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221.
棉铃虫病毒杀虫乳悬剂的生产及其药效试验 总被引:5,自引:1,他引:4
成功研制出棉铃虫病毒(NPV)杀虫乳悬剂,改进了生产工艺和设备,建立了棉铃虫的室内品系,提高了生产效率,建立了产品的检测方法,提高了产品质量,促使棉铃虫病毒杀虫剂商品开发获得成功。大田试验证明,病毒乳悬剂的防治效果,相当于当前推广的化学农药,优于原病毒可湿性粉剂。相同剂量(0.53一1.07×10(10)PIB/公顷)的病毒乳悬剂可使虫口平均减退91.7%,而病毒可湿性粉剂为83.7%。 相似文献
222.
酪氨酸羟化酶基因载体-pCMVTH 质粒的构建及在大鼠骨骼肌内的表达 总被引:4,自引:0,他引:4
为用转基因方法治疗巴金森氏病大鼠模型,本研究采用分子克隆技术,将合成多巴胺的关键酶-酪氨酸羟化酶(TH)的基因,克隆进入以巨细胞病毒CMV为启动子的载体质粒内,经限制性内切酶定位分析证实该重组的DNA质粒的可靠性。携带TH基因的PCMVTH质粒以LIPO-FECTIN介导,在培养的原代骨骼肌细胞中高效表达。本研究为进一步用转基因的细胞植入脑内以治疗巴金森氏病打下一定基础。 相似文献
223.
PCR法快速检测临床标本中结核杆菌DNA 总被引:2,自引:0,他引:2
应用聚合酶链反应(PCR)快速检测临床标本(脑脊液、胸水、腹水、血、痰液)中的结核杆菌DNA,特异性扩增片段123bp,为结核杆菌的特异性重复序列IS6110部分基因。PCR检测人型结核杆菌的敏感性达10fgDNA。临床标本的PCR检测阳性率(23.3%)明显高于抗酸染色涂片(2.9%)和细菌培养(5.7%)的阳性率(P〈0.05)。通过设立对照系统及对扩增产物酶切分析,表明该法无假阴性结果(特异 相似文献
224.
复合氨基酸在临床上的应用越来越被人们重视,我们利用水解猪血粉的方法得到含17种氨基酸的复合液,配制成滴眼剂用于多种原因引起的眼角膜溃疡疾病的治疗研究取得了较好的效果。 相似文献
225.
利用KCN、H_2O2和SDS的选择性反应引起的SOD同工酶谱带变化即可鉴别粗抽提液中的SOD同工酶类型;用这种方法对五株不同种根霉的鉴别实验表明,它们均不同程度地含有Cu,Zn型和Mn型两种SOD,前者约占80%左右,后者只占20%左右。用邻苯三酚自氧化法对样品中SOD活性测定结果与在同工酶谱上的鉴别结果基本一致。 相似文献
226.
用苯甲基磺酰氟(PMSF)和H_2Se相继处理铜锌超氧化物岐化酶(Cu,Zn-SOD),将酶分子中的丝氨酸(Ser)转化为硒代半胱氨酸(SeCys),从而引入了谷胱甘肽过氧化物酶(GPX)的催化基团,使其在SOD酶活性大部分保留的情况下,具有GPX活性,其GPX活力是PZ51活力的30倍。研究了双功能酶的最佳制备条件,包括PMSF的剂量、反应最适温度及H_2Se处理时间等,并用电子能谱、DTNB等方法测定了双功能酶的硒含量;测定了双功能酶对不同底物的米氏常数及双功能酶的荧光光谱、紫外吸收光谱及稳定性。 相似文献
227.
The effect of gossypol on the activities of 10 acrosomal enzymes of the rabbit sperm was evaluated. Acrosin, Azocoll proteinase, neuraminidase, and arylsulfatase were significantly inhibited or completely inactivated by 12–76 μM gossypol. Hyaluronidase, β-glucuronidase, and acid phosphatase were inhibited only at a higher concentration of gossypol (380 μM). Phospholipase C, alkaline phosphatase, and β-N-Acetyl glucosaminidase were not inhibited even at 380 μM gossypol. Gossypol was found to be a noncompetitive inhibitor of arylsulfatase with a Ki of 120 μM. The inhibition was reversible and dose-dependent. As the acrosomal enzymes were more sensitive to the inhibition by gossypol compared to sperm enzymes involved in glycolysis or energy production, these assays may serve as a more reliable indicator for monitoring the occurence of gossypol-induced sterility. © 1995 Wiley-Liss, Inc. 相似文献
228.
Gloria Giacomini Santo V. Nicosia Beatriz O. Saunders Caroline Fultz X. Sun Valerio M. Jasonni 《In vitro cellular & developmental biology. Animal》1995,31(4):300-309
Summary The ovarian mesothelium (OM) represents the tissue of origin of ovarian epithelial cancer. To gain insight into the regulation
of this tissue, OM organoids and submesothelial ovarian stromal cells (SC) were isolated from New Zealand White rabbits by
a stepwise tissue dispersal technique, while granulosa cells (GC) were aspirated from mature follicles (14±4 groups/animal).
OM and SC dispersal were sequentially accomplished by: a) 1-h incubation in collagenase type I (300 U/ml), gentle scraping
of the ovarian surface, and 1 g sedimentation of OM organoids (equivalent to 0.93±0.40 × 106 cells/animal) on 5% bovine serum albumin (BSA); b) 2-h incubation in pronase-collagenase (0.5%–300 U/ml) under periodical
resuspension and gentle scraping of SC (1.40±0.25 × 106/animal) from OM-denuded ovaries. After a week-long in vitro expansion, OM cells (OMC) were cultured alone and with SC or
GC within monocameral vessels or bicameral transfilter vessels in serumless, fibronectinrich (4μg/ml) HL-1 medium. After 7
d of contact cell-cell interaction, cytokeratin-positive OMC became surrounded by fibroblastoid, vimentin-positive SC or by
cytokeratin and vimentin-weakly positive GC. Filter-bound OMC humorally interacting with underlying SC or GC displayed a biphasic,
epithelioid and spindle, morphology with universal cytokeratin expression. Bromo-2′-deoxyuridine (BrdU) immunoperoxidase revealed
mean cell proliferation indices of 14.88% for OMC cultured alone, 11.21% and 19.39% for OMC cultured with GC or SC in monocameral
dishes, and 15.25% or 22.47% for OMC cultured in bicameral vessels over GC or SC, respectively. This model provides an experimental
tool for investigating the unexplored role of stromal-mesothelial interaction in OM pathobiology. 相似文献
229.
230.
Analysis of RIM11, a yeast protein kinase that phosphorylates the meiotic activator IME1. 总被引:16,自引:11,他引:5
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Many yeast genes that are essential for meiosis are expressed only in meiotic cells. Known regulators of early meiotic genes include IME1, which is required for their expression, and SIN3 and UME6, which prevent their expression in nonmeiotic cells. We report here the molecular characterization of the RIM11 gene, which we find is required for expression of several early meiotic genes. A close functional relationship between RIM11 and IME1 is supported by two observations. First, sin3 and ume6 mutations are epistatic to rim11 mutations; prior studies have demonstrated their epistasis to ime1 mutations. Second, overexpression of RIM11 can suppress an ime1 missense mutation (ime1-L321F) but not an ime1 deletion. Sequence analysis indicates that RIM11 specifies a protein kinase related to rat glycogen synthase kinase 3 and the Drosophila shaggy/zw3 gene product. Three partially defective rim11 mutations alter residues involved in ATP binding or catalysis, and a completely defective rim11 mutation alters a tyrosine residue that corresponds to the site of an essential phosphorylation for glycogen synthase kinase 3. Immune complexes containing a hemagglutinin (HA) epitope-tagged RIM11 derivative, HA-RIM11, phosphorylate two proteins, p58 and p60, whose biological function is undetermined. In addition, HA-RIM11 immune complexes phosphorylate a functional IME1 derivative but not the corresponding ime1-L321F derivative. We propose that RIM11 stimulates meiotic gene expression through phosphorylation of IME1. 相似文献