苦荞R2R3-MYB转录因子调控原花青素生物合成的研究

基于苦荞花期转录组数据,该研究筛选并克隆获得一个黄酮代谢相关的MYB类转录因子,并命名为FtMYB23。该基因ORF框长879bp,编码292个氨基酸;系统进化树分析显示,FtMYB23与SG5-MYB亚家族成员聚为一簇,属于典型的R2R3-MYB型转录因子。β-半乳糖苷酶滤纸分析表明,其具有转录激活活性。FtMYB23过表达转基因拟南芥株系的表型分析表明,3个阳性株系的种皮颜色均呈现出比野生型更深的褐色,其叶中原花青素含量均极显著增加(P 0.01),分别为野生型的4.68、3.5和2.8倍。qRT-PCR分析表明,转基因拟南芥中黄酮合成相关的AtCHS、AtCHI、AtF3H、AtF3′H、AtFLS、AtDFR和AtBAN等基因的表达量显著升高(P 0.05),而AtTT12的表达量极显著降低(P 0.01)。研究认为,FtMYB23作为典型的Subgroup5-MYB(SG5-MYB)激活型转录因子,通过促进黄酮合成途径早期关键酶基因的表达,从而提高原花青素的合成与积累。     

一个Ⅰ型遗传性淋巴水肿中国家系的VEGFR3基因的新突变方式

通过对国人Ⅰ型遗传性淋巴水肿一家系分子遗传学检测,报告VEGFR-3基因新突变。首先在Ⅰ型遗传性淋巴水肿对该家系进行致病基因的连锁分析,然后用DNA直接测序方法进行基因突变分析。连锁分析和单倍体分析确定该家系致病基因位于5q35.3,与Ⅰ型遗传性淋巴水肿连锁。VEGFR-3基因突变分析发现了一个新的错义突变D1055V,该错义突变在家系中共分离,且在100个正常对照组中未发现该序列改变。本研究首次报告了国内Ⅰ型遗传性淋巴水肿VEGFR-3基因新的错义突变D1055V,丰富了VEGFR-3基因基因突变谱,为今后开展遗传性淋巴水肿的基因诊断和遗传咨询奠定基础。     

Detection of a new mutation (T1140C) in a patient with Hunter syndrome from Guangdong,China

This study identified mutations of the idumate-2-suffatase (IDS) gene in a patient with Hunter syndrome,and established a basis for the diagnosis of the prenatal gene of Hunter syndrome.Urine glyeosaminoglycan (GAG) assay was used to make the preliminary diagnosis of mucopolysaccharidosis type H.Polymerase chain reaction (PCR) from dried blood spots and DNA sequencing were applied to analyze hotspot mutations in exons 9,3 and 8 of the IDS gene in the proband and his parents.A new missense mutation (T1140C) in exon 8 of the IDS gene was found by using DNA sequencing.This mutation caused a substitution of codon 339 from CTA (leucine) to CCA (praline).The patient is a hemizygote,and his mother is a heterozygote.The new missense mutation results in a change in the primary and tertiary structure of the IDS protein.It is possible that this mutation severely impairs enzymatic activity and is the underlying basis for the pathology seen in this patient with Hunter syndrome.     

Specific on-plate enrichment of phosphorylated peptides for direct MALDI-TOF MS analysis

An on-plate specific enrichment method is presented for the direct analysis of peptides phosphorylation. An array of sintered TiO 2 nanoparticle spots was prepared on a stainless steel plate to provide porous substrate with a very large specific surface and durable functions. These spots were used to selectively capture phosphorylated peptides from peptide mixtures, and the immobilized phosphopeptides could then be analyzed directly by MALDI MS after washing away the nonphosphorylated peptides. beta-Casein and protein mixtures were employed as model samples to investigate the selection efficiency. In this strategy, the steps of phosphopeptide capture, purification, and subsequent mass spectrometry analysis are all successfully accomplished on a single target plate, which greatly reduces sample loss and simplifies analytical procedures. The low detection limit, small sample size, and rapid selective entrapment show that this on-plate strategy is promising for online enrichment of phosphopeptides, which is essential for the analysis of minute amount of samples in high-throughput proteome research.     

抗逆转录病毒药对孕育期雌鼠心血管影响*

目的: 评价抗逆转录病毒药对孕育期雌性大鼠心血管功能及某些生化指标的影响。方法: SD大鼠9周龄雌鼠19只、10周龄雄鼠6只,9只/10只雌鼠与3只雄鼠合1笼,共2笼,分为正常对照组(CON)、高效抗逆转录病毒治疗组(HARRT)。其中CON组雌性大鼠每天早、晚生理盐水 (10 ml/kg)灌胃,HARRT组雌性大鼠灌等容积抗逆转录病毒药(AZT 31.25 mg/kg +3TC 15.63 mg/kg +LPV/r (41.67/10.42) mg/kg),连续3个月。记录雌性大鼠体重、存活情况;检测超声心动图,多导生理记录仪检测动脉血压、心脏血流动力学参数;相应试剂盒检测血糖、血脂四项、心肌酶及肝酶;Masson染色及透射电镜分别观察心肌胶原纤维和心肌细胞超微结构。结果: CON组雌性大鼠均存活(9/9),HARRT组雌性大鼠存活6只(6/10);与CON组比较,HAART组雌性大鼠体重减少(P＜ 0.01);LVDd、IVST、LVPWT、LAD增加(P＜0.05);动脉舒张压增加(P＜0.05)、LVP +dP/dt_max减少(P＜0.01);TG减少、Glu增加(P＜0.05)、CK减少(P＜0.01)、GOT减少(P＜0.05);心肌组织胶原纤维增多,心肌细胞超微结构异常。结论: 抗逆转录病毒药可导致孕育期雌性大鼠心血管病变。     

落叶阔叶林反照率的时间变化与影响因素

反照率原位测量对生态系统能量收支及其遥感应用至关重要,但目前坡面地形反照率的测量方式有局限且可见光与近红外波段反照率时间变化的差异尚不清楚。本研究以东北地区帽儿山森林生态站的落叶阔叶林为例,探究入射和反射太阳辐射(SR,300～2800 nm)、光合有效辐射(PAR,400～700 nm)、近红外辐射(NIR,700～2800 nm)的反照率时间变化特征及其影响因子,同时分析了两种辐射表安装方式反照率的差异。结果表明: 晴天SR和NIR反照率日变化呈上下午不对称的U型曲线,但PAR从早到晚递增;阴天反照率均先急剧下降后趋于稳定。平行于坡面测量增大了反照率的日均值,但缓和了SR、NIR反照率日不对称的现象。从整个生长季来看,SR、NIR与PAR反照率水平测量时最大值分别为0.16、0.27和0.11,最小值分别为0.07、0.11和0.03。SR和NIR反照率季节变化均为先增大后减小(7月为峰值),PAR则相反,SR反照率主要受NIR而不是PAR控制。各波段反照率季节变化的影响因子按照贡献率排序为宽带归一化植被指数(61.7%～78.5%,可表征叶面积指数)>太阳高度角(15.4%～36.9%)>晴空指数(0.4%～36.9%)。     

NAMPT regulates PKM2 nuclear location through 14-3-3ζ: Conferring resistance to tamoxifen in breast cancer

The resistance against tamoxifen therapy has become one of the major obstacles in the clinical treatment of breast cancer. Nicotinamide phosphoribosyltransferase (NAMPT) is an essential enzyme catalyzing nicotinamide adenine dinucleotide biosynthesis and is important for tumor metabolism. The study here sought to explore the effect of NAMPT on breast cancer survival with tamoxifen conditioning. We found that NAMPT was highly expressed in breast cancer cells compared with normal mammary epithelial cells. Inhibition of NAMPT by FK866 inhibited cell viability and aggravated apoptosis in cancer cells treated with 4-hydroxytamoxifen. NAMPT overexpression upregulated 14-3-3ζ expression. Knockdown of 14-3-3ζ reduced cell survival and promoted apoptosis. Activation of Akt signaling, rather than ERK1/2 pathway, is responsible for 14-3-3ζ regulation by NAMPT overexpression. Furthermore, NAMPT overexpression led to PKM2 accumulation in the cell nucleus and could be dampened by 14-3-3ζ inhibition. In addition, NAMPT overexpression promoted xenografted tumor growth and apoptosis in nude mice, while 14-3-3ζ inhibition attenuated its effect. Collectively, our data demonstrate that NAMPT contributes to tamoxifen resistance through regulation of 14-3-3ζ expression and PKM2 translocation.     

Retracted: miR-150 might inhibit cell proliferation and promote cell apoptosis by targeting LMO4 in Burkitt lymphoma

This study aimed at investigating the effect of microRNA-150 (miR-150) on cell proliferation of Burkitt lymphoma and its molecular mechanism. Gene expression analysis was applied to identify target genes of miR-150 in Burkitt lymphoma cell line ST486 based on the dataset from the Gene Expression Omnibus (GEO) datasets GSE86432. miRNA mimics, inhibitor and small interfering RNA (siRNA) were fluorescently labeled by Cy3, whereas plasmid vector was labeled by EGFP. Cells were viewed by fluorescence microscope and transfection efficiency was evaluated through fluorescent cell percentage. Quantitative real-time polymerase chain reaction analysis (qRT-PCR) and western blot were applied to detect the expression level of miR-150 and LMO4. Cell proliferation, cell cycle, and apoptosis were explored by CCK-8, flow cytometry. Targeting relationship was validated by the Luciferase reporter assay. Tumor xenograft and immunohistochemical analysis were conducted in nude mice model. In Burkitt lymphoma cells, miR-150 expression was significantly lower than normal ones, whereas the expression of LMO4 was upregulated. miR-150 might inhibit cell proliferation and promoted apoptosis in Burkitt lymphoma deterioration by downregulating LMO4. The results of tumor xenograft further confirmed the role of miR-150 in Burkitt lymphoma. Targeting LMO4 is a significant mechanism by which miR-150 suppresses cell growth and promotes apoptosis in Burkitt lymphoma cells, thus may provide a novel target for Burkitt lymphoma therapy in the future.     

Proteomic identification of hippocalcin and its protective role in heatstroke-induced hypothalamic injury in mice

Heatstroke is a devastating condition that is characterized by severe hyperthermia and central nervous system dysfunction. However, the mechanism of thermoregulatory center dysfunction of the hypothalamus in heatstroke is unclear. In this study, we established a heatstroke mouse model and a heat-stressed neuronal cellular model on the pheochromocytoma-12 (PC12) cell line. These models revealed that HS promoted obvious neuronal injury in the hypothalamus, with high pathological scores. In addition, PC12 cell apoptosis was evident by decreased cell viability, increased caspase-3 activity, and high apoptosis rates. Furthermore, 14 differentially expressed proteins in the hypothalamus were analyzed by fluorescence two-dimensional difference gel electrophoresis and identified by matrix-assisted laser desorption ionization time-of-flight mass spectrometry. Expression changes in hippocalcin (HPAC), a downregulated neuron-specific calcium-binding protein, were confirmed in the hypothalamus of the heatstroke mice and heat-stressed PC12 cells by immunochemistry and western blot. Moreover, HPAC overexpression and HPAC-targeted small interfering RNA experiments revealed that HPAC functioned as an antiapoptotic protein in heat-stressed PC12 cells and hypothalamic injury. Lastly, ulinastatin (UTI), a cell-protective drug that is clinically used to treat patients with heatstroke, was used in vitro and in vivo to confirm the role of HPAC; UTI inhibited heat stress (HS)-induced downregulation of HPAC expression, protected hypothalamic neurons and PC12 cells from HS-induced apoptosis and increased heat tolerance in the heatstroke animals. In summary, our study has uncovered and demonstrated the protective role of HPAC in heatstroke-induced hypothalamic injury in mice.     

Atomistic modelling of interface structure and deformation mechanisms in the Al/GaN multilayer under compression

The properties of ohmic contact and thermal boundary conductance between Al and GaN have been studied extensively, but the interface structures and deformation mechanisms in the Al/GaN multilayer can be rarely found in literatures. By molecular dynamics (MD) simulations, we systematically studied the interface structures and structural deformations in the Al/GaN multilayer. Two kinds of interface structures are identified according to the different terminal surfaces of GaN; glide-set terminal interface and shuffle-set terminal interface. Further analysis shows that interface has the maximum stress and misfit lines have the maximum stress values, which serve as the dislocation sources in the Al layer due to the larger stress in the interface. The mechanical responses of the Al/GaN multilayer exhibit a minor stage and some distinctive drops in the stress–strain curve. The first stage is associated with the dislocation nucleation from the interface. Upon further compression, more slip systems appear in the Al layer and dislocation nucleation in GaN could induce drops in curves. Meanwhile, the multiplications of dislocations cause strain hardening behaviours.