Expression of Escherichia coli Min system in Bacillus subtilis and its effect on cell division

In both rod-shaped Bacillus subtilis and Escherichia coli cells, Min proteins are involved in the regulation of division septa formation. In E. coli , dynamic oscillation of MinCD inhibitory complex and MinE, a topological specificity protein, prevents improper polar septation. However, in B. subtilis no MinE is present and no oscillation of Min proteins can be observed. The function of MinE is substituted by that of an unrelated DivIVA protein, which targets MinCD to division sites and retains them at the cell poles. We inspected cell division when the E. coli Min system was introduced into B. subtilis cells. Expression of these heterologous Min proteins resulted in cell elongation. We demonstrate here that E. coli MinD can partially substitute for the function of its B. subtilis protein counterpart. Moreover, E. coli MinD was observed to have similar helical localization as B. subtilis MinD.     

Polyspermy in angiosperms: Its contribution to polyploid formation and speciation

Polyploidization has played a major role in the long‐term diversification and evolutionary success of angiosperms. Triploid formation among diploid plants, which is generally considered to be achieved by fertilization of an unreduced gamete with a reduced one, has been accepted as a means of polyploid production. In addition, it has been supposed that polyspermy also contributes to the triploid formation in maize, wheat, and some orchids; however, such a mechanism has been considered uncommon because reproducing the polyspermic situation and unambiguously investigating developmental profiles of polyspermic zygotes are difficult. To overcome these problems, rice polyspermic zygotes have been successfully produced by electrofusion of an egg cell with two sperm cells, and their developmental profiles have been monitored. The triploid zygotes progress through karyogamy and divide into two‐celled embryos via a typical bipolar mitotic division; the two‐celled embryos further develop into triploid plants, indicating that polyspermic plant zygotes, unlike those of animals, can develop normally. Furthermore, progenies consisting of triparental genetic materials have been successfully obtained in Arabidopsis through the pollination of two different kinds of male parents with a female parent. These different pieces of evidence for development and emergence of polyspermic zygotes in vitro and in planta suggest that polyspermy is a key event in polyploidization and species diversification.     

Seasonal dynamic of plant phenophases in Beijing—A case study in Beijing Botanical Garden

季节性是北京植物景观的典型特征, 而个体物候是植物景观季节动态的基础。该研究基于北京植物园内120种落叶树种的周年物候数据, 对北京植物景观的物候季节动态进行分析。物候观测以中国物候观测法为标准, 采用a、b、c三级物候代码进行物候记录; 数据分析以二十四节气中的候(5日)为基本时间变量, 基于频率分布型法探究北京物候季节划分及其物候构成动态, 基于SPSS 20.0频数分布统计等探究各类物候现象发生期及持续期的时间分布特征等。物候季节划分及物候构成特征结果为: 6-19候为春, 物候期发生频数占全年总量的54.03%, 以发芽、展叶、开花为主要物候特征, 后期有少数树种结果; 20-45候为夏, 物候量占全年的12.95%, 此期全部观测树种完成展叶, 春花树种进入结果期, 并有较少夏花开放及秋色叶出现; 46-59候为秋, 物候量占全年的27.19%, 以秋色叶及落叶物候为主并伴有较少结果和开花物候发生; 60候至次年春季起始前为冬, 其中60-72候物候量仅占全年的0.6%, 全为落叶物候。各类物候期的时间分布特征如下: 展叶物候期分布于3-23候, 华北珍珠梅(Sorbaria kirilowii)、旱柳(Salix matsudana)等展叶最早, 展叶期平均持续3.27候。秋色物候期分布于40-63候, 49-56候为最佳观赏期, 蒙椴(Tilia mongolica)、山杏(Armeniaca sibirica)等最早显秋色; 秋色期平均持续8.2候, 卫矛(Euonymus alatus)、接骨木(Sambucus williamsii)等秋色期较长。叶幕期平均持续44.2候, 糯米条(Abelia chinensis)、旱柳、棣棠(Kerria japonica)等叶幕期最长。花物候期分布于1-53候, 始花期为1-41候, 盛花期平均发生于始花后1.81候, 8-23候为集中观赏期, 蜡梅(Chimonanthus praecox)、迎春(Jasminum nudiflorum)、榆(Ulmus pumila)、毛白杨(Populus tomentosa)等开花最早, 木香薷(Elsholtzia stauntoni)开花最晚; 花期平均持续 6.7候, 华北珍珠梅、木槿(Hibiscus syriacus)、紫薇(Lagerstroemia indica)等夏秋开花树种花期最长。果物候期分布于8-59候, 榆、郁香忍冬(Lonicera fragrantissima)等果实成熟最早; 持果期平均持续29.0候, 果实宿存树种及黑果荚蒾(Viburnum melanocarpum)、‘金叶’风箱果(Physocarpus opulifolius ‘Luteus’)等具有较长的果实观赏期。与20世纪80年代同类研究结果对比分析, 北京2017年的物候季节与30年前相比, 入春提早1候, 夏季延长4候, 入秋延后3候, 秋季缩短2候, 且不同季节持续期长短的差距加大。     

Factors promoting sustained divisions of mesophyll protoplasts isolated from dihaploid clones of potato (Solanum tuberosum L.) and a cytological analysis of regenerated plants

A culture protocol has been developed for mesophyll protoplasts isolated from various dihaploid clones of potato. A special effort was made to promote the growth of initially dividing cells to form cell colonies and calli. An increase in plating efficiency in 3 different dihaploid clones and one doubled dihaploid clone was obtained after serial dilution of cultures with a suitable amount and type of medium at different stages of cell colony development. Plating on a refined semi-solid medium after 14 days of culture further improved both the yield and the quality of calli obtained. The refined plating medium also enhanced shoot regeneration ability from 67 to 90% in one of the dihaploid clones (67:9). The refined culture protocol could also be used without causing a decrease in plating efficiency at a low population density adjusted after 3 days of culture. The ploidy level of plants regenerated from dihaploid protoplasts were determined by chromosome counting and DNA analysis by flow cytometry. Most of the plants were aneuploid or tetraploid although, some dihaploid plants were obtained after protoplast culture of 2 dihaploid clones derived from the same cultivar (cv. Stina).Abbreviations BA benzyladenine - 2,4-D dichlorophenoxyacetic acid - GA₃ gibberellic acid - NAA naphthaleneacetic acid     

Cell division events are essential for embryo patterning and morphogenesis: studies on dominant-negative cdc2aAt mutants of arabidopsis

During plant development, cell division events are coordinately regulated, leading to specific growth patterns. Experimental evidence indicates that the morphogenetic controls that act at the vegetative plant growth stage are flexible and tolerate distortions in patterns and frequencies of cell division. To address questions concerning the relationship between cell division and embryo formation, a novel experimental approach was used. The frequencies of cell division were reduced exclusively during embryo development of Arabidopsis by the expression of a dominant cdc2a mutant. The five independent transgenic lines with the highest levels of the mutant cdc2a affected embryo formation. In the C13 line, seeds failed to germinate. The C1, C5 and C12 lines displayed a range of distortions on the apical-basal embryo pattern. In the C3 line, the shoot apical meristem of the seedlings produced leaves defective in growth and with an incorrect phyllotactic pattern. The results demonstrate that rates of cell division do not dictate cellular differentiation of embryos. Nevertheless, whereas cell divisions are uncoupled from vegetative development, they are instrumental in elaborating embryo structures and modulating embryo and seedling morphogenesis.     

衣藻叶绿体分裂基因CrFtsZ1在E.coli中的表达

FtsZ蛋白在细菌的分裂中起着重要作用,能够在分裂位点形成一个环状结构而控制细菌的分裂过程。细胞内FtsZ蛋白浓度的明显降低或异常升高均可阻断正常的细胞分裂过程进而导致丝状菌体的产生。为了研究衣藻叶绿体分裂基因ftsZ的功能,构建了衣藻CrFtsZ1的原核表达重组质粒。试验结果表明,衣藻ftsZ的表达严重影响了大肠杆菌的分裂,初步证明衣藻FtsZ蛋白不仅与E．coli FtsZ蛋白在序列上相似,而且也有着相似的功能,同时这一结果也为真核细胞中质体的内共生起源提供了直接的证据。     

不同温度下酿酒酵母细胞分裂周期蛋白Cdc5在有丝分裂中的分子动力学研究

[目的] 探究不同温度下酿酒酵母细胞分裂周期蛋白Cdc5蛋白在有丝分裂中的分子动力学变化。[方法] 本研究以酿酒酵母（Saccharomyces cerevisiae）为材料,采用活细胞成像的方法,探究Cdc5蛋白在不同温度下在酿酒酵母有丝分裂过程中的精细分子动力学变化;通过测量OD₅₉₅绘制生长曲线图,看其宏观的分裂情况是否与微观下Cdc5蛋白的分子动力学变化一致;利用流式细胞术检测细胞的细胞周期变化的情况。[结果] 在胞质分裂时,Cdc5蛋白从母细胞进入子细胞,并在芽颈处发生聚集。25℃条件下细胞中Cdc5蛋白在芽颈处的聚集时间长,37℃条件下Cdc5蛋白在芽颈处聚集时间短,两者间存在显著差异;但两个温度下,细胞中Cdc5蛋白的表达量没有显著性差异。同时,温度也会影响Cdc5蛋白在降解过程中的动力学行为,包括Cdc5蛋白在母细胞与子细胞中荧光强度峰值出现的次数和时间。生长曲线结果显示,酿酒酵母单一细胞分裂周期的变化影响了其宏观的细胞生长,且酵母分裂速度越快,子细胞长宽比越小;细胞周期结果表明,37℃下Cdc5蛋白的动力学变化与酿酒酵母细胞周期变化一致,酿酒酵母细胞周期从G₀/G₁期进入S期,亦加速了酿酒酵母的分裂。[结论] 本研究首次探究了不同温度下酿酒酵母有丝分裂中Cdc5蛋白的精细分子动力学及对应的酵母的宏观生长情况,结果表明温度会对Cdc5蛋白的动力学产生影响,且其精细分子动力学与酿酒酵母的分裂速度成正相关,该结果为进一步研究其在细胞有丝分裂中的功能提供了前期研究基础。     

成年大鼠纹状体、边缘区和苍白球的计算机三维结构重建

应用计算机图形技术在大鼠脑的连续冠状切片Nissl染色的基础上通过Onyx2超级图形工作站对大鼠脑的纹状体进行了三维重建。结果提示：大鼠纹状体由尾壳核、苍白球和边缘区三部分组成,其中边缘区位于尾壳核和苍白球之间,被二完全包绕;尾壳核呈近似的内凹半球形,嘴尾径最大的为6.2mm;背腹径最大为4.9mm;宽度（冠状平面上的内外径)为3.5mm。从嘴侧到尾侧随着脑平面的增宽,尾壳核逐渐向外侧（即靠近外轮廓的方向）移位。苍白球呈块形,嘴尾径最大为4.4mm,背腹径最大为2.6mm,宽度（冠状平面上的内外径）最大为1.5mm。位于尾壳核的内侧,除内侧外基它三个方向均被尾壳核包绕。边缘区呈现一个片状扇形结构,嘴侧背腹径大,最大为2.2mm,宽约0.17mm;尾侧背腹径小,为0.8mm,宽约0.13mm。同属壳核和苍白球一样,从嘴侧到尾侧随着脑平面的增宽边缘区亦逐渐向外侧（即靠近外轮廓的方向）移位,其移位的幅度亦明显大于脑平面增宽的幅度;整个边缘区从嘴侧到尾侧呈均匀变化,其片状逐渐变宽,长度（背腹径）逐渐变小,从而形成一个盘状结构。     

PTP-S2, a nuclear tyrosine phosphatase, is phosphorylated and excluded from condensed chromosomes during mitosis

PTP-S2 is a tyrosine specific protein phosphatase that binds to DNA and is localized to the nucleus in association with chromatin. It plays a role in the regulation of cell proliferation. Here we show that the subcellular distribution of this protein changes during cell division. While PTP-S2 was localized exclusively to the nucleus in interphase cells, during metaphase and anaphase it was distributed throughout the cytoplasm and excluded from condensed chromosomes. At telophase PTP-S2 began to associate with chromosomes and at cytokinesis it was associated with chromatin in the newly formed nucleus. It was hyperphosphorylated and showed retarded mobility in cells arrested in metaphase. In vitro experiments showed that it was phosphorylated by CK2 resulting in mobility shift. Using a deletion mutant we found that CK2 phosphorylated PTP-S2 in the C-terminal non-catalytic domain. A heparin sensitive kinase from mitotic cell extracts phosphorylated PTP-S2 resulting in mobility shift. These results are consistent with the suggestion that during metaphase PTP-S2 is phosphorylated (possibly by CK2 or a CK2-like enzyme), resulting in its dissociation from chromatin.     

医疗机构分工协作研究综述

尽管政策鼓励医疗机构开展分工协作,但关于分工协作的内容、必要性缺乏研究,没有厘清整合与分工协作的关系,部分效果评价存在一些问题,更缺乏从宏观层面介绍国外开展医疗机构分工协作的情况。文章从医疗机构分工协作定义、分工协作必要性、存在的问题和动力机制、模式效果评价以及国外医疗整合现况等5个方面予以分析,并提出了值得研究的问题。