chondroitin sulfate. Overall, the
highest affinities were observed with intact heparan sulfate proteoglycans:
laminin-1's affinities for the proteoglycans cerebroglycan (glypican-2),
glypican-1 and syndecan-3 were 300- to 1800-fold stronger than its affinity
for brain heparan sulfate. In contrast, the affinities of fibroblast growth
factor-2 for cerebroglycan and for brain heparan sulfate were similar.
Interestingly, partial proteolysis of cerebroglycan resulted in a >400-
fold loss of laminin affinity. These data support the views that (1)
GAG-binding proteins can be differentially sensitive to variations in GAG
structure, and (2) core proteins can have dramatic, ligand-specific
influences on protein-proteoglycan interactions.
相似文献
88.
89.
90.
Summary Young leaves ofNicotiana tabacum were fixed in glutaraldehyde-formaldehyde followed by osmium tetroxide. The fine structure of dividing cells was studied. Before prophase a band of microtubules was observed between the nucleus and the cell wall at a position judged as the future plane of division. The microtubules in the band are 4–6 units deep and relatively closely packed, giving sections of the band a characteristic appearance. Micro-tubules of the mitotic spindle, the phragmoplast, and the preprophase band are morphologically similar. Some of the microtubules of the mitotic spindle and the phragmoplast have an undulate appearance. It is suggested that the undulate microtubules may have been fixed at a time when microwaves were traveling along them. The cell plate is formed by a fusion of small smooth surfaced vesicles and small coated vesicles. Fusion of small vesicles results first in larger vesicles and then in a meshwork of new cell-wall material surrounded by new regions of plasma membrane. Most of the vesicles are derived from dictyosomes and may be produced before and during prophase as well as during later stages of division. The ER may also contribute some vesicles to the cell plate. 相似文献