山豆根叶片光合特性对光强和干旱的响应

山豆根(Euchresta japonica)为我国II级重点保护野生植物。该研究通过设置不同遮阴网的层数和采用不同浓度的聚乙二醇溶液浇灌,探讨了山豆根光合特性对光强和干旱的响应。结果表明, 山豆根叶片的饱和光强为683.06~907.07mmol/(m²·s); 单层遮阴处理叶片的最大电子传递速率和最大净光合速率整体高于双层遮阴处理,其中单层遮阴且未进行干旱处理的叶片最大电子传递速率和最大净光合速率最高,分别为55.36和6.73mmol/(m²·s);相同遮阴条件下,叶片的最大净光合速率及其对应的饱和光强均随干旱程度增加整体呈下降趋势;单层遮阴条件下的蒸腾速率和水分利用效率均整体高于双层遮阴条件下的。不同处理下叶片光系统II的实际光化学效率、光化学猝灭系数以及非光化学猝灭系数等整体上均无显著差异(P>0.05)。山豆根属半阳生植物,其叶片利用弱光能力较强,植株具有较强的耐干旱能力。因此,建议在开展野外回归、迁地保护、人工栽培等工作时,进行适当遮阴处理并保持充足的土壤含水量。     

Promoting effect of IFN-γ on the expression of LPS-induced IL-12 p40 and p35 mRNA in murine suppressor macrophages

We detected the expression of IL-12 p40/p35 mRNA by semi-quantitative RT-PCR and silver staining, and studied the molecular interaction between the IL-12 expression and the NF-κB activation induced by LPS and IFN-γ/LPS in murine peritoneal suppressor macrophages (MPSMs). It was found that IFN-γ strongly enhanced the LPS-induced IL-12 p40 and p35 mRNA expression. Both p40 and p35 mRNA levels were approximately equal. IFN-γ also greatly promoted the LPS-induced secretion of IL-12 p70 in MPSMs. The Proteasome Inhibitor I (PSI) could block the expression of IL-12 p40 and p35 mRNA, and the degradation of κBα induced by LPS or LPS/IFN-γ. EMSA showed that LPS could augment the NF-κB binding activity to p40 promoter DNA. However, IFN-γ could neither enhance the LPS-induced NF-κB activity nor promote the degradation of kBa. Taken together, the data suggest: (i) IFN-γ/LPS could strongly induce the expression of IL-12 p40 and p35 mRNA; both the expression levels were equal; this phenomenon coincided wit     

Promoting effect of IFN-γ on the expression of LPS-induced IL-12 p40 and p35 mRNA in murine suppressor macrophages

We detected the expression of IL-12 p40/p35 mRNA by semi-quantitative RT-PCR and silver staining, and studied the molecular interaction between the IL-12 expression and the NF-eB activation induced by LPS and IFN-γ/LPS in murine peritoneal suppressor macrophages (MPSMs). It was found that IFN-γ strongly enhanced the LPS-induced IL-12 p40 and p35 mRNA expression. Both p40 and p35 mRNA levels were approximately equal. IFN-a also greatly promoted the LPS-induced secretion of IL-12 p70 in MPSMs. The Proteasome Inhibitor I (PSI) could block the expression of IL-12 p40 and p35 mRNA, and the degradation of IκBα induced by LPS or LPS/IFN-γ. EMSA showed that LPS could augment the NF-κB binding activity to p40 promoter DNA. However, IFN-γ could neither enhance the LPS-induced NF-κB activity nor promote the degradation of IκBα. Taken together, the data suggest: (i) IFN-γ/LPS could strongly induce the expression of IL-12 p40 and p35 mRNA; both the expression levels were equal; this phenomenon coincided with the high-level secretion of IL-12 p70 induced by IFN-γ/LPS; (ii) NF-κB signal pathway is essential for IFN-γ/LPS to induce IL-12 mRNA expression; (iii) by blocking the degradation of IκB, the PSI suppresses the IL-12 p40/p35 mRNA expression induced by LPS and IFN-γ/LPS; (iv) NF-κB signal may not be involved in the mechanism by which IFN-γ enhanced the expression of the LPS-induced IL-12 p40/p35 mRNA. The first two authors contributed equally to this work.     

水稻中央细胞发育期间超微结构变化的观察

本文通过透射电镜对水稻受精前胚囊中央细胞发育过程中超微结构的变化进行观察。结果表明,八核胚囊形成后很快就进行细胞化形成7个细胞,其中刚形成的中央细胞由1个大液泡、2个极核（珠孔端和合点端各1个）和一些含有丰富细胞器的胞质组成。中央细胞以后的发育主要是极核的发育和极核周围胞质的变化。极核发育经历以下过程：a．2个核都膨大呈“椭圆”形。核周围胞质呈不对称分布。b．2个核分别向胚囊中央移动并相互靠近。之后2个极核调整排列方式,由纵排（即与胚囊纵轴平行）变成横排。此时期有细胞质“桥”联结珠孔端卵器、2个极核和合点端反足细胞器。c．横排的极核移向卵器,并排列于卵细胞之上。此时胚囊未明显膨大,但极核相靠近的两边核膜有许多处已形成“融合桥”,核周围的胞质也起较大的变化,如质体内淀粉消失和光面内质网增加等。极核进一步发育直至胚囊成熟期间,极核排列方式及其周围胞质组成未观察到明显的变化,但胚囊体积明显增大。     

Double-gating mechanism and diversity of an adenosine triphosphate (ATP)-sensitive K+ channel in neurons acutely dissociated from rat neocortex

Classically, ion channels are classified into 2 groups: chemical-sensitive (ligand-gated) and voltage sensitive channels. Single ATP-sensitive K⁺ (K-ATP) channel currents were recorded in acutely dissociated rat neocortical neurons using patch clamp technique. A type of K-ATP channel has been found to be gated not only by intracellular ATP, but also by membrane potential (V_m), and proved to be a novel mechanism underlying the gating of ion channels, namely bi-gating mechanism. The results also show that the K-ATP channels possess heterogeneity and diversity. These types of K-ATP channels have been identified in 40.12% of all patches, which are different in activation-threshold and voltage-sensitivity. The present experiment studied the type-3 K-ATP channel with a unitary conductance of about 80 pS in detail (n = 15). Taking account of all the available data, a variety of K-ATP channels are suggested to exist in body, and one type of them is bi-gated by both chemical substances and membrane potentials. This property of the K-ATP channels may be related to their pathophysiological function. Project supported by the National Natural Science Foundation of China and Natural Science Foundation of Guangdong Province     

新一代植物表型组学的发展之路

随着多种植物全基因组测序的完成, 科研人员越来越认识到植物表型研究的重要性, 并将其提升至“组学”的高度。植物表型组学是研究植物生长、表现和组成的科学, 能够有效追踪基因型、环境因素和表型之间的联系, 是突破未来作物学研究和应用的关键领域。该文介绍了植物表型采集分析经历的从手工测量计数的初始阶段到特定测量工具的辅助阶段再到高通量表型组学3个阶段; 提出了推动植物表型采集分析发展的3个要素: 表型组学研究设施、表型采集技术及图像数据分析方法; 进而详细阐述了表型组学设施的发展、国际上代表性的设施平台情况以及表型采集传感器和图像数据分析方法的发展, 并展望了植物表型组学未来的研究方向。     

茶树嫩枝扦插的高效方法

茶(Camellia sinensis)是世界上最重要的饮料作物之一, 随着种植面积的扩大, 茶苗的需求量也日益增加。传统的扦插育苗方式存在着生根难、周期长和取材难等问题, 因此优化扦插生根的方法十分重要。该研究以较易获得、但传统方法难以生根的绿色嫩枝为扦插材料, 首先对培养介质进行改良。与土培和水培相比, 利用海绵培养可以使茶树幼嫩插穗在1个月之内快速生根, 生根率达32.2%。其次, 对海绵培方法做进一步优化, 确定一芽一叶的幼嫩短穗生根潜力更佳; 同时, 添加生根粉能够促进茶树茎部愈伤组织与根系的形成, 其中1.25 g?L ^-1生根粉处理48小时对茶树扦插快速生根最有效, 生根率达42.0%。综上, 通过优化培养介质和扦插材料以及适当添加生根粉等措施, 建立了一种茶树高效嫩枝扦插生根的方法。该方法能够显著缩短嫩枝插穗的生根时间, 突破了扦插材料的限制, 有效降低了扦插成本, 具有重要的应用前景。