角速度计检测信号数字滤波处理的研究

我们曾采用压电式陀螺仪角速度计检测行走车辆的角速度。但由于行走车发动机的振动、路面不平等因素的影响，在获得的信号中混有噪声，因而存在一定的误差。为了提高检测信号精度，有必要消除器器声。我们针对上述问题，采用数字滤波的软件实现方法来消除噪声，提高检测精度。对由实验所获得的数据进行了有、无数字滤波处理的对比分析，获得了较好的结果。这表明本研究通过软件的方法，既提高了检测精度，又降低了硬件成本。     

Identification by isoelectric focusing of creatine kinase-MM isoforms in the plasma and striated muscle of pigs

Total creatine kinase (CK) and CK-MM isoforms were determined in plasma and longissimus dorsi muscle extracts from normal pigs. Based on their total CK activity, the pigs were divided into two groups. Pigs of group 1 (n=16) had a mean plasma total CK of 298±16 U/L and the distribution of the CK-MM isoforms was 65.7±2.5% CK-MM₃, 18.9±1.6% CK-MM₂ and 15.3±1.5% CK-MM. In group 2 (n=18; 826±75 U/L total CK) four isoforms were observed: 3.1±0.9% CK-MM, 67.9±3.0% CK-MM₃, 21.5±2.3% CK-MM₂ and 7.5±1.3% CK-MM₁. The differences between the two groups of pigs were significant (p<0.001) for CK-MM₁ and the presence of CK-MM. Four CK-MM isoforms were also detected in longissimus dorsi muscle homogenates: 45.6±8.1% CK-MM, 32.6±11.7% CK-MM₃, 16.6±2.3% CK-MM₂ and 5.1±2.8% CK-MM₁. The release of CK-MM isoforms from muscle into plasma seems to be unrelated to the concentration of these isoforms in striated muscle.     

Expression of receptor tyrosine kinases VEGFR-1 (FLT-1), VEGFR-2 (KDR), EGFR-1, PDGFRa and c-Met in canine primary brain tumours

Inhibition of tumour growth and angiogenesis by targeting key growth factor receptors is a promising therapeutic strategy for central nervous system tumours. Characterization of these growth factor receptors in canine primary brain tumours has not been done. Using quantitative real‐time TaqMan polymerase chain reaction (PCR), we evaluated the expression of messenger RNA (mRNA) for five tyrosine kinase growth factor receptors (vascular endothelial growth factor receptor [VEGFR]‐1, VEGFR‐2, endothelial growth factor receptor [EGFR]‐1, platelet‐derived growth factor receptor a [PDGFRa], and c‐Met) relative to normal cerebral cortex in 66 spontaneous canine primary brain tumours. Increased expression of VEGFR‐1 and VEGFR‐2 mRNA was greatest in grade IV astrocytomas (glioblastoma multiforme) and grade III (anaplastic) oligodendrogliomas. EGFR‐1 mRNA expression was more consistently increased than the other receptors in all tumour types, while increased PDGFRa mRNA expression was mostly restricted to oligodendrogliomas. The similarities in increased expression of these tyrosine kinase growth factor receptors in these canine tumours, as compared to data from their human counterparts, suggest that common molecular mechanisms may be present.     

西门塔尔牛肌内和皮下脂肪miRNA表达谱及miR-27b靶基因分析

【目的】通过分析西门塔尔牛肌内脂肪和皮下脂肪差异表达miRNA,及对重要的候选miRNA-27b进行靶基因预测及相关生物信息学分析,探索miRNA在动物肌内脂肪生长、发育过程中的作用及其调控机制。【方法】利用miRNA微阵列芯片技术对肌内脂肪和皮下脂肪miRNA表达谱进行检测和分析以筛选差异表达miRNA;qRT-PCR方法验证4个在肌内脂肪显著高表达的候选miRNAs;采用Targetscan生物信息学计算方法预测目标miR-27b（对肌内脂肪沉积可能起重要调节作用）的靶基因,并对靶基因进行GO注释描述、富集分析及KEGG富集。【结果】miRNA芯片分析发现肌内脂肪和皮下脂肪共有88个差异表达极显著miRNA（P＜0.01）。候选的4个在肌内脂肪高表达miRNAs（miR-140、miR-145、miR-143、miR-27b）的qRT-PCR检测结果与芯片分析结果具有很好的一致性。KEGG富集显示,目标miR-27b的预测靶基因在MAPK、Wnt、Hedgehog、TGF-beta、GnRH等信号通路中显著富集,其中在MAPK信号通路中富集度最高。【结论】牛肌内脂肪和皮下脂肪组织中确实存在一些差异表达的miRNAs,某些重要的在差异高表达miRNA（如miR-27b）可能以独特的通路（如MAPK信号）来调节牛肌内脂肪的形成过程。     

采用花粉管通道法将蛋白激酶基因导入玉米自交系的研究

通过花粉管通道法将ZmPtil,ZmPtil-1,ZmCIPK2三种蛋白激酶基因植物表达载体分别导入玉米自交系吉444,经草丁膦筛选后得40株抗性植株,通过PCR检测其中28株为PCR阳性植株,平均转化率为1.33％,最后收获11株转基因植株.干旱条件下通过对转基因T1植株的单株籽粒产量、千粒重两个指标进行差异显著性和...     

调亏灌溉下酿酒葡萄耗水特性及水分生产函数研究

为了确定酿酒葡萄的水分生产函数,以酿酒葡萄"梅鹿辄"为供试品种,采用滴灌的方式,以不同生育期土壤水分水平为试验因素,对酿酒葡萄不同生育期进行亏水处理,测定不同生育期土壤含水率、耗水量、产量及水分利用效率,研究了不同生育期、不同土壤水分状况对酿酒葡萄耗水量和产量的影响。结果表明,土壤水分对酿酒葡萄产量的影响规律为浆果膨大期最大,其次是开花期、着色成熟期、抽蔓期,萌芽期最小;通过对Jensen模型与Blank模型进行计算比较,发现在该试验中Jensen模型更为合理,且得出不同生育期水分生产函数的敏感指数为:浆果膨大期开花期着色成熟期抽蔓期萌芽期,与酿酒葡萄耗水规律一致;在萌芽期、抽蔓期及着色成熟期的土壤水分保持在田间持水率的60%~65%左右不会造成酿酒葡萄减产,而在浆果膨大期进行充分供水,既可获得高产,也使水分利用效率达到较高水平。     

应用ISSR标记分析12份臂形草种质的遗传差异

选用17条ISSR引物分析12份臂形草种质遗传差异,结果表明:臂形草种质问的多态性高,17条引物产生了286条DNA片段,其中280条具有多态性,多态性比率高达97.90%;每个引物可扩增出6～23条DNA片段,平均16.8条,种质问遗传相似系数变化范围为0.486～0.968,平均值为0.681;通过聚类分析可将12份臂形草种质分为两类:一类为巴拉草和湿生臂形草,其余品种则聚为另一类.     

USP14 regulates H2O2 induced oxidative stress in H9c2 cells

AIM:To evaluate the effect of inhibiting ubiquitin-specific protease 14(USPl4) activity on oxidative stress induced by H₂O₂ of H9c2 cells.METHODS:The H9c2 cells were incubated with H₂O₂ at 25 μmol/L for 2 h to establish the oxidative stress injury model.The cells were divided into control group,H₂O₂ group,IU1 group (25 μmol/L or 50 μmol/L) and IU1+H₂O₂ group.The H9c2 cells activity was measured by MTS assay.The level of intracellular reactive oxygen species (ROS) and cell survival rate were analyzed by flow cytometry assay.The changes of the mitogen-activated protein kinase (MAPK) family related proteins were detected by Western blot.RESULTS:Compared with control group,the cell activity and the viability rate in H₂O₂ group were decreased (P<0.05),while the intracellular ROS,the protein levels of Bax/Bcl-2,P53,p-ERK1/2,p-JNK and p-P38 were increased (P<0.05).Compared with H₂O₂ group,the cell activity and the viability rate of the H9c2 cells in IU1+H₂O₂ group were increased (P<0.05),while the intracellular ROS,the protein levels of Bax/Bcl-2,P53,p-ERK1/2,p-JNK and p-P38 were decreased (P<0.05).CONCLUSION:Inhibition of USPl4 activity reduces the oxidative stress injury of the H9c2 cells.The mechanism may be related to inhibition of the MAPK signaling and down-regulation of apoptosis related proteins.     

G protein signalling involved in host recognition and mycoparasitismrelated chitinase expression in Trichoderma atroviride

Mycoparasitic species of Trichoderma are commercially applied as biological control agents against various fungal pathogens. The mycoparasitic interaction is host specific and includes recognition, attack and subsequent penetration and killing of the host. Investigations on the underlying events revealed that Trichoderma responds to multiple signals from the host (e.g. lectins or other ligands such as low molecular weight components released from the host's cell wall) and host attack is ac…     

茶树蛋白激酶基因CsCIPK的克隆与表达特性分析

以茶树品种‘龙井43’作为材料,利用RT-PCR方法,从茶树的cDNA中克隆得到1个编码蛋白激酶的基因,命名为CsCIPK。序列分析表明,CsCIPK开放阅读框长度为1 341 bp,编码446个氨基酸,蛋白质分子量为414234。蛋白功能域预测和多重对比显示,CsCIPK蛋白含有1个保守的N端激酶结构域和1个相对不保守的C端调节结构域,即丝氨酸/苏氨酸激酶结构域和NAF结构域。理化性质、亲/疏水性、无序化分析显示,CsCIPK属于疏水性蛋白,理论等电点为7.04,有4段无序化区域,其二级结构分析显示主要由α螺旋、不规则卷曲组成。通过实时荧光定量PCR对‘龙井43’和‘安吉白茶’中的CsCIPK表达特性进行分析。结果显示‘龙井43’中CsCIPK的相对表达量在高温、干旱及盐处理4 h、低温处理24 h时达到最高。‘安吉白茶’中CsCIPK的相对表达量在高温及盐处理4 h、低温及干旱处理1h时达到最高。CsCIPK在‘龙井43’的根中,‘安吉白茶’茎中表达量最高。不同浓度的GA和IBA处理‘龙井43’茶苗,结果显示0.2 mmol·L-1 GA处理后,CsCIPK表达量先升高后下降,6 d时处理组为对照组的62倍;0.6 mmol·L-1 IBA处理后,CsCIPK的表达量在3 d时显著高于对照组;不同浓度GA和IBA处理后,9 d时CsCIPK表达量均显著低于对照。