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61.
Electron Microscopy of Tissue Culture Cells Infected with Brucella abortus 总被引:1,自引:0,他引:1 下载免费PDF全文
Betty A. Hatten Shyi Yi Huang M. L. Schulze S. Edward Sulkin 《Journal of bacteriology》1971,108(1):535-544
Thin sections of hamster kidney tissue cultures were examined by electron microscopy over a 7-day period after infection with Brucella abortus 3183. Numerous bacteria and structures resembling L-forms were present both intracellularly and extracellularly after the first 24 hr of infection. Most intracellular microorganisms were enclosed by a cytoplasmic membrane, but in a few instances no limiting membrane was detected. After 4 to 7 days, fewer microorganisms were present, and most normal-appearing bacteria were intracellular, particularly in antibiotic-treated cultures. Structures typical of Brucella L-forms were extracellular at the latter time intervals. Several structures were observed in cells from infected cultures whose relationship to the infecting organisms is not known. These consisted of various membranous structures within cytoplasmic vacuoles, myelin-like structures surrounding occasional intracellular organisms, and small bodies present within vacuoles and extracellularly. The latter structures observed throughout the experimental period appeared to occur more frequently as the duration of the infection increased. 相似文献
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Siân SE Cox Mark van der Giezen Sarah J Tarr Mark R Crompton Jorge Tovar 《BMC microbiology》2006,6(1):45-16
Background
Giardia intestinalis is a parasitic protozoan and major cause of diarrhoeal disease. Disease transmission is dependent on the ability of the parasite to differentiate back and forth between an intestine-colonising trophozoite and an environmentally-resistant infective cyst. Our current understanding of the intracellular signalling mechanisms that regulate parasite replication and differentiation is limited, yet such information could suggest new methods of disease control. Phosphoinositide-3 kinase (PI3K) signalling pathways have a central involvement in many vital eukaryotic processes, such as regulation of cell growth, intracellular membrane trafficking and cell motility. Here we present evidence for the existence of functional PI3K intracellular signalling pathways in G. intestinalis. 相似文献65.
Prenatal maternal psychological distress increases risk for adverse infant outcomes. However, the biological mechanisms underlying this association remain unclear. Prenatal stress can impact fetal epigenetic regulation that could underlie changes in infant stress responses. It has been suggested that maternal glucocorticoids may mediate this epigenetic effect. We examined this hypothesis by determining the impact of maternal cortisol and depressive symptoms during pregnancy on infant NR3C1 and BDNF DNA methylation. Fifty-seven pregnant women were recruited during the second or third trimester. Participants self-reported depressive symptoms and salivary cortisol samples were collected diurnally and in response to a stressor. Buccal swabs for DNA extraction and DNA methylation analysis were collected from each infant at 2 months of age, and mothers were assessed for postnatal depressive symptoms. Prenatal depressive symptoms significantly predicted increased NR3C1 1F DNA methylation in male infants (β = 2.147, P = 0.044). Prenatal depressive symptoms also significantly predicted decreased BDNF IV DNA methylation in both male and female infants (β = −3.244, P = 0.013). No measure of maternal cortisol during pregnancy predicted infant NR3C1 1F or BDNF promoter IV DNA methylation. Our findings highlight the susceptibility of males to changes in NR3C1 DNA methylation and present novel evidence for altered BDNF IV DNA methylation in response to maternal depression during pregnancy. The lack of association between maternal cortisol and infant DNA methylation suggests that effects of maternal depression may not be mediated directly by glucocorticoids. Future studies should consider other potential mediating mechanisms in the link between maternal mood and infant outcomes. 相似文献
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Jason Lehto Stephen Sulkin Suzanne Strom Darcie Johnson 《Journal of experimental marine biology and ecology》1998,230(2):851-224
Newly-hatched larvae of the brachyuran crab, Hemigrapsus oregonensis, were raised in the laboratory on an autotrophic dinoflagellate (Prorocentrum micans), a heterotrophic dinoflagellate (Noctiluca milaris), a green alga (Dunaliella tertiolecta), an unfed control, and a fed control of Artemia sp. nauplii. Larvae also were fed preparations of seagrass detritus that had been cultured both to promote microbial colonization and to discourage it. Detrital diets were used both alone and in combination with sub-optimal applications of Artemia sp. nauplii. Larvae raised on P. micans showed survival to zoeal stage II equal to those raised on the Artemia sp. nauplii control, although development was delayed. Larvae raised on N. milaris showed substantial (34.7%) survival to zoeal stage II; however survival was lower and development slower than for Artemia sp. nauplii-fed larvae. Survival on D. tertiolecta was less than 3%. Larvae fed microbially-enriched detritus showed a delay in mortality as compared to unfed controls. No larvae fed solely on detritus survived to zoeal stage II. When larvae were fed a sub-optimal diet of Artemia nauplii, supplemented by detrital particles, survival to zoeal stage II increased, although not to the level shown by Artemia-fed larvae in optimal application. Development was not accelerated over the sub-optimal diet in either treatment. The potential for larval crabs to utilize a wide variety of potential prey immediately upon hatching is significant given their susceptibility to early starvation. Such omnivory also suggests a trophic link between carbon sources of the microbial loop and crab larvae. 相似文献
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Non-acidic inhibitors and embryo dormancy in Taxus baccata L. Embryo dormancy of Taxus baccata is eliminated when the embryos are continuously kept in sterile nutritive liquid medium. After 3 weeks of culture, an important non-acidic inhibitory complex can be extracted from this liquid medium. At least three substances are involved: two pigments and a compound with some properties that suggest xanthoxin. These substances are neither found in embryos taken directly from the seeds, nor in liquid medium after 8 days of culture, which is the time necessary and sufficient to allow germination after transfer on agar medium. Such behaviour is quite different from that of ABA previously studied and indicates that these non-acidic inhibitors appear late during the culture and are not directly involved in embryo dormancy. 相似文献
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