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991.
João Lavrado Kaamil Gani Pedro A. Nobre Sofia A. Santos Paula Figueiredo Dinora Lopes Virgílio do Rosário Jiri Gut Philip J. Rosenthal Rui Moreira Alexandra Paulo 《Bioorganic & medicinal chemistry letters》2010,20(19):5634-5637
Quindolone derivatives, designed to target the malaria parasite digestive vacuole and heme detoxification pathway, have been synthesized by reaction with 2-chloro-N,N-diethylethanamine. This reaction gave N,O-, N,N- and O-alkylated products containing one or two basic side-chains. The compounds were evaluated for antiplasmodial activity against the chloroquine-resistant Plasmodium falciparum W2 strain and for cytotoxicity in HepG2 A16 hepatic cells. By incorporating alkylamine side chains and chlorine atoms in the quindolone nucleus we transformed the inactive tetracyclic parent quindolones into moderate or highly active and selective antimalarial compounds. The most active and selective compound, 5c, showed an IC50 = 51 nM for P. falciparum and a selectivity ratio of 98. 相似文献
992.
Richardson M Pimenta AM Bemquerer MP Santoro MM Beirao PS Lima ME Figueiredo SG Bloch C Vasconcelos EA Campos FA Gomes PC Cordeiro MN 《Comparative biochemistry and physiology. Toxicology & pharmacology : CBP》2006,142(3-4):173-187
The proteomes of the venoms of the Brazilian wandering "armed" spiders Phoneutria nigriventer, Phoneutria reidyi, and Phoneutria keyserlingi, were compared using two-dimensional gel electrophoresis. The venom components were also fractionated using a combination of preparative reverse phase HPLC on Vydac C4, analytical RP-HPLC on Vydac C8 and C18 and cation exchange FPLC on Resource S at pH 6.1 and 4.7, or anion exchange HPLC on Synchropak AX-300 at pH 8.6. The amino acid sequences of the native and S-pyridyl-ethylated proteins and peptides derived from them by enzymatic digestion and chemical cleavages were determined using a Shimadzu PPSQ-21(A) automated protein sequencer, and by MS/MS collision induced dissociations. To date nearly 400 peptides and proteins (1.2-27 kDa) have been isolated in a pure state and, of these, more than 100 have had their complete or partial amino acid sequences determined. These sequences demonstrate, as might be expected, that the venoms of P. reidyi and P. keyserlingi (Family: Ctenidae) both contain a similar range of isoforms of the neurotoxins as those previously isolated from P. nigriventer which are active on neuronal ion (Ca(2+), Na(+) and K(+)) channels and NMDA-type glutamate receptors. In addition two new families of small (3-4 kDa) toxins, some larger protein (>10 kDa) components, and two serine proteinases of the venom of P. nigriventer are described. These enzymes may be responsible for some of the post-translational modification observed in some of the venom components. 相似文献
993.
994.
目的研究高纯度大豆卵磷脂对中国仓鼠肺细胞(cHL)染色体畸变作用。方法测定高纯度大豆卵磷脂对CHL细胞的半数抑制浓度(IC50),根据IC50设立不同剂量组,进行正式试验,分别观察高纯度大豆卵磷脂接触CHL6h,24h及加S9后6h染色体的畸变情况,根据标准进行结果判定。结果染毒6h,24h及加S9后染毒6h染色体畸变为阴性。结论高纯度大豆卵磷脂不能引起CHL细胞染色体产生畸变作用。 相似文献
995.
Marta D. Mendes Helena Trindade A. Cristina Figueiredo José G. Barroso Susana S. Fontinha Luis G. Pedro 《Biochemical Systematics and Ecology》2009
Chemical and genetic differences of 11 individuals of Angelica lignescens and 3 individuals of Melanoselinum decipiens were studied to determine whether volatile components could be used as taxonomical markers and to examine the correlation between molecular and chemical markers. The volatiles were isolated from each individual by distillation–extraction and analyzed by gas chromatography (GC) and gas chromatography–mass spectrometry (GC–MS). The same plants were analyzed by Inter Simple Sequence Repeat (ISSR) using 14 arbitrary primers. The main component of volatile fraction isolated from vegetative aerial parts of A. lignescens was limonene (57–86%) while in M. decipiens the main components detected were β-pinene (38–47%) and sabinene (1–33%). Cluster analyses based both on the chemical composition of volatile fraction and on molecular markers grouped the 14 accessions in two main groups, corresponding to each of the two species under study. Considering the species together, a moderate Pearson's correlation of r = 0.61 was obtained between the two analyses. 相似文献
996.
Helicobacter pylori induces chronic inflammation of the gastric mucosa, but only a proportion of infected individuals develop peptic ulcer disease or gastric carcinoma. Reasons underlying these observations include differences in bacterial pathogenicity as well as in host susceptibility. Numerous studies published in the last year provided new insight into H. pylori virulence factors, their interaction with the host and consequences in pathogenesis. These include the role of bacterial genetic diversity in host colonization and persistence, outer membrane proteins and modulation of adhesin expression, new aspects of VacA functions, and CagA and its phosphorylation-dependent and -independent cellular effects. This article will also review the recent novel findings on the interactions of H. pylori with diverse host epithelial signaling pathways and events involved in the initiation of carcinogenesis, including genetic instability and dysregulation of DNA repair. 相似文献
997.
Jeremy A. Dodsworth Lei Li Shiping Wei Brian P. Hedlund John A. Leigh Paul de Figueiredo 《Applied and environmental microbiology》2010,76(16):5644-5647
Escherichia coli transforms the methanogenic archaeon Methanococcus maripaludis at frequencies ranging from 0.2 × 10−6 to 2 × 10−6 per recipient cell. Transformation requires cell-to-cell contact, oriT, and tra functions, is insensitive to DNase I, and otherwise displays hallmarks of conjugation.Conjugal transfer of DNA involves a specific set of transfer (tra) functions that mediate the mobilization of DNA containing an origin of transfer (oriT) from a donor to a recipient in a process requiring cell-to-cell contact (9). While conjugation is often very efficient between members of a given species or genus, it can also occur at a lower efficiency between phylogenetically distant microorganisms with structurally distinct cell surfaces. Escherichia coli, for example, mediates conjugal transfer of DNA to such diverse bacterial recipients as cyanobacteria (23), spirochetes (14), and a variety of Gram-positive bacteria (17, 22); E. coli even mediates conjugal DNA transfer to members of the domain Eukarya, such as to Saccharomyces cerevisiae (6) and mammalian (20) cells. Because of its broad range of potential recipients, conjugation has proven to be a valuable genetic tool (11) and may be an important mechanism of horizontal gene transfer and a driver of genome evolution (7). Conjugation-like DNA transfer has also been demonstrated in members of the domain Archaea (5, 15). However, conjugation between Bacteria and Archaea has not been demonstrated, despite the observation that many whole-genome sequences of Archaea harbor DNA that appears to be of bacterial origin (7).To investigate whether conjugation can occur between Bacteria and Archaea, the RP4 (IncPα group) conjugal-transfer system was used to attempt to mobilize DNA from E. coli to the anaerobic, methanogenic archaeon Methanococcus maripaludis strain S2 (21). The RP4 system was selected because previous work demonstrated that this plasmid supports the transfer of DNA from E. coli to phylogenetically distant recipients, including yeast (3) and mammalian (20) cells. Additionally, E. coli has been shown to successfully conjugate with strictly anaerobic bacterial strains (22). M. maripaludis was chosen as a recipient because it has growth parameters similar to those of E. coli and has readily available selectable markers (1). For all the experiments described, M. maripaludis was grown in liquid or solid (excluding cysteine) McCas medium (12), supplemented with 2.5 μg/ml puromycin (Pur) where appropriate, using standard anaerobic techniques (2). All plating for conjugation experiments, except for determination of viable-E. coli cell counts, was performed in an anaerobic chamber (Coy, Grass Lake, MI) with an atmosphere of 5:5:90 H2-CO2-N2. E. coli was grown in Difco LB medium (Becton-Dickinson, Sparks, MD) supplemented where appropriate with 50 μg/ml kanamycin sulfate (Kan) and ampicillin (Amp).To interrogate conjugal DNA transfer between E. coli and M. maripaludis, a set of vectors that either contained or lacked cis-acting sites required for mobilization by RP4 transfer functions were constructed (Table (Table1).1). Each of these vectors contained a Pur resistance (Purr) gene cassette (pac) (4) flanked by ∼0.5 kb DNA homologous to regions 5′ and 3′ of the M. maripaludis nrpR gene (nrpR::pac), which allows for selection by Pur in M. maripaludis and provides sites for homologous recombination into the nrpR locus of the M. maripaludis chromosome. This construct was selected because it has previously been used to transform M. maripaludis to Pur resistance by recombination into the nrpR locus using a polyethylene glycol (PEG)-mediated transformation protocol (10, 18). After it was demonstrated that plasmids of the appropriate genotypes support conjugation from donor strain E. coli S17-1, which contains the RP4 trans-acting transfer (tra) functions on the chromosome via an integrated RP4-2-Tc::Mu-Km::Tn7 cassette (16), to E. coli recipient cells (Table (Table1;1; see also the supplemental material), we investigated whether these same donor strains could support DNA transfer to M. maripaludis.
Open in a separate windowaFrom pBBR1MCS-2 (8) for pTAP1 to -4 or RP4 (13) for pTAP6 (see the supplemental material).bIndicates whether recipient growth was observed (yes) or not (no) under appropriate selection conditions for transconjugants (see the supplemental material).cAverage of results from 3 experiments.dOnly one colony was observed in three experiments.eNo colonies observed.fAll vectors were based on pCR2.1 (Ampr Kanr) and contained nrpR::pac.For initial conjugation experiments, 20-ml cultures of E. coli donor cells were pelleted by centrifugation, resuspended in 5 ml of the recipient culture, and transferred to 28-ml serum tubes under anaerobic conditions (see the supplemental material). Sealed tubes were removed from the chamber, centrifuged for 10 min at 750 × g, and returned to the anaerobic chamber, and cell pellets were resuspended in 1 ml of McCas medium without sulfide. Aliquots (10 to 50 μl) of the concentrated donor-recipient mixture were spread on Pur-containing McCas medium plates, and dilutions were plated on nonselective LB and McCas medium plates to determine total counts of viable cells of the donor and recipient, respectively. Preliminary experiments indicated that, although E. coli remained fully viable during at least the first 4 h of coincubation with M. maripaludis on McCas medium plates (data not shown), significant growth was not observed; thus, no selection against the donor strain was necessary. Plates were incubated at 37°C for 1 day (LB medium) or 4 days (McCas medium), and colonies were counted. In a series of three experiments, only two Pur-resistant M. maripaludis colonies were observed when the mob-negative vectors pTAP2, -3, and -5 were used (Table (Table1).1). When these were restreaked onto selective McCas medium plates, either no or very poor growth occurred, suggesting that these were not true transformants. In contrast, many M. maripaludis colonies were observed when vectors that were capable of being mobilized to an E. coli recipient were used (pTAP1, -4, and -6) (Table (Table1).1). For these vectors, frequencies of transformation ranged from 0.2 × 10−6 to 2 × 10−6 per recipient cell, suggesting that the Pur-resistant colonies arose due to conjugation. These are similar to frequencies of RP4-mediated conjugation from E. coli to diverse recipients, such as yeast (6) and Clostridium spp. (22).To confirm that the Pur-resistant colonies obtained in these experiments were indeed transformed with the nrpR::pac-containing vector, randomly selected colonies (5 each from matings using pTAP1 and pTAP4 or 19 from pTAP6) were screened by PCR and Southern hybridization (see the supplemental material). PCR using primers complementary to the 3′ or 5′ end of the pac cassette and to the M. maripaludis genome 3′ or 5′ of nrpR (outside the regions of homology in nrpR::pac) as well as Southern blots using a region of the pac gene as a probe indicated that all tested strains contained nrpR::pac recombined at the nrpR locus (Fig. (Fig.1).1). Approximately half of the strains were the result of double-crossover events, i.e., replacement of genomic nrpR with nrpR::pac.Open in a separate windowFIG. 1.Genetic analysis of M. maripaludis transformants. (A) A schematic diagram of the nrpR gene and flanking region in the M. maripaludis genome and the nrpR::pac region of the gene replacement constructs pTAP1, pTAP4, and pTAP6, harboring mob-oriT-rep, mob-oriT, and RP4-oriT, respectively (open boxes). Primers for PCR analyses are shown with arrowheads, and the probe for Southern analysis is indicated. gDNA, genomic DNA. (B) Southern blot and PCR analyses of DNA extracted from putative pTAP1, pTAP4, and pTAP6 transformants of M. maripaludis. Arrows indicate the signature band (6.3 kb) for double crossover (c/o), 5′ crossover, and 3′ crossover. Positive and negative PCR amplifications are shown as “+” and “−,” respectively. WT, wild-type M. maripaludis S2; MM500, nrpR deletion mutant generated by PEG-mediated transformation with an nrpR::pac-containing construct (10).Using the pTAP6 vector (GenBank accession no. HM536627), a series of controls were performed to determine whether transformation was a result of conjugation. Matings were performed as described above, except that donor and recipient cells were pelleted and resuspended separately, coming into contact only when plated on McCas medium plus Pur agar. This is essentially the “combined spread plate” method described by Walter et al. (19) and was used to simplify interpretation of results. To determine whether the mobilization functions present in S17-1 were required, E. coli strain DH5α (tra mutant) transformed with pTAP6 was used as a donor. To determine whether donor cells must be viable, concentrated S17-1(pTAP6) was heated to 80°C for 20 min under anaerobic conditions prior to being plated, which decreased donor viable counts >10,000-fold (<105/ml). To test if transformation could be achieved with naked DNA (via natural competence of M. maripaludis) and if the transferred plasmid must be inside the donor cell, 4 μg purified pTAP6 was plated along with S17-1 containing no intracellular plasmid. To test for inhibition by DNase, 250 U (0.2 ml of 1,250 Kunitz units/ml in McCas medium) of DNase I (Sigma, St. Louis, MO) was spread on plates immediately prior to plating; the efficacy of DNase under assay conditions was confirmed (see the supplemental material). To determine if cell-to-cell contact was required, 20-μl aliquots of the donor and recipient were spread either on the same or opposite sides of a 0.45-μm nylon filter laid on the plate surface. In all other cases, 20-μl aliquots of donor and recipient cells were spread on a section of the plate ∼50 mm in diameter, consistent with the size of the nylon filters. Transformants were observed only with live S17-1(pTAP6) as a donor, with or without DNase on plates and only when the donor and recipient were not separated by the nylon filter, at frequencies ranging from 0.4 × 10−6 to 2 × 10−6 per recipient cell or 0.5 × 10−6 to 3 × 10−7 per donor cell (Table (Table22).
Open in a separate windowaAll data are from a single experiment, where each treatment was performed in quadruplicate. Approximately 8 × 107 recipient cells were used, with donor/recipient ratios ranging from 7:1 to 13:1. NA, not applicable.bThe number of Purr M. maripaludis colonies observed on each plate.cEfficiency represents the mean number of Purr colonies per viable recipient cell (±standard error of the mean). When no Purr colonies were observed, the efficiency is shown as being less than the calculated efficiency observed from one Purr colony ± the error in determining the total number of viable recipients.In summary, this work demonstrated that the transformation of M. maripaludis by E. coli displayed all of the hallmarks of conjugation: oriT was required in cis on the plasmid to be transferred, mobilization functions were required in the donor cell, the plasmid had to be inside the donor cells, donor cells had to be viable, cell-to-cell contact was required, and DNase I had no effect on the transformation. This shows that conjugation between Bacteria and Archaea can occur, thereby expanding the phylogenetic range of recipients that can be transformed using the RP4 conjugal-transfer system. Although the process described here is less efficient than standard PEG-mediated transformation of M. maripaludis (18), it is less laborious and may be useful for routine transformation of this methanogen. This approach may also prove fruitful for establishing genetic systems in other methanogens and Archaea. 相似文献
TABLE 1.
Transformation of M. maripaludis by E. coli| Plasmidf | Locus(i) from mobilizable plasmida | Predicted mobilization phenotype | Mediates conjugation to E. coli recipient?b | No. of Purr colonies per 108M. maripaludis cellsc |
|---|---|---|---|---|
| pTAP1 | mob-oriT-rep | Mob+ | Yes | 24 |
| pTAP2 | rep | Mob− | No | <1d |
| pTAP3 | oriT-rep | Mob− | No | <1d |
| pTAP4 | mob-oriT | Mob+ | Yes | 51 |
| pTAP5 | None | Mob− | No | 0e |
| pTAP6 | oriT region | Mob+ | Yes | 175 |
TABLE 2.
Requirements for transformation of M. maripaludis by E. colia| E. coli donor | Plasmid in donor | Treatment | No. of Purr colonies observedb | Efficiency per recipient (n = 4)c |
|---|---|---|---|---|
| S17-1 | pTAP6 | None | 28, 27, 26, 32 | (3.8 ± 0.8) × 10−7 |
| S17-1 | pTAP6 | 250 U DNase I spread on plates | 24, 26, 16, 52 | (3.9 ± 1.3) × 10−7 |
| S17-1 | pTAP6 | Both donor and recipient plated on a 0.45-μm filter | 129, 170, 180, 167 | (2.1 ± 0.5) × 10−6 |
| S17-1 | pTAP6 | Donor and recipient separated by a 0.45-μm filter | 0, 0, 0, 0 | < (3.3 ± 0.7) × 10−9 |
| S17-1 | pTAP6 | Heat-killed donor (80°C for 20 min) | 0, 0, 0, 0 | < (3.3 ± 0.7) × 10−9 |
| S17-1 | pTAP5 | None | 0, 0, 0, 0 | < (3.3 ± 0.7) × 10−9 |
| DH5α (Tra−) | pTAP6 | None | 0, 0, 0, 0 | < (3.3 ± 0.7) × 10−9 |
| S17-1 | None | Purified pTAP6 (4 μg) plated with donor | 0, 0, 0, 0 | < (3.3 ± 0.7) × 10−9 |
| None | NA | No donor | 0, 0, 0, 0 | < (3.3 ± 0.7) × 10−9 |
| S17-1 | pTAP6 | No recipient | 0, 0, 0, 0 | NA |
998.
Donald SA McLeod 《The Clinical biochemist. Reviews / Australian Association of Clinical Biochemists》2010,31(1):9-19
This paper provides an overview on the biology, monitoring and management of differentiated thyroid cancer (DTC), with particular attention to issues of relevance to clinical chemistry. The incidence of DTC appears to be increasing and management strategies are evolving as we learn more about its natural history and response to therapy. Clinical chemistry techniques play a central role in these protocols. Technical limitations inherent in current monitoring tools can hamper follow-up, although progress is being made. The molecular basis of DTC is being delineated with the potential to develop new strategies for diagnosis, monitoring and management of this condition. 相似文献
999.
Silva AC Spina AM Lemos MF Oba IT Guastini Cde F Gomes-Gouvêa MS Pinho JR Mendes-Correa MC 《Memórias do Instituto Oswaldo Cruz》2010,105(6):770-778
In this study, we evaluated the hepatitis B virus (HBV) genotype distribution and HBV genomic mutations among a group of human immunodeficiency virus-HBV co-infected patients from an AIDS outpatient clinic in S?o Paulo. HBV serological markers were detected by commercially available enzyme immunoassay kits. HBV DNA was detected using in-house nested polymerase chain reaction and quantified by Cobas Amplicor. HBV genotypes and mutations in the basal core promoter (BCP)/pre-core/core regions and surface/polymerase genes were determined by sequencing. Among the 59 patients included in this study, 55 reported prior use of lamivudine (LAM) or tenofovir. HBV DNA was detected in 16/22 patients, with a genotype distribution of A (n = 12,75%), G (n = 2,13%), D (n = 1,6%) and F (n = 1,6%). The sequence data of the two patients infected with genotype G strongly suggested co-infection with genotype A. In 10 patients with viremia, LAM-resistance mutations in the polymerase gene (rtL180M + rtM204V and rtV173L + rtL180M + rtM204V) were found, accompanied by changes in the envelope gene (sI195M, sW196L and sI195M/sE164D). Mutations in the BCP and pre-core regions were identified in four patients. In conclusion, genotype G, which is rarely seen in Brazil, was observed in the group of patients included in our study. A high prevalence of mutations associated with LAM-resistance and mutations associated with anti-HBs resistance were also found among these patients. 相似文献
1000.