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排序方式: 共有171条查询结果,搜索用时 15 毫秒
71.
以10 mmol/L CaCl2溶液处理滨梅幼苗叶片后,置于培养箱于(40±2)℃高温、光照强度(1 200±50)μmol·m-2·s-1下培养,定期测定有关生理生化指标,以探讨外源Ca2+对高温强光胁迫下滨梅幼苗的保护效应.结果显示:(1)与蒸馏水处理组相比,Ca2+处理使高温强光胁迫下滨梅幼苗叶片的脯氨酸含量显著升高,可溶性糖含量变化不明显,根系活力小幅降低;Ca2+处理有效抑制了高温强光下膜透性的加大,提高和保护了Ca2+-ATPase的活性.(2)采用Ca2+螯合剂EGTA或钙调素拮抗剂TFP对滨梅幼苗叶片同法处理并同条件胁迫时,与Ca2+处理相比,滨梅幼苗的脯氨酸、可溶性糖含量、Ca2+-ATPase活性和根系活力均明显下降,膜透性加大.研究表明,Ca2+处理能提高滨梅幼苗对高温强光的耐受性;Ca2+信号系统参与了胁迫过程中的渗透物质和Ca2+-ATPase活性等的调节. 相似文献
72.
Xu XM Carlson BA Irons R Mix H Zhong N Gladyshev VN Hatfield DL 《The Biochemical journal》2007,404(1):115-120
Selenophosphate synthetase (SelD) generates the selenium donor for selenocysteine biosynthesis in eubacteria. One homologue of SelD in eukaryotes is SPS1 (selenophosphate synthetase 1) and a second one, SPS2, was identified as a selenoprotein in mammals. Earlier in vitro studies showed SPS2, but not SPS1, synthesized selenophosphate from selenide, whereas SPS1 may utilize a different substrate. The roles of these enzymes in selenoprotein synthesis in vivo remain unknown. To address their function in vivo, we knocked down SPS2 in NIH3T3 cells using small interfering RNA and found that selenoprotein biosynthesis was severely impaired, whereas knockdown of SPS1 had no effect. Transfection of SPS2 into SPS2 knockdown cells restored selenoprotein biosynthesis, but SPS1 did not, indicating that SPS1 cannot complement SPS2 function. These in vivo studies indicate that SPS2 is essential for generating the selenium donor for selenocysteine biosynthesis in mammals, whereas SPS1 probably has a more specialized, non-essential role in selenoprotein metabolism. 相似文献
73.
Strain improvement and metabolic flux analysis in the wild-type and a mutant Lactobacillus lactis strain for L(+)-lactic acid production 总被引:3,自引:0,他引:3
The effects of initial glucose concentration and calcium lactate concentration on the lactic acid production by the parent strain, Lactobacillus lactis BME5-18, were studied. The results of the experiments indicated that glucose and lactate repressed the cell growth and the lactic acid production by Lactobacillus lactis BME5-18. A L(+)-lactic acid overproducing strain, Lactobacillus lactis BME5-18M, was screened by mutagenizing the parent strain with ultraviolet (UV) light irradiation and selecting the high glucose and lactate calcium concentration repression resistant mutant. Starting with a concentration of 100g L(-1) glucose, the mutant produced 98.6 g L(-1) lactic acid after 60 h in flasks, 73.9% higher than that of the parent strain. The L(+)-lactic acid purity was 98.1% by weight based on the amount of total lactic acid. The culture of the parent strain could not be analyzed well by conventional metabolic flux analysis techniques, since some pyruvate were accumulated intracellularly. Therefore, a revised flux analysis method was proposed by introducing intracellular pyruvate pool. Further studies demonstrate that there is a high level of NADH oxidase activity (12.11 mmol mg(-1) min(-1)) in the parent strain. The molecular mechanisms of the strain improvement were proposed, i.e., the high level of NADH oxidase activity was eliminated and the uptake rate of glucose was increased from 82.1 C-mmol (g DW h)(-1) to 98.9 C-mmol (g DW h)(-1) by mutagenizing the parent strain with UV, and therefore the mutant strain converts mostly pyruvate to lactic acid with a higher productivity (1.76 g L(-1) h(-1)) than the parent strain (0.95 g L(-1) h(-1)). 相似文献
74.
太湖日本沼虾野生群体遗传结构的微卫星分析 总被引:3,自引:0,他引:3
利用8个高度多态性的微卫星位点分析了太湖日本沼虾野生群体的遗传结构.结果表明:在15个群体中至少有3个位点经Bonferroni校正后显示杂合不足,显著偏离了HardyWeinberg平衡;15个群体中观测杂合度均大于0.683,显示出较高的遗传多样性水平,但其波动明显,如太湖东、南部的渡口和陆巷等群体的遗传多样性高于西、北部的华庄和洋渚等群体;突变-漂移平衡分析结果显示,15个群体中部分位点杂合显著过剩,偏离了突变-漂移平衡,且近期曾经历过瓶颈效应,群体数量曾经下降;群体间AMOVA分析表明,太湖日本沼虾群体间遗传分化程度较低(FST=0.011),98.9%的遗传变异来自群体内,1.1%来自群体间,并没有形成显著的遗传结构,在种质资源保护和管理上可视作一个单元;华庄与吴塘门群体间DA遗传距离达到0.206,已接近种间分类界限,故太湖日本沼虾种质资源可持续利用工作仍须深入的研究. 相似文献
75.
改变培养基碳源复壮草菇退化菌种 总被引:1,自引:0,他引:1
碳源是草菇重要的营养源之一,草菇菌种在添加葡萄糖的传统PDA上长期继代会导致菌种退化。本研究用蔗糖、果糖、甘露醇、海藻糖代替PDA中的葡萄糖,对草菇原种(D0)和退化菌株(D1-D3)进行复壮。结果表明:改变碳源对D0影响不显著。蔗糖、果糖、甘露醇、海藻糖均可提高D1-D3的气生菌丝密度、菌丝生长速度和生物量,诱导厚垣孢子产生,并增加菌丝多糖和蛋白质含量;有效抑制了活性氧O2 -·、H2O2的积累;提升了超氧化物歧化酶(SOD)和过氧化物酶(POD)活性,但过氧化氢酶(CAT)活性变化不显著;且菌种退化程度越高,复壮效果越好,海藻糖的效果最佳。与对照组相比,海藻糖处理组使退化最严重的D3的菌丝生长速度和生物量分别提高了75.00%和66.67%,多糖和蛋白质含量分别增加了22.49%和16.58%;O2 -·和H2O2分别降低了12.50%、12.83%;POD和SOD分别提高了33.33%和255.56%。本研究通过改变培养基的碳源,有效复壮了草菇退化菌种的菌丝特性;也为延缓食用菌菌种退化研究提供参考。 相似文献
76.
Mei-Zhu Wu Bing-Quan Xu Xiao-Zheng Zhang Sha Liu You-Ping Luo Xue-Ming Zhou Guang-Ying Chen 《化学与生物多样性》2023,20(5):e202300338
Two new guaiane-type sesquiterpenes dysodensiols J and L, one new natural product dysodensiol K together with four known biogenetically related guaiane-type sesquiterpenes were isolated from the stems of Fissistigma oldhamii. Their structures were elucidated by detailed analysis of NMR, HR-ESI-MS, IR and Optical rotations data. Compound 1 contains an uncommon five-membered ether ring. The inhibitory effect of all compounds on the proliferation of primary synovial cells was evaluated. Compound 3 showed inhibitory activity with an IC50 value of 6.8 μM. Compounds 5–7 exhibited moderate inhibitory activity with IC50 values of 23.8, 26.6, and 27.1 μM, respectively. 相似文献
77.
Kim JY Carlson BA Xu XM Zeng Y Chen S Gladyshev VN Lee BJ Hatfield DL 《Biochemical and biophysical research communications》2011,(4):814-819
GDP dissociation inhibitor (GDI) plays an essential role in regulating the state of bound nucleotides and subcellular localizations of Rab proteins. In our previous study, we showed that OsGDI3 facilitates the recycling of OsRab11 with a help of OsGAP1. In this study, we show that OsGDI3 complement the yeast sec19-1 mutant, a temperature-sensitive allele of the yeast GDI gene, suggesting that OsGDI3 is a functional ortholog of yeast GDI. To obtain further knowledge on the function of OsGDI3, candidate OsGDI3-interacting proteins were identified by yeast two-hybrid screens. OsMAPK2 is one of OsGDI3 interacting proteins from yeast two-hybrid screens and subject to further analysis. A kinase assay showed that the autophosphorylation activity of OsMAPK2 is inhibited by OsGDI3 in vitro. In addition, ectopic expressions of OsGDI3-in Arabidopsis cause reductions at the level of phosphorylated AtMPK in phosphorylation activity. Taken together, OsGDI3 functions as a negative regulator of OsMAPK2 through modulating its kinase activity. 相似文献
78.
Li-Xiao Sun Hui Qian Meng-Yu Liu Ming-Hua Wu Yun-Yun Wei Xue-Ming Zhu Jian-Ping Lu Fu-Cheng Lin Xiao-Hong Liu 《Environmental microbiology》2022,24(3):1076-1092
Magnaporthe oryzae is an important plant pathogen that causes rice blast. Hse1 and Vps27 are components of ESCRT-0 involved in the multivesicular body (MVB) sorting pathway and biogenesis. To date, the biological functions of ESCRT-0 in M. oryzae have not been determined. In this study, we identified and characterized Hse1 and Vps27 in M. oryzae. Disruption of MoHse1 and MoVps27 caused pleiotropic defects in growth, conidiation, sexual development and pathogenicity, thereby resulting in loss of virulence in rice and barley leaves. Disruption of MoHse1 and MoVps27 triggered increased lipidation of MoAtg8 and degradation of GFP-MoAtg8, indicating that ESCRT-0 is involved in the regulation of autophagy. ESCRT-0 was determined to interact with coat protein complex II (COPII), a regulator functioning in homeostasis of the endoplasmic reticulum (ER homeostasis), and disruption of MoHse1 and MoVps27 also blocked activation of the unfolded protein response (UPR) and autophagy of the endoplasmic reticulum (ER-phagy). Overall, our results indicate that ESCRT-0 plays critical roles in regulating fungal development, virulence, autophagy and ER-phagy in M. oryzae. 相似文献
79.
不同海拔火绒草叶绿体超微结构的比较 总被引:13,自引:0,他引:13
利用透射电镜对生长于青藏高原东北部3个不同海拔地区(2300m、2700m和3800m)的火绒草叶绿体超微结构进行了比较观察。结果发现,随着海拔的升高,叶绿体结构差异明显。海拔2300m处,叶绿体呈扁船形,沿细胞壁分布,基粒片层排列整齐,片层可达32层;海拔2700m处,叶绿体呈扁船形,沿细胞壁分布,基粒片层排列不规则,片层下降到十几层,类囊体出现轻微膨大;海拔3800m处,叶绿体呈圆形,位于细胞中央,基粒片层则严重扭曲,片层只有几层,类囊体膨大严重,出现脂质小球。研究表明,火绒草叶绿体结构的变化是对逆境的一种适应,是青藏高原特殊生态条件长期胁迫的结果。 相似文献
80.
Homo sapiens J domain protein (HSJ1) is a J-domain containing co-chaperone that is known to stimulate ATPase activity of HSP70 chaperone, while it also harbors two ubiquitin (Ub)-interacting motifs (UIMs) that may bind with ubiquitinated substrates and potentially function in protein degradation. We studied the effects of HSJ1a on the protein levels of both normal and the disease--related polyQ-expanded forms of ataxin-3 (Atx3) in cells. The results demonstrate that the N-terminal J-domain and the C-terminal UIM domain of HSJ1a exert opposite functions in regulating the protein level of cellular overexpressed Atx3. This dual regulation is dependent on the binding of the J-domain with HSP70, and the UIM domain with polyUb chains. The J-domain down-regulates the protein level of Atx3 through HSP70 mediated proteasomal degradation, while the UIM domain may alleviate this process via maintaining the ubiquitinated Atx3. We propose that co-chaperone HSJ1a orchestrates the balance of substrates in stressed cells in a Yin-Yang manner. 相似文献