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361.
Moravej A Rasouli M Kalani M Asaei S Kiany S Najafipour S Koohpayeh A Abdollahi A 《Molecular biology reports》2012,39(6):6907-6914
Lymphotoxin-α (LT-α) and interleukin-1beta (IL-1β) are proinflammatory cytokines playing important roles in immunity against
Leishmania infection and the outcome of the disease. As cytokine productions are under the genetic control, this study tried to find
any probable relationship between these cytokine gene polymorphisms and the susceptibility to visceral leishmaniasis in Iranian
pediatric patients. Ninety-five pediatric patients involved with visceral leishmaniasis and 128 non-relative healthy people,
from the same area as the patients, were genotyped for LT-α (+252A/G) and IL-1β (+3953T/C and −511T/C) gene polymorphisms
using polymerase chain reaction-restriction fragment length polymorphism (PCR–RFLP). There was not found any significant differences
in allele and genotype frequencies of LT-α (+252A/G) and IL-1β (+3953) among the study groups. However, the frequency of IL-1β
−511TT genotype was higher in the controls (P = 0.0004) while the frequency of IL-1β −511CC genotype and C allele were higher in the patients (P = 0.008 and P = 0.00006, respectively). Furthermore, IL-1β CC (−511/+3953) haplotype was more frequent in VL patients compared with the
controls (P = 0.0002) and the distribution of TT haplotype was higher in the controls compared with the patients (P = 0.003). In conclusion, based on the results, IL-1β −511C allele, CC genotype and CC (−511/+3953) haplotype could be considered
as the susceptibility factors for visceral leishmaniasis while IL-1β −511TT genotype, T allele and TT haplotype (−511/+3953)
might be counted as the influential factors for resistance to the disease. 相似文献
362.
Zoleykha Asadi Mojtaba Fathi Elham Rismani Zahra Bigdelou Behrooz Johari 《Cell biology international》2021,45(5):1001-1014
363.
Seied Ali Hosseini Tafreshi Mansour Shariati Mohammad Reza Mofid Mojtaba Khayam Nekui 《In vitro cellular & developmental biology. Plant》2011,47(5):561-568
A highly promising procedure to obtain seedlings of Taxus baccata L. has been developed, which involves a combination of in vitro embryo culture and growth under hydroponic conditions. Embryos isolated from freshly collected seeds were 100% sterile, even
though the seeds were not treated with acid or soaked in water prior to culturing. The embryo germination level of non-leached
seeds was slightly lower (85%) than those leached in running water for 7 d (100%). The leached embryos germinated with extended
roots while the non-leached embryos had abnormal shapes. The embryos cultured on media supplemented with an absorbent (PVP
or activated charcoal) had extended roots and shoots and were a larger size without any browning, as compared to those grown
without the supplement; activated charcoal gave better results. There were no significant differences in germination rates
of T. baccata embryos between the media with differing strengths of macronutrients; however, for further development of the shoot, it was
necessary to sub-culture the seedlings in MS in the light. To obtain seedlings with longer roots, they had to be maintained
in one-half strength MS in darkness. Approximately 90% of the plants survived when grown hydroponically for 2 mo. The surviving
plants showed well-extended roots and were a good starting material for genomic, proteomic, and conservational studies as
well as Taxol permeabilization investigations. 相似文献
364.
Fekete É Fekete E Irinyi L Karaffa L Árnyasi M Asadollahi M Sándor E 《Microbiological research》2012,167(5):283-291
Botrytis cinerea has been described as a species complex containing two cryptic species, referred to as groups I and II. The first B. cinerea group I strains outside of Western Europe were collected in Hungary in 2008 from strawberry and rape plants. Sympatric B. cinerea cryptic species were analyzed using a population genetic approach and phenotypic markers. Statistically significant, but moderate population differentiation was found between the two groups in Hungary. Group I was originally typified by the lack of the transposable elements Boty and Flipper. However, all the Hungarian group I isolates carried the Boty element and one isolate additionally contained Flipper, indicating a much wider genetic variation than previously believed. Vegetative compatibility analyses showed that twelve of the thirteen B. cinerea group I isolates studied belonged to a unique vegetative compatibility group (VCG), but VCGs overlapped between groups. Phenotypic markers such as fenhexamid resistance or asexual spore size were found unsuitable to differentiate between the cryptic species. The results did not confirm the complete separation of the two cryptic species, previously determined with genealogical concordance of the phylogenetic species recognition using multiple gene sequences, and suggest instead the possibility of information exchange between them. 相似文献
365.
Abbas Tanhaeian Farajollah Shahriari Ahmadi Mohammad Hadi Sekhavati Mojtaba Mamarabadi 《Probiotics and antimicrobial proteins》2018,10(4):787-793
Lactoferrin is the most dominant protein in milk after casein. This protein plays a crucial role in many biological processes including the regulation of iron metabolism, induction and modulation of the immune system, the primary defense against microorganisms, inhibiting lipid peroxidation and presenting antimicrobial activity against various pathogens such as parasites, fungi, bacteria, and viruses. The major antimicrobial effect of lactoferrin is related to its N-terminal tail where different peptides for instance lactoferricin and lactoferrampin which are important for their antimicrobial abilities are present. The growth rate of bacterial cells in camel milk is lower than that of the cow milk due to having more antimicrobial compounds. In this study, we have fused a codon-optimized partial camel lactoferrcin and lactoferrampin DNA sequences in order to construct a fused peptide via a lysine. This chimeric 42-mer peptide consists of complete and partial amino acid sequence of camel lactoferrampin and lactoferricin, respectively. Human embryonic kidney 293 (HEK-293) cells were used for synthesizing this recombinant peptide. Finally, the antibacterial activities of this constructed peptide were investigated under in vitro condition. The result showed that, all construction, cloning and expression processes were successfully performed in HEK-293. One His-tag tail was added to the chimera in order to optimize the isolation and purification processes and also reduce the cost of production. Additionally, His-tag retained the antimicrobial activity of the chimera. The antimicrobial tests showed that the growth rate in the majority of bacterial plant pathogens, including gram negative and positive bacteria, was inhibited by recombinant chimera as the level of MIC values were evaluated between 0.39 and 25.07 μg/ml for different bacterial isolates. 相似文献
366.
Abdollahi Mohammad Reza Kianersi Farzad Moosavi Sayyed Saeed Dastan Dara Asadi Sepideh 《Journal of Plant Growth Regulation》2023,42(2):759-770
Journal of Plant Growth Regulation - Fennel (Foeniculum vulgare Mill.), a medicinal plant from the Apiaceae, is used in traditional medicine. For the first time in F. vulgare, partial cDNA of two... 相似文献
367.
368.
Plasmonics - In this paper, formation of dark plasmon-soliton in a plasmonic photonic crystal fiber (PPCF) structure is predicted and analyzed by the use of the generalized nonlinear... 相似文献
369.
370.
Moosavi-Movahedi AA Amani M Moosavi-Nejad SZ Hashemnia S Ahmad F Floris G Mura A Rezaei-Tavirani M Hakimelahi GH Saboury AA Yousefi R 《Bioscience, biotechnology, and biochemistry》2007,71(7):1644-1649
The relationships between the structural and energetic domains of lentil seedling amine oxidase (LSAO) were investigated using modifiers that target the active site and the carbohydrate moiety of the enzyme. An irreversible inhibitor, aminoguanidine, specifically modified the active site of the lentil enzyme, whereas sodium metaperiodate cleaves carbohydrate moieties covalently bound to the native enzyme. Differential scanning calorimetry (DSC) measurements were made on the modified LSAOs. Deconvolution of the reversible thermal DSC profiles of the modified enzyme gave three subpeaks (energetic domains), each of which was assigned to one of the three structural domains of the native protein. Our results led us to conclude that deglycosylation of LSAO has no effect on thermal stability, whereas binding of the inhibitor imparts more stability to the enzyme. 相似文献