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131.
影响山羊体外受精的因素 总被引:5,自引:0,他引:5
以屠宰山羊卵母细胞为材料研究了公羊个体、附睾不同部位精子、成熟培养和受精时卵丘存在与否、卵丘扩展程度及卵龄对山羊体外受精的影响。结果表明 :1)不同公羊精液在受精、卵裂和桑椹 /囊胚率上都有显著差异 ;2 )附睾尾精子和鲜精的受精、卵裂和桑椹 /囊胚率无显著差异 ,但显著高于附睾体和附睾头精子 ;3)成熟培养 2 4和 2 7h卵母细胞的的桑椹胚 /囊胚率显著高于培养 2 1和 30h卵母细胞 ;4 )卵丘扩展 3和 4级卵母细胞受精和桑椹胚 /囊胚率显著高于扩展 0和 1级卵母细胞 ;5 )成熟培养前机械去卵丘严重影响卵母细胞体外受精和桑椹胚 /囊胚率 ;6 )受精前完全去掉卵丘显著影响桑椹胚 /囊胚率 相似文献
132.
OEP及卵黄浓度对蓝狐冻融精子质量的影响 总被引:6,自引:0,他引:6
人工采取 6只优质芬兰雄性蓝狐精液 ,利用不同OEP及卵黄含量的Tris 果糖 -柠檬酸钠稀释液稀释 ,制成细管冻精 ,透射电镜下观察精子冷冻前后质膜和顶体超微结构 ,荧光免疫方法检测不同培养时间冻融精子的质量。结果表明 ,蓝狐精子顶体外膜双层膜的厚度为 0 0 2 0 μm ,冷冻 -解冻过程中易发生质膜膨胀、顶体外膜融合现象。顶体产生的囊泡分两种类型 ,一种是体积较大的中空囊泡 ,平均直径为 1 2 5 μm。另一种是体积较小的实体囊泡 ,内充满顶体内容物 ,平均直径为 0 83μm ,两种囊泡的数量不定。OEP能有效抑制顶体囊泡形成 ,影响顶体囊泡类型、体积大小及囊泡数量 ,添加适宜剂量OEP能使顶体囊泡的体积明显缩小 ,囊泡的总数及中空囊泡的数量显著降低。蓝狐冻融精子质量与OEP及卵黄剂量有关 ,在卵黄存在的前提下 ,OEP有利于维持冻融过程中质膜 (5 6 3% )、顶体的完整性 (5 7 8% ) ,显著提高冻融精子活力 (5 4 7% )。在蓝狐精液稀释液中 ,OEP、卵黄的适宜含量分别为 1 %、 2 0 % 相似文献
133.
植物病毒协生作用及其分子机理 总被引:1,自引:0,他引:1
植物病毒协生作用分布广,是造成农作物减产的重要原因之一,抗病毒转基因植物中协生作用的出现,严重限制了基因工程植物的商品化生产。本文对植物病毒协生作用的类型和特点、协生作用中病毒与病毒、病毒与环境间的相互作用及其分子机制进行了阐述。 相似文献
134.
目的:研究精子非整倍体染色体与男性不育之间的关系。方法:用荧光原位杂交(FISH)技术,对12个不育患精子的染色体进行了研究,其中,10例少,弱,畸精症患为A组,2例正常或接近正常的样品为B组,另有2例正常健康献精为对照组,原位杂交采用染色体XY和18号探针,每个个体记数1000个精子,结果:杂交总有效率为98%,在B组男性不育XY和18号的二体频率为0.30%和0.30%,与对照组相比(0.15%,0%)无显差别,XY和18号失体的精子为0.15%和0%,与对照组(0%,0.15%)也无显差别,而A组的XY和18号染色体二体率为1.13%和0.96%,失体为1.13%和1.6%,与前两组相比,差异有显性,估算总的非整倍体率:A组为42.44%,B组为6.05%,对照组为2.59%,前与后两组相比,差异有显性,结论:不育患精子的染色体具有显的非整倍体性。 相似文献
135.
136.
137.
最近几年来 ,由于光子计数的发展 ,在弱光通量测定方面有了新的突破 ,动植物有机体在正常的生理状态下 (暗反应 ) ,它们的细胞、细胞器以及动物的肝脏、血液均有光子释放 ,同时由于光通量极弱 ,所以通常称为“超弱化学发光” ,它可以反映有机体基质代谢的综合活动 ,提供活体细胞物理化学反应或更复杂反应的信息 ,是生物体的化学发光 ,即有机物氧化过程中产生的激态分子 ,变到较低状态时 ,以光子形式释放能量。本文研究表明 ,奶山羊的精子存在有超弱化学发光现象 ,精子的超弱化学发光与活力呈强正相关 ,相关系数为 0 .932 5(P <0 .0 5) ,与… 相似文献
138.
精子特异性乳酸脱氢酶(LDH—C4)在精子的运动和存活等生理活动中起着重要的作用。研究表明,LDH—C4接种鼠、兔等能够降低动物的生育率。通过RT—PER方法从布氏田鼠睾丸总RNA中克隆出编码抗原决定簇的LDH—C4基因片断;采用T—A克隆的方法将其插入到pCR3.1载体中构建重组载体pCR3.1—bvLDH—C4′,测序结果表明克隆的基因片断与已知小鼠相应片断有83%的序列同源。通过质脂体法转染HeLa细胞,RT—PCR证实其可在mRNA水平有效表达;通过肌肉接种BAIB/c小鼠,RT-PER结果表明其在体内也可有效表达。 相似文献
139.
绵羊胞内单精子注射技术 总被引:7,自引:0,他引:7
In this study, the possibility of sheep transgenesis by intracytoplasmic sperm injection (ICSI) was assessed. In experiment 1, activation of ovine oocytes matured in vitro in preparation for ICSI has been investigated with 3.42 mmol/L Ca2+ treatment, ionomycin alone and ionomycin followed by 6-dimethylaminopurine (DMAP) after 3-h delay (group 1, 2 and 3, respectively). After activation, the oocytes were then cultured in SOFaaBSA medium. Cleavage rates were significantly (P<0.05) different among three groups (18.4%, 91.8% and 71.7%, respectively). In additional culture, no parthenotes in group 1, whereas 11% and 17.4% in group 2 and 3 developed to the blastocyst stage. Therefore we used the third activation method in the following ICSI tests. In experiment 2, development of ovine oocytes after ICSI was investigated. Thawed semen from two rams was separated by Percoll centrifugation and was used for ICSI or in vitro fertilization (IVF) trails. A total of 71.8% of oocytes reached the 2-cell stage following living sperm injection, which was significantly (p>0.05) different from those following IVF (41.4%) and sham-ICSI (30.2%). After seven days' culture, no sham-injected oocytes developed into the blastocyst stage, although 7% in ICSI and 16.1% in IVF-oocytes developed into the blastocyst stage, but there was no significant difference in ICSI and IVF groups (p>0.05). In the further study, the possibility of sheep transgenesis by ICSI was assessed. After coinjection of ovine oocytes matured in vitro with dead sperm cold to -20 degrees C and exogenous DNA encoding green fluorescent protein (GFP), seventy-three percent of coinjected oocytes developed to 2-cell stage (33/45) and two of them were transgene-expressing embryos. Among ten embryos at the 16-cell stage, all embryonic cells in one transgenic embryo still expressed GFP. Four coinjected blastocysts were thawed and transferred to the uterine of the two progesterone-synchronized recipient ewe. No pregnancies were detected on the 60th day. These results suggested sheep transgenic embryos could be produced by ICSI and further studies should be performed. 相似文献
140.
蟋蟀精子表面LCA及ConA结合糖复合物的分布变化 总被引:8,自引:0,他引:8
LCA and ConA-binding glycoconjugates on cricket (Teleogryllus emma) sperm surface were detected with fluorescence microscope after FITC labelling for better understanding of the distribution of glycoconjugates during spermatogenesis and spermiogenesis. FITC-LCA and FITC-ConA were bound on the spermatocytes, and their distribution changes in the process of spermiogenesis were observed .In the testis sperm, FITC-LCA and FITC-ConA were mainly bound on the head and neck region. That is different from the mark pattern of spermatophore sperm, in which the nucleus, neck region and front of the tail showed obvious fluorescence mark, especially the acrosome complex and neck region exhibited stronger mark. The mark patterns of FITC-LCA and FITC-ConA were similar,though the former was distinctly clearer than the latter. But a little difference still exists in both of them. For example in the ninth stage of spermatid, FITC-LCA mark is located on the spermatid head and neck region, and FITC-ConA mark on the spermatid head, neck and front of the tail region. When fixed germ cells were treated with PBS instead of lectin solution, or fixed cells were incubated with lectin solution, which have been treated with 0.1 mol/L specific sugar inhibitor, i.e.α-D-mannose for FITC-LCA and FITC-ConA, and α-D-glucose for FITC-ConA, no mark was observed on the cells. Those results indicate that FITC-LCA conjugated glycoconjugates has the α-D- mannose residue, and FITC-ConA conjugated glycoconjugates has the α-D-mannose and α-D-glucose residue. The investigations show that the changes in glycoconjugates distribution of cricket sperm is similar to those of other insects and mammals. The evidence exhibit that a common rule of the glycoconjugates distribution on the sperm surface is followed by most of animal sperm which may relate to the function of sperm physiology. 相似文献