Plastin在肿瘤中的研究进展CSCD

Plastin是一种肌动蛋白结合蛋白,可与纤维状肌动蛋白结合,使纤维状肌动蛋白相互交联形成紧密的束状结构,起到稳定细胞肌动蛋白骨架以及调节细胞运动的作用。Plastin家族有三种亚型,组织特异性地在哺乳动物体内不同组织细胞中表达,并且在肿瘤内异常表达。研究Plastin家族蛋白与肿瘤之间的关系在肿瘤早期诊断和基因治疗方面都有重要的理论指导意义。本文综述了近年来关于Plastin家族蛋白分子结构、功能特点以及在肿瘤中作用等的相关研究,为该领域的研究提供一定的参考。     

植物肌动蛋白解聚因子ADF的研究进展

肌动蛋白解聚因子/丝切蛋白(actin depolymerizing factor,ADF/cofilin)是一种重要的肌动蛋白结合蛋白。在植物细胞中,ADF/cofilin通过与肌动蛋白相结合,在植物生长发育以及响应外界刺激方面起着重要的作用,以此对各种动态生命活动进行调控。该文对国内外近年来有关ADF/cofilin家族的序列结构特征及定位,与肌动蛋白的互作机制、促进细胞生长、抗生物和非生物逆境胁迫能力等的生物学功能,以及磷酸化作用、环境pH、PIP2对其功能影响的调控模式和作用机制进行了综述,为ADF/cofilin新的抗逆功能机制解析提供参考。     

植物驱动蛋白:从微管阵列到生理活动调控

驱动蛋白(kinesin)是以微管为轨道的分子马达,其催化ATP水解为ADP,将贮藏在ATP分子中的化学能高效地转化为机械能,在细胞形态建成、细胞分裂、细胞运动、胞内物质运输和信号转导等多种生命活动中发挥重要作用。对植物驱动蛋白的研究落后于动物和真菌,其原因不仅由于植物进化出独有的驱动蛋白家族,而且其家族成员数量远多于动物驱动蛋白。该文主要总结了驱动蛋白在微管阵列动态组织,包括周质微管和有丝分裂早前期微管带、纺锤体及成膜体中的角色和功能,以及其对植物生理活动的调控作用。同时对重要经济作物大豆(Glycine max)中的驱动蛋白进行了系统分析、分类及功能预测,发现大豆驱动蛋白数量庞大。结合公共数据库中大豆转录组数据,对部分大豆驱动蛋白进行功能预测,以期对大豆及其它作物驱动蛋白功能研究提供线索和启示。     

玉米成蛋白家族的鉴定与生物信息学分析

成蛋白(formins)在细胞骨架的调控中起着关键作用,并通过该过程参与细胞的动态调控。研究成蛋白对进一步了解真核细胞的生长和形态变化具有重要意义。但玉米(Zea mays)作为一种重要的农作物,其成蛋白家族并未被系统性鉴定以及分析。因此,本文通过对两种模式植物水稻(Oryza sativa)和拟南芥(Arabidopsis thaliana)的成蛋白进行同源性分析,鉴定出玉米中22个成蛋白家族成员,其氨基酸数目为300～1 699 aa,蛋白分子量为36 376.32～184 309.82 kDa,等电点为6.88～9.76。基于它们的结构域组成,这些成员可以分为16个植物Ⅰ类成蛋白,6个植物Ⅱ类成蛋白。亚细胞定位和蛋白互作网络分析结果表明,玉米成蛋白主要定位在细胞质膜上,且主要与抑制蛋白(profilin)以及ROP(rho-related GTPases from plants)蛋白互作。GO功能富集网络分析表明,玉米成蛋白主要参与细胞骨架的组成以及介导肌动蛋白聚合过程。顺式作用元件分析结果表明,玉米成蛋白基因受生长素、赤霉素等激素以及光照、昼夜节律、温度等环境因子的调控,并且都...     

Plastin在肿瘤中的研究进展

Plastin是一种肌动蛋白结合蛋白,可与纤维状肌动蛋白结合,使纤维状肌动蛋白相互交联形成紧密的束状结构,起到稳定细胞肌动蛋白骨架以及调节细胞运动的作用。Plastin家族有三种亚型,组织特异性地在哺乳动物体内不同组织细胞中表达,并且在肿瘤内异常表达。研究Plastin家族蛋白与肿瘤之间的关系在肿瘤早期诊断和基因治疗方面都有重要的理论指导意义。本文综述了近年来关于Plastin家族蛋白分子结构、功能特点以及在肿瘤中作用等的相关研究,为该领域的研究提供一定的参考。     

WRKY转录因子功能研究进展

植物各种诱导型基因的表达主要受特定的转录因子在转录水平上的调控.转录因子结构和功能的研究近年来成为植物分子生物学、细胞分子生物学和分子遗传学研究领域的重要内容.WRKY转录因子在拟南芥中有74个成员,水稻中有100多个成员,在生物胁迫及非生物胁迫方面发挥着非常重要的作用.该文就近年来国内外关于WRKY转录因子家族的结构与起源进化和在植物损伤、衰老、发育及代谢等过程中参与的调控功能,以及在植物防御反应中对防御相关基因表达的调控及参与的植物激素类信号途径等方面的研究进展进行了综述,为全面解析WRKY转录因子家族的结构与功能提供了新的视点.     

钙结合蛋白对花粉生长发育调控研究进展

植物钙结合蛋白存在于花粉管中,通过直接或间接结合Ca~(2+),定位膜结构,形成Ca~(2+)信号通道,发生信号转导,对花粉发育及花粉管的生长起到调控作用。目前已明确以钙调蛋白(CAM)、钙依赖型蛋白激酶(CDPK)、类钙调蛋白(CML)、类钙调素B类蛋白(CBL)和激酶蛋白(CIPK)为主的植物钙结合蛋白在调控花粉发育及花粉管生长方面的重要作用。该文主要对近年来国内外已经明确的各类钙结合蛋白家族以及家族成员间不同的作用机理的研究进展进行综述,并举例阐述了钙结合蛋白家族中各类成员对花粉管特定的作用方式及调控作用,最后对今后相关领域的研究前景进行了展望。     

凝溶胶蛋白基因的生物学功能及其应用研究进展

凝溶胶蛋白(gelsolin,GSN)是Gelsolin/Villin超家族的核心成员,是一种多功能的钙依赖性肌动蛋白结合蛋白,在细胞中Ca^2+和PIP2等多因素的调控下,对细胞凋亡、吞噬功能、肌动蛋白微丝切割、细胞信号转导等方面起着重要的作用。近年来,凝溶胶蛋白还被频繁用于相关疾病的预防、诊断与治疗,但其在调控细胞凋亡、炎症等病理生理中的作用机制还存在些许争议。本研究综述了凝溶胶蛋白的结构特点、生物学功能以及对疾病的诊断和治疗,旨在了解凝溶胶蛋白在生物医学及动物科学等领域的应用以及未来凝溶胶蛋白的发展前景。     

植物多肽信号分子CLE家族

动物中存在众多多肽信号分子,它们在信号转导方面发挥重要作用。近几年,对植物中多肽信号分子的研究取得了重大突破,它们积极参与调控植物生长发育的众多过程,同时也表明多肽信号分子在细胞之间的"交流"过程中发挥作用在进化上是保守的。CLE(CLAVATA3/EMBRYO SURROUNDING REGION)家族是目前植物领域研究较热的多肽信号分子家族,通过对拟南芥CLV3和百日草TDIF等CLE多肽信号分子的研究发现,CLE蛋白在成为有功能活性的信号分子之前,存在翻译后蛋白剪切和修饰的过程,这方面与动物中多肽信使的成熟过程相似。对CLE家族成员的分子特征、生物学功能、翻译后的加工修饰和研究中出现的问题进行综述,并对本领域未来的发展方向作出展望。     

植物膜联蛋白(Annexin)的研究进展

植物膜联蛋白属于D类膜联蛋白是在植物中的一类钙和磷脂结合蛋白。植物膜联蛋白约占植物总蛋白含量的0.1%,与动物膜联蛋白在分子量、氨基酸序列及Ca~(2+)与磷脂结合的能力上,都拥有较高的同源性。植物膜联蛋白的亚细胞定位具有多样性,与胞质Ca~(2+)浓度、细胞所处pH、植物组织及外界环境有关。植物膜联蛋白的表达具有组织特异性,且受到各种生物及非生物因子在转录及翻译后水平的调控。植物膜联蛋白具有与植物肌动蛋白结合、参与钙离子通道形成、膜动力学功能、具有ATPase/GTPase及过氧化物酶活性等生物功能,在植物生长发育及响应逆境胁迫过程中起重要作用。本综述从植物膜联蛋白的进化、结构、亚细胞定位、表达调控和生物学功能方面进行综述,旨在为深入研究植物膜联蛋白的功能及其应用提供参考。     

微流控芯片技术在细胞生物学研究中的应用进展

20世纪90年代以来,微流控芯片技术得到了快速发展。由于具有小型化、集成化、高通量、低消耗、分析快速等特点,微流控芯片作为一种新型的生物学研究平台,能够提供传统方法不具备的精细和可控制的细胞研究条件,在细胞生物学研究领域中得到了广泛关注。该文主要介绍其在细胞培养、分选、裂解、计数、凋亡检测、迁移、单细胞捕获、细胞间作用等方面的研究进展。     

Efficient and Innocuous Live‐Cell Delivery: Making Membrane Barriers Disappear to Enable Cellular Biochemistry

The confluence of protein engineering techniques and delivery protocols are providing new opportunities in cell biology. In particular, techniques that render the membrane of cells transiently permeable make the introduction of nongenetically encodable macromolecular probes into cells possible. This, in turn, can enable the monitoring of intracellular processes in ways that can be both precise and quantitative, ushering an area that one may envision as cellular biochemistry. Herein, the author reviews pioneering examples of such new cell‐based assays, provides evidence that challenges the paradigm that cell penetration is a necessarily damaging and stressful event for cells, and highlights some of the challenges that should be addressed to fully unlock the potential of this nascent field.     

Ultrastructural evidence for two-cell and three-cell neural pathways in the tentacle epidermis of the sea anemone Aiptasia pallida.

Sensory and ganglion cells in the tentacle epidermis of the sea anemone Aiptasia pallida were traced in serial transmission electron micrographs to their synaptic contacts on other cells. Sensory cell synapses were found on spirocytes, muscle cells, and ganglion cells. Ganglion cells, in turn, synapsed on sensory cells, spirocytes, muscle cells, and other neurons and formed en passant axo-axonal synapses. Axonal synapses on nematocytes and gland cells were not traced to their cells of origin, i.e., identified sensory or ganglion cells. Direct synaptic contacts of sensory cells with spirocytes and sensory cells with muscle cells suggest a local two-cell pathway for spirocyst discharge and muscle cell contraction, whereas interjection of a ganglion cell between the sensory and effector cells creates a local three-cell pathway. The network of ganglion cells and their processes allows for a through-conduction system that is interconnected by chemical synapses. Although the sea anemone nervous system is more complex than that of Hydra, it has similar two-cell and three-cell effector pathways that may function in local responses to tentacle contact with food.     

The role of glutamine, serum and energy factors in growth of enterocyte-like cell lines

Background: Glutamine is routinely added to most cell cultures. Glutamine has been found to be the preferential nutrient to the rapidly replicating intestinal mucosa, but whether this is a metabolic effect or due to other properties of this amino acid is not determined. To study the importance of glutamine on the growth of two enterocyte-like cell lines, the effects of depriving the media or supplementing it with glutamine were assessed in media with different serum and energy supplements. Methods: CaCo-2 and HT-29 cells were grown in serum-free medium, with fetal bovine or synthetic serum, and with or without glucose or galactose. The glutamine content was varied between 0 and 4 mM. All growth assays were performed in triplicate by counting in a hemocytometer. Results: Both cell lines were dependent of serum factors for growth, but displayed distinct requirements on glutamine supplementation. Glutamine was an obligate supplement with dose-dependent correlation to growth (r=0.87, p<0.01) for CaCo-2 cells cultured in synthetic, but not in fetal bovine serum. In HT-29 cells, the correlation between glutamine and growth was significant (r=0,68, p<0,05) only in fetal bovine serum in the absence of galactose. Conclusion: This study shows that glutamine has different growth stimulating effects on two enterocyte-like cell lines studied. This could reflect different modes of action of glutamine on proliferation and differentiation in an enterocyte cell population.     

Of mice, frogs and flies: generation of membrane asymmetries in early development

Embryonic development begins with cleavage of the fertilized egg. Cleavage comprises two major processes: cytokinesis and formation of a polarized epithelial cell layer. The focus of this review is comparison of the generation of membrane polarity during embryonic cleavage in three different developmental model systems. In mammalian embryos, as exemplified by analysis of the mouse, generation of distinct membrane domains is uncoupled from cleavage divisions and is initiated in a specific developmental phase, called compaction. In Xenopus laevis embryos, generation of polarized blastomeres occurs simultaneously with cytokinesis. The origin of specific membrane domains of X. laevis polar blastomeres, however, can be traced back to oogenesis. Finally, in Drosophila melanogaster, generation of polarized cells occurs at cellularization. The relevance of cell adhesion, cell junctions and cytocortical scaffolds will be discussed for each of the model systems. Despite enormous morphologic differences, the three models share many common features; in particular, many important molecular interactions are conserved.     

微囊化K562细胞生长周期及代谢特性的研究

以K562细胞为模型,分别进行微囊化和游离培养,运用流式细胞术考察两种培养体系下细胞周期和生长代谢变化;建立数学模型,模拟了两种培养体系下细胞的生长活性和代谢特性。实验发现：微囊化培养过程中的K562细胞处于DNA合成期（S期）的百分含量显著高于游离培养,并且细胞保持较高的增殖活性。模型计算表明,所建模型动力学参数能够很好地描述微囊化和游离两种培养体系下细胞的代谢情况;对细胞活性的理论计算表明,微囊化的细胞具有较高的增殖和代谢活性,同时细胞能够较长时间保持此活性;模型参数表明,两种培养体系下,葡萄糖对细胞生长的影响无显著差别 (k^Free_L≈k^APA_L),乳酸对游离培养细胞的生长具有明显抑制作用,但对微囊化培养细胞抑制作用较小(kFreeL>≈kAPAL)。     

哺乳动物体细胞核移植中供体细胞的研究进展

在哺乳动物体细胞核移植中,供体细胞是影响其效率的主要因素之一。供体细胞的类型、细胞周期、细胞的培养代数、冷藏与冷冻处理,以及供体动物的性别、年龄等都可能影响核移植胚胎的发育。根据现有资料,简要综述了在哺乳动物体细胞核移植中有关供体细胞的研究进展。     

Engineering Cardiac Cell Junctions In Vitro to Study the Intercalated Disc

Abstract

This review article discusses a recent work using engineered cardiac cells to study the function of the intercalated disc putting emphasis on mechanical and electrical coupling.     

Perivascular cells for regenerative medicine

Mesenchymal stem/stromal cells (MSC) are currently the best candidate therapeutic cells for regenerative medicine related to osteoarticular, muscular, vascular and inflammatory diseases, although these cells remain heterogeneous and necessitate a better biological characterization. We and others recently described that MSC originate from two types of perivascular cells, namely pericytes and adventitial cells and contain the in situ counterpart of MSC in developing and adult human organs, which can be prospectively purified using well defined cell surface markers. Pericytes encircle endothelial cells of capillaries and microvessels and express the adhesion molecule CD146 and the PDGFRβ, but lack endothelial and haematopoietic markers such as CD34, CD31, vWF (von Willebrand factor), the ligand for Ulex europaeus 1 (UEA1) and CD45 respectively. The proteoglycan NG2 is a pericyte marker exclusively associated with the arterial system. Besides its expression in smooth muscle cells, smooth muscle actin (αSMA) is also detected in subsets of pericytes. Adventitial cells surround the largest vessels and, opposite to pericytes, are not closely associated to endothelial cells. Adventitial cells express CD34 and lack αSMA and all endothelial and haematopoietic cell markers, as for pericytes. Altogether, pericytes and adventitial perivascular cells express in situ and in culture markers of MSC and display capacities to differentiate towards osteogenic, adipogenic and chondrogenic cell lineages. Importantly, adventitial cells can differentiate into pericyte‐like cells under inductive conditions in vitro. Altogether, using purified perivascular cells instead of MSC may bring higher benefits to regenerative medicine, including the possibility, for the first time, to use these cells uncultured.     

Mammalian testis: a target of in vivo electroporation

Mammalian spermatogenesis consists of three biologically significant processes: stem cell self-renewal and differentiation, meiosis, and haploid cell morphogenesis. Understanding the molecular mechanisms behind these processes might provide clues to the puzzle of species preservation and evolution, and to treatments for male infertility. However, few useful in vitro systems exist to investigate these processes at present. To elucidate these mechanisms, in vivo electroporation of the testis might be a convenient option. Since DNA solution can be injected into the seminiferous tubule via the rete testis, similar to germ cell transplantation, it is easy to transfect expression vectors into various differentiated germ cells and supporting Sertoli cells with adequate electric shock. Unfortunately, it is difficult to create transgenic animals using this method because of its low efficiency. However, gain- and loss-of-function assays, promoter assays, and tagged-protein behavior assays can be conducted with this technique, as in in vitro culture systems.