Ion Implantation Hampers Pollen Tube Growth and Disrupts Actin Cytoskeleton Organization in Pollen Tubes of Pinus thunbergii

Pollen grains of Pinus thunbergii Parl. （Japanese black pine） were implanted with 30 keV nitrogen ion beams and the effects of nitrogen ion implantation on pollen tube growth in vitro and the organization of actin cytoskeleton in the pollen tube cell were investigated using a confocal laser scanning microscope after fluorescence labeling. Treatment with ion implantation significantly blocked pollen tube growth. Confocal microscopy showed that ion implantation disrupted actin filament cytoskeleton organization in the pollen tube. It was found that there was a distinct correlation between the inhibition of pollen tube growth and the disruption of actin cytoskeleton organization, indicating that an intact actin cytoskeleton is essential for continuous pollen tube elongation in Pinus thunbergii. Although the detailed mechanism for the ion-implantation-induced bioeffect still remains to be elucidated, the present study assumes that the cytoskeleton system in pollen grains may provide a key target in response to ion beam implantation and is involved in mediating certain subsequent cytological changes.

ITF对PAF引起的肠上皮细胞骨架F-actin破坏的抑制作用

目的:探讨血小板活化因子(PAF)对肠上皮细胞骨架F-actin的影响以及肠三叶因子(ITF)对此影响的抑制作用.方法:体外培养人结肠腺癌细胞株Caco-2,分为4组.对照组:不加刺激物及干预因素;实验组:加入PAF,终浓度分别为0、50、100和200nmol/L,作用24h;PAF100nmol/L,分别作用0、2、4、8、12、24、48h;ITF预防组:先加入ITF0.3mol/L,30min后加入PAF100nmol/L;ITF治疗组:先加入PAF100nmol/L,30min后加入ITF0.3mol/L,24h后进行实验.应用跨上皮电阻(TEER)反映肠上皮细胞屏障通透性;免疫荧光染色法观察F-actin的定位、重排以及形态学变化;流式细胞术对F-actin蛋白进行定量分析.结果:给予50nmol/LPAF,作用8-12h即可引起TEER的下降,PAF100nmol/L作用24h,TEER降到最低点,与对照组相比,差异显著(232.75/cm2±15.74/cm2vs346.75/cm2±26.69/cm2,P<0.01);预防或治疗性给予ITF,TEER有所恢复,与模型组相比,差异显著(313.75/cm2±18.28/cm2,299/cm2±13.16/cm2vs232.75/cm2±15.74/cm2,均P<0.01).TRITC-phalloidin直接免疫荧光染色显示正常Caco-2细胞,F-actin主要环绕于细胞周边,排列紧密圆滑,无明显间隙,细胞界限清晰.PAF100nmol/L作用24h后,F-actin出现重排,断裂,周边肌动蛋白丝带模糊,部分细胞出现横跨细胞的应力纤维结构.预防或治疗性给予ITF后,具有正常F-actin染色的细胞比例增加,周边肌动蛋白丝带逐渐清晰,胞质内应力纤维减少,但环点状断裂未完全修复.预防组作用更强.以TRITC-phalloidin的相对平均荧光强度表示F-actin的含量,经流式细胞仪检测发现PAF100nmol/L作用24h后,F-actin含量明显减少(218.56±23.18vs425.35±40.31,P<0.01),给予ITF后F-actin的含量有所增加,与模型组相比差异显著(391.76±58.57,360.86±8.68vs218.56±23.18,均P<0.01),但仍低于对照组.结论:PAF可以改变肠上皮细胞骨架F-actin的定位及定量,从而影响肠上皮细胞屏障功能;ITF可以通过抑制F-actin重排,恢复F-actin蛋白定量而稳定细胞骨架.

F-actin重构对树突状细胞形态和功能影响的研究进展

树突状细胞(Dendritic cells,DCs)是目前发现的最有效的抗原提呈细胞,在启动和放大先天性及适应性免疫应答中发挥重要的作用。在其整个生命过程中,它的细胞形态、迁移与黏附、抗原捕获及抗原提呈等多方面与细胞骨架的动态重构存在密切的关系。细胞骨架的动态重构是一个由多种细胞骨架蛋白共同参与调节的复杂的结构体系,随着研究的不断深入,人们对这种结构体系的认知越来越清晰。基于这些研究,本文综述了纤维状肌动蛋白(Filamentous actin,F-actin)重构对树突状细胞形态和功能的影响。

腺病毒介导的shRNA下调PTEN表达对活化肝星状细胞骨架蛋白F-actin的影响

目的:探讨腺病毒介导的shRNA下调第10号染色体缺失的磷酸酶张力蛋白同源物(PTEN)基因表达对体外培养的活化肝星状细胞(HSC)纤丝状肌动蛋白(F-actin)的影响。方法:体外培养大鼠活化HSC(HSCT6),将携带靶向PTEN的RNA干扰序列[短发夹RNA(shRNA)]并表达绿色荧光蛋白(GFP)的重组腺病毒AdshRNA/PTEN及仅表达GFP的对照空病毒Ad-GFP转染HSC,实时荧光定量PCR及Western blotting实验检测HSC的PTEN mRNA及蛋白表达;利用激光扫描共聚焦显微镜检测HSC的形态、F-actin的分布及荧光强度、伪足以及应力纤维的变化,并采用钙荧光探针Rhod-2/AM负载检测HSC内Ca^(2+)浓度的变化。实验分为对照(control)组(在腺病毒转染步骤以DMEM代替腺病毒液)、Ad-GFP组(转染表达GFP的空病毒Ad-GFP)和Ad-shRNA/PTEN组(转染重组腺病毒Ad-shRNA/PTEN)。结果:靶向PTEN的shRNA成功转染体外活化HSC,显著下调HSC的PTEN mRNA及蛋白表达(P<0.05);PTEN表达下调使活化HSC呈星形向四周伸展,F-actin排列紧密规则,数量增多,伪足充分向外伸展,应力纤维丝增长增粗;Ad-shRNA/PTEN组F-actin的荧光强度较control组及Ad-GFP组显著增强(P<0.05),而control组与Ad-GFP组间差异无统计学显著性;Ad-shRNA/PTEN组HSC内Ca^(2+)浓度较control组及Ad-GFP组明显升高(P<0.05),而control组与Ad-GFP组间差异无统计学显著性。结论:PTEN表达下调使体外活化肝星状细胞骨架蛋白F-actin的形成及细胞骨架的重构增强,并增加了HSC内的Ca^2浓度。

洋水仙花粉和花粉原生质体中肌动蛋白微丝分布变化的共焦显微镜观察

用荧光标记的鬼笔环肽作为肌动蛋白微丝的探针,结合共焦显微镜技术,观察了洋水仙(Narcissus cyclamineus)花粉及花粉原生质体中微丝骨架的分布变化情形。在水合而未萌发的花粉粒中,存在于周质的微丝束多数与花粉粒的长轴呈直角排列。但在萌发沟部位,微丝束的排列则呈网状。在花粉粒的周质至中央部位,微丝束形成另一种形式的网络,在结构上比在萌发沟部位的网络疏松。当花粉开始萌发时,存在于花粉粒内的微丝束逐步转变为平行排列状,并向花粉管伸长的方向延伸和聚集。在脱壁后的花粉原生质体内,微丝束经过重组形成一个结构复杂和排列紧密的网络。原生质体经低渗爆破处理或Triton X-100等过程抽提离析,在遗留下来的膜层上仍然可以见到微丝束残迹,显示微丝与膜层关系密切。用双染法同时显示微管和微丝,表明两者的分布有重叠现象,说明微管和微丝骨架的分布并不是随机的,而可能是由同一种结构或机制控制着。

肺炎链球菌触发肺Ⅱ型上皮细胞微丝肌动蛋白重排的钙信号转导机制

目的通过体外实验研究肺炎链球菌(S.pn)是否可通过肺型上皮细胞(A549)钙信号转导途径触发微丝肌动蛋白(F-actin)细胞骨架重排,进而导致S.pn对A549细胞的侵袭。方法采用F-actin特异性FITC-phalloidin荧光染料,观察S.pn作用A549细胞前后F-actin细胞骨架重排情况,以重排百分率表示;用F-actin细胞骨架重排抑制剂细胞松弛素D预处理A549细胞,观察S.pn对A549细胞的侵袭;使用Ca2+信号转导抑制剂dantrolene预处理A549细胞,观察其与F-actin细胞骨架重排百分率间是否存在剂量依赖关系;用Fura-2/AM荧光探针负载A549细胞后测定S.pn粘附A549细胞30、60、90 min的胞内[Ca2+]i。结果S.pn作用A549细胞后,经FITC-phalloidin荧光染色,F-actin细胞骨架呈黄绿色块状聚集;F-actin细胞骨架重排抑制剂细胞松弛素D可明显降低S.pn对A549细胞的侵袭,在其浓度为0.25 μg/ml时,未得到可测的细菌数;Ca2+信号转导抑制剂可部分抑制A549细胞F-actin细胞骨架重排,且与F-actin细胞骨架重排百分率间存在量效关系;S.pn粘附A549细胞30、60、90 min后的胞内[Ca2+]i高于对照[(187.4±17.3 nmol/L)],并达到饱和,分别为(487.5±38.1)、(548.2±35.6)和(557.2±47.5)nmol/L。结论S.pn可通过Ca2+细胞信号转导途径触发A549细胞F-actin细胞骨架重排,进?

Formins蛋白的结构及其功能

Form ins蛋白是一类结构蛋白,它的生物学功能与肌动蛋白密切相关。其基本结构除了FH 1和FH 2结构域以外,动物和真菌中还具有FH 3、双螺旋结构域等等,而在植物中则没有。根据蛋白N端有无信号肽和跨膜结构域,植物中的Form ins蛋白被典型地分为I、II二类。Form ins蛋白分布广泛,在拟南芥和水稻中分别预测出有21个和16个Form ins蛋白的存在。Form ins蛋白的生物学功能主要表现在参与了肌动蛋白的组装以及作为信号传递链的组成部分。

小鼠树突细胞成熟前后的形态及其微丝蛋白的适应性改变

目的研究树突细胞(DC)成熟前后的形态及其微丝蛋白的适应性变化。方法经重组小鼠粒细胞-巨噬细胞集落刺激因子、白细胞介素-4诱导小鼠骨髓单核细胞为未成熟树突细胞,培养至第6天时,用脂多糖(LPS)诱导成熟树突细胞(mDC),在倒置相差显微镜和荧光显微镜下观察并前后对比分析细胞在成熟前后的表面突起和内部微丝蛋白的变化。结果 mDC高表达CD11c、MHC-Ⅱ和CD86。成熟前的DC体积较小,随着细胞的成熟,直径逐渐增大。成熟过程中,DC表面突起逐渐增多、变粗且变长,呈怒张状,在第7天达到高峰,以后突起逐渐松弛变软,最后又回复至短细、稀疏状态。微丝蛋白主要集中于细胞膜和触突上,其平均荧光强度在LPS刺激24h后最高,48h后明显降低;细胞内F-肌动蛋白在成熟过程中逐渐减低,LPS刺激16h后达高峰,以后细胞内又重新出现F-肌动蛋白的表达,且与细胞膜、突起间基本均匀一致。结论树突细胞体积增大,突起增多增长,密度加大,旨在尽可能地增大细胞的表面积,最大限度地发挥DC提取、抗原呈递的功能;细胞核增大,暗示细胞核在抗原的处理、加工过程中发挥着重要的作用。

肾小球足细胞骨架蛋白的研究进展

足细胞是肾小球滤过屏障的重要组成部分,结构独特复杂。足细胞的细胞骨架决定着其形态、结构及对环境刺激的应答能力。足细胞突起部分由初级及次级突触构成。初级突触中的细胞骨架主要有微管与中间丝,次级突触即足突骨架则由肌动蛋白微丝组成。足细胞骨架蛋白受损会导致蛋白尿及肾小球疾病。而与细胞骨架成分有关的肾小球疾病,均可能在此亚细胞结构上寻找到治疗靶点。

The Role of Host Cytoskeleton in Flavivirus Infection

The family of flaviviruses is one of the most medically important groups of emerging arthropod-borne viruses. Host cell cytoskeletons have been reported to have close contact with flaviviruses during virus entry, intracellular transport, replication, and egress process, although many detailed mechanisms are still unclear. This article provides a brief overview of the function of the most prominent flaviviruses-induced or-hijacked cytoskeletal structures including actin, microtubules and intermediate filaments, mainly focus on infection by dengue virus, Zika virus and West Nile virus. We suggest that virus interaction with host cytoskeleton to be an interesting area of future research.

New Insights into Dynamic Actin-Based Chloroplast Photorelocation Movement

Chloroplast movement is essential for plants to survive under various environmental light conditions. Photo- tropins--plant-specific blue-light-activated receptor kinases--mediate the response by perceiving light intensity and direction. Recently, novel chloroplast actin （cp-actin） filaments have been identified as playing a pivotal role in the directional chloroplast photorelocation movement. Encouraging progress has recently been made in this field of research through molecular genetics and cell biological analyses. This review describes factors that have been identified as being involved in chloroplast movement and their roles in the regulation of cp-actin filaments, thus providing a basis for reflection on their biochemical activities and functions.

The kinesin-like proteins, KAC1/2, regulate actin dynamics underlying chloroplast light-avoidance in Physcomitrella patens

In plants, light determines chloroplast position; these organelles show avoidance and accumulation re- sponses in high and low fluence-rate light, respectively. Chloroplast motility in response to light is driven by cytoskeletal elements. The actin cytoskeleton mediates chloroplast photorelocation responses in Arabidopsis thali- ana. In contrast, in the moss Physcomitrella patens, both, actin filaments and microtubules can transport chloroplasts. Because of the surprising evidence that two kinesin-like proteins （called KACs） are important for actin-dependent chloroplast photorelocation in vascular plants, we wanted to determine the cytoskeletal system responsible for the function of these proteins in moss. We performed gene- specific silencing using RNA interference in P. patens. We confirmed existing reports using gene knockouts, that PpKAC1 and PpKAC2 are required for chloroplast dispersion under uniform white light conditions, and that the two proteins are functionally equivalent. To address the specificcytoskeletal elements responsible for motility, this loss-of- function approach was combined with cytoskeleton-targeted drug studies. We found that, in P. patens, these KACs mediate the chloroplast light-avoidance response in an actin filament- dependent, rather than a microtubule-dependent manner. Using correlation-decay analysis of cytoskeletal dynamics, we found that PpKAC stabilizes cortical actin filaments, but has no effect on microtubule dynamics.

宿主细胞骨架与内膜网络重构调控病毒复制

病毒性疾病的日益频繁暴发严重危害全球人类健康和经济发展.病毒感染的一个共同特征是重塑宿主细胞的膜结构和细胞骨架结构,形成用于病毒基因组复制的特化亚细胞结构,称为病毒工厂.不同的病毒可能会挟持不同的宿主细胞器进行膜修饰形成形态各异的复制工厂,包括病毒质体、小球体、双膜囊泡、管状体和细胞核病毒工厂.三种细胞骨架微丝、微管、中间丝形态在病毒复制过程中也会发生剧烈重塑,形成笼状结构包裹病毒工厂,包括肌动蛋白环、微管笼和中间丝笼.本文系统描述了病毒复制阶段病毒工厂的形成过程及细胞骨架组分和膜组分的形态学变化,重点阐述了三种细胞骨架及其相关蛋白在病毒工厂建立过程中的物质运输、物理支撑、和生化调控功能,简要介绍了相关研究技术手段,并讨论了病毒感染背景下病毒组分-细胞内膜-细胞骨架三者相互作用的重要性和未来研究方向.

冠状病毒与宿主细胞骨架相互作用的研究进展

冠状病毒是所有RNA病毒中基因组最大的正链RNA病毒,仅感染脊椎动物,与多种动物和人类的疫病有关。在冠状病毒入侵、细胞内复制、组装、运输及出芽释放过程中,宿主细胞骨架与冠状病毒密切接触。本文对冠状病毒诱导或劫持的细胞骨架结构(包括肌动蛋白、微管和中间纤维)机制作简要概述,为进一步深入研究细胞骨架在病毒感染中的作用机制提供参考。

At FH16, an Arabidopsis Type II Formin, Binds and Bundles both Microflaments and Microtubules, and Preferentially Binds to Microtubules

Formins are well-known regulators that participate in the organization of the actin cytoskeleton in organisms. The Arabidopsis thaliana L. genome encodes 21 formins, which can be divided into two distinct subfamilies. However, type II formins have to date been less well characterized. Here, we cloned a type II formin, AtFH16, and characterized its biochemical activities on actin and microtubule dynamics. The results show that the FH1 FH2 structure of AtFH16 cannot nucleate actin polymerization efficiently, but can bind and bundle microfilaments. AtFH16 FHIFH2 is also able to bind and bundle microtubules, and preferentially binds microtubules over microfilaments in vitro, in addition, AtFH16 FHIFH2 co-localizes with microtubules in onion epidermal cells, indicating a higher binding affinity of AtFH16 FHIFH2 for microtubules rather than microfilaments in vivo. In conclusion, AtFH16 is able to interact with both microfilaments and microtubules, suggesting that AtFH16 probably functions as a bifunctional protein, and may thus participate in plant cellular processes.

细胞骨架在植物抗锈病中的作用

锈菌是真菌中一个很大的类群,由锈菌侵染引起的病害可造成世界范围内大多数重要作物锈病的大流行和严重的产量损失。细胞骨架包括微管和微丝,在植物生命活动中担负着复杂的生理功能。越来越多的实验证明,细胞骨架在植物抗锈病中起着重要的作用。该文着重对国内外有关植物与锈菌相互作用过程中细胞骨架重组、活性氧积累、过敏性坏死反应发生、细胞骨架结合蛋白功能、细胞信号转导方面的研究进展进行综述,为深入了解植物抗锈性遗传机制并最终应用于植物锈病的防治奠定基础。

Cytoskeletal changes in diseases of the nervous system

The neuronal cytoskeleton not only provides the structural backbone of neurons, but also plays a fundamental role in maintaining neuronal functions. Dysregulation of neuronal architecture is evident in both injury and diseases of the central nervous system. These changes often result in the disruption of protein trafficking, loss of synapses and the death of neurons, ultimately impacting on signal transmission and manifesting in the disease phenotype. Furthermore, mutations in cytoskeletal proteins have been implicated in numerous diseases and, in some cases, identified as the cause of the disease, highlighting the critical role of the cytoskeleton in disease pathology. This review focuses on the role of cytoskeletal proteins in the pathology of mental disorders, neurodegenerative diseases and motor function deficits. In particular, we illustrate how cytoskeletal proteins can be directly linked to disease pathology and progression.