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饲喂硬脂酸和癸酸对工蜂合成10-HDA的影响 被引量:2
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作者 刘丽 杨晓慧 王瑞明 《西北农业学报》 CAS CSCD 北大核心 2016年第7期973-978,共6页
为探讨硬脂酸和癸酸对工蜂合成10-HDA及其生物合成相关酶基因表达的影响,在工蜂基础日粮中添加不同质量分数的硬脂酸和癸酸,采用高效液相色谱法和半定量RT-PCR技术测定不同日龄段工蜂上颚腺10-HDA的合成量和相关酶基因的表达量。结果显... 为探讨硬脂酸和癸酸对工蜂合成10-HDA及其生物合成相关酶基因表达的影响,在工蜂基础日粮中添加不同质量分数的硬脂酸和癸酸,采用高效液相色谱法和半定量RT-PCR技术测定不同日龄段工蜂上颚腺10-HDA的合成量和相关酶基因的表达量。结果显示,工蜂日粮中添加不同质量分数的硬脂酸和癸酸可在一定程度上提高工蜂上颚腺10-HDA的产量,在工蜂5、10、15日龄时,w=5%硬脂酸组和w=1%癸酸组10-HDA的合成量均显著高于空白组(P<0.05),且全期10-HDA产量的平均值分别较空白组提高11.82%和13.37%。另外,w=5%硬脂酸组和w=1%癸酸组能使工蜂上颚腺10-HDA的分泌高峰提前,由原来的20日龄分别提前至15日龄和10日龄。同时,添加硬脂酸和癸酸后,工蜂在15日龄前的ETF-β和KAT基因表达量均增加。表明,硬脂酸和癸酸可影响工蜂10-HDA生物合成相关酶基因的表达,促进工蜂上颚腺合成10-HDA,在短时间内提高10-HDA的产量。 展开更多
关键词 硬脂酸 癸酸 10-HDA etf-β KAT 高效液相色谱
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REGULATION OF THE INTERFERON-INDUCIBLE PROTEIN KINASEPKR AND2'5' OLIGOADENYLATE SYNTHETASE BY A CATALYTICALLY  INACTIVE PKR M
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作者 校秋蓉 《Journal of Pharmaceutical Analysis》 CAS 1995年第2期191-191,共1页
The interferon-inducible double-stranded RNA-dependent protein kinase PKR has been suggested to function as a turnour suppressor gene product.Catalytically inactive mutants of PKR give rise to a tumourigenic phenotype... The interferon-inducible double-stranded RNA-dependent protein kinase PKR has been suggested to function as a turnour suppressor gene product.Catalytically inactive mutants of PKR give rise to a tumourigenic phenotype when overexpressed in NIH-3T3 fibroblasts and this has been attributed to a dominant negative effect on only inhibits the protein kinase activity of wild-type PKR but is also inhibitory towards another dotlblestranded RNA-dependent enzyme,the 40kDa form of 2'5'oligoadenylate synthetase. Inhibition of both wile-type PKR or 2'5' oligoadenylate synthetase is reversed by adding higher concentrations of double-stranded RNA. These results suggest competition between PKR K296R and wild-type PKR or 2'5' oligoadenylate synthetase for limiting amounts of dublestranded RNA. Moreover,the data imply that the tumourigenic effect of this PKR mutant could be due to inhibition of additional pathways requiring low levels of double-strandeed RNA for activation and cannot be unambiguously attributed to inhibition of endogenous PKR itself. 展开更多
关键词 dsRNA 1 etf-2 INTERFERON PKR 1 2'5'-oligoadenylate synthetase
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